Opioid Peptides: An Update Editors: Rao S. Rapaka, Ph.D. Division of Preclinical Research National Institute on Drug Abuse Bhola N. Dhawan, M.D. Central Drug Research Institute Lucknow, India NIDA Research Monograph 87 1988 U.S. DEPARTMENT OF HEALTH AND HUMAN SERVICES Public Health Service Alcohol, Drug Abuse, and Mental Health Administration National Institute on Drug Abuse 5600 Fishers Lane Rockville, Maryland 20857 For sale by the Superintendent of Documents, U.S. Government Printing Office Washington, D.C. 20402 5483090Y PUBL NIDA Research Monographs are prepared by the research divisions of the National Institute on Drug Abuse and published by its Office of Science. The primary objective of the series is to provide critical reviews of research problem areas and techniques, the content of state-of-the-art conferences, and integrative research reviews. Its dual publication emphasis is rapid and targeted dissemination to the scientific and professional community. Editorial Advisors MARTIN W. ADLER, Ph.D. Temple University School of Medicine Philadelphia, Pennsylvania SYDNEY ARCHER, Ph.D. Rensselaer Polytechnic Institute Troy, New York RICHARD E. BELLEVILLE, Ph.D. NB Associates, Health Sciences Rockville, Maryland KARST J. BESTEMAN Alcohol and Drug Problems Association of North America Washington, D.C. GILBERT J. BOTVIN, Ph.D. Cornell University Medical College New York, New York JOSEPH V. BRADY, Ph.D. The Johns Hopkins University School of Medicine Baltimore, Maryland THEODORE J. CICERO, Ph.D. Washington University School of Medicine St. Louis, Missouri MARY L. JACOBSON National Federation of Parents for Drug-Free Youth Omaha, Nebraska REESE T. JONES, M.D. Langley Porter Neuropsychiatric Institute San Francisco, California DENISE KANDEL, Ph.D. College of Physicians and Surgeons of Columbia University New York, New York HERBERT KLEBER, M.D. Yale University School of Medicine New Haven, Connecticut RICHARD RUSSO New Jersey State Department of Health Trenton, New Jersey NIDA Research Monograph Series CHARLES R. SCHUSTER, Ph.D. Director, NIDA THEODORE M. PINKERT, M.D, J.D. Acting Associate Director for Science, NIDA Parklawn Building, 5600 Fishers Lane, Rockville, Maryland 20857 Opioid Peptides: An Update ACKNOWLEDGMENT This monograph is based upon papers and discussion from the Indo-U.S. Conference on Recent Progress in the Chemistry and Biology of Biologically Active Peptides With Emphasis on Opioid Peptides, held in Lucknow, India, on February 25-27, 1987. The conference was jointly sponsored by the National Institute on Drug Abuse; the Department of Science and Technology, Government of India; Central Drug Research Institute, Lucknow; and the Indian National Science Academy. COPYRIGHT STATUS The figures on pages 28 and 54 are copyrighted and are reproduced with the permission of the copyright holders. Further reproduction of this copyrighted material is permitted only as part of a reprinting of the entire publication or chapter. For any other use, the copyright holder's permission is required. All other material in this volume is in the public domain and may be used or reproduced without permission from the Institute or the authors. Citation of the source is appreciated. The U. S. Government does not endorse or favor any specific commercial product or company. Trade, proprietary, or company names appearing in this publication are used only because they are. considered essential in the context of the studies reported herein. DHHS publication number (ADM)89-1604 Printed 1988 NIDA Research Monographs are indexed in the Index Medicus. They are selectively included in the coverage of American Statistics Index, BioSciences Information Service, Chemical Abstracts, Current Contents, Psychological Abstracts, and Psychopharmacology Abstracts. iv Preface To bring into focus the rapidly expanding areas of research associated with the opioid peptides, an Indo-U.S. Symposium was held in February 1987 at the Central Drug Research Institute (CDRI), Lucknow, India. This symposium was organized by the National Institute on Drug Abuse (NIDA) and the CDRI and was jointly funded by NIDA; CDRI; the Department of Science and Technology, Government of India‘ and the National Academy of Sciences, New Delhi. A number of individuals were responsible for the success of this conference. MWe especially acknowledge the help of Dr. Phil Schambra, Science attache, U.S. Embassy (India); Mrs Linda A. Vogel, Associate Director for Management and Program Coordination, Office of International Health; Dr. George V. Coelho, Chief, International Activities Program, ADAMHA; at NIDA, Dr. James C. Cooper, Associate Director for Medical and International Affairs; Dr. Marvin Snyder, Director, Division of Preclinical Research; and Dr. Richard L. Hawks, Chief, Research Technology Branch; and at CDRI, Dr. R. Raghubir and Mr. K.L. Gupta. Selected papers from this symposium have appeared as a research monograph published by the CDRI, entitled Recent Progress in Chemistry and Biology of Centrally Acting Peptides. Other" presentations from the symposium, along with contributions from invited authors, comprise the present monograph. We are grateful to all the contributors for their cooperation in preparing this publication. We hope that this volume will serve as a useful reference source on various aspects of the medicinal chemistry, pharmacology, and biochemistry of opioid peptides and will provide new incentives for drug abuse researchers in the opioid peptide field. Rao S. Rapaka Bhola N. Dhawan Contents Preface Neuropeptides, A Personalized History Sidney Udenfriend. : a Synthesis and Biological Activity of Novel Met-enkephalin Analogs Krishna B. Mathur; Balaram J. Dhotre; Shubh D. Sharma; Ram Raghubir; Gyanendra K. Patnaik; and Bhola N. Dhawan . Approaches to Studying Structure-Activity Relationships in Peptide Hormones Through the Expression of Synthetic Genes John W. Taylor. “« $ ww BW BB Ee = X-Ray Diffraction Studies of Enkephalins and Opiates Jane F. Griffin and G. David Smith . Conformational Analysis of Cyclic Opioid Peptide Analogs Peter W. Schiller and Brian C. Wilkes . ns Conformational Studies of Dermorphin V. Renugopalakrishnan and Rao S. Rapaka Use of Molecular Biological Methods to Study Neuropeptides Michael J. Brownstein Three Technical Approaches for Cloning Opioid Receptors Curtis A. Machida; John Salon; David Grandy; James Bunzow; Paul Albert; Eric Hanneman; and Olivier Civelli Effects of Opioid Peptides on Human Neuroblastoma Cells Wolfgang Sadee; Victor C. Yu; and Gunther Hochhaus. Analgesia and Neuropeptides David J. Mayer. Mechanism of Development of Tolerance and Dependence to Opioids in Neuroblastoma x Glioma Hybrid Cells and Mice Shail K. Sharma; Madhav Bhatia; and Ranju Ralhan Development of Spinal Substrate for Nociception in Man Veena Bijlani; Tilat A. Rizvi; and S. Wadhwa. vii . 20 . 41 . 60 . 74 . 83 « 93 «111 .118 BY .167 Differential Effects of Opioid Peptides Administered Intra- cerebrally in Loci of Self-Stimulation Reward of Lateral Hypothalamus and Ventral Tegmental Area-Substantia Nigra Jitendra Singh and T. Desiraju + ®» ow 9 Peptides and Thermoregulation R. Shukla and Bhola N. Dhawan. Endogenous Opioids and Immune Responses: An Experimental Study P. K. Mediratta; N. Das; V. S. Gupta; and P. Sen An Update of Selected Topics in the Biology and Chemistry of Opioid Peptides Rao S. Rapaka; Bhola N. Dhawan; and V. Renugopalakrishnan List of NIDA Research Monographs . viii .180 -J92 .209 217 +233 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D., eds. National Institute on Drug Abuse, 1988 Neuropeptides, A Personalized History Sidney Udenfriend, Ph.D. The full significance of the important roles in neurobiology played by peptides is still emerging. It seems that each day we read of the discovery and characterization of new peptides in extracts of neural tissue. In fact the chemical structures of neuropeptides are now elucidated before their biological significance becomes apparent. What is responsible for this rapidly growing field are the recent advances in microprotein chemistry and molecular biology. Therefore a brief history of peptide chemistry is important to understand how we have advanced in so relatively short a period of time in our ability to isolate and characterize trace amounts of peptides in biological extracts. In this review, I will not differentiate between small peptides and large peptides (proteins). I will also discuss peptides in the nervous system as well as in the endocrine system because of the interrelationship of these two systems. The earliest neuroactive substances to be characterized were the amines and substituted amines--first acetylcholine, then adrenaline, noradrenaline, and serotonin. Although dopamine was known for some time, it was considered to be an intermediate rather than a neuroregulator in its own right until somewhat later. However, in some of the earliest studies (late forties and early fifties) it was recognized that other substances were active in nerve and muscle preparations that were not amines and whose activities were destroyed by proteases. In 1950 peptide chemistry was still emerging as a discipline. While synthetic chemists could synthesize small peptides, methods for their purification, even from synthetic mixtures, were not yet very efficient. Sequencing of peptides had not yet been introduced. In fact, there was still controversy as to whether each peptide and protein was a stoichiometric entity (i.e., had a unique and invariable sequence) or whether a given protein or peptide was composed of molecules each varying somewhat from the other but the average being fairly constant for that peptide. The dipeptides carnosine and anserine had been isolated from muscle. Homocarosine, the GABA analog of carnosine, was found to be uniquely present in brain. However, the high concentration (mg of peptide per g of 1 tissue) and small size of these compounds required no unusual methodology. The first findings that specific proteins have an invariant molecular composition came from end-group analysis when it was shown that the same protein isolated from highly diverse species always had the same amino terminus. Not until the late 1950s, after Fred Sanger had devised a method for elucidating the amino acid sequence of a protein and applied it to insulin, was it generally conceded that all proteins and peptides had exact molecular compositions. Several years later, Vincent du Vigneaud isolated and characterized oxytocin and vasopressin from extracts of the posterior pituitary gland. It should be noted, however, oxytocin and vasopressin are present in relatively large amounts in the pituitary gland (ca 1 pmole/g). Column chromatography became generally available in the late fifties, and Edman introduced the manual procedure for sequencing peptides at about the same time. These procedures were used in the isolation and characterization of angiotensin and bradykinin. In the late sixties Roger Guillemin and Andrew Schally used similar procedures to isolate TRH from hypothalamus. However, the hormone was so potent that to isolate the amounts needed at the time for analysis and sequencing (ca 50 nmoles) they had to extract tons of tissue. This was very costly and time consuming and required all the patience and skill of these two outstanding scientists. At about the same time many other biologically active factors that were apparently peptide in nature were also reported--substance P, many growth factors, including nerve growth factor, and a host of lymphokine activities including the interferons. Isolation and characterization of these had to await newer developments. Several major discoveries and advances in technology in the late sixties and seventies, advances that are still continuing today, completely changed our approach to dealing with biologically active peptides. High performance liquid chromatography (HLPC) with ultrasensitive detection systems made it possible to achieve many thousandfold degrees of purification in a relatively few steps and with relatively small amounts of material. The continued improvement in sensitivity and speed of commercial automated sequenators now make it possible to determine the primary structure of a modest sized peptide within a day, starting with 100 pmole or less of pure material. With monoclonal antibody techniques, it is now possible to prepare specific antibodies to a biologically active peptide while it is still present in a crude mixture. These monoclonal antibodies can then be used for rapid purification of the peptide. With monoclonal antibodies it is frequently unnecessary to actually isolate the biologically active peptide to determine its sequence. When expression vectors are used for cloning the cDNA derived from the tissue of interest, monoclonal antibodies can be used for clone selection. Sequencing is then carried out on specific cDNA from which the primary structure of the peptide precursor can be deduced. Having isolated and determined the sequence of a peptide or its cDNA, the peptide can be readily synthesized for further study. The synthetic peptide can then be used to prepare site directed polyclonal antibodies, which provide additional tools for studying the localization and regulation of that peptide. I would like to briefly discuss some of the developments in the chemistry and biology of neuropeptides that took place in the Roche Institute of Molecular Biology over the past 20 years. Although the structures of oxytocin and vasopressin were already known, it was Sachs and Takabatake (1964) who first demonstrated that each of these was produced as part of a larger polypeptide containing the neurophysin sequence. This information laid the groundwork for the subsequent cloning and sequencing of the cDNAs for oxytocin- neurophysin and vasopressin-neurophysin (Richter 1987). The dipeptide carnosine, which was originally considered to be restricted to muscle, was found to be present in the olfactory bulb by Margolis (1974). Carnosine is now considered to be a transmitter with a presynaptic site of action. This peptide along with the enzyme carnosine synthetase and the degradative enzyme carnosinase are now used as markers of olfactory nerves and to monitor nerve regeneration. Margolis has also isolated, sequenced, and cloned a protein that is uniquely expressed in the olfactory mucosa (Keller and Margolis 1976). In my own laboratory (Bohlen et al 1975) we developed HPLC and introduced the fluorescent reagent, fluorescamine, for high sensitivity. These procedures made possible many studies that were subsequently carried out in our Institute and elsewhere. Shortly after the discovery of the enkephalins, my colleagues and I used the fluorescamine HPLC procedure in the discovery of the prescursor of beta-lipotropin (Rubinstein et al. 1978a). Chromatograms of pituitary extracts revealed a B-endorphin-containing peptide that was larger than beta-lipotropin, about 30K. This appeared simultaneously with the report of Mains et al. (1977), who found that the 30K protein also contained within it the sequence of ACTH. We coined the name proopiocortin for this common precursor of B-endorphin and ACTH. Subsequently, to emphasize the sequences of MSH in the 30K protein, it was renamed pro-opiomelanocortin, now better known as POMC. In their studies in cell culture, Mains and Eipper found that POMC was produced as a glycosylated protein. For this reason it was generally believed that all forms of POMC are glycosylated and that the latter may have something to do with biological activity. However, we showed that in vivo glycosylation is highly variable from individual to individual within a given species. In pituitaries taken from individual camels, we showed that in some glands isolated POMC was almost entirely in the glycosylated form while in others the molecule contained little or no glycosyl residues (Kimura et al. 1979). Apparently in the case of POMC as in other proteins and peptides the significance of glycosylation remains to be determined. It is of interest that Rubinstein, who had isolated POMC, subsequently used the same procedures in my laboratory in collaboration with Pestka to isolate a-interferon from human leukocytes (Rubinstein et al. 1978b). This represented the first purification and characterization of any form of interferon and quite a feat because the amount of interferon in these cells was very small. Although interferon was discovered in the early fifties and many had tried to purify it over the years, it was not until 1978 with the availability of these newer peptide methods that its purification and characterization were achieved. Getting back to the enkephalin pentapeptides, many believed that they were derived from POMC However, we reasoned that POMC could not give rise to free Leu-enkephalin since it did not contain that sequence. Furthermore, although the B-endorphin derived from POMC contained a Met-enkephalin sequence at its amino terminus, there was no known processing site adjacent to this sequence that could lead to its processing to Met-enkephalin. For those reasons we decided to look for other enkephalin-containing compounds that could serve as precursors. We devised a bioassay that involved homogenizing tissue, then treating the extract with trypsin followed by carboxypeptidase B. By analogy with other peptide precursors, we felt that there was a good possibility that the enkephalin sequence within its precursor would be bracketed by pairs of Lys and/or Arg residues, i.e., -Lys-Arg-enkephalin-Lys-Lys. Trypsin cleaves basic residues at their carboxyl termini and would be expected to cleave out a hexapeptide, enkephalin-Lys or enkephalin-Arg. The latter would be converted to free enkephalin by the carboxypeptidase and so detectable by the binding assay. The first application of the above procedure to guinea pig and rat striatum revealed many large peptides from which both Met- and Leu-enkephalin were released on treatment with the two proteases (Lewis et al. 1978). Following a report that bovine adrenal medulla is rich in enkephalins (Schultzberg et al. 1978), we turned to that tissue from which we isolated and sequenced about ten different enkephalin-containing peptides, some containing within them as many as four enkephalin sequences (Lewis et al. 1980). Others contained both Met- and Leu-enkephalin. Even before these enkephalin-containing peptides were characterized, we had demonstrated the presence in brain and adrenal medulla of a very large peptide which, on treatment with trypsin and carboxypeptidase B, yielded approximately six Met-enkephalin residues per Leu-enkephalin residue. This led to the concept of a multivalent proenkephalin. It appeared that proenkephalin like POMC was a polyprotein, one containing the sequences of more than one active peptide, and that these sequences were designed to be released by processing. The many enkephalin-containing peptides that we had isolated and sequenced at the time were like pieces of a jigsaw puzzle. Although we had most of the pieces, some were still missing and their exact order was not clear. However, one of the pieces, Peptide F, contained a sequence that showed no degeneracy at the nucleic acid level, enabling us to make an excellent cDNA probe. The same probe was used by us (Gubler et al. 1982) and by Numa and his colleagues (Noda et al. 1982) to clone and sequence bovine proenkephalin. The latter was indeed shown to contain six [Metlenkephalin and one [Leulenkephalin sequence as predicted from the peptides we had jsolated. Two of the sequences were designed to be processed out as heptapeptides. With POMC and proenkephalin sequenced, there still remained two [Leulenkephalin-containing peptides that were present in the posterior pituitary and whose sequences did not appear in either of these precursors. These were a-neoendorphin (Kangawa et al. 1981) and dynorphin (Goldstein and Ghazarossian 1980). It was already apparent that a third enkephalin-containing precursor must exist. Before it was characterized we (Kilpatrick et al. 1982) and Fischli et al. (1982) independently isolated and characterized a third [Leulenkephalin-containing peptide (rimorphin) and showed it to be present in posterior pituitary extracts in amounts comparable to a-neoendorphin and dynorphin. Using the sequence information provided by these peptides, Numa's laboratory cloned and sequenced their precursor, prodynorphin (Kakidani et al. 1982). The significance of the redundancy of enkephalin precursors is still not clear, nor are the exact functions of these neuropeptides known. Later, Howells in my laboratory cloned and sequenced rat proenkephalin cDNA (Howells et al. 1984) so that we would be able to study the biology of the opioid peptides in the species that has been used most in studies on opiate drugs. We used the cDNA, antibodies, and HPLC in many different ways. Proenkephalin derived peptides and the corresponding mRNA were found in several nonneural tissues including the heart ventricles (Howells et al. 1986) and the testis and ovary (Kilpatrick et al. 1985) as well. They are also present in the intestine and pancreas. It is apparent that the biological functions of proenkephalin derived peptides, like those of many other neuropeptides, are not limited to the central nervous system. Adrenal proenkephalin transcription and translation are markedly increased by denervation (Howells et al. 1984; Lewis et al. 1981) and are apparently under the control of glucocorticoids (Yoburn et al. 1987; Mocchetti et al. 1985). Brain proenkephalin transcription and translation are increased by several centrally acting drugs (Tang et al. 1983; Romano et al. 1987). Antibodies to opioid peptides had been used to trace the proenkephalin innervation in the CNS. However, a more precise and complete localization of proenkephalin neurons in the brain was recently carried out with the corresponding rat cDNA. The in situ hybridization studies were carried out by Howells in my laboratory in collaboration with Pfaff and his colleagues (Harlan et al. 1987). In situ hybridization methods utilizing cDNA are becoming more sensitive and may even be more specific than immunocytochemistry. The latter visualizes nerve bodies as well as fibers, whereas hybridization visualizes nerve bodies exclusively. When dealing with antibodies directed to small molecules, such as the opioid peptides or the catecholamines, diffusion may limit the precision of localization by immunocytochemistry. Localization of macromolecules, whether precursors, specific enzymes, or specific mRNA, is generally more precise. I will conclude with two recent examples of the advances that modern biotechnology has brought to the neurosciences. In the Tate sixties Guillemin had to use tons of beef hypothalami to isolate hundreds of nanomoles for characterizing the first releasing factor, TRH. More recently Guillemin's laboratory was able to isolate a few hundred picomoles of growth hormone releasing factors from several grams of human tissue (Guillemin et al. 1982). This was sufficient for sequencing. Shortly thereafter, in collaboration with Roche scientists they cloned the corresponding cDNA (Gubler et al. 1983). A fraction of the amount of tissue was used, and purification and sequencing were accomplished on far less material and in a much shorter time. Horecker, while at our Institute, had shown that extracting tissues with 6M guanidine hydrochloride prevents proteolysis (Hannappel et al. 1982). Under these conditions most larger proteins are denatured and precipitate and supernatant solutions contain peptides that are characteristic of a tissue and are not experimental artifacts. A brain extract prepared in this manner yields many peptides on HPLC. Some of these peptides are present in other tissues and are probably known. Others are unique to brain. When Morgan applied this extraction procedure along with HPLC to different portions of the brain, the resulting chromatographic eluates contained relatively few peptides. Two of the unidentified minor components in extracts of cerebellum when isolated and sequenced were shown to be unique molecules and limited to the cerebellum (Slemmon et al. 1984). These two related peptides, which he named cerebellins, are localized in Purkinje cells (Slemmon et al. 1985). The cerebellins are now used as markers for maturation of these cerebellar cells. No doubt many other "minor peptides" present in extracts recovered from specific brain areas will prove to be of interest. One of the most interesting developments relating to peptides in the brain concerns oncogene products. Oncogenes were originally discovered through their association with tumors, and the translations products of oncogenes are considered to be aberrant versions of normal regulatory proteins or peptides. Protooncogenes code for normal proteins the functions of which are still being determined. Morgan and Curran in our Institute showed that the c-fos protooncogene is rapidly and transiently induced by receptor-ligand interaction and by agents that affect voltage dependent calcium channels (Morgan and Curran 1986). The magnitude of these effects is modulated by pharmacologic agents. More recently they applied immunocytochemical methods to c-fos protooncogene induction as a means of determining the exact cells in brain where specific drugs act. With all the advances that have been made in methodology and instrumentation and with our increasing knowledge of how proteins and peptides are made, there is still a great future for peptide research in neurobiology. REFERENCES Bohlen, P.; Stein, S.; Stone, J.; and Udenfriend, S. Automatic monitoring of primary amines in preparative column effluents with fluorescamine. Anal Biochem 67:438-445, 1975. Fishcli, W.; Goldstein, A.; Hunkapillar, M.W.; and Hood, L. Isolation and amino acid sequence analysis of a 4,000-dalton dynorphin from porcine pituitary. Proc Natl Acad Sci USA 79:5435-5437, 1982. Goldstein, A., and Ghazarossian, V.E. Immunoreactive dynorphin in pituitary and brain. Pro Natl Acad Sci USA 77:6207-6210, 1980. Gubler, U.; Monahan, J.J.; Lomedico, P.T.; Bhatt, R.S.; Collier, K.J.: Hoffman, B.J.; Bohlen, P.; Esch, F.; Ling, N.; Zeytin, F.; Brazeau, P.; Poonian, M.S.; and Gage, P.L. Cloning and sequence analysis of cDNA for the precursor of human growth hormone- releasing factor, somatocrinin. Proc Natl Acad Sci USA 80:4311-4314, 1983. Gubler, J.; Seeburg, P.; Gage, L.P.; and Udenfriend, S. Molecular cloning establishes proenkephalin as precursor of enkephalin- containing peptides. 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Kakidani, H.; Furutani, Y.; Takahashi, H.; Noda, M.; Morimoto, Y.; Hirose, T.; Asai, M.; Inayama, S.; Nakanishi, S.; and Numa, S. Cloning and sequence analysis of cDNA for porcine beta- neoendorphin/dynorphin precursor. Nature 298:245-249, 1982. Kangawa, K.; Minamino, N.; Chino, N.; Sakakibara, A.; and Matsuo, H. The complete amino acid sequence of alpha-neo-endorphin. Biochem Biophys Res Commun 99:871-878, 1981. Keller, A., and Margolis, F.L. Isolation and characterization of rat olfactory marker protein. J Biol Chem 251:6232-6237, 1976. Kilpatrick, D.L.; Howells, R.D.; Noe, M.; Gailey, L.C.; and Udenfriend, S. Expression of preproenkephalin-like mRNA and its peptide products in mammalian testis and ovary. Proc Natl Acad Sci USA 82:7467-7469, 1985. Kilpatrick, D.L.; Wahlstrom, A.; Lahm, H.W.; Blacher, R.; and Udenfriend, S. Rimorphin, a unique, naturally occurring [Leulenkephalin-containing peptide found in association with dynorphin and alpha-neo-endorphin. Proc Natl Acad Sci USA 79:6480-6483, 1982. Kimura, S.; Lewis, R.V.; Gerber, L.D.; Brink, L.; Rubinstein, M.; Stein, S.; and Udenfriend, S. Purification to homogeneity of camel pituitary pro-opiocortin, the common precursor of opioid peptides and corticotropin. Proc Natl Acad Sci USA 76:1756-1759, 1979. Lewis, R.V.; Stein, S.; Gerber, L.D. Rubinstein, M.; and Udenfriend, S. High molecular weight opioid-containing proteins in striatum. Lewis, R.V.; Stern, A.S.; Kilpatrick, D.L.; Gerber, L.D.; Rossier, J.; Stein, S.; and Udenfriend, S. Marked increases in large enkephalin-containing polypeptides in the rt adrenal gland following denervation. J Neurosci 1:80-82, 1981. Lewis, R.V.; Stern, A.S.; Kimura, S.; Rossier, J.; Stein, S.; and Udenfriend, S. An about 50,000-dalton protein in adrenal medulla; A common precursor of [Metl- and [Leulenkephalin. Science 208: 1459-1461, 1980. Mains, R.E.; Eipper, B.A.; and Ling, N. Common precursor to corticotropins and endorphin. Proc Natl Acad Sci USA 74:3014-3018, 1977. Margolis, F. Carnosine in the primary olfactory pathway. Science 184:909-911, 1974. Mocchetti, I.; Guidotti, A.; Schwartz, J.P.; and Costa, E. Reserpine changes the dynamic state of enkephalin stores in rat striatum and adrenal medulla by different mechanisms. J Neurosci 5:3379-3385, 1985. Morgan, J.I., and Curran, R. The role of ion fluxes in the control of c-fos expression. Nature 322:552-555, 1986. Noda, M.; Furutani, Y.; Takahashi, H.; Toyosato, M.; Hirose, T.; Inayama, S.; Nakanishi, S.; and Numa, S. Cloning and sequence analysis of cDNA for bovine adrenal preproenkephalin. Nature (London) 295:202-206, 1982. Romano, G.; Shivers, B.D.; Harlan, R.E.; Howells, R.D.; and Pfaff, D.W. Haloperidol increases proenkephalin mRNA levels in the caudate-putamen of the rat: A quantitative study at the cellular level using in situ hybridization. Molec Brain Res 2:33-41, 1987. Richter, D. Biochemistry and biology of vasopressin, oxytocin, and their corresponding neurophysins. In: Udenfriend, S., and Meienhofer, J., eds. The Peptides, Vol. 8. New York: Academic Press, 1987. pp. 41-75. Rubinstein, M.; Stein, S.; and Udenfriend, S. Characterization of pro-opiocortin, a precursor to opioid peptides and corticotropin. Rubinstein, M.; Rubinstein, S.; Familletti, P.C.; Gross, M.S.; Miller, R.S.; Waldman, A.A.,; and Pestka, S. Human leukocyte interferon purified to homogeneity. Science 202:1289-1290, 1978b. Sachs, H., and Takabatake, Y. Evidence for a precursor in vaso- pressin biosynthesis. Endocrinology 75:943-948, 1964. Schultzberg, M.; Lundber, J.M.; Hokfelt, T.; Terenius, L.; Brandt, J.; Elde, R.P.; and Goldstein, M. Enkephalin-like immunoreactivity in gland cells and nerve terminals of the adrenal medulla. Neuroscience 3:1169-1186, 1978. Slemmon, J.R.; Blacher, R.; Danho, W.; Hempstead, J.; and Morgan, J.I. Isolation and sequencing of two novel cerebellum-specific peptides. Proc Natl Acad Sci USA 81:6866-6870, 1984. Slemmon, J.R.; Danho, W.; Hempstead, J.; and Morgan, J.I. Cerebellin, a quantifiable marker for Purkinje cell maturation. Proc Natl Acad Sci USA 82:7145-7148, 1985. Tang, R.; Costa, E.; and Schwartz, J.P. Increase in proenkephalin mRNA and enkephalin content of rat striatum after daily injection of haloperidol for 2 to 3 weeks. Proc Natl Acad Sci USA 80:3841-3844, 1983. Yoburn, B.C.; Franklin, S.0.; Calvano, S.E.; and Inturissi, C.E. Regulation of rat adrenal medullary enkephalins by glucocorticoids. Life Sci 40:2495-2503, 1987. AUTHOR Sidney Udenfriend, Ph.D. Roche Institute of Molecular Biology Building 102--340 Kingsland Street Nutley, New Jersey 07110, U.S.A. Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D., eds. National Institute on Drug Abuse, 1988 Synthesis and Biological Activity of Novel Met-enkephalin Analogs Krishna B. Mathur, Ph.D.; Balaram J. Dhotre, Ph.D.; Shubh D. Sharma, Ph.D.; Ram Raghubir, Ph.D; Gyanendra K. Patnaik, Ph.D.; and Bhola N. Dhawan, M.D. INTRODUCTION The discovery of enkephalins (Hughes 1975) ushered in a new’ era in which peptides emerged as a novel class of potent analgesics. Soon after their isolation and characterization was reported by Hughes et al. (1975), the search for other endogenous peptides possessing opioid activity was further intensified and several of them could be isolated from different mammalian tissues and fluids within a short span of time (Rossier 1982). Almost simultaneously, structure-activity relationship studies on these pentapeptides were undertaken in a number of labora- tories, primarily with the object of getting a synthetic peptide that could be utilized as a pain reliever in clinical practice (Morley 1980, 1983; Hansen and Morgan 1984). Endeavors of this sort were also started at this Institute, and the interesting results obtained by us are being briefly reviewed in this communication. RATIONALE FOR THE DESIGN OF ANALOGS Since the analgesia evoked by enkephalins was found to be only weak and transient after they were injected directly into the cerebral ven- tricles (Chang et al. 1976; Belluzzi et al. 1976), our emphasis was mainly on the design and synthesis of such analogs of enkephalins that would elicit profound and long-lasting analgesia even after their administration by the systemic routes. For designing new congeners, special care was also taken while introducing novel structural features in the molecules so that the resulting peptides could be synthesized rather conveniently even on a large scale when required. At the very outset, we were struck by the finding that (-endorphin, which is a 31 amino acid peptide having the Met-enkephalin sequence at its N-terminus (Li and Chung 1976; Bradbury et al. 1976), produces a powerful and long-lasting analgesia even after intravenous (i.v.) injection (Tseng et al. 1976). It is nearly 100 times more potent than morphine by intracerebroventricular (i.c.v.) route and 3 to 4 times as potent as morphine when administered intra- venously (Li and Chung 1976; Tseng et al. 1976). Based on a comparison of the analgesic properties of g-endorphin and two synthetic congeners 10 of Met-enkephalin whose N- and C- termini were stabilized against enzymatic degradation (Pert et al. 1976; Bradbury et al. 1977), Bradbury et al. (1976) and Cox et al. (1976) suggested that the high order of activity of B-endorphin was not merely due to its being impervious to brain enzymes. According to them, it could be more of a reflection of its higher binding affinity with the opioid receptors that might be arising from the sequence of amino acids that extends from its N- terminal pentapeptide (Bradbury et al. 1977). If that was true, derivatiza- tion of the terminal carboxy function of Met-enkephalin to get alkyl- amides could be expected to lead to derivatives that would not only be resistant to the attack of carboxypeptidases, but would also possess higher binding affinity for the opioid receptors due to enhanced hydro- phobicity at the C-terminus (Beddell et al. 1977). Moreover, the presence of alkyl chains in these derivatives was also expected to increase their overall lipophilic character so that their penetration through the blood- brain barrier would be possible (Belluzzi et al. 1978). To investigate this hypothesis, a series of alkylamides of Met-enkephalin were synthesized and examined for their morphinomimetic activity. As reported earlier, all the newly synthesized compounds of this series exhibited marked opioid activity (Patnaik et al. 1982). The most active compounds were, however, the n-propyl and isopropyl amide derivatives. Encouraged by the initial results, we launched the synthesis of another series of alkylamides in which the N-terminus of the pentapeptides was also protected against the atack of brain enzymes (Hambrook et al. 1976). In this series, the Gly” residue of enkephalins was replaced by D-Ala as Pert et al. (1976) and Beddell et al. (1977) had already, demonstrated that such a substitution not only protected the Tyr -Gly~ bond against cleavage by aminopeptidases but also potentiated the receptor-binding affinity of the peptides. As expected, all the pentapeptides thus obtained showed more pronounced and sustained antinociceptive activity following intracerebral (i.c.) administration (Mathur et al. 1979). The most promis- ing compounds here again were the isopropyl- and n-propyl derivatives. With a view to further optimize the morphine-like activity of these pentapeptide derivatives, we proceeded in two ways. On the one hand, a few substituted hydrazides of (D-Ala“, Met”)-enkephalin were synthesized as we found that the hydrazide derivative (11) was twice as potent an analgesic as the corresponding amide, (compd. 10, table 2). On the other hand, we decided to substitute Phe" in peptides 3 and 4 (table 1) with a MePhe residue so that the Gly -Phe’ bond would be stabilized against the action of enkephalinases (Schwartz et al. 1981; Gorenstein and Snyder 1980) and the hydrophobic site provided by the phenyl ring of Phe’ would be retained in the molecules for interaction with the opiate receptors (Gorin et al. 1980). The incorporation of this modification could be expected to yield highly potent and systemically active peptides (Romer et al 1977; Romer and Pless 1979). The sulfoxides of derivatives 5 and 6 were also syn- thesized (compds. 7 and 8, table 1) for studying their activity profile. 11 TABLE 1 Comparative Morphine-Like Activity of New Enkephalin Analogs Relative S.No. Compound Molar, Potency Analgesia GPI Gc) 5. Tyr-Gly-Gly-Phe-Met-NH.C 3H, (n) 0.82 0.52 2 C,H, (0) 2.88 0.36 3. __D-Ala _C3H,(n) 2.53 4.55 4. CH, (i) 8.84 5.60 5. MePhe C,H, (n) 24.17 30.00 6. CH, (0) 716.08 12.95 2 Met(0)__C3H.(n) 20.85 24.78 8. C,H, (0) 353.62 19.06 9. Gly- __C4H,() 706.09 2.98 - Tyr-Gly-Gly-Phe-Met 0.01 2.00 - Morphine hydrochloride 1.00 1.00 ED, Morphine analgesia in mice(i.c.): 0.11:0.01 ug; ICs, (1073M):5.7:0.07mg/ml TABLE 2 Analgesic Activity of (D-Ala2, Met”)-Enkephalin Amide and Hydrazides in mice (i.c.) S.No. Compound M pLRliive ny 10. Tyr-D-Ala-Gly-Phe-Met-NH,, 0.31 11. NH.NH,, 0.56 12, NH.NH.C H 21.52 - Tyr-Gly-Gly-Phe-Met 0.01 - Morphine hydrochloride 1.00 EDg, Morphine analgesia: 0.10 + 0.01 pug 12 It is evident from the lar potencies of peptides 6 and 8 (table 1) that the oxidation of Met” residue to Met(0) leads to a drastic reduction of the intrinsic activity of the parent peptide (Raghubir st al. 1982). An attempt was, therefore, made to substitute the Met” side-chain of analog 6 by other stereochemically equivalent side-chains by replace- ment of the thiomethylene group of Met with an amide residue and several analogous peptides were obtained (Sharma 1983). In addition, the side-chain of Met” was altogether deleted in one of the analogs. As discussed in the subsequent sections, some highly potent systemically active enkephalin analogs could thus be obtained. Finally, a few analogs in which Nval, D-Nval and Gly residues were incorporated as the fifth amino acid and their carboxy functions were derivatized as isopropylamide or phenyl hydrazide were also synthesized in an effort to get an analog which may be more selective for the &-subtype of opiate receptors. The synthetic strategies and biological activities of some of the more promising analogs of enkephalin obtained under this study are being discussed in the following sections. SYNTHESIS OF PEPTIDES All the enkephalin analogs were synthesized in the solution phase by well-established procedures peptide synthesis. In general, coupling of amino acids and peptides” was achieved by the DCC/HOBt, mixed anhydride and 2,4,5-trichlorophenyl ester methods. Except in the case of Met-enkephalin alkylamides, where the carboxy function of Met was initially protected by p-nitrobenzyl group, methyl or ethyl esters were employed for protecting the carboxyl groups. The «-NH. functions of amino acids and intermediate peptides were protected either with a carbobenzoxy (Z) or t-butyloxycarbonyl (Boc) group. The cleavage of Boc group was accomplished by treatment of the protected derivatives with TFA, HCOOH or HCl/dioxane in presence of ethanedithiol and anisole. Z-group was removed either by hydrogenolysis over Pd/C or by catalytic transfer hydrogenation using HCOOH as the hydrogen donor. The synthetic strategy for getting alkylamides of Met-enkephalin involved sequential peptidation of Met-ONBzl with appropriate Boc-amino acid- 2,4,5-trichlorophenylesters to get the protected pentapeptide Boc-Tyr- Gly-Gly-Phe-Met-ONBzl. Treatment of this pentapeptide ester with the required amines followed by cleavage of Boc group from the resulting amides gave the desired analogs (Dhotre et al. 1984). The synthesis of alkylamides of (D-Ala’, Met)-enkephalin was also carried out in a stepwise manner starting from Met-ONBzl in the same way ‘as described for Met-enkephalin alkylamides (Dhotre and Mathur 1984). An alternate strategy involving (3+2) fragment condensation technique was also adopted for the synthesis of peptides of this series as well as for the n-and isopropylamides of (D-Ala”, MePhe’, Met )- enkephalin (figure 1). In this procedure, the C-terminal dipeptide ester Boc-Phe-Met-OMe or Boc-MePhe-Met-OMe was synthesized by either DCC/HOBt or mixed anhydride method and converted into the required alkylamides via the free peptide acid. The N-terminal tripeptide fragment was coupled with the appropriate C-terminal dipgptide alkylamides via the 2-4-5-trichlorophenyl ester for getting (D-Ala“, Met”)-enkephalin 13 alkylamides and via the mixed anhydride for getting (D-Ala?, MePhe®, Met”)-enkephalin propylamides 5 and 6. Synthesis of Tyr-D-Ala-Gly- MePhe-Gly-NH.C, H(i) (compd.9) was also achieved in the same fashion by coupling thé ‘N-terminal tripeptide with MePhe-Gly-NH.C H(i). The sulfoxides 7 and 8 (table 1) could be obtained by direct oxidation of compounds 5 and 6 using approximately IN H.,0 in acetic acid (Raghubir et al. 1982). 22 Tyr D-Ala Gly Aaa Bbb Z wrens OH Hosier OE z DCC/HOBt | (5p, Boc— OH H-l—OMe HBr/AcOH Mixed anhydride or DCC/HOBt Boc+—OH H OEt Boc OMe Bog | DCC/HOBt OEt foc), NEOH, | on Mixed anhydride NaOH Boc NHR HCOOH/SH¢ (CH,),-SH Boc OH H NHR Boc NHR 1) Formic acid/Ethanedithiol- Anisole v 2) Neutralization Tyr-D-Ala-Gly-Aaa-Bbb-NH.R FIGURE 1 Synthetic Strategy For Various Enkephalin Analogs Aaa:Phe or MePhe; Bbb: Met or Gly; R: n-propyl or isopropyl Various (D-Ala2, Met”)-enkephalin hydrazides (table 2) were synthesized by a slightly modified procedure. The common intermediate Boc-Tyr- D-Ala-Gly-Phe-Met-OMe, was obtained first by coupling the mixed anhydride of Boc-Tyr-D-Ala-Gly with Phe-Met-OMe. Treatment of the pentapeptide ester with hydrazine hydrate directly gave the correspon- ding hydrazide which was deblocked with HCl/dioxane to give the compound ll. For the synthesis of the phenyl hydrazide 12, the penta- peptide ester, mentioned above, was hydrolyzed and the resulting acid 14 coupled with phenylhydrazine by the mixed anhydride procedure (Sharma 1983). Cleavage of the Boc group by treatment with HCOOH gave the final product. Homogeneity of all the peptides was checked by chromatography including HPLC. BIOLOGICAL ACTIVITY Morphinomimetic activity of all the newly synthesized analogs of enke- phalin was examined both in vitro and in vivo. For in vitro tests, the electrically stimulated myenteric plexus-longitudinal muscle preparation of guinea pig ileum (GPI) was prepared from adult guinea pigs of either sex as described by Kosterlitz and Watt (1968). Graded concentrations of various compounds were added to the bath and agonist activity cal- culated from inhibition of the contraction (IC., values). Morphine hydro- chloride and Met-enkephalin were used as” standard for comparison. Naloxone antagonism was used to investigate the specificity of action. For assaying analgesic activity of peptides, the method of Eddy and Leimbach (1953) was employed using mice of either sex in groups of 10 for each dose. The compounds were administered in graded doses intracerebrally (i.c.) and the control group received an equal volume of normal saline by the same route. Percentage of animals showing analgesia was determined at each dose level and ED 0 calculated accord- ing to Finney's Probit analysis (1952). Morphine hydPochloride and Met- enkephalin were used as standard drugs and naloxone was used to anta- gonize the analgesic effect. The relative molar potencies of some of the more promising analogs of enkephalin obtained by us in analgesia and GPI tests are presented in tables 1 and 2. As mentioned earlier, the most active compounds among the alkylamides of Met-enkephalin were the n-propyl and isopropyl- amide derivatives, being 80 and 270 times more potent than the parent pentapeptide in the analgesia test. Lengthening and shortening of the alkyl chain was found to have an adverse effect on the antinociceptive activity. However, the most potent compound of this series in the GPI test was the n-hexyl amide, its activity being 12 times higher than the isopropylamide (Patnaik et al. 1982). In the (D-Ala?, Met”)-enkephalin alkylamide series too, the highest order of analgesic activity was exhibited by the isopropylamide (compd.4) followed by the n-propylamide (compd.3). It can be seen that replacement of Gly” with D-Ala has led to a threefold increase in the activity of these peptides (Mathur et al. 1979). Peptides 3 and 4 are approximately 240 and 800 times more potent than Met-enkephalin on a molar basis. Here again, there is no correlation in the in vivo and in vitro activities of compounds. The most active derivative of this , series in the GPI test was the ethylamide. The hydrazide of (D-Ala“®, Met” )-enkephalin was found to be twice as potent as the corresponding amide. When the hydrazide nitrogen was substituted with alkyl groups, no significant change in the activity was observed. In the case of phenyl hydrazide, however, a substantial enhancement of analgesic activity was achieved (table 2). It is nearly 2,000 times more active than Met-enkephalin. 15 When Phe” was substituted by a MePhe residue in the propylamides 3 and 4, highly potent analogs could be obtained. The antinociceptive activity of peptides 5 and 6 is nearly 12 and 80 times higher than that of compounds 3, and ths respectively. As compared to Met-enkephalin, (D-Ala®, MePhe’, Met”)-enkephalin isopropylamide is nearly 70,000 times more potent as an analgesic (Raghubir et al. 1982). The correspond- ing sulfoxide retains only half the activity of the parent peptide. It has, however, been found to be active even when administered by systemic routes. This is in conformity with the results obtained by R38mer et al. (1977) and Rdmer and Pless (1979). 5 The most significant finding of this study is that the side chain of Met” in (D-Ala“, MePhe’, Met”)-enkephalin isopropylamide does not seem to play any role in the manifestation of the opioid activity of this analog. As such, the Met, residue ycan de replaced by Gly without any loss of activity. (D- Ala”, MePhe’,Gly”)-Enkephalin isopropylamide is, in fact, a highly potent analog and elicits profound and longer-lasting analgesia even after systemic administration (Raghubir et al. 1984). Both the systemically active compounds mentioned above have been taken up for detailed investigation, and their pharmacological profile is discussed elsewhere (Raghubir et al. 1988). We have also, found that the corresponding phenyl hydrazide, (D-Ala“, MePhe’, Gly”’)-enkephalin phenyl hydrazide, is comparatively more selective for é-subtype of opiate receptor. CONCLUDING REMARKS It is evident from this review that incorporation of such structural modifications that would inhibit metabolic deactivation of enkephalins and enhance their receptor-binding affinity leads to peptides that show a high order of antinociceptiye activity after systemic administration. The aromatic side chain of Phe” in enkephalins plays an impprtang role in the manifestation of opioid activity. Stabilization of Gly” -Phe peptide bond against the action of enkephalinases, so that the hydrophobic site for receptor interaction provided by the Phe residue is not lost, enhances the activity of peptides remarkably. Introduction of hydrophobic chains at the C-terminus of the pentapeptides certainly has a favorable effect on their activity, but the presence of such groups that would lead to an optimum hydrophobicity of the solvent, facing part of the molecule is most desirable. The deletion of Met side-chain withoyt causing any loss in the biological activity of the analog (D-Ala“, MePhe’, Met” )-enkephalin isopropylamide may be viewed in this context. It is now well established that enkephalins play several important roles in the CNS in addition to their role in the process of analgesia. They are known to be involved in learning and behavior, modulation of other neuropeptides and putative neurotransmitters, modulation of neuro- endocrinal activities and central control of autonomic activities. It will be useful to study the effect of the modified enkephalins on these central parameters as well. This may provide useful leads for potential drugs/tools beyond their present significance in analgesia. 16 FOOTNOTES 1 communication no.4192 from Central Drug Research Institute, Lucknow, India. 2 Abbreviations for amino acid and peptide derivatives are according to IUPAC-IUB Commission on biochemical nomenclature, Biochemistry 11:1726,1972; other abbreviations are: DCC, NN-dicyclohexylcarbodii- mide; HOBt, l-hydroxy-benzotriazole; TFA, trifluoroacetic acid. REFERENCES Beddell, C.R.; Clark, R.B.; Hardy, G.W.; Lowe, L.A.; Ubatuba, F.B.; Vane, J.R.; Wilkinson, S.; Chang, K.J.; Cuatrecasas, P.; and Miller, R.J. Structural requirements for opioid activity of analogues of the enkephalins. Proc R Soc Lond B198:249-265, 1977. Belluzzi, J.D.; Grant, N.; Garsky, V.; Sarantakis, D.; Wise, C.D.; and Stein, L. Analgesia induced in vivo by central administration of enke- phalin in rat. Nature 260:625-626, 1976. Belluzzi, J.D.; Stein, L.; Dvonch, W.; Dheer, S.; Gluckman, M.l; and McGregor, W.H. Enhanced analgesic activity of D-Ala” enkephalinamides following D-isomer substitutions at position five. Life Sci 23:99-104, 1978. Bradbury, A.F.; Smyth, D.C.; Snell, C.R.; Birdsall, N.J.M.; and Hulme, E.C.C-fragment of lipotropin has a high affinity for brain opiate receptors. Nature 260:793-795, 1976. Bradbury, A.F.; Smyth, D.G.; Snell, C.R.; Deakin, J.F.W.; and Wendlandt, S. Comparison of the analgesic properties of lipotropin C-fragment and stabilized enkephalins in the rat. Biochem Biophys Res Commun 74:748-754, 1977. Chang, J.-K.; Fong, B.T.W.; Pert, A.; and Pert, C.B. Opiate receptor affinities and behavioral effects of enkephalin: Structure activity relationship of ten synthetic peptide analogues. Life Sci 18:1473- 1482, 1976. Cox, B.M.; Goldstein, A.; and Li, C.H. Opioid activity of a peptide, B-lipotropin-(61-91), derived from A-lipotropin. Proc Natl Acad Sci USA 73:1821-1823, 1976. Dhotre, B.J., and Mathur, K.B. Design and synthesis of enkephalin analogues: Part II- Synthesis of (D-Ala®, Met”)-enkephalin alkylamides having morphinomimetic activity. Indian J Chem 23B:1231-1236, 1984. Dhotre, B.J.; Chaturvedi, S.; and Mathur, K.B. Design and synthesis of enkephalin analogues: Part I-Synthesis of Met-enkephalin alkylamides with enhanced analgesic potency. Indian J Chem 23B:828-833, 1984. Eddy, N.B., and Leimbach, D. Synthetic analgesics II. Dithienylbutenyl and dithienylbutylamines.J Pharmacol Exp Ther 107:385-393, 1953. Finney, D.J. Probit Analysis. Cambridge: University Press, 1952. Gorenstein, C., and Snyder, S.H. Enkephalinases. Proc R Soc Lond B210: 123-132, 1980. 17 Gorin, F.A.; Balasubramanian, T.M.; Cicero, T.J.; Schwietzer, J.; and Marshall, G.R. Novel analogues of enkephalin: identification of func- tional groups required for biological activity. J Med Chem 23:1113- 1122, 1980. Hambrook, J.M.; Morgan, B.A.; Rance, M.J.; and Smith, C.F.C. Mode of ‘deactivation of the enkephalins by rat and human plasma and rat brain homogenates. Nature 262:782-783, 1976. Hansen, P.E., and Morgan, B.A. Structure-activity relationships in enke- phalin peptides. In: Meienhofer, J., and Udenfriend, S., eds. The Peptides. Vol.6. New York: Academic Press, 1984, pp.269-321. Hughes, J. Isolation of an endogenous compound from the brain with pharmacological properties similar to morphine. Brain Res 88:295- 308, 1975. Hughes, J.; Smith, T.W.; Kosterlitz, H.W.; Fothergill, L.A.; Morgan, B.A.; and Moris, H.R. Identification of two related pentapeptides from the brain with potent opiate agonist activity. Nature 258:577- 579, 1975. Kosterlitz, H.W., and Watt, A.J. Kinetic parameters of narcotic agonists and antagonists with particular reference to N-allylnoroxymorphone (naloxone). Br J Pharmacol 33:266-276, 1968. Li, C.H., and Chung, D. Isolation and structure of an untriacontapeptide with opiate activity from camel pituitary glands. Proc Natl Acad Sci USA 73:1145-1148, 1976. Mathur, K.B.; Dhotre, B.J.; Raghubir, R.; Patnaik, G.K.; and Dhawan, B.N. Morphine like activity of some new Met-enkephalin analogues. Life Sci 25:2023-2028, 1979. Morley, J.S. Structure-activity relationships of enkephalin-like peptides. Annu Rev Pharmacol Toxicol 20:81-110, 1980. Morley, J.S. Chemistry of opioid peptides. Br Med Bull 39:5-10, 1983. Patnaik, G.K.; Raghubir, R.; Mathur, K.B.; Dhotre, B.J.; and Dhawan, B.N. Opioid activity of some new Met-enkephalin analogues. Indian J Pharmacol 14:15, 1982. 2 Pert, C.B.; Pert, A.; Chang, J.K.; and Fong, B.T.W. (D-Ala“)-Met-enkepha- linamide: A potent long-lasting synthetic pentapeptide analgesic. Science 194:330-332, 1976. Raghubir, R.; Patnaik, G.K.; Sharma, S.D.; Mathur, K.B.; and Dhawan, B.N. Antinociceptive activity of new Met-enkephalin analogues- Importance of the side chain of fifth amino acid. Indian J Pharmacol 16(1):35, 1984. Raghubir, R.; Sharma, S.D.; Mathur, K.B.; Patnaik, G.K.; Sriynal, R.Gy; and .Dhawan, B.N. Pharmacological profile of some (D-Ala”, MePhe’, Met~)-enkephalin-alkylamides, new potent analogues of Met-enkephalin. In: Dhawan, B.N., ed. Advances in the Biosciences. Vol.38.Current Status of Centrally Acting Peptides. Oxford: Pergamon Press, 1982. pp.61-68. Raghubir, R.; Patnaik, G.K.; Sharma, S.D.; Mathur, K.B.; and Dhawan, B.N. Pharmacological profile of two new analogues of Met-enkephalin In: Dhawan, B.N., and Rapaka, R.S., eds. Recent Progress in Chemistry and Biology of Centrally Acting Peptides, Central Drug Research Institute, Lucknow, 1988. pp.167-174. Romer, D., Buscher, H.H.; Hill, R.C.; Pless, J.; Bauer, W.; Cardinaux, F. Closse, A.; Hauser, D.; and Huguenin, R. A synthetic enkephalin analogue with prolonged parenteral and oral analgesic activity. Nature .268:547-549, 1977. 18 Romer, D.; and Pless, J. Structure activity relationship of orally active enkephalin analogues as analgesics. Life Sci 24:621-624, 1979. Rossier, J. Opioid peptides have found their roots. Nature 298:221-222, 1982. Sa Schwartz, J.-C.; Malfroy, B.; and Baume, S.D.L. Biological inactivation of enkephalins and the role of enkephalin-dipeptidyl-carboxypeptidase (enkephalinase) as neuropeptidase. Life Sci 29:1715-1740, 1981. Sharma, S.D. Studies in the synthesis of peptides with possible biological activities. Ph.D dissertation: 196-218, 1983. Tseng, L.F.; Loh, H.H.; and Li, C.H. p-Endorphin as a potent analgesic by intravenous injection. Nature 263:239-240, 1976. AUTHORS Krishna B. Mathur, Ph.D. Balaram J. Dhotre, Ph.D. Shubh D. Sharma, Ph.D. Ram Raghubir, Ph.D. Gyanendra K. Patnaik, Ph.D. Bhola N. Dhawan, M.D. Central Drug Research Institute Lucknow 226001, India 19 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D, eds. National Institute on Drug Abuse, 1988 Approaches to Studying Structure- Activity Relationships in Peptide Hormones Through the Expression of Synthetic Genes John W. Taylor, Ph.D. INTRODUCTION The primary structures of a very large number of peptide hormones having diverse pharmacological properties have now been elucidated. In order to understand the func- tions of these peptides and to exploit their potential as pharmaceutical agents, it is essential to study structure-activity relationships in each case. To this end, the tech- niques of peptide synthesis have commonly been applied, allowing the direct preparation of deletion analogues and analogues incorporating natural and nonnatural amino acid sub- stitutions. However, many peptide hormones are too large to consider extensive investi- gations of the role of individual amino-acid residues, as the preparation of multiple ana- logues in this way would be too time-consuming and expensive, and even the synthesis of the natural structure alone may represent a significant synthetic achievement or produce material that is too poorly characterized to be useful (Clark-Lewis et al. 1986). In such cases, the alternative approach of employing synthetic genes and recombinant DNA technology is becoming increasingly more attractive as new methods in this area are developed. The latter approach consists of three main stages: (a) the assembly from synthetic oligonucleotides of a gene coding for the peptide hormone being studied; (b) the preparation of mutant genes coding for the desired hormone analogues; (c) the efficient expression of the original and mutant genes in overproducing cells from which the hor- mone analogues are recovered and purified. Compared to peptide synthesis, this approach has the major advantage that all possible deletion analogues or single residue substitution analogues may be prepared simply and rapidly, at little extra cost, by muta- tion of the original gene once it has been assembled. Furthermore, the purity of the final peptide products prepared in this way, and the likelihood that they will be contaminated with pharmacologically active impurities, is not a function of the size of the hormone or its amino acid composition, as it is when direct chemical synthesis is employed. The purpose of this article is to review the methods that are currently available for preparing peptide hormones by gene expression in Escherichia coli and to discuss how they might be employed to perform structure-activity analyses. OLIGONUCLEOTIDE SYNTHESIS AND GENE CONSTRUCTION Oligomeric DNA must be synthesized in order to construct a gene that codes for the desired peptide hormone and can be incorporated into a suitable plasmid vector for expression. In addition, synthetic oligonucleotides are employed in the subsequent site- directed mutagenesis of that gene and the sequence characterization of all of the gene constructs produced, as described below. There are two synthetic strategies in common use, each involving the stepwise addition of protected nucleotides to the 5' end of the 20 oO o oO + 0 | & 0=P-0 HNEt, O-Ph-Cl DMT-O4 o B, Tetrazole + : MSNT, 3-Nitrotriazole 1 P-N(iPr), NC.C,H,0 DMT-0— 0 B, 1 DMT-04 0 B, c 0 : 1 NG.CpH40-0 NGO: 0: P==0 i O— 0B 0— o B 7 0B » I, H,0, 0 d Lutidine S ® FIGURE 1 Oligonucleotide synthesis by the phosphite method (A) and the phosphate method (B). Oligonucleotides are built up on a solid phase support through the repetitive application of these reactions for each base addition. DMT, dimethoxytrityl; MSNT, 1-(mesitylene-2- sulfonyl)-3-nitro-1,2,4-triazole. growing oligonucleotide chain which is anchored to a solid support at its 3' end (reviewed by Itakura et al. 1984 and Sonveaux 1986). The two methods are distinguished by the use of either a phosphite analogue of the nucleotide (a phosphoramidite) in the addition step which is subsequently oxidized to the phosphate form, or the introduction of the protected nucleotide in the phosphate form directly (figure 1). After completion of the final synthetic cycle, the base- and phosphate backbone-protecting groups are removed, and the linkage to the solid support is cleaved to yield the crude oligonucleotide. If an automated synthesizer is employed under optimal conditions, the synthesis of oligonu- 21 cleotides as long as 100 bases may be achieved. However, manual syntheses that employ apparatus as simple as a small syringe are quite adequate for the preparation of oligonucleotides up to 20 bases long. Purification of the correct oligonucleotides from crude synthetic mixtures may be achieved by HPLC on ion-exchange or reversed-phase columns, or by electrophoresis through polyacrylamide gels under denaturing conditions (Sonveaux 1986). The HPLC methods are suitable for oligonucleotides shorter than about 20 bases long and can be used for larger quantities, but often require the assumption that the major product from the synthesis is the correct one. In contrast, polyacrylamide gel electrophoresis can readily provide adequate poeain of oligonucleotides 10-100 bases long in sufficient quantities for the uses described here, and can be performed on multiple samples simulta- neously in the presence of reliable standards to identify the desired products. The solid supports that are most commonly used are derivatized silica, which is useful for preparing relatively large quantities of shorter oligonucleotides, and derivatized con- trolled-pore glass, which gives higher yields per synthetic cycle and is more useful for the present purposes (Sonveaux 1986). In addition, however, Helmut Blocker's group has demonstrated that paper disks may also be used as a solid support for oligonucleotide synthesis (Frank et al. 1983). If these disks are used in conjunction with a synthetic apparatus that incorporates one reaction vessel dedicated to the addition of each of the four base types, then the simultaneous synthesis of multiple oligonucleotides (as many as 40 is reasonable) having unique base sequences can be achieved by numbering the paper disks and resorting them between the four reaction vessels after each successive base addition. Both the phosphite and the phosphate chemistries have been applied to this process, which can result in considerable savings in time and expensive synthetic reagents (Frank et al. 1983; Matthes et al. 1984; Ott and Eckstein 1984). In our labora- tory, for example, we have successfully employed the phosphoramidite chemistry to the simultaneous manual synthesis on paper disks of 12 unique oligonucleotides that ranged from 13 to 19 bases in length. These were then purified in a few hours from the crude synthetic products by simultaneous electrophoresis on a single polyacrylamide gel in sufficient quantities and purities for use in oligonucleotide-directed mutagenesis or DNA sequencing experiments. An analysis of the crude and purified products of these synthe- ses by gel electrophoresis and autoradiography, after 5'-end labelling with ATP-y-32P and polynucleotide kinase, is presented in figure 2. Since the preparation of each mutant gene coding for a new peptide hormone analogue requires a unique oligonucleotide of this size range, the application of Blocker's approach should be particularly useful in this regard. Several semisynthetic approaches to the assembly of the double-stranded DNA com- prising the synthetic gene and its incorporation into a double-stranded plasmid or phage DNA vector may be considered. Most commonly, both strands of the gene are synthe- sized in their entirety as oligonucleotide fragments that have overlapping base comple- mentarities. These oligonucleotides are enzymatically phosphorylated at their 5' ends, and then annealed together and ligated using T4 DNA ligase and ATP. The resulting segment of double-stranded DNA is designed to have unpaired "sticky ends" that allow another enzymatic ligation into vector DNA linearized with a restriction enzyme that produces complementary "sticky ends." This approach, illustrated in figure 3, can be refined by (a) the use of two restriction enzymes producing different "sticky ends" so that the orientation of the inserted DNA is unambiguous, and (b) using the synthetic DNA in excess over the vector (about five- to tenfold has given us good results) and leaving the oligonucleotides that provide the 5' ends of the synthetic gene unphosphorylated so that ligation of either the insert or the vector to itself is minimized. Using this approach, synthetic genes can be efficiently assembled into vectors in segments of 100-300 base pairs, punctuated by unique restriction enzyme sites (for examples, see Ferretti et al. 22 CRUDE PURIFIED FIGURE 2 Analysis of the products from a manual synthesis of twelve unique oligonucleotides. The oligonucleotides were synthesized simultaneously on individual paper disks using the phos- phite method. They were then desalted on Sep-Pak Cig cartridges (Waters Co. Lid.), and then purified by electrophoresis on a 20% polyacrylamide gel and desalted again, as before. The crude (left panel) and gel-purified (right panel) synthetic products were analyzed by autoradiography, after 5-end labelling with 32P and electrophoresis on a 15% gel. The oligomers ranged in length from thirteen to nineteen base residues, as follows (left to right): 18mer; 14mer; 18mer; 17mer; 18mer; 18mer; 19mer; 18mer; 16mer; 19mer; 18mer; 13mer. 23 C a oh a EA va S SJ ed | Vv J © a V Vector Phosphorylated oligonucleotides Restriction (1) Anneal LL (2) Ligate with T4 es! ligase and ATP Synthetic gene rr Transform cells and Gi) grow on agar plates Vector FIGURE 3 Assembly of a synthetic gene and its incorporation into a vector. For best results, the oligonucleotides at the 5-end of each strand (in this case, | and V) are left unphosphory- lated, and the "sticky ends" of the synthetic gene are different, so that the vector must be cut with two restriction enzymes that produce complementary "sticky ends." 1986 and von Bodman et al. 1986). Thus, a synthetic gene coding for a given peptide hormone can usually be assembled in a single step. Oligonucleotides about 50 bases long and overlaps of about 8-12 bases appear to provide the most reliable combination for obtaining the correct annealing and ligation and the fewest sequence errors after cell transformation and characterization of the amplified products. We have also found that it is quite reliable to perform the two ligation steps simultaneously, by adding both the vector and ligase directly to the annealed oligonucleotides. The use of longer oligonu- cleotides can result in more sequence errors, since there will inevitably be more impurities present from their synthesis even after purification, and the use of shorter oligonu- cleotides and/or overlaps makes the design of unique overlapping segments difficult and increases the difficulties of obtaining correct annealing. Nevertheless, synthetic genes have been successfully assembled from shorter oligonucleotides prepared by the paper disk method of Blocker described above (Grundstrom et al. 1985; Brodin et al. 1986). Two other notable strategies have been employed. First, the approach of ligating the synthetic oligonucleotides one strand at a time was successful in a synthesis where the presence of a repeated codon made direct assembly of the duplex difficult (Smith et al. i In this case, the oligonucleotides comprising one strand only were phosphorylated with kinase. These were then ligated together after annealing to the unphosphorylated overlapping oligonucleotides comprising the opposite strand. After denaturing this mix- ture, the ligated strand was then purified by polyacrylamide gel electrophoresis. This process was performed simultaneously for the second strand, and the two purified strands were then annealed and ligated into the vector in a separate step. The second alternative strategy is one in which oligonucleotide synthesis is minimized by limiting the synthesis to longer overlapping single-stranded segments of the gene, so that the gaps between the overlaps can be filled enzymatically using a suitable polymerase and the 24 deoxynucleotide triphosphates (NTPs), before the segments are ligated. This approach has also been quite successfully employed (see, for example, Bergmann et al. 1986) but is generally found to be less reliable due to the difficulties of obtaining correct annealing and strand synthesis. MUTAGENESIS The preparation of peptide hormone analogues for structure-function analysis requires that the synthetic gene coding for the natural structure be mutagenized. This may be achieved in a random or partially random fashion by a number of chemical or physical methods, including treatments with sodium bisulfite, nitrous acid, hydrazine or UV light, that involve damaging the DNA so that its sequence is incorrectly repaired or replicated upon cell transformation giving rise to mutant progeny (Myers et al. 1985). Alternatively, restriction enzyme recognition sites purposefully introduced into the synthetic gene at strategically useful points may be exploited to introduce more specifically chosen muta- tions. In this case, either the DNA is cleaved in one strand only by restriction enzyme digestion under suboptimal conditions and then "misrepaired" enzymatically (Shortle et al. 1982), or else two such restriction sites are employed in order to cut out a "cassette" of double-stranded DNA that can then be replaced by any new "cassette" consisting of synthetic oligonucleotides (Lo et al. 1984). The most universally applicable methods, however, involve oligonucleotide-directed mutagenesis (Zoller and Smith 1983). In these methods, a synthetic oligonucleotide carrying a mismatch near the center of its sequence to direct the desired mutation is annealed to its partially complementary sequence on a single-stranded vector carrying the gene or gene fragment to be mutagenized. This oligonucleotide is then used to prime the synthesis of the entire complementary strand in vitro, using a DNA polymerase and each of the deoxynucleotide triphosphates (dNTPs). Competent cells are transformed with the resultant heteroduplex DNA and spread out on agar plates, giving rise to both forms of the DNA, from which the desired mutant form must be selected (figure 4a). In principle, all types of mutations of the target DNA sequence are achievable in this way, including deletions, additions, and substitutions of one or more bases, and there are no limitations on the sites that are accessible to change. It is necessary ony that the vector carrying the gene can be prepared in the single-stranded form, and that a suitable mismatched primer oligonucleotide can be designed and synthesized so that it will anneal specifically to the correct site on the gene. Since most expression vectors are double-stranded plasmids, the requirement for the single-stranded form usually necessitates a subcloning step, where the gene or gene fragment to be mutagenized is cut out by restriction enzyme digestion and transferred to a single-stranded bacteriophage such as one of the convenient M13 vectors adapted by Messing and coworkers to contain multiple cloning sites (Messing 1983). Once the mutant has been prepared, the gene can then be transferred back to the original plasmid for the purposes of expression. In some cases, however, this process has been simplified either through the use of phage vectors for expression directly (Wilkinson et al. 1983), or through the use of plasmid expression vectors of the pEMBL type, which are normally double-stranded but contain the origin of replication of M13 phage DNA and can readily be prepared in the single-stranded form upon infection of the plasmid-carrying cells with phage (Dente et al. 1983). The requirement for specific annealing of the mismatched oligonucleotide to the desired site usually presents no problems in cases involving the addition, deletion, or substitution of a single codon. It is usually sufficient to place the mismatched bases at least eight bases from either end of the oligonucleotide, and the precise arrangement can be further optimized for specific annealing to the correct site through the use of commercially available computer programs designed for this purpose. The major difficulty in oligonucleotide-directed mutagenesis is often the identification, after cell transformation with the heteroduplex DNA, of the plaques of phage-infected cells that contain the mutant phage. E. coli cells have a DNA mismatch repair system 25 A (1) © 2) (+)-strand ; Colonies on Mismatched DNA agar plate B “) () 3 © : ©) ee Ri. (+)-strand Mismatched DNA, Gapped DNA phosphorothioate (-)-strand | 3) ¢) 7 (4) Characterize mutants “ by sequencing directly Colonies on agar plate Phosphorothioate DNA, both strands mutated FIGURE 4 Oligonucleotide-directed mutagenesis using M13 vectors. (A) The unmodified procedure of Zoller and Smith (1983): (1) Mismatched primer extension with the Klenow fragment of DNA polymerase | and the dNTPs; ligation with T4 DNA ligase and ATP. (2) Trans- formation of competent cells and colony growth on agar plates. (B) The phosphoro- thioate method (Sayers and Eckstein 1987): (1) Mismatched primer extension with Klenow, dATP, dGTP, dTTP and dCTP-a-S; ligation with T4 ligase and ATP. (2) Nicking with Nci I; gapping with exonuclease Ill in the 3' to 5' direction, or with A exonu- clease or theT7 gene 6 exonuclease in the 5' to 3' direction, as appropriate. (3) Repair with DNA polymerase |, the dNTPs, T4 ligase and ATP. (4) Transformation and colony growth. that depends upon the action of the dam methylase, which labels DNA in vivo by methy- lation of GATC sequences, in order to recognize the original (methylated) viral (+)- strand and correct mismatches that were introduced into the (-)-strand during synthesis in vitro (Kramer et al. 1984a). The efficiency of this system is dependent on the type of mismatch introduced, but it typically reduces the frequency of occurrence of the mutant phage to about 10% of the plaques, and much lower frequencies are quite common (Taylor et al. 1985a). Furthermore, most of the plaques containing mutant phage that were obtained by plating out transformed cells directly are contaminated by the presence of the nonmutant form and must be replated at least once to ensure that the pure mutant form is obtained. Since the mutagenesis of a hormone gene in a phage vector 26 carried by E. coli cells will not normally result in a recognizable change in plague pheno- type, the mutant phage obtained by this method must be identified by screening a large number of plaques with a hybridization assay using the 32P-labelled mismatched oligonu- cleotide (which is perfectly complementary to the mutant page DNA). This assay involves transferring the plaques obtained in a mutagenesis experiment onto nitrocellulose filter paper, denaturing the phage and then hybridizing the radiolabelled oligonucleotide to the exposed immobilized phage DNA. Mutant and nonmutant phage are then distinguished by autoradiography after washing the nitrocellulose paper in a high salt buffer at successively higher temperatures. The radiolabel is washed off the samples of nonmu- tant phage at lower temperatures (Zoller and Smith 1983). In order to avoid the time-consuming hybridization screening step described above and eliminate the use of high specific activity 32P radiation, a number of modified mutagene- sis procedures have been developed that increase the frequency of occurrence of the mutants to a point where they may be conveniently identified and characterized directly by DNA sequencing. For this purpose, it is necessary to increase the efficiency of the mutagenesis to a point where the random selection for sequencing of only two or three plaques from each experiment will result in a high probability of identifying the desired mutant in a pure form. The relationship between the mutagenesis efficiency and the number of plagues that must be screened to achieve a satisfactory 90% probability of success is graphically illustrated in figure 5 (Kramer et al. 1982). Clearly, any method that will be useful in this regard needs to achieve reliable efficiencies of mutagenesis that are higher than about 50%. Only a few methods are adequate in this regard. These methods depend upon either selecting against the original DNA sequence in the (+)-strand of the heteroduplex in vivo, after transformation, or eliminating the original DNA sequence in that strand in vitro, before transformation. Selection against the (+)-strand in vivo has been successfully achieved in different ways. Kunkel (1985) has shown that single-stranded M13 vectors carrying cloned genes may be prepared in host cells deficient in dUTPase (dut =) and uracil glycosylase (ung =) to contain several deoxyuridine residues per molecule in place of the normal thymidine residues. When this DNA is used as the template to produce heteroduplex DNA in the normal way, transformation into ung + cells results in glycosylation and excision of the uracil moieties, creating multiple abasic sites and a consequent strong selection against the original (+)-strand molecules during the subsequent replication. The result is that more than 50% of the plaques obtained from these transformed cells contain progeny phage that are the desired mutants derived from the (-)-strand sequence. In a similar manner, the amber nonsense mutation or the Eco K restriction site have been exploited as genetic markers that may be incorporated into the (+)-strand of M13 DNA when it is prepared in a suitable suppressor-carrying or Eco K ~ host, respectively (Carter et al. 1985). In these approaches, selection against the (+)-strand of the heteroduplex DNA that is subsequently prepared in vitro requires an additional mismatch in the (-)-strand opposite the marker, so that transformation into a suppressor-deficient or Eco K- restricting host, as appropriate, will select against progeny derived from the (+)-strand only. The simplest way to achieve this double mismatch is to use two mismatched oligonucleotides simultaneously to prime the (-)-strand synthesis in vitro. In this case, the oligonucleotide annealed to the site of the genetic marker would be identical for all the mutations directed by the second mismatched primer in the normal way, so that little extra synthetic effort is required. Other, more difficult approaches involving the prepa- ration of heteroduplex, gapped DNA have also been applied to these selection methods (Kramer et al. 1984b). Again, the typical mutation efficiencies appear to be about 50%, although higher efficiencies have been reported, so that all of the preceding methods for in vivo selection against the nonmutant strand appear to allow the use of DNA sequencing methods to identify and characterize the mutants generated directly. 27 12 - 10 ~ w - S 8 - oo © oo S 6 > 0 £ 4 - =] = 2 = 0 T T Y T y T r T v 1 0 20 40 60 80 100 Mutation Efficiency (%) FIGURE 5 Relationship between the number of phage plaques that must be screened to have a 90% probability of identifying a mutant and the efficiency of the mutagenesis method used. (Adapted from Kramer et al. 1982. Copyright 1982, IRL Press, Ltd.) Most recently, my coworkers and | in Fritz Eckstein's laboratory have developed a very efficient method for oligonucleotide-directed mutagenesis that takes the alternative approach of eliminating the original (+)-strand sequence opposite the mismatched primer in the heteroduplex DNA, before it is used to transform competent cells (Taylor et al. 1985a; Nakamaye and Eckstein 1986; Sayers and Eckstein 1987). In this approach, the mismatched oligonucleotide primer is annealed to the (+)-strand of the M13 vector DNA with its cloned insert in the normal way, and then the in vitro synthesis of the comple- mentary (-)-strand is performed with the dCTP in the reaction mixture entirely substi- tuted by its at-thiophosphate analogue, dCTP-o.-S. The a-thiophosphate analogues of the natural dNTPs are diastereomeric and all of the DNA polymerases that have been investigated to date readily accept the Sp diastereomer of each dNTP-a.-S as a sub- strate, incorporating it into DNA with inversion of configuration about the phosphorus atoms almost as efficiently and accurately as for the unmodified dNTPs (Burgers and Eckstein 1979). The product of this in vitro synthesis is, therefore, heteroduplex cova- lently closed circular DNA that contains in its (-)-strand the desired mutant sequence, as well as phosphorothioate internucleotidic linkages of the Rp configuration on the 5' side of each dCMP base residue (figure 4b). Phosphorothioate-substituted M13 DNA has similar physicochemical characteristics to the natural DNA and retains its infectivity upon transformation of competent host cells, but also has the property of being resistant to linearization by restriction enzymes, particularly those which cleave their recognition sequences on the 5' side of the base type that was substituted by its c.-thiophosphate analogue in the synthesis. Indeed, for about one-third of the restriction enzymes that we have tested, linearization that requires cleavage of a phosphorothioate linkage appears to be completely blocked (Taylor et al. 1985b). However, these enzymes are still able to hydrolyse the unsubstituted (+)-strand of the phosphorothioate DNA quite efficiently in the normal way, to produce double-stranded DNA with a single "nick" placed specifically in the (+)-strand at the restriction enzyme cleavage site. We have exploited this prop- erty of the Nci | restriction enzyme in order to specifically hydrolyse the (+)-strand of the heteroduplex DNA containing dCMPS-substitutions in the if at recognition sites of the type shown below. 28 (+)-strand: ~~ 5'-CC/GGG-3' (-)-strand: 3-GGC/CC-5' Nci | normally cleaves the internucleotidic linkage on the 5' side of the central base residue in both strands of such sequences, as indicated, but in this case cleavage of the (-)- strand is blocked. The nicks that are generated in the (+)-strand can then be used as starting points for its digestion in the 3' to 5' direction, using the enzyme exonuclease Il. This digestion occurs at a reproducible rate of about 100 bases per minute in all of the DNA sample simultaneously, provided that the correct buffer conditions and excess of the exonuclease are used. When digestion has proceeded to a point safely beyond the desired point of mutagenesis (opposite the mismatched primer i the gapped DNA can be repaired by polymerization with dNTPs, using the mutated sequence of the (-)-strand as the template to produce phosphorothioate DNA having the desired mutant sequence in both strands (figure 4b). In a number of trial base-substitution mutagenesis experiments, where mutant M13 DNA prepared in this way was used to transform com- petent cells, 80% - 90% of the plaques obtained were consistently found to contain the ig mutant phage uncontaminated by the unmutated form (Nakamaye and Eckstein 1986). Based on the above results, the phosphorothioate DNA approach promises to be the most efficient of the enhanced oligonucleotide-directed mutagenesis methods, and it requires only a few hours of additional manipulations over the basic protocol and has no special requirements for unusual host cells or vectors. The dNTP-o.-S analogues are commercially available and give satisfactory results when used as the racemic mixtures directly. Furthermore, all of the potential limitations of this approach appear to present no additional difficulties and it should be applicable to every mutagenesis problem. For example, other restriction enzymes besides Nci | may be employed for the nicking reac- tion (in conjunction with the appropriate c.-thiophosphate nucleotide analogue); the exonu- clease Ill digestion and subsequent repair reactions are efficient over a range of several thousand bases; and gapped DNA may also be prepared by digestion from a nick in the Jpposie 5' to 3' direction, using either A exonuclease or the T7 gene 6 exonuclease (Sayers and Eckstein 1987). Thus, one or more appropriate restriction enzyme recogni- tion site present at any position in the vector or cloned gene is probably a sufficient prerequisite for the method and one that is easily satisfied. In the case of Nci I, the recognition sequence described above is present in all of the M13 vectors and the alternative Nci | site, where the (+)-strand sequence is 5'-CCCGG-3', does not seem to interfere when it is also present, because its cleavage in the (-)-strand is also blocked by the dCMPS substitution (Nakamaye and Eckstein 1986). Initial experiments (Sayers and Eckstein 1987) indicate that deletion mutagenesis is also just as efficient using these methods, despite the expected difficulty of digesting the loop of unpaired bases in the (+)- strand opposite the mismatched primer during the gapping step. (The third alternative of insertion mutagenesis, in which the heteroduplex phosphorothioate DNA will have an unpaired loop in its (-)-strand, is expected to be straightforward.) Finally, we have failed to detect any unexpected mutations in addition to those that were directed by the mis- matched oligonucleotides during our extensive characterization by sequence analysis of the mutants generated by these procedures. This indicates that the phosphorothioate DNA in the (-)-strand is a suitable template for accurate DNA synthesis by DNA poly- merase | during repair of the gapped DNA in the final step of the in vitro manipulations. The high efficiency of the phosphorothioate DNA method for mutagenesis suggests that new approaches to the rapid preparation of large numbers of mutants of a given peptide or protein might be possible. Nearly all of the DNA that is prepared in vitro contains the mutant sequence that is determined by the mismatched primer oligonucleotide. There- fore, the use of oligonucleotides that contain degenerate positions would allow the effi- 29 cient single-step preparation of, for example, mutants of an enzyme in which an active site residue is replaced by all other possible naturally occurring amino-acid residues. The subsequent identification and characterization of these mutants would be very rapid, because it could be performed directly by DNA sequencing. Alternatively, multiple spe- cific mutations at many different sites could be generated very rapidly by combining this mutagenesis method and direct sequence analysis with the paper disk approach of Helmut Blocker to synthesize the large number of mismatched oligonucleotides that would be required. This should be extremely useful in the characterization of structure-activity relationships in the larger peptide hormones that we are considering here, particularly when i are available for the efficient expression and purification of the mutants generated. EXPRESSION AND PURIFICATION The most important aspects of the expression of a synthetic gene in E. coli cells and the purification of the protein product are the requirements for efficient transcription of the gene and subsequent translation of the mRNA; the location, structure, and stability of the peptide product; and the possible methods by which it, and any mutants of interest, might be separated from the other protein constituents of the host cells. These subjects have been reviewed extensively elsewhere (Gold et al. 1981; Wetzel and Goeddel 1983; Marston 1986), and the present discussion will focus on the particular problems that are associated with the preparation of peptide hormones and their analogues, and the approaches to solving those problems that have been adopted to date. Various factors are known to affect the efficiency of transcription and translation, sometimes dramatically. These include the strength of the promoter, the structure of the ribosome-binding site and its position relative to the translation start codon (usually AUG) on the mRNA, the stability of the mRNA, and the presence of transcription atten- uators near the end of the open reading frame of the message. There are also strong correlations between codon usage in E. coli genes and the levels to which the correspond- ing proteins are expressed, which suggest that expression levels are determined by the codon-anticodon interaction energies and by tRNA abundancies (Grosjean and Fiers 1982). Unfortunately, there appear to be no absolute rules governing the precise choices that must be made in order to optimize these many factors for efficient expression. The approach that most researchers have adopted has been to employ the best natural systems, either directly or through the design of consensus structures. Thus, trp, lac, Ipp, AP and pho A promoters and ribosome-binding sites have all been employed directly, or in synthetic combinations such as the tac hybrid derived from trp and lac (De Boer et al. 1982) or the rac hybrid derived from rrnB and lac (Boros et al. 1986), which appear to be stronger than their parent structures. The design of hybrid or consensus promoters and ribosome-binding sites does not, however, always lead to better expres- sion systems (see, for example, Deuschle et al. 1986). Most of the promoters that are commonly employed also offer the advantage of being inducible, for example by temperature shift (AP) or addition of a metabolite (systems based on trp and lac ). This allows gene expression to be switched on at the most advantageous time, which is particularly important in cases where the protein produced is detrimental to the cell. The codons chosen to design a synthetic gene are usually taken from tabulations of the most abundant tRNAs (lkemura 1981), or the most abundant codons in highly expressed genes (Yarus and Folley 1985), although exceptions are often made so that convenient restriction enzyme recognition sites can be built in. The importance of this consideration was highlighted by the use of a synthetic gene that had been optimized in this manner to produce bovine growth hormone (Seeburg et al. 1983). The synthetic gene was ex- pressed at much higher efficiency than the natural mammalian gene had been. Additional empirical rules governing codon choice have also been suggested (Yarus and Folley 1985). 30 Unfortunately, it is possible that the choices made at this stage of the design of an expression system may result in quite unpredictable problems that are difficult to identify or solve: if certain DNA sequences cause the RNA polymerase to slow or stop, this may result in premature dissociation of the transcription complex and truncation of the mes- sage; or, if protein folding occurs concomitant with translation, other sequences may disrupt this process through their effects on the rate of translation of the mRNA on the ribosome, and incorrectly folded products may result. Even less information is available regarding mRNA stability and how it can be enhanced. Although stability might be related to secondary structure formation throughout the message, as well as, possibly, its overall length, experiments suggest that the structure of the 5' end is critical. Again, the approach to this problem has been to employ natural sequences in the 5' untranslated region that are taken from stable systems. In the case of the T4 gene 32 message, for example, the 5' sequence has been shown to confer stability on unstable sequences that are fused downstream to it. This property has been exploited in the design of a plasmid vector employing the promoter region and start codon of that gene and requiring phage T4 infection for expression (Duvoisin et al. 1986). In the expression of foreign proteins in E. coli cells, the stability of the product within the cells is an especially important consideration. Such expression has been shown to turn on the production of the lon protease and other gene products regulated by the hip R gene product associated with the heat shock response, leading to much higher rates of prote- olytic degradation than normal (Goff and Goldberg 1985), and the use of lon- and hip R mutant host strains is certainly helpful in this regard (Buell et al. 1985). Whether these responses are triggered by particular "foreign" amino acid sequences, or by incorrectly folded structures, or some other mechanism is responsible is not presently known. In addition, the half-lives of proteins that are endogenous to the cells vary themselves over a wide range, indicating that there are mechanisms for targetting proteins for degrada- tion that are normally in effect and might act on an overexpressed foreign protein also. E. coli has a large number of proteolytic enzymes that might participate in these pro- cesses, and are vital to the normal functioning of the cell (Swamy and Goldberg 1981). Empirical correlations suggest a strong relationship between the half-life of a protein in E. coli and its N-terminal amino acid sequence. In particular, the "PEST" hypothesis sug- gests that sequences rich in Pro, Glu, Ser, and Thr will be most highly susceptible to degradation (Rogers et al. 1986). Alternatively, procaryotic cells may have a mecha- nism for protein turnover that is similar to the ubiquitin-associated mechanism that appears to operate in eucaryots, in which case an important determinant of the half-life will be the N-terminal residue itself, with Arg, Lys, Asp, Leu, and Phe directing the most rapid degradation, and Met, Ser, Ala, Thr, Val, and Gly dictating the greatest resis- tance to degradation (Bachmair et al. 1986). Proteolytic degradation of the desired product is, perhaps, the most difficult problem attendant to the production of smaller peptides such as the peptide hormones. Their direct expression is usually followed by their rapid degradation, so that large quantities can never accumulate. This is almost certainly because these peptides are too small to fold into a stable globular structure, and their extended flexible conformations can readily fit into the typical active-site groove of a broad-specificity protease. The first success- ful solution to this problem, and the approach that is still most commonly applied, was to express the peptides as part of a much larger fusion protein by splicing the corresponding synthetic gene in frame to the end of the gene coding for a highly expressed protein that could act as an intracellular carrier. In this way, somatostatin, 3-endorphin, and both the A and B chains of insulin were separately produced, each fused to a point near the C terminus of B-galactosidase (ltakura et al. 1977; Shine et al. 1980; Goeddel et al. 1979). Expression was directed under the control of the strong inducible lac promoter and the peptides were recovered from the purified fusion protein by proteolytic (B-endorphin) or 3 chemical (somatostatin and the insulin chains) cleavage at specific amino-acid residues engineered into the structure for this purpose. The fusion protein approach solves a number of the problems discussed above simultane- ously, provided that the carrier protein is normally expressed at a high level in E. coli and it is being used as the N-terminal portion of the hybrid. At the RNA level, the structure around the ribosome-binding site should already be optimized for transcription, translation, and mRNA stability, and codon usage for most of the rest of the message should also be correct. After translation, the N-terminal amino acids should be consistent with the requirements in that region for a stable protein in vivo. There are additional advantages in relation to the purification procedures. First, the production of a larger protein aids in its direct identification by polyacrylamide gel electrophoresis, since the identification and visualization of small peptides by these techniques is difficult. This usually eliminates the need for antibodies directed against the desired peptide in order to follow its expression and purification. If enzymatic carrier proteins such as B-galactosidase or alkaline phos- phatase are used, activity can often be assayed directly on agar plates by colorimetric methods. Second, affinity columns can often be designed that target the carrier portion of the fusion protein during purification. Such affinity columns are usually constructed using antibodies to the carrier protein or, if it is an enzyme, inhibitors may be employed more conveniently. Affinity chromatography based on the carrier is a particularly important asset when multiple mutants of the peptide portion are being prepared, since the purification procedures should be identical in each case. Finally, procaryotic proteins are synthesized in vivo with N-formyl-Met at the N terminus which is usually cleaved from the mature protein during posttranslational processing. However, overexpressed foreign proteins are often produced with the N-terminal Met deformylated but still attached or incompletely removed, and the factors that govern the processing are not understood. The fusion protein strategy, with the carrier portion at the N terminus, therefore eliminates this potential problem also. To date, many small peptides in addition to those mentioned above have been expressed using the gene fusion strategy. These include antigenic determinants from hepatitis B fused to B-galactosidase and expressed under control of the /ac promoter (Charnay et al. 1980), or fused to B-lactamase (trp promoter; Edman et al. 1981); influenza virus antigens fused to B-galactosidase (lac promoter; Davis et al. 1981); hirudin fused to p- galactosidase (lac or AP, promoters; Bergmann et al. 1986); TGFa fused to 17 residues of the trp LE protein and promoter (Winkler et al. 1986); calcitonin fused to interferon-y (AP, promoter; Ivanov et al. 1987); and 27-desamidosecretin fused to B- galactosidase (lac promoter; Sumi et al. 1984). Frequently, these fusion proteins are insoluble within the cellular environment, even when produced at low levels, possibly as a result of incorrect folding of the carrier. This results in the formation of intracellular aggregates or inclusion bodies consisting predominantly of the fusion protein. These structures can often be isolated by centrifugation, and subsequently dispersed under denaturing conditions, as reviewed recently by Marston (1986), with considerable advan- tages in the purification strategy. In a number of cases, the fusion approach is unsatisfactory, either because recovery from the inclusion bodies is difficult, because a soluble fusion protein is desired (when the peptide is to be used directly as an antigen) or, very commonly, because proteolytic degradation of the peptide component still occurs, leading to impure products and a low yield. In these cases, proteins such as alkaline phosphatase, Omp A or B-lactamase, which have N-terminal signal- or leader-peptide extensions that direct their translocation across the cytoplasmic membrane and subsequent release into the periplasmic space, have been useful as alternative carriers. When correct transport and processing by signal peptidase occurs, large quantities of the fusion protein can accumulate in the periplasm, where precipitation has not generally been encountered, although proteolytic 32 degradation can still be a problem. Since relatively few E. coli proteins are present in the periplasm, and its contents can usually be selectively released by osmotic shock, secre- tion to the periplasm is also advantageous in terms of purification (Marston 1986). Examples of peptides that have been prepared in this way include human proinsulin, which was fused to N-terminal fragments of B-lactamase (Chan et al. 1981), and the Met27 analogue of human GRF, which was fused to the phosphate-binding protein, pho S (Anba et al. 1987). However, when a-neoendorphin was fused to alkaline phosphatase near its C terminus, transport or release into the periplasm was unexpectedly blocked (Ohsuye et al. 1983). On the other hand, it is often possible to dispense with the mature carrier pro- tein entirely and simply connect the synthetic peptide directly to a signal peptide sequence with its signal peptidase recognition site intact. Thus, for example, human EGF and hirudin have both been expressed, transported across the cytoplasmic membrane and released into the periplasm after correct signal peptidase cleavage, through their fusion to the alkaline phosphatase signal peptide (Oka et al. 1985; Dodt et al. 1986); human growth hormone was similarly processed under the direction of the alkaline phosphatase signal peptide or its own (eukaryotic) signal peptide (Gray et al. 1985); and proinsulin was secreted into the periplasm by fusion to the B-lactamase signal peptide (Chan et al. 1981), or through the correct transport and processing of the preproinsulin gene product (Talmadge et al. 1980). In a small number of cases, the processed peptides have been found predominantly in the extracellular medium, indicating that they have passed through the outer cell membrane also. These include B-endorphin, which had been fused to the Omp F signal peptide and an additional 12 amino-acid residues, and was subject to proteolytic degradation at its C terminus (Nagahari et al. 1985), and human growth hormone (Kato et al. 1987) and a-fibrinogen (Lord 1985), each of which had been fused to B-lactamase signal peptides. In the human growth hormone study, passage across the outer membrane was promoted by additional weak expression of the kil gene, which makes the outer cell wall permeable without cell lysis, suggesting that passive diffusion across this membrane occurred. The large size of a-fibrinogen (molecular weight 67,000) would seem to preclude passive diffusion, indicating that other mechanisms of transloca- tion across the outer membrane may also be important. However, extensive degradation of this protein was demonstrated, and the method of detection employed was dependent only on the presence of a short peptide fragment at its N terminus, so that passive diffusion across the relatively porous outer membrane might explain the extracellular presence of all three of these peptides. Whatever the mechanism, transport to the extracellular medium appears to yield smaller quantities of these peptides than can be obtained from intracellular fractions, and is not necessarily advantageous in terms of purification. Unless an endogenous proteolytic cleavage system such as the signal peptide/signal pep- tidase system described above is accurately exploited, the fusion protein strategy to peptide production requires that a specific cleavage reaction must be devised for the release of the target peptide from the fusion protein. This step is performed after cell lysis and, usually, after some initial purification. Several site-specific methods for such peptide backbone cleavages have been employed, all of them requiring that a "recognition site" consisting of one or more residues be engineered into the fusion protein on the N- terminal side of the scissile peptide bond. In most cases, the structural requirements for these sites are limited to the N-terminal side of that bond only. Since many biologically active peptides do not tolerate N- or C-terminal modifications to their natural structures, and given the additional possibility that peptides may be produced in E. coli with an addi- tional Met at their N termini (see above), this situation is ideal for recovery of a precise peptide structure if that peptide is positioned at the C terminus of a fusion construct. The cleavage methods can be divided into three categories: chemical, enzymatic at a single specific residue, and enzymatic at sites defined by a specific sequence of residues. Three chemical methods have been employed. Cleavage on the C-terminal side of Met 33 residues using cyanogen bromide has often been used to release peptides that contain no additional Met residues from fusion protein products (Itakura et al. 1977; Goeddel et al. 1979). Occasionally, the target peptide sequence has been modified in order to meet this requirement, as in the case of [Thr59]insulin-like growth factor | fused to an eight residue leader peptide (Peters et al. 1985). The cyanogen bromide reaction is usually carried out in 70% formic acid, and is therefore often useful for cleavages that must be performed under denaturing conditions such as those involving insoluble products in inclusion bodies, although additional denaturating agents such as urea or guanidinium thiocyanate are often added. A second chemical method, used to cleave Trp E-bovine growth hormone fusion proteins at Asp-Pro bonds, is acid pH treatment (Szoka et al. 1986). Again, the conditions require 70% formic acid, and often a denaturing agent is added, but elevated temperatures are also required. Although this method has the advantage of greater selectivity because it requires a two-residue site, it results in a cleaved peptide with an N-terminal Pro and may not always be efficient or specific for the Asp-Pro bond. Fur- thermore, there are reports that some Asp-Pro bonds are quite resistant to acidolysis, even under forcing conditions where extensive side reactions are occurring (see, for example, Allen et al. 1985). The third chemical method is similar to the second, consisting of cleavage at Asn-Gly bonds by hydroxylamine treatment at pH 9 and elevated tem- perature. This method was recently used to release human insulin-like growth factor from the C-terminal end of an IgG-binding domain of staphylococcal protein A, after the intact fusion protein had been purified on an IgG-Sepharose affinity column (Moks et al. 1987). Its general applicability remains to be determined. Enzymatic cleavages at single-residue sites include the reported use of clostripain to cleave C-terminal to Arg in an a.-chloramphenicol acetyltransferase-calcitonin fusion protein (see Marston 1986), and trypsin cleavage of B-endorphin from B-galactosidase, also C-terminal to Arg, after the fusion protein had been treated with citraconic anhy- dride to provide temporary protection of the Lys residues in B-endorphin from cleavage (Shine et al. 1980). In this category, the Staphylococcus aureus V8 protease is also potentially useful in that cleavage by this enzyme can be limited to sites C-terminal to Glu residues, even in the presence of Asp residues, under specific buffer conditions (Houmard and Drapeau 1972). This specificity has not yet been exploited, but might well be applicable to the production of a wide variety of active hormone analogues that have been engineered to replace any internal Glu residues with Asp. Such substitutions repre- sent very minor changes in peptide structure, and they might often have little effect on pharmacological activities. There are, at present, only two enzymes having recognition sites comprised of several amino-acid residues that have been exploited for the recovery of peptides from a fusion product. Collagenase cleaves collagen at multiple sites having a consensus structure - Pro-Xxx-Gly-Pro-Yyy-, with cleavage occurring on the C-terminal side of both of the unspecified residues. In one example of the early application of this cleavage reaction, Germino and Bastia (1984) designed a plasmid to express a fusion protein consisting of B-galactosidase at the N terminus, connected to the plasmid R6K initiator protein via a 60 residue segment of chicken proa-2 collagen containing several potential collagenase cleavage sites. They were then able to purify this protein by affinity chromatography based on the B-galactosidase segment and recover the R6K initiator, which is normally rapidly degraded in E. coli, after collagenase-catalyzed hydrolysis of the linker at multiple sites. The final product, however, was probably extended from the N terminus of the R6K initiator by about 10 residues of the linker, and may have been heterogeneous. More satisfactory results have been obtained by Nagai and Thegersen (1984) to recover human B-globin from a hybrid with Ac-II protein, and by Steven Benner's group (Nambiar et al. 1987) to cleave B-galactosidase-linked ribonuclease A, using the action of blood coagulation factor Xa to cleave at the C-terminal end of its consensus linker -lle-Glu-Gly- Arg-. In this case, the enzyme does not appear to require the three-dimensional structure 34 of its normal substrate for efficient cleavage, which probably contrasts with the re- quirements of collagenase, and the products obtained appeared to be homogeneous and devoid of unwanted N-terminal extensions, although in neither case was any sequence characterization performed. As one final note, it is worth pointing out that the potential utility of any enzymatic method is limited by the purity of the enzyme preparation, and contaminating proteolytic activities are often a problem. The utility of fusion constructs for enhancing the stability of overexpressed peptides in vivo and for simplifying their purification has stimulated a number of researchers to design novel systems for these purposes that do not involve natural carrier proteins. In several cases, the use of multiple fused copies of the target peptide has been shown to enhance its stability and recovered yield. For example, three copies of the proinsulin gene were found to be optimal for resistance to proteolysis when they were fused directly to the tac promoter, and two copies were optimal when fusion to the lac promoter plus a small fragment of the B-galactosidase gene was tested (Shen 1984). The repeated proinsulin gene segments were connected by linkers coding for the amino acid sequence - Arg-Arg-Asn-Ser-Met-, with the expectation that the correct proinsulin peptide could be recovered by cyanogen bromide cleavage followed by proteolytic digestion with trypsin and carboxypeptidase B. A similar strategy has been employed for the production of Met-enkephalin (Hostomsky et al. 1985). This opioid peptide was released from a fusion product consisting of 11 copies of the peptide connected by -Arg-Arg- linkers and fused to part of the SV40 small-t antigen, after trypsin and carboxypeptidase B digestion, as indicated by RIA and guinea-pig ileal assays. A substance P analogue having a C-termi- nal homoserine amide was also successfully prepared from overexpressed fusion proteins containing 4, 16 and 64 copies of the corresponding C-terminal Met analogue (Kempe et al. 1985). These were fused together between part of the A cro repressor on the N- terminal side and B-galactosidase on the C-terminal side. In this case, the substance P analogue was obtained by cyanogen bromide cleavage to release multiple copies of the C- terminal homoserine lactone analogue, which were converted to the desired [HSe'1]substance P with a C-terminal amide, as in the natural hormone, by treatment with 30% ammonium hydroxide. This last approach is likely to prove useful for the preparation of many other peptide hormone analogues where a C-terminal amide is required for activity. Another approach taken by Sung et al. (1986) to optimize the production of proinsulin was the addition of different homo-oligomeric peptides at its N terminus. As discussed above, this tactic is likely to affect the efficiency of expression as a result of modifications to the 5' end of the mRNA structure, in addition to affecting the lifetime of the peptide in vivo as a result of the effects of the N-terminal amino-acid residues on endogenous mechanisms for targetting protein degradation. In this investigation, hexamers of Ala, Asn, Cys, Gin, His, Ser, or Thr were found to produce the highest yields, and the yields for the(Ala)g- and (Ser)g-modified constructs were indeed found to be strongly dependent on the specific choice of codons used, indicating the importance of the structure of the ribosome-binding site on the mRNA. The use of poly-Arg fused to the C terminus of an overexpressed protein has also been explored as an aid to purification (Smith et al. 1984). This method was applied to the production in E. coli of human growth hormone (urogastrone) as a fused protein with 14 residues of the trp E protein at its N terminus and a C-terminal tail of 5 Arg residues. After expression, the fusion protein was purified from the cell lysate by cation-exchange chromatography, where it eluted after the bulk of the bacterial proteins on a salt gradient. The poly-Arg tail could be removed by carboxypeptidase B digestion. In our laboratory, we are attempting to exploit the potential amphiphilic nature of many peptide hormones and other biologically active peptides, and the general propensity of these structures to form organized aggregates in aqueous solution (Taylor and Kaiser 35 FIGURE 6 Schematic diagram of the structure of a helix bundle protein consisting of four amphiphilic a helices. Fusion proteins of this type, designed to incorporate amphiphilic peptide hor- mones at their C termini (shaded segment), might be resistant to proteolysis in E. coli. 1986), in order to generate fusion proteins that are specifically designed to include the peptide hormone as an integral part of their globular structure. For example, many of the intermediate-sized flexible peptide hormones can form amphiphilic o-helical segments (Taylor and Kaiser 1986). These peptides might be incorporated into globular fusion protein structures consisting of multiple near-parallel helices similar to the four-helix bundles commonly found in natural proteins (Weber and Salemme 1980), if they were connected to repeated segments of peptide sequences designed to form idealized amphiphilic helices (figure 6). Such tailor-made structures are expected to be soluble and more resistant to proteolytic degradation than the randomly connected fusion proteins usually are. 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The purification of fully active recombinant transforming growth factor a. produced in Escherichia coli. J Biol Chem 261:13838- 13843, 1986. Yarus, M., and Folley, L.S. Sense codons are found in specific contexts. J Mol Biol 182:529-540, 1985. Zoller, M.J., and Smith, M. Oligonucleotide-directed mutagenesis of DNA fragments cloned into M13 vectors. Methods Enzymol 100:468-500, 1983. ACKNOWLEDGMENTS Oligonucleotide synthesis, purification, and analysis was performed by Ms. G.V. Babiera. Funding support was provided by the National Institute on Drug Abuse through P.H.S. grant DA 04197. AUTHOR John W. Taylor, Ph.D. Laboratory of Bioorganic Chemistry and Biochemistry The Rockefeller University 1230 York Avenue New York, New York 10021, U.S.A. 40 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D., eds. National Institute on Drug Abuse, 1988 X-Ray Diffraction Studies of Enkephalins and Opiates Jane F. Griffin, Ph.D., and G. David Smith, Ph.D. The conformation or conformations of the enkephalins responsible for biological activity, that is, the conformation assumed at the receptor and resulting in the transduction of a message, has been of enormous interest since the enkephalins were first isolated by Hughes and Kosterlitz (1975). These pentapeptides with sequence Tyr-Gly-Gly-Phe-Leu(Met) have many degrees of conformational freedom due to peptide chain flexibility, centered in the four ¢ and five y torsional rotations, and side-chain flexibility from the x rotations of the Tyr', Phe! and Leu® or Met® residues. How does the opioid receptor(s) recognize a flexible linear pentapeptide, the relatively inflexible fused ring morphine-like compounds and the other families of drugs with which it interacts? What are the chemical moieties recognized by the receptor(s) and how are they arranged in three dimensions? Do the different opioid receptor subtypes bind different low energy conformations of the endogenous compounds or induce them into an "active” conformation? Since 1975 the conformations of enkephalin have been studied by every available spectroscopic technique in a variety of solvents and in the solid state, by more traditional biochemical structure/activity studies, by theoretical methods and by single crystal X-ray diffraction techniques. These studies have been reviewed in an excellent chapter by Schiller (1984). A more detailed review of the crystallographic literature appears in a previous monograph in this series (Camerman and Camerman 1986). This review will concentrate on the enkephalin structures determined by X-ray diffraction techniques since that paper was published, and on certain aspects of the structures which were not highlighted in the previous review. The results of X-ray diffraction studies on some morphine analogues with interesting opioid activity profiles will also be discussed. INFORMATION OBTAINED FROM X-RAY DIFFRACTION STUDIES The results of an X-ray diffraction study are a set of atomic coordinates, unit cell constants and space group. Calculations made from the above information provide not only geometric details on the compound under 41 study, precise bond distances, valency angles and torsion angles, but also intramolecular and intermolecular hydrogen bond geometry. The interactions that represent the forces holding molecular crystals together are exactly the same forces that are responsible for substrate-receptor binding: electrostatic interactions between charged groups, hydrogen bonds between functional groups, hydrophobic interactions and dipolar interactions. Thus the bioactive compound in the crystal lattice is a model of the substrate in a set of complementary surroundings. Determination of different crystalline forms, polymorphs and solvates, of the same material show different gross intermolecular interactions that can be related back to interactions in solution. Stable patterns of aggregation and even solvation present in solution persist in the crystalline Lok Thus, multiple determinations of the same compound (either more than one molecule in the asymmetric unit or different crystalline forms) give information on conformational flexibility, stable aggregates, patterns of solvation, and intermolecular interactions. Main-Chain Conformation There have been three X-ray crystallographic studies of [Leu®] enkephalin and two studies of the same crystalline form of [Met®]enkephalin. The crystal data on these structures is given in table 1. The structures labelled LE;,, ME,, (Griffin et al., 1985, 1986a), ME,,, and MEBr,,, the [(4-bromo-Phet | analogue of [Met® Jenkephalin (Doi et al., 1987b) have been determined since the previous review. Structures ME;, and ME,,, are two independent studies on crystals that appear to vary only in the amount of water present (see table 1). Previously, the crystal structures of the [(4-bromo-Phe*] analogue of [Leu®]enkephalin and a few other analogues with individual amino acid replacements have also been determined. These compounds and the main-chain conformations observed in each of these studies are given in table 2. Two conformations predominate, a 8 turn centered on Gly?Gly® and a family of extended conformations. Solution spectra have for the most part been interpreted as Shaving that there are both extended and folded conformations in solution; the folded conformation most frequently found by interpretation of spectra is a g turn centered on Gly3Phe?, a conformation not yet observed in the solid state. Khaled (1986) has pointed out some of the limitations in magnetic resonance studies of peptides: (1) assignments are complicated in a molecule containing a recurring amino acid residue such as in enkephalin with two adjacent glycine residues; (2) a controversy exists regarding the interpretation of the temperature dependence of NH protons. These assignments are used to distinguish inter- and intramolecular hydrogen bonds. The presence of the type I' g-turn conformation of enkephalin, centered on Gly?Gly* and characterized by a Phe NH to O=C Tyr! hydrogen bond, observed in the solid state studies of [Leu®]enkephalin and analogues (table 2) has been reported in only one spectroscopic study, enkephalin amides complexed with 18-crown-6-ether in chloroform (Beretta et al. 1984). 42 ev TABLE 1 Crystal data on enkephalins. [Leu’]enkephalin [Met3]enkephalin LER)? LE(E4)P LE(E2)°¢ ME(E2)cr® ME(E2’)9:°® MEBr(E2)¢ Space Group C2 P2, P2, P2, PZ, Pl Z 16 8 4 4 4 2 No. independent mol./ asym. unit 4 4 2 2 2 2 solvent/ asym. unit 6 H,0 8H,0, 8C,H,NO, 0.5H,0 10.6H,0 10 H,0 4.5 H,0 X Vol. (A3) 13501 8459 2999 3448 3413 1730 No. observations 8869 10942 3180 5056 6037 5908 No. obs. > 2 sigma 5430 5965 3004 4725 4407 5270 a (A) 24.861 18.720 11.549 11.607 11.592 11.619 b (A) 17.084 24.732 15.587 17.987 17.871 11.609 c (4) 31.937 20.311 16.673 16.519 16.480 12.943 alpha (°) 93.92 beta (°) 95.54 115.9 92.19 91.24 91.23 96.10 gamma (°) 86.99 2 Smith and Griffin 1978; Blundell et al. 1979. b Rarle et al. 1983; Camerman et al. 1983. © Griffin et al. 1985, 1986a. Subsequent to this report of structures LE(E2) and ME(E2), Mastropaolo et al. (1986, 1987) reported the independent structure determination of the same structures using the same X-ray diffraction data of Blundell. The report that the [Met®]enkephalin crystals were grown from ethanol/water (Mastropaolo et al. 1986) is incorrect. The experimental details of crystallization and data collection from Blundell’s laboratory are given in Griffin et al. 1986a. d Doi et al. 1987b. © ME(E2) and ME(E2’) are two independent studies on crystals that appear to vary only in the amount of vater present. Note the almost identical cell parameters, differing by 34 A3 in unit cell volume. TABLE 2 Conformations of enkephalin and enkephalin analogues from X-ray crystallographic determinations. Peptide Tyr-Gly-Gly-Phe-Leu- 2H, O (Smith and Griffin, 1978) Tyr-Gly-Gly-Phe-Leu- 2H, O, 2C,H,NO,X (Karle et al. 1983) Tyr-Gly-Gly-Phe-Leu- 0.5 H,O (Griffin et al. 1986a) Tyr-Gly-Gly-Phe-Met- 5.3 H,O (Griffin et al. 1986a) Tyr-Gly-Gly-Phe-Met- 5.0 H,O (Doi et al. 1987b) Tyr-Gly-Gly-(4Br)Phe-Leu- 2.5H, 0 (Ishida et al. 1984) Tyr-Gly-Gly-(4Br)Phe-Met- 2.3H,O (Doi et al. 1987b) Tyr-D-Nle-Gly-Phe-NleS- 2.5H, O, C,H, OH (Stezowski et al. 1985) Tyr-Gly-Gly-Phe- DMSO,2H, O (Fournie-Zaluskie et al. 1977) Gly-Gly-Phe-Leu- H,O (Fournie-Zaluskie et al. 1977) BOC-Tyr-Gly-Gly-(4Br)Phe-MetOH (Doi et al. 1984) BOC-Aib-Aib-Phe-MetNH, - DMSO (Prasad et al. 1983) BOC-Gly-Gly-Phe Ethyl Ester (Ishida et al. 1983) Conformation Intramolec. H-bonds type I’ g-bend Ney, t0 Op, (Gly-Gly) Tyr Phe Extended None antiparallel g-sheets Extended None antiparallel g-sheets Extended None antiparallel g-sheets Extended None antiparallel g-sheets type I’ g-bend Neyo 10 Oy, (Gly-Gly) Tyr Phe Extended None type II’ g-bend Nppe t0 Op, (D-Nle-Gly) Ny, t0 Oy, type I’ g-bend Ngy, 10 Op, (Gly-Gly) Extended None Extended None antiparallel B-sheets 3,5 Helix N,,, t0 Oy, Nyoe O aib type I' B-bend None (Gly-Gly) a4 Extended Main-Chain Conformations The six independent observations of [Leu® enkephalin, 4 molecules in LE, and 2 molecules in LE_,, in the extended conformation are superimposed in figure la. The two independent molecules of [Met® enkephalin (ME,,) are superimposed in figure 1b. The peptide chains observed in LE_,, but particularly in the three [Met®] structures are unusually planar. is is apparent by examination of the &,Y torsion angles for the [Met® Jenkephalin structures and [Leu enkephalin (LE;,) versus the extended conformations seen in LE_, (see table 3). The main-chain torsion angles of the dimer of [4-bromo-Phe? ,Met® enkephalin (MEBr,,) are remarkably similar to those in ME;, and ME_,, even though the space group and the amount of solvent water in the crystal are different. The &/Y torsion angles for Gly? and Gly? in the three [Met®] structures indicate an unusually extended conformation, all the values lie between + 160° and + 180°. The &/¥ values for the Phe! residue in the [Met®]enkephalin structures (six observations) are almost invariant, —154° + 4°/155° + 4°, and lie in the ideal B-sheet region; the values in the [Leu® Jenkephalin structures show greater variability, especially in LE,,. The Met residues are in two slightly different conformations, —~138°/157° and —-155°/170°. These results could be interpreted to indicate less flexibility in the main chain of [Met® |- versus [Leu®]enkephalin, but the small size of the data base imposes caution in drawing this conclusion. Side-Chain Conformation In addition to the ¢,y torsion angle values, which define main-chain conformation, table 3 contains the X torsion angles, which describe the Tyr, Phe, Leu, and Met side-chain conformations in the B-sheet enkephalin structures. The x* values for the Tyr and Phe side chains in the [Met enkephalin structures are almost invariant, both close to +60° (six observations of each). This is in contrast to the values observed in the [Leu® enkephalin structures: Tyr =~ +60° (three observations), 180° (three); Phe = —-60° (five), 180° (one). If the side-chain conformation observed in the extended structures is compared with that observed in the type I' B-turn [Leu’] structures, LEg, and [(4-bromo)Phe? Leu’ Jenkephalin, the major difference is in X* of Tyr: = -60° in the B-turn forms and = +60° and 180° in the extended forms; x* of Phe is = —60° in the B turn structures, similar to the major conformer in the g-sheet [Leu® Jenkephalin structures. In summary, in this admittedly small sample, the side-chain conformations in [Leu®]- versus [Met® Jenkephalin are distinguished by mutually exclusive Phe x* values. The [Leu®] structures have x! of Phe = —60°, 180°, while the [Met®] structures have x* of Phe values = +60°. The extended versus g-turn structures have mutually exclusive values for Tyr x*, —-60° (B turn), and +60°, 180° (extended). INTERMOLECULAR INTERACTIONS The [Met®]enkephalin structures consist of dimers forming infinite anti- 45 FIGURE 1 (a) A stereo view of a least-squares superposition of the six crystallographically observed extended conformations of [Leu® Jenkephalin. The 21 main chain atoms were fit. (b) A stereo view of a least-squares superposition of the two crystallographically observed extended conformations of [Met®Jenkephalin in ME;,. Each methionine residue is observed in two distinct conformations; one is dashed. 46 parallel B-sheets with varying amounts of water molecules per dimer. The two crystallographically independent molecules of the dimer are remarkably similar with respect to both main-chain and tyrosine and phenylalanine side- chain conformations (table 3). In both ME;, and ME;,, each methionine side chain is disordered, and the disordered conformations are different in the two independent molecules (see table 3). The disorder appears to be the result of close contacts between methionine side chains in adjacent independent molecules. The amount of solvent in the unit cell appears to affect the methionine side-chain conformation. In the dimer the nitrogen and carbonyl of Gly? and Phe! of one molecule are hydrogen bonded to the carbonyl and nitrogen of Phe! and Gly?, respectively, of the other molecule (figure 2). Additional hydrogen bonds connect adjacent dimers and form head-to-tail (N,,. to O,,.) connections, which join crystallographically equivalent molecules related by translation. The [Leu®Jenkephalin structure LE,, is made up of planar g-sheets arranged similarly to those in the [Met®] structures. However, the side chains are oriented differently in the two independent molecules (see table 3). There is only one molecule of water per dimer of [Leu®]enkephalin versus 10.6 and 10.0 in ME, and ME,,,, respectively. The packing is more compact than is observed in the other two [Leu®] forms. The one water molecule is tetrahedrally coordinated; it donates two hydrogen bonds to the two independent leucyl carboxyl groups and accepts two hydrogen bonds from the hydroxyl groups of two independent tyrosine side chains. In the [Met® Jenkephalin structures ME, and ME,,, the distance between B- sheets is approximately 9.0 A (one-half the b axis), while the value observed in the [Leu enkephalin structure is 7.8 A. As a result of this increase in interplanar spacing, the unit cell of [Met®]enkephalin accommodates additional water molecules. Comparison of the g-Sheet Forms The asymmetric unit, that is, repeating unit, is a dimer in structures Li ME, ,» ME;,, and MEBr,, and a tetramer in LE;,. The dimers are similar in all four structures; two independent molecules form an antiparallel g-sheet with four hydrogen bonds, N(Gly?), to O(Phe*),, N(Phe!), to O(Gly?),, N(Gly?), to O(Phe*),, N(Phe!), to O(Gly?),, where A and B refer to the two independent molecules. e dimers are joined in head-to-tail fashion, with identical dimers related by translation forming infinite ribbons. These ribbons are joined to adjacent ribbons by antiparallel hydrogen bonds translated by approximately 1/2 the length of the peptide. Therefore, dimers adjacent in the plane of the B-sheet hydrogen bond across the head-to-tail connections (see figure 2). The B-sheets thus formed are not pleated in the normal direction, that is, along the peptide chain. Instead the chains are very flat and extended, and the pleat is perpendicular to the direction of the peptide chain. The asymmetric unit in LE;, is a tetramer; two of the four molecules, A and B, form a dimer similar to the one described above for the dimeric structures with respect to hydrogen bonding. The other two molecules of the tetramer, C and D, are rotated 180° in the plane of the B-pleated sheet and form a7 FIGURE 2 Packing pattern of [Met® Jenkephalin ME, , showing the B-sheet structure. This pattern is common to the three [Met®] structures. Water is shown as large circles. The water structure is not common to the three structures. @ FIGURE 3 Comparison of the g-sheet formed in [Leu® Jenkephalin, LE,,, left, and LE_,, right. The dimer common to both structures is outlined. 48 hydrogen bonds with one another and with B and the translationally related A molecules through the peptide C=0 and NH groups. The tetramers form a continuous B-pleated sheet along a. These sheets are connected to translationally related sheets along c, forming an infinite B sheet in the ac plane. The sheets are separated from one another by solvent, much of it disordered. The distance between the sheets is 12.4A (1/2 b) and there is no interaction between the side-chain residues of adjacent sheets. The side-chain residues pack quite differently in the space between adjacent g sheets in the two [Leu®] structures, LE;, and LE;, (see figure 3). In LE;, there is a layer of solvent molecules separating the side-chains of the g-sheets adjacent along b. The structure is a sandwich layered along b, the bottom slice is a B-sheet, followed by a side-chain layer forming hydrogen bonds (Tyr) and hydrophobic interactions (Leu and Phe) to the next layer, solvent, which in turn forms hydrogen bonds and hydrophobic interactions to the side-chain layer from the top B-sheet, the final slice. Because in LE,, the dimer formed by molecules C and D is rotated 180° in the plane of the sheet with respect to the AB dimer, all three side-chain residues from the plane at y = 0.25 and three from the plane at y =~ 0.75 pack in the space between sheets separated by b/2. In LE;,, on the other hand, the residues between the planes consist of tyrosyl and leucyl side-chains from one sheet and phenylalanyl residues from the sheet separated by b/2. These form relatively tight hydrophobic interactions connecting the B-sheets along b. Packing of the g-Turn Form The asymmetric unit in the g-turn form LEg is a tetramer (see figure 4). The two central molecules form a hydrogen-bonded dimer, the N-terminus of each is hydrogen-bonded to the tyrosyl hydroxyl of the other. Molecules one and three are connected by three water molecules forming bridging hydrogen bonds between them. Molecules two and four are almost identical to one and three. These tetrameric units are repeated in three dimensions by the symmetry operations of the space group. The interactions between separate tetramers are mainly hydrophobic; the two-fold axis is surrounded by Phe and Leu side-chains (see figure 4b). In the g-turn structure there are two intramolecular hydrogen bonds that connect the Tyr and Phe groups of each of the four independent molecules, N(Tyr) to O(Phe) 2.79-2.84 A and N(Phe) to O(Tyr), 2.99-3.10 A. The six water molecules take part in a variety of interactions. Two water molecules form a bridge between the Phe! carbonyl oxygen and the Leu® carboxy oxygen of one molecule. In each of the four independent molecules, both the Gly? nitrogen and the Gly* carbonyl oxygen are hydrogen bonded to water molecules. There are patterns of solvation common to more than one of the enkephalin crystal structures; that is, water molecules bind to the same atoms even though the packing in the structures may vary. The waters common to more than one structure are given in table 4. 49 09 TABLE 3 Main-chain and side-chain torsion angles of extended forms [Leu®]enkephalin [Met®]enkephalin LE(E4)? LE(E2) ME(E2) ME(E2’) MEBr(E2) A B C D A B A B A B A B [Tyr?] 135 154 155 137 140 162 164 165 165 165 159 166 [Gly?] -144 151 141 -131 -147 172 -179 -171 -166 178 -170 172 114 -155 -157 142 156 -176 -174 167 164 -174 166 -167 [Gly3] -122 154 174 -144 -154 -167 171 -164 -163 170 -160 -165 132 =151 -170 131 162 165 -175 163 161 -173 165 -170 [Phe?] -122 -128 -119 -147 -160 -145 -157 -152 -150 -157 -150 -158 139 130 149 152 134 152 159 153 153 157 150 157 [Leu®] -79 -72 -141 -141 -141 -143 [Met®] -138 -155 -154 -138 -158 -137 176 167 137 151 143 150 154 172 172 157 169 160 [Tyr!] 177 70 53 169 175 62 71 63 63 69 58 68 -86,93 -86,99 -85,101 71,-102 83,-92 -84,95 -89,87 -88,89 -89 -89 -90 -86 [Phe?] -63 -55 -71 -68 -169 -69 69 62 63 68 53 65 87,-95 87,-88 -82,98 -91,93 66,-112 -75,104 -83,97 -87,97 96*> -83 96*> -81 [Leu®] -64 -62 -171 -80 170 67 [Met] -175 69 65 129 64 -55 173 165 -168 179 -173 154 168 168 160 -158 -152 -160 -67 -69 68 63 64 -93 58° 152° 155° -130° 53 -67 -58 125 82 142 89¢ 90¢ 68¢ -47¢ 2 Refer to table 1 for crystallographic form and references. A, B, C, D refers to independent molecules in the crystallographic asymmetric unit, tetramer in LE(E4), dimer in LE(E2) and ME(E2) forms. ® Values reported in Doi et al. (1987b). Convention requires the smaller number to be reported, which must be = 85, but lacking published coordinates it is impossible to calculate these values. © Disordered methionine side chains; C(y), S(§) and C(g) are disordered in ME(E2), A and B, and ME(E2’), A and B. [ BETA TURN TETRAMER (b) FIGURE 4 (a) Stereo view of the tetramer that makes up the asymmetric unit in LEg. Large circles are water molecules. (b) Stereo view of the packing of a unit cell, 16 molecules, in LEg. Note the hydrophobic holes formed by tyrosyl, phenylalanyl, and leucyl residues. 51 TABLE 4 Common patterns of solvation in enkephalin crystal structures: atoms of enkephalin molecules hydrogen-bonded to water. LEg LE,, LE,, ME," CO (leu?) CO (leu®) CO (lewd) CO (met5) OH(tyr') OH(tyr') OH(tyr*) OH(tyr?) N* (tyr) N* (tyr!) C=0(gly’) C=0(gly*) C=0(phe?) C=0(phe?) C=0(phe?) * The authors do not have the crystallographic coordinates for ME,,, and MEBTr,,, so the solvent structure cannot be calculated. Conformation of Enkephalin at the u and § Receptor Since the demonstration of the existence of multiple forms of opioid receptors, arguments have been made that the u and § subtypes bind different conformations of the endogenous opioids. Soos et al. (1980) suggested this on the basis of CD spectra on the enkephalins and enkephalin analogues. Raman spectra was interpreted as showing more folded conformations of [Leu® Jenkephalin than [Met®]enkephalin in aqueous solution and DMSO (Renugopalakrishnan et al. 1985). The observed solid state conformations led to the proposal that [Leu® enkephalin binds to the u receptor in a folded conformation and [Met® enkephalin to the § in an extended conformation (Ishida et al. 1984). Recently Doi et al. (1987b) suggested that a pair of g- bend molecules of enkephalin can mimic the g-sheet dimer, placing similar functional groups in the same regions of three-dimensional space, and bind to the § receptor. In a subsequent paper the same group (Doi et al. 1987a) suggested that the g-turn monomer and the extended dimer could each bind to both 1 and 8 subtypes of the opioid receptor. They based this conclusion on computer graphics and empirical energy studies of the two conformations, adjusting the tyrosyl and phenylalanyl side chains on both conformations to superimpose the analogous residues in the same regions of three-dimensional space. This hypothesis requires further testing by biochemical techniques. The B-turn structure of [Leu®]enkephalin was initially proposed to be the biologically active conformation (Smith and Griffin. 1978). The conclusion was based on a least-squares superposition of the B-turn conformation of enkephalin with the structures of morphine, etorphine and PET, 7-[1-phenyl- 3-hydroxybutyl-3]-endoethenotetrahydrothebaine, the latter two superactive agonists. In addition, the fact that the ¢,y torsion angles of Gly? place the conformation in a region of conformational space allowed for D-amino acids, and D-Ala? substituted enkephalins had been shown to be very active, supported the proposal. These arguments were made before the existence of opioid receptor subtypes was demonstrated and the selectivity of the 52 individual subtypes shown experimentally. The activity of etorphine and the tetrahydrothebaines at both u and § opioid receptor subtypes, however, has not been accounted for in the suggestion that u and § subtypes bind different conformations of the enkephalins. The fully extended conformation of a small peptide can form the maximum number of intermolecular hydrogen bonds. In going from the extended form to the type I' B-turn conformation centered on Gly?Gly®, the enkephalin molecule decreases the number of hydrogen bonding groups available for receptor interactions and increases the wo hydrophobicity. This may be relevant to the conformation assumed at the receptor(s), since the morphine- and tetrahydrothebaine-like molecules are more hydrophobic than enkephalin. OPIATE DRUGS Naltrexone Derivatives O24 FUNALTREXAMINE «- and B-Funaltrexamine («- and B-FNA) are naltrexone derivatives differing only in chirality at C6. Both compounds bind to the u opioid receptor in mouse vas deferens (MVD) and guinea pig ileum (GPI) preparations, but only the B-epimer binds irreversibly, presumably by forming a covalent bond to the receptor. For this reason, B-FNA has been used to irreversibly block p receptors in order to isolate the binding characteristics of § receptors in GPI and MVD preparations, and § and « sites in brain homogenate preparations. A two-step recognition process had been proposed to account for the different binding characteristics of «- and B-FNA for the u receptor; both bind in the first recognition step but only the B-epimer is in the proper orientation for the second recognition step which results in alkylation. The crystal structures of «- and B-FNA suggested a possible explanation for the observed differences (Griffin et al. 1986b). The two compounds have almost identical conformations in the fused rings with the exception of the C ring; the B-epimer has a chair conformation and the o-epimer a twist-boat conformation, resulting in the fumaramate side chain being equatorial to the C ring in both cases. Analysis of the superposition of the two structures 53 FIGURE 5 Stereo view of the superposition of the crystallographically observed structures of «- and B-funaltrexamine, with the proposed sites of receptor interaction. The first recognition step involves the phenol ring, the phenol hydroxyl, and the charged nitrogen. The second recognition step involves the fumaramate group and possibly the amino nitrogen at C6 (from Griffin et al., 1986b, Copyright 1986, American Chemical Society). 54 revealed that the fumaramate groups occupied the same region with respect to the naltrexone frame in both structures, but the conjugated fumaramate roups were oriented orthogonal to one another. A close oxygen contact (O3 rom a symmetry related molecule) to the double bond carbon (C23) observed in the crystal structure was used to model this second recognition site and explain the failure of the «-epimer to irreversibly bind to the receptor (see figure 5). The conformation of the C ring of naltrexone derivatives appears to be sensitive to substitution at C6. The crystal structure of the 6a-amino derivative of naltrexone, 6a-oxymorphamine (Lever et al. 1985) confirmed their conclusions based on *H NMR that the C ring in the 6x-amino epimer is in a twist-boat conformation and in the 6B-epimer is a chair. As in the FNA structures this places the 6 substituent in the equatorial position in both epimers. Comparison of the C ring torsion angles in «-FNA and 6o- oxymorphamine shows they have almost identical conformations. Acylmorphinans Although the phenolic hydroxyl group is considered essential to activity in morphine and structurally related analogues, its presence results in rapid inactivation when given by oral route. Mohacsi et al. (1985) have reported the crystal structure of a C3-acyl morphinan that retains morphine-like analgesic activity even when administered orally. The O3 atom could be serving as a hydrogen bond acceptor, since the phenolic oxygen in morphine can act as both donor and acceptor of hydrogen bonds. The oxygen to nitrogen distance in the acylmorphinan structure is 7.94 A, whereas in the 30 crystal structures containing the morphine five fused-ring system in the Cambridge Structural Database (Allen et al. 1979), the value of the distance ranges from 6.77 to 7.16 A, average 7.03(11) A. Conformations of the Morphine Fused-Ring System Brown et al. (1983) reported that the conformation of morphine in the crystal is different from that in aqueous solution, and that the latter is the one "available for receptor binding,” although no evidence or explanation for this assertion was included in the report. Their study was based on a comparison of the high resolution *3C NMR spectra of solid morphine sulfate versus solid morphine free base, solid morphine sulfate versus morphine sulfate dissolved in D,0O, and morphine sulfate dissolved in D,O at 22°C and 70°C. Their data were interpreted as showing a minor component of the nitrogen invertoisomer in solution, the nitrogen methyl went from equatorial to axial, and the inversion was associated with a "greater freedom of motion in the piperidine ring than previously believed.” They speculated that the downfield chemical shifts of the spectral lines assigned to C2, C7, C11, C15, and C16 on going from solution to solid were due to interactions in the solid state between these atoms and the sulfate group. The authors did not identify the crystalline polymorph they were examining. Solid state spectral studies should always verify the identity of the crystals studied by means of b5 powder or single crystal X-ray diffraction to determine cell constants and space group. Without this information, no meaningful comparison can be made between the spectral studies and crystallographic results. The change in chemical shifts are difficult to explain from the crystal structure of morphine, 0.5 SO,, 2.5 H,O (Wongweichintana et al. 1984); although C2, C15, and C16 show close contacts to sulfate oxygens in the crystal (3.39 to 3.49 4), C7 and C11 do not, while C3 and the N-methyl carbon also show short contacts. The Cambridge Structural Database (Allen et al. 1979) contains 30 crystal structure determinations of compounds that contain the morphine five fused- ring framework. In this data base the methyl substituent on the piperidyl nitrogen is always observed equatorial and there is little evidence for great freedom of motion in the piperidine ring especially at C15 and C16. The Bipstidy) ring is always a chair, and the torsion angle C13-C15-C16-N only varies from -47° to -57° in the entire sample, average 51.2 (2.0)°. The main region of flexibility is ring C, and the changes in ring C conformation can be correlated with changes in chemical constitution, either a double bond at C6, C7 or C7, C8, or the substitution of a nitrogen on C6, as discussed above. There are also changes in the three carbon-nitrogen bonds of the piperidyl nitrogen correlated with whether the structure is the free base or salt. SUMMARY Information on intramolecular geometry, low energy conformations, hydrogen bonds, both intramolecular and intermolecular, and preferred intermolecular interactions is obtained from single crystal X-ray diffraction experiments. Structure determinations of crystals with more than one molecule in the asymmetric unit and of different crystalline forms provide information on conformational flexibility and stable aggregation states. The single crystal X-ray diffraction studies of enkephalin have demonstrated a number of minimum energy conformations of the main chain and side chains, a type I’ B turn centered on Gly?Gly* and a number of extended main-chain conformations. In the studies of native enkephalins, dimers and tetramers form repeating units, and some patterns of solvation are observed in more than one form. Certain conformations and interactions proposed on the basis of solution spectroscopic studies have yet to be observed in the solid state. Efforts should be made to grow different crystalline forms of the enkephalins and to determine the solid state structure of enkephalin analogues that exhibit high selectivity for a particular opioid receptor subtype. Crystallographic studies of opiate dup with selective activity profiles at different receptor subtypes can give information on the features responsible for active site differentiation between the subtypes of opioid receptor. Analysis of the crystallographic data base of 30 compounds containing the five fused-ring morphine moiety indicate that: (1) the methyl group on the 56 piperidyl nitrogen prefers the equatorial position, (2) the conformation of the piperidyl ring is a relatively invariant chair conformation, (3) C-ring conformation depends on the chemical constitution of the C-ring and substitution at C6. REFERENCES Allen, F.A.; Bellard, S.; Brice, M.D.; Cartwright, B.A.; Doubleday, A.; Higgs, H.; Hummelink, T.; Hummelink-Peters, B.G.; Kennard, O.; Motherwell, W.D.S.; Rodgers, J.R.; and Watson, D.G. The Cambridge Crystallographic Data Centre: Computer-based search, retrieval, analysis and display of information. Acta Cryst B35:2331-2339, 1979. Beretta, C.A.; Parrilli, M.; Pastore, A.; Tancredi, T.; and Temusi, P.A. Experimental simulation of the environment of the opioid receptor. A 500 MHz study of enkephalins in CDCl,. Biochem Biophys Res Commun 121:456-462, 1984. Blundell, T.L.; Hearn, L.; Tickle, I.J.; Palmer, R.A.; Morgan, B.A.; Smith, G.D.; and Griffin, J.F. Crystal structure of [Leu®]enkephalin. Science 205:220, 1979. Brown, C.E.; Roerig, S.C.; Fujimoto, J.M.; and Burger, V.T. The structure of morphine differs between the crystalline state and aqueous solution. J Chem Soc Chem Commun 1983: 1506-1508, 1983. Camerman, A, and Camerman, N. Conformational features of the opioid peptides in the solid state: A review of X-ray crystallographic research. In: Rapaka, R.S.; Barnett, G.; and Hawks, R.L., eds. Opioid Peptides: Medicinal Chemistry. National Institute on Drug Roe Research Monograph 69. DHS Pub. No. (ADM) 86-1454. Washington, D.C.: Supt. of Docs., U.S. Govt. Print. Off., 1986. pp. 351-363. Camerman, A.; Mastropaolo, D.; Karle, I.L.; Karle, J.; and Camerman, N. Crystal structure of leucine-enkephalin. Nature 306:447-450, 1983. Doi, M.; Ishida, T.; Inoue, M.; Fujiwara, T.; Tomita, K.-i.; Kimura, T.; and Sakakibara, S. Three-dimensional structure of monoanionic methionine-enkephalin: X-ray structure of tert-butyloxycarbonyl-Tyr-Gly- Gly-(4-bromo)Phe-Met-OH. FEBS Lett 170:229-231, 1984. Doi, M.; Tanaka, M.; Ishida, T.; and Inoue, M. The three-dimensional similarity between a dimeric antiparallel extended structure and a g-turn folded form of enkephalin. FEBS Lett 213:265-268, 1987a. Doi, M.; Tanaka, M.; Ishida, T.; Inoue, M.; Fujiwara, T.; Tomita, K-i.; Kimura, T.; Sakakibara, S.; and Sheldrick, G.M. Crystal structures of[Met®] and [(4-bromo)Phe*, Met>]enkephalins: formation of a dimeric antiparallel g-structure. J Biochem 101:485-490, 1987b. Fournie Zaluskie, M-C.; Prange, T.; Pascard,C.; and Roques, B.P. Enkephalin related fragments. Conformational studies of the tetrapeptides Tyr-Gly-Gly-Phe and Gly-Gly-Phe-X (X = Leu, Met) by X- ray and 'H NMR spectroscopy. Biochem Biophys Res Commun 79:1199-1206, 1977. TF Griffin, J.F.; Langs, D.A.; Smith, G.D.; Blundell, T.L.; Tickle, L.J.; and 57 Bedarkar, S. The crystal structures of [Met®Jenkephalin and a third form of [Leu®]enkephalin: Observations of a novel pleated g-sheet. Proc Natl Acad Sci USA 83:3272-3276, 1986a. Griffin, J.F.; Langs, D.A.; Smith, G.D.; Van Roey, P.V.R.; Blundell, T.L.; Tickle, 1.J.; and Hearn, L. The crystal structures of [Met®]enkephalin and a third form of [Leu®]enkephalin. Abstracts of the Annual Meeting of the American Crystallographic Association, Stanford University, Stanford, California, Series 2, Volume 13, Abstract No. PC36, p. 61, 1985. Griffin, J.F.; Larson, D.L.; and Portoghese, P.S. Crystal structures of a- and B-funaltrexamine: conformational requirement of the fumaramate moiety in the irreversible blockage of u opioid receptors. J Med Chem 29:778-783, 1986b. Hughes, J.; Smith, T.W.; Kosterlitz, H.W.; Fothergill, L.A.; Morgan, B.A.; and Morris, H.R. Identification of the two related pentapeptides from the brain with potent opiate agonist activity. ~~ Nature (London) 258:577-579, 1975. Ishida, T.; Kenmotsu, M.; Mino, Y.; Inoue, M.; Fujiwara, T.; Tomita, K-i.; Kimura, T.; and Sakakibara, S. X-ray diffraction studies of enkephalins, crystal structure of [4’-bromo)Phe! ,Leu®Jenkephalin. Biochem J 218:677-689, 1984. Ishida, T.; Tanabe, N.; and Inoue, M. Structure of tert- butoxycarbonylglycylglycyl-L-phenylalanine ethyl ester, C,,H,,N,O,. Acta Cryst C39:110-112, 1983. Khaled, M.A. Conformations of opioid peptides as determined by nuclear magnetic resonance and related spectroscopies. In: Rapaka, R.S.; Barnett, G.; and Hawks, R.L., eds. Opioid Peptides: Medicinal Chemistry. National Institute on Drug Abuse Sa Monograph 69. DHHS Pub. No. (ADM) 86-1454. Washington, D.C.: Supt. of Docs., U.S. Govt. Print. Off., 1986. pp. 266-290. Karle, 1.L.; Karle, J.; Mastropaolo, D.; Camerman, A.; and Camerman, N. [Leu’ Jenkephalin: Four cocrystallizing conformers with extended backbones that form an antiparallel g-sheet. Acta Cryst B39:625-637, 1983. Lever, O.W., Jr.; Bhatia, A.V.; and Chang, K.-J. Opioid receptor interactions and conformations of the 6a and 68 epimers of oxymorphamine. Solid-state structure of 6a-oxymorphamine. J Med Chem 28:1652-1656, 1985. Mastropaolo, D.; Camerman, A.; and Camerman, N. Crystal structure of methionine-enkephalin. Biochem Biophys Res Commun 134:698-703, 1986. Mastropaolo, D.; Camerman, A.; Ma, L.Y.Y.; and Camerman, N. Crystal structure of an extended-conformation leucine-enkephalin dimer monoydrate. Life Sciences 40:1995-1999, 1987. Mohacsi, E.; O’Brien, J.; Blount, J.; and Sepinwall, J. Acylmorphinans. A novel class of potent analgesic agents. J Med Chem 28: 1177-1180, 1985. Prasad, B.V.V.; Sudha, T.S.; and Balaram, P. Molecular structure of Boc- Aib-Aib-Phe-Met-NH,- DMSO. A fragment of a biologically active enkephalin analogue. J Chem Soc Perkin I 1983:417-421, 1983. Renugopalakrishnan, V.; Rapaka, R.S.; Collete, T.W.; Carriera, L.A.; and Bhatnagar, R.S. Conformational states of Leu®- and Met>-enkephalins in solution. Biochem Biophys Res Commun 126:1029-1035, 1985. 58 Schiller, P.W. Conformational analysis of enkephalin and conformation- activity relationships. In: Udenfriend, S., and Meienhofer, J., eds. The Peptides: Et sis, S ihegis Biology. Vol. 6. New York: Academic ress, 1984. pp. 219- Smith, G.D., ols Griffin, J.F. Conformation of [Leu Jenkephalin from X- ray diffraction: Features important for recognition at opiate receptor. Science 1091714. 1216, 1978. Soos, J.; Berzetei, 1.; Bajusz, S.; and Ronai, A.Z. Correlation between circular on, data and ‘biological activities of 2,5 substituted enkephalin analogues. Life Sciences 27:129-133, 1980. Stezowski, J.J.; Eckle, E.; and Bajusz, S. A crystal structure determination for Tyr-D- -Nle- -Gly-Phe- NleS [NleS=MeCH, CH, CH, CH(NH,)SO,H]: An active synthetic enkephalin analogue. Tr Chém Soc Chem Commun 1985:681-682, 1985. Wongweichintana, C.; Holt, E.M.; and Purdie, N. Structures of morphine methyl iodide monohydrate, « H,,NO,)*.I".H,0, and di(morphine) dihydrogensulfate pentahydrate 20¢,, ,oNO, y SO, 2-5H,0. Acta Cryst C40:1486-1490, 1984. AUTHORS Jane F. Griffin, Ph.D. G. David Smith, Ph.D. Molecular Biophysics Department Medical Foundation of Buffalo, Inc. 73 High Street Buffalo, New York 14203, U.S.A. 59 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D, eds. National Institute on Drug Abuse, 1988 Conformational Analysis of Cyclic Opioid Peptide Analogs Peter W. Schiller, Ph.D., and Brian C. Wilkes, Ph.D. INTRODUCTION Extensive conformational studies of the enkephalins [H-Tyr-Gly- Gly-Phe-Met(or Leu)-OH] by various spectroscopic techniques and by X-ray diffraction analysis revealed that these linear pentapeptides are highly flexible molecules capable of assuming a number of both folded and extended conformations of comparably low energy (Schiller 1984). In fact, it has been demonstrated quite convincingly that in solution enkephalin exists in a conformational equilibrium (Fischman et al. 1978). It has, therefore, become clear that conformational studies of these small opioid peptides and of many of their analogs are unlikely to provide any insight into their bioactive (receptor-bound) conformation(s). Furthermore, the conformational flexibility of the enkephalins is most likely the reason for their lack of specificity toward the different opioid receptor classes (un, 6, n) because conformational adaptation to the various receptor topographies is possible. Thus, even though the enkephalins preferentially bind to the 6-receptor, they also have quite good affinity for the wu-receptor and, therefore, are only moderately &-receptor selective. CONFORMATIONALLY RESTRICTED ANALOGS OF OPIOID PEPTIDES The conformational flexibility of opioid peptides can be reduced through incorporation of conformational constraints. In recent years conformationally restricted analogs of enkephalin have been synthesized with two goals in mind. First, such analogs are more amenable to a meaningful conformational analysis since because of their relatively rigid structure they are unlikely to undergo major conformational changes upon binding to the receptor and, therefore, information about the bioactive conformation at the various opioid receptors can be obtained. Second, the introduction of conformational constraints may result in improved receptor selectivity, because the conformationally restricted analog may have good affinity for one receptor type but may no longer be able to undergo a conformational change necessary to 60 bind to another receptor class. Local conformational restrictions in enkephalins have been achieved either at particular peptide backbone positions (e.g., through N®- or C®- methylation or through incorporation of small ring structures) or in selected side chains (e.g., through substitution of a dehydroamino acid) (for a review, see Schiller 1984). However, the most drastic restriction of the overall conformational space available to the peptide has been realized through the design and synthesis of cyclic enkephalin analogs. Three families of biologically active cyclic opioid peptide analogs have been synthesized to date. A cyclic enkephalin analog was first prepared through substitution of D-a, 7Y- diaminobutyric acid (A,bu)” in position 2 of the peptide sequence followed by cyclization between the side chain amino group of Abu and the C-terminal carboxyl group (DiMaio and Schiller 1880). The resulting analog, H-Tyr-cyclo[-D-A, bu-Gly-Phe-Leu-] (figure 1, compound 2), containing a fairly rigid l4-membered ring structure, turned out to be moderately p-receptor selective (Schiller and DiMaio 1982). Pharmacologic comparison of 2 with a corresponding open-chain analog revealed that its u-receptor preference is a direct consequence of the conformational restriction introduced through ring closure and, furthermore, permitted the fundamental conclusion that p- and 6-opioid receptors differ indeed from one another in their conformational requirements toward peptide ligands (Schiller and DiMaio 1982). Homologs of 2 (compounds 1, 3, and 4) were obtained through variation of the side chain length in position 2 and also were found to display moderate preference for p-receptors over 6- receptors (DiMaio et al. 1982). On the other hand, a diastereomer of cyclic peptide 2, H-Tyr-cyclo[-D-A bu-Gly-Phe-D- Leu-], was non selective (Mierke et al. 1987). Several partial retro-inverso analogs of 2 were found to be very potent and pu- selective (figure 1, structures 2b and 2c), whereas both diasteromers of 2d showed very weak activity (Bermag et al. 1983; Richman et al. 1985), presumably because the Gly -Phe peptide bond is important for binding to the receptor. A second class of cyclic enkephalin analogs was obtained through side chain-to-side chain cyclization between a D-Cys and a D- or L-Cys residue substituted in positions 2 and 5 of the peptide sequence, respectively (Schiller et al. 1981). The resulting cystine-containing analogs H-Tyr-D-Cys-Gly-Phe-L(or D)-Cys-X (5) were highly potent and showed either no receptor selectivity (X= NH, ) or moderate 6-receptor selectivity (X = OH) (Schiller et al. 1985a). The Trp analog H-Tyr-D-Cys-Gly-Trp-D-Cys-NH, (6) displayed an ctivity profile similar to that of the corresponding Phe parent compound (Schiller 1983). Replacement of the half-cystine residues in positions 2 and/or 5 with penicillamine residues resulted in compounds (7-7c) with markedly improved &-receptor selectivity (Mosberg et al. 1983). The configurational requirements of cyclic analogs 4 and 5 at the residues in positions 1, 2, 4, and 5 of the peptide sequence were 61 29 R-7yz-D-a,0r-Cly-Phe-lauy R~Tyr~D-a,bu-Gly-Phe-Léuy HeTyr=Deaapu~ClyPhe~D-Lau, HeIyr=DeCla=ClynPhe-Laty H-Tyr -D-A,bu-Gly-gPhe-L(or D)emleny H-Tyr-D-A,bu-gGly-L(or D)-mPhe-Leu F-Tyr-D-Ori-Qly he Tauy Hn TyE~Dulye Gl ysrneslovy Hn 290 =D=0rg=Gly=Prea1lor D)-Cys-X H-Tyr-D-Cys-Gly-Trp-D-Cys-NH, fe FIGURE 1 H-Tyr-D-Pen-Gly-Phe-L(or D)-Cys-NH, isin) H-Tyr-D-Pen-Gly-Phe-L(or D)-Cys-OH ia rain) He7yr D080) y= Phe~Llor D)-Pen-OH H-Tyr-D-Pen-Gly-Phe-L(or D)-Pen-OH br cr —— 2 H-Tyr-D-Orn-Phe-D-Asp-NH meer J H-Tyr-D-Orn-Phe-Asp-NH Ce 2 H-Tyr-D-Asp-Phe-Orn-NH, H-Tyr-D-Orn-Phg-Asp-NH, H-Tyr-L-Orn-Phe-Asp-NH LY 2 H-Tyr -D-Orn-Phe (NMe) -Asp-NH, fe Structural Formulas of Cyclic Opioid Peptide Analogs an) 12) (13) found to be the same as those of the corresponding residues in linear enkephalins (Schiller and DiMaio 1983). This finding as well as other structure-activity data obtained with these compounds indicated that corresponding moieties in these cyclic and linear enkephalin analogs interact with the same subsites on the receptor. It can thus be concluded that both H-Tyr-cyclo[-D- Lys-Gly-Phe-Leu-] and H-Tyr-D-Cys-Gly-Phe-Cys-NH, have the same mode of binding to the receptor eT enkephalins. Another family of side chain-to-side chain cyclized opioid peptide analogs was obtained through amide bond formation between the side chain amino and carboxyl groups of appropriately substituted Orn (or Lys) and Asp (or Glu) residues (Schiller and Nguyen 1984; Schiller et al. 1985b, 1987). Among the various cyclic lactam analogs of this type prepared, H-Tyr-D-Orn-Phe-Agp- NH (8) turned out to be potent and highly p-selective. The latter analog contains a rather rigid 13-membered ring structure and a Phe residue in the 3-position as it is the case with the dermorphins and the B-casomorphins. Among several prepared analogs of 8, H-Tyr-D-Orn-Phe-D-Asp-NH, (9 and H-Tyr-D-Asp-Phe- Orn-NH, (10) showed the same high M-sélectivity as the parent compound, whereas H-Tyr-D-Orn-Phg-Asp-NH, (11) was less u- selective due to reduced affinity for the pu-receptor. Analogs H- Tyr-L-Orn-Phe-Agp-NH, (12) and H-Tyr-D-Orn-Phe (NMe ) -Agp-NH, (13) showed very weak activity. Taken together, the structure- activity data obtained with analogs of H-Tyr-D-Orn-Phe-Asp-NH indicated that the mode of binding of the latter peptide is identical with that of the dermorphins but different from that of the B-casomorphins (Schiller et al. 1987). CONFORMATIONAL ANALYSIS OF CYCLIC OPIOID PEPTIDE ANALOGS Side Chain-to-End Group Cyclized Enkephalin Analogs The conformational behavior of the cyclic prototype analog H-Tyr- cyclo[-D-A,bu-Gly-Phe-Leu-] (2) has been investigated by various groups, using a variety “of theoretical and experimental techniques. In a first theoretical conformational analysis, a molecular mechanics approach was used to determine low energy conformers of 2 (Hall and Pavitt 1984a). Th loyest energy conformer obtained was characterized by a Gly” -Phe type II' bend, and it was suggested by the authors that the same type of bend might also be present in the receptor-bound conformation of linear enkephalins. Furthermore, some of the low energy conformers found showed a transannular hydrogen bond between the side chain NH of A,bu and the A,bu carbonyl group. Another energy minimization soudy of cyclic analog 2 resulted in a number of low energy conformers that contained either relatively planar ring structures stabilized by intramolecular hydrogen bonds (B- turns or C, structures) or twisted ring structures devoid of any hydrogen bonds (Maigret et al. 1986). Furthermore, the author postulated that the tyramine portion of Tyr and the Gly carbonyl group in 2 might correspond to the tyramine portion and the C-ring hydroxyl group contained in morphine. It was then 63 attempted to impose spatial overlap of these pharmacophoric moieties with those in the rigid morphine molecule through conformational adaptation of each one of the low energy conformers of cyclic peptide 2. This was possible at a relatively low energy expenditure (6 kcal/mol) with only one of the low energy conformers and resulted in a tilted structure tha was characterized by intramolecular. hydrogen bonds from Leu"-NH to A,bu-CO (B-bend) and from Gly -NH to Tyr -CO (C structure). $e was suggested that the latter conformation sight represent the bioactive one at the u-receptor, since the 6 kcal/mol increase in energy as a consequence of the imposed fit could certainly be compensated for by favorable binding interactions at the receptor. It must be realized, however, that this proposed model depends entirely on the authors' somewhat arbitrary choice of the pharmacophore. In a third study, both computer simulations and Ling spectroscopy were employed to determine the conformation(s) of cyclic analog 2 (Mammi et al. 1985). The performed molecular dynamics study showed that the ring structure of 2 is not entirely rigid but fluctuates about a few equilibrium conformations. The most stable ring conformations were found to be stabilized by transannular hydrogen bonds implicated in the formation of C. structures. The carried out energy minimization study resulted in one lowest energy conformer characterized. by hydrogeg bonds from A bu, (side chain)-NH to A, bu-CO, from Leu” -NH to Gly -CO and from ty -NH to Tyr -CO. The ring strugture of another obtained low energy conformer also showed a Leu -NH-— OC- Gly~ hydrogen bond, whereas the A, bu side chain NH was hydrogen- bonded to the Phe -CO rather than to the A bu-CO. Determination of the temperaturg dependence of the amide proton chemical shifts (g6/dT) in the "HNMR study perforged with cyclic analog 2 in ["H_IDMSO revealed that both the Leu NH and the side chain NH of A,bu may be involved in hydrogen bond formation. These results are consistent with the hydrogen bonding patterns obtained in the energy minimization and suggest that the solution conformation of 2 may indeed be stabilized by the transannular hydrogen bonds observed in the calculated lowest energy conformers. It is obvious that the results of these various conformational studies on «cyclic analog 2 have not yet led to a consensus concerning a possible unique bioactive conformation at the receptor. Clearly, the most important finding of these endeavors is the realization that the ring structure in 2 still retains some flexibility and that the various intramolecular hydrogen bonds observed are constantly formed, broken, and re- formed again, as shown most conclusively in the molecular dynamics study. In a recent study, the conformational behavior of H-Tyr-cyclo[-D- A,bu-Gly-Phe-Leu-] (2) was compared with that of its diastereomer with Leu” in the D-configuration (analog 2a), using gain a combination of computer simulations and “HNMR in [“H_]DMSO (Mierke et al. 1987). The obtained results showed that, in 64 contrast to the tan? peptide, the conformation of the Petey? analog is not stabilized by any intramolecular hydrogen bonds. Furthermore, the NMR data (T, relaxation time measurements) and molecular dynamics study indicated that both the peptide backbone and the side chains in 2a are considerably more flexible than in 24 In particular, the computer simulation carried out for 20 Picoseconds reyealed that the important intramolecular distance between the Tyr and Phe. aromatic rings remains constant (~20 Rf) in the case of the L-Leu” analog, whereas considerable variation of that same distance with time (5-16 %) is seen in the case of the D-Leu analog. It was concluded that the more rigid conformation and the relatively large and fixed distance between the Tyr™ and Phe aromatic rings of analog 2 may be responsible for its yu-receptor preference, whereas the lack of receptor selectivity shown by 2a may be due to its comparatively higher structural flexibility. The same approach was also used to investigate the conformational behavior of partial retro-inverso analogs of 2, characterized by a reversed amide bond in three different positions of the ring structure (figure 1, compounds 2b, 2c, and 2d). Various transannular hydrogen bonds, giving rise to C, structures or also C, and C structures, were detected in the computer simulation e2udy g00 were found to be compatible with the results of the NMR temperature perturbation study, which permitted the identification of hydrogen-bonded amide protons. No PB-turns were observed, as the conformational restriction introduced through ring closure renders the formation of a 4-1 hydrogen bond energetically unfavorable. In all analogs the side chains of the Phe and Leu residues were found to be very flexible, whereas the Tyr side chain appeared to exist primarily in the trans conformation (x,~ 180°), which was favored by more than 3 kcal/mol over gauche conformations. Hall and Pavitt (1985) compared the low energy conformations of H-Tyr-cyclo[-D-A,pr-Gly-Phe-Leu-] (1) and H-Tyr-cyclo[-D-Orn-Gly- Phe-Leu-] (3) with those of H-Tyr-cyclo[-D-A,bu-Gly-Phe-Leu-] (2), using the same molecular mechanics approach as in their original study of 2 (Hall and Pavitt 1984a). This investigation resulted in a number of low energy ring conformations common to all three analogs, which differed from one another primarily in the orientation of a particular amide bond. Several of 5 thege conformations contained a type II' bend centered on Gly -Phe , and it was speculated that one of these might represent the bioactive conformation at the regeptor. Kessler et al. (1985) performed a "H NMR study in ["H_]JDMSO with H-Tyr-cyclo[-D- Orn-Gly-Phe-Leu-] (3) and H-Tyr-cyclo[-D-Lys-Gly-Phe-Leu-] (4). The obtained NMR data indicated that cyclic analog 3 has a relatively rigid ring conformation, and the determination of the temperature dependence of the amide proton chemical shifts (dé /dT) suggested the gxistence of two tyansannular hydrogen bonds (Leu”-NH -0C-Gly~ (y-turn) and Orn“-N®H-0C-Orn“). The analogous y-turn and A, bu-NYH- OC-A,bu hydrogen bond had also been observed with cyclic analog 2" in the conformational study described above (Mammi et al. 1985). In comparison with 3, the ring conformation in cyclic analog 4 was found to be considerably 65 more flexible. The d&/dT values and coupling constants determined with 4 suggested the existence of a B-turn centered on Phe -Leu” ang stabilized by a hydrogen bond betyeen the N®H group of D-Lys and the carbonyl group of Gly . The ring conformation of analog 3 defined by the two hydrogen bonds detected in this study formed the basis for a recent computer- modeling study aimed at determining topological similarities between this cyclic peptide and 7-a-[(1R)-1-hydroxy-l-methyl-3- phenylpropyl]-6,l4-endo-ethenotetrahydrooripavine (PEO) (DiMaio et al. 1986). Side Chain-to-Side Chain Cyclized Enkephalin Analogs Using the molecular mechanics approach, Hall and Pavitt (1984b) performed a theoretical conformational analysis of the potent, non selective egkephalin analogs H-Tyr-D-Cys-Gly-Phe-D(or L)-Cys- NH, (5). A Gly -Phe type II' bend was indicated by the obtained results, as it had been the case with the H-Tyr-cyclo[-D-Xxx-Gly- Phe-Leu-] analogs analyzed in the same manner by these authors (see above). However, comparison of the l4-membered ring structures in these two cyclic peptides with the l4-membered ring of H-Tyr-cyclo[-D-A bu-Gly-Phe-Leu-] (2) indicated a higher structural flexibility in the case of the cystine-containing analogs, which may explain their lack of receptor preference. In a conformational study by fluorescence techniques, the tyrosine fluorescence quantum yield determined with H-Tyr-D-Cys-Gly-Phe-D- Cys-NH, was found to be 2.5 times lower than that of the linear analog H-Tyr-D-Ala-Gly-Phe-Met-OH (Schiller 1983), presumably due to the quenching effect of the adjacent disulfide group, which is known to occur at distances of less than 6 between the Tyr phenol ring and the -S-S moiety. This observation suggested the existence of an energetically favorable intramolecular complex between the phenol ring and the disulfide group, which would result in an interaction energy of about 1 kcal/mol at an optimal distance of 3.5 8 between the plane of the aromatic ring and one of the sulfur atoms. On the basis of these findings and arguments, a close interaction between the tyrosine side chain and the disulfide bridge in H-Tyr-D-Cys-Gly-Phe-D-Cys-NH, was proposed. inglet-singlet energy transfer between the phenol ring of Tyr and the indole moiety of Trp was measured in the analog H-Tyr-D-Cys-Gly-Trp-D-Cys-NH, (6). Evaluation of the determined fluorescence parameters on the basis of F8rster's equation resulted in an average intramolecular distance of 9.7 0.2 R between the two aromatic rings contained in 6. This mean distance is nearly identical with the average Tyr -Trp distance (9.5 * 0.3 8) in the linear enkephalin analog H-Try-D-Ala-Gly- Trp-Met-OH, which was determined by the same technique. The conformations of the two non selective cystine-containing analogs H-Tyr-D-Cys-Gly-Phe-L-C -NH, and H-Tyr-D-Cys-Gly-Phe-D- Cy,s-NH (structures > were compared with those of the related 6- selective Pen -containing analogs H-Tyr-D-Pen-Gly-Phe-L-C -NH, and H-Tyr-D-Pen-Gly-Phe-D-Cys-NH, (structures 7) in a HNMR study carried out in D,0 (Mosberg and Schiller 1984)7 Similar chemical 2 66 shifts, d&/dT values, and coupling constants were observed for corresponding penicillamine and cysteine containing analogs, indicating similar overall conformations. However, the obtained NMR, data suggested that, in comparison with the corresponding Cys~ analogs, the Pen analogs show higher structural rigidity in the C-terminal part of the molecule, which may explain their 6- receptor selectivity. The determined temperature dependences of the amide proton chemical shifts did not indicate the existence of intramolecular hydrogen bonds in any of these four cyclic analogs. The large chemical shift difference obgerved for the two penicillamine methyl resonances in both Pen analogs are indicative of a ring current effect caused by the tyrosyl aromatic moiety and, as in the case of H-Tyr-D-Cys-Gly-Phe-D-Cys NH,, (see above), suggest a close proximity between the Tyr aromatic ring and the disulfide moiety. The same type of NMR analysis was then performed with six penicillamine-containing cyclic enkephalin analogs (structures 7a, 7b, and Je), all of which display 6-receptor selectivity (Mosberg 1987) Some variation in various NMR parameters was observed even between compounds that displayed similar potency and receptor selectivity. These findings were interpreted to indicate that these analogs must contain the crucial pharmacophoric elements in a similar spatial disposition, presumably as a congequence of the observed conformational flexibility of the Gly~ residue, which allows for conformational compensation. Measurement of the temperature dependence of the amide proton chemical shifts indicated that most amide protons in these analogs were fully exposed to the golvent. The exceptions were the D-Pen,. amide protons in [D-cys , D-Pen Jenkephalin and [D-Pen”, D-Pen” Jenkephalin, which showed low d&/dT values, indicating a possible involvement in an intramolecular hydrogen bond. Interestingly, very good aggeement of all NMR parageters was observed between [D-Cys~, D-Pen” Jenkephalin and [D-Pen or Dw Pen” Jenkephalin, suggesting very similar conformations of these two compounds. The latter analog is about six times more &- receptor selective than the former as a consequence of its poor affinity for the p-receptor. These regults indicate that the improved 6-receptoy selectiyity of [D-Pen”, D-Pen”Jenkephalin as compared to [D-Cys”, D-Pen” Jenkephalin is not due to a different conformational behavior byt rather to the presence of the gem dimethyl group of the Pen” residue, which causes more severe steric interference at the p-receptor than at the 6-receptor. Belleney et al. (1987) performed a comparative Linn study with H-Tyr-D-Pen-Gly-Phe-Pen-OH and H-Tyr-D-Thr-Gly-Phe-Leu-Thr-OH (DTLET) in | He JDMSO. In contrast to the data obtained by Mosberg (1987) with H-Tyr-D-Pen-Gly-Phe-Pen-OH in D,0, low d6/dT values were observed for the Tt chenionl shifts of both L-Pen™ and Gly in the case of the cyclic peptide. These data were interpreted to indicgte that the conformation(s) of H-Tyr-D- P n-Gly-Phe-L-Pen-OH, in [ Hg JDMSO might contain two turns; either a y-turn around Phe or a gII' turn centered gn Gly -Phe in the C-terminal region and a y-turn centered on Pen in the N-terminal 67 region. In the case of DTLET, the obtained d6/dT values also suggested the existence of a y-turn and a B-turn in the N- and C- terminal region of the peptide, respectively, and, thus, H-Tyr-D- Pen-Gly-Phe-Pen-OH and DTLET appear to have similar backbone ToreatTons in DMSO. This type of backbone conformation together with the similar arrangement of the Tyr~ and Phe side chains in both the cyclic and the linear peptide was suggested to be responsible for the observed preferential interaction with the 6-receptor. Furthermore, the authors proposed on the basis of these models that the two threonine methyl groups in DTLET might play the same role in the interaction with the receptor as the gem dimethyl groups of the two Pen residues in the cyclic peptide. Cyclic Lactam Analogs Containing the Phenylalanine Residue in the 3-Position Recently, Wilkes and Schiller (1987) applied a systematic procedure for the determination of the allowed low energy conformations of the highly p-receptor selective cyclic analog H- Tyr-D-Orn-Phe-Asp-NH, (8), using the software package SYBYL (Tripos Associates, St. Louis, MO). A comprehensive grid searc of the 13-membered zing structure of 8 lacking the exocyclic Tyr residue and the Phe” side chain resulted in only four low energy conformers. These four conformations showed considerable similarity, being all fairly round and flat. The three amide bonds within the ring were generally either perpendicular to the plane of the ring or slightly tilted toward the ring center, but no linear tyansannular hydrogen bonds were observed. The exocylic Tyr residue and Phe” side chain were then added to these four low energy conformers and an extensive energy minimization was carried out with each ong of them. The obtained results indicated that the Tyr and Phe side chains enjoy considerable orientational freedom but nevertheless only a limited number of low energy side chain configurations were found. The lowest energy conformer obtained by this approach was characterized by a tilted stacking arrangement of the two aromatic rings (figure 2, structure 8). However, several other conformers with different side chain configurations were found to be only slightly higher in energy (1 kcal/mol or less above the energy minimum). This conformational analysis has recently been extended to several 13-membered ring cyclic analogs related to 8, which show considerable diversity in their u-receptor affinity and selectivity (figure 1, compounds 9-13) (Wilkes and Schiller 1988). Again, the analyses performed with the bare ring structures resulted in no more than four low energy conformers (within 2 kcal/mol of the lowest energy structure) in all cases. The gross topological features of all the low energy ring conformations observed with these analogs were similar to those of the low energy conformers of the cyclic parent peptide 8. Thus, in all cases no transannular hydrogen bonds were found. Only two low energy ring conformations were obtained in the case of compound 11, indicating that the additional conformational 68 H 8 10 12 FIGURE 2 Lowest Energy Conformers of Cyclic Opioid Peptide Analogs 8, 10, 12 and 13. 69 constraint introduced by N-methylation of the Phe? residue led to a further incyease in structural rigidity. After addition of the exocyclic Tyr™ residue and the Phe” side chain to the low energy ring conformations of analogs 9-13, low energy side chain configurations were again determined by extensive energy minimization (figure 2). The two potent and p-selective analogs 9 and 10 showed a tilted stacking arrangement of the two aromatic rings “in their lowest energy conformations similar to that observed in the lowest energy conformer of 8. Among the analogs with reduced p-receptor affinity, compound 11 showed a lowest energy conformation characterized by a fully stacked parallel arrangement of the two aromatic rings rather than a tilted stacking interaction. Analysis of the weak u-agonist 12 revealed that chiral inversion at the 2-position precludes a Tow energy stacking configuration. The lack of stacking of the aromatic rings observed in the low energy conformers of the weakly active analog 13 appears to be due to steric interference of the bulky N-methyl group at the 3-position residue. Taken together, these results suggest that a specific tilted stacking interaction of the aromatic rings in the 1- and 3-position of cyclic opioid peptide 8 and its analogs may represent an important structural requirement for binding at the p-receptor. However, it should be kept in mind that other side chain configurations were found to be only slightly higher in energy and that a change in side chain conformations could occur upon binding to the receptor at an energy expense, which could be compensated for by part of the binding energy. CONCLUSION Conformational studies of three families of cyclic opioid peptide analogs carried out to date have revealed that the ring structures contained in these compounds are not entirely rigid but, depending on the type and size of the ring, undergo more or less extensive conformational fluctuations. Nevertheless, the results of the performed molecular mechanics and molecular dynamics studies indicate that these structural fluctuations are relatively minor in the case of 13- or l4-membered rings and that the various low energy ring conformers observed for a given cyclic analog do not differ very much in their overall shape from one another. As expected, the results of various conformationa analyses indicate that the exocyclic Tyr residue and the Phe side chain still enjoy considerable orientational freedom. In order to determine the distinct conformational requirements of the u- and the 6-receptor, it will be necessary to prepare and characterize cyclic opioid peptide analogs in which the conformational freedom of these important pharmacophoric moieties is restricted in various ways. FOOTNOTES 1 \bbreviations: A bu, a, y-diaminobutyric acid; A,pr, ©, B- diaminopropionic acid; DTLET, H-Tyr-D-Thr-Gly-Phe-Leu-Thr-OH; NMR, nuclear magnetic resonance; Pen, penicillamine; Phe(NMe), N®-methylphenylalanine; Phg, phenylglycine. 70 REFERENCES Belleney, J.; Roques, B.P.; and Fournié-Zaluski, M.-C. Comparison of conformational properties of linear and cyclic 6 selective opioid ligands DTLET (Tyr-D-Thr-Gly-Phe-Leu-Thr) and DPLPE (Tyr-c[D-Pen-Gly-Phe-Pen]) by “H n.m.r. spectroscopy. Int J Peptide Protein Res 30:356-364, 1987. - Berman, J.M.; Goodman, M.; Nguyen, T.M.-D.; and Schiller, P.W. Cyclic and acyclic partial retro-inverso enkephalins: mu receptor selective enzyme resistant analogs. Biochem Biophys Res Commun 115:864-870, 1983. DiMaio, J., and Schiller, P.W. A cyclic enkephalin analog with high in vitro opiate activity. Proc Natl Acad Sci USA 77:7162- 7166, 1980. == DiMaio, J.; Nguyen, T.M.-D.; Lemieux, C.; and Schiller, P.W. Synthesis and pharmacological characterization in vitro of cyclic enkephalin analogues: Effect of conformational constraints on opiate receptor selectivity. J Med Chem 25:1432- 1438, 1982. TT DiMaio, Jes Bayly, C.I.; Villeneuve, G.; and Michel, A. Topological similarities between a cyclic enkephalin analogue and a potent opiate alkaloid: A computer-modeling approach. J Med Chem 29:1658-1663, 1986. E: Fischman, A.J.; Riemen, M.W.; and Cowburn, D. Averaging of e, and ©, in [5-leucyl]-enkephalin. FEBS Lett 94:236-240, 1978. Hall, D., and Pavitt, N. Conformation of a cyclic tetrapeptide related to an analog of enkephalin. Biopolymers 23:1441-1455, 1984a. Hall, D., and Pavitt, N. Conformation of cyclic analogs of enkephalin. II. Analogs containing a cystine bridge. Biopolymers 23:2325-2334, 1984b. Hall, D., and Pavitt, N. Conformation of cyclic analogs of enkephalin. III. Effect of varying ring size. Biopolymers 24:935-945, 1985. Kessler, H.; HY1lzemann, Ga} and Zechel, C. Peptide conformations. 33. Conformational analysis of cyclic enkephalin analogs of the type Tyr-cyclo-(-NY-Xxx-Gly-Phe- Leu-). Int J Peptide Protein Res 25:267-279, 1985. Maigret, B.; Fournié-Zaluski, R.-E.; Roques, B.; and Premilat, S. Proposals for the up-active conformation of the enkephalin analog Tyr-cyclo(-NY-D-A,bu-Gly-Phe-Leu-). Mol Pharmacol 29:314-320, 1986. = Mammi, N.J.; Hassan M.; and Goodman, M. Conformational analysis of a cyclic enkephalin analogue by “HNMR and computer simulations. J Am Chem Soc 107: 4008-4013, 1985. Mierke, D.F.; Lucietto, P.; Schiller, P.W.; and Goodman, M. Comparative conformational analysis of two diastereomeric cyclic enkephalin analogues by “HNMR and computer simulations. Biopolymers 26:1573-1586, 1987. Mosberg, H.I. "H n.m.r. investigation of conformational features of cyclic, penicillamine-containing enkephalin analogs. Int J Peptide Protein Res 29:282-288, 1987 = Mosberg, H.I., and Schiller, P.W. "H n.m.r. investigation of conformational features of cyclic enkephalinamide analogs. Int J Peptide Protein Res 23:462-466, 1984. 71 Mosberg, H.I.; Hurst, R.; Hruby, V.J.; Gee, K.; Yamamura, H.I.; Galligan, J.J.; and Burks, T.F. Bis-penicillamine enkephalins possess highly improved specificity toward 6 opioid receptors. Proc Natl Acad Sci USA 80:5871-5874, 1983 (and references cited therein). Richman, S.J.; Goodman, M.; Nguyen, T.M.-D.; and Schiller, P.W. Synthesis and biological activity f linear and cyclic enkephalins modified at the Gly -Phe amide bond. Int J Peptide Protein Res 25:648-662, 1985. Ee, = Schiller, P.W. Fluorescence study on the conformation of a cyclic enkephalin analog in aqueous solution. Biochem Biophys Res Commun 114:268-274, 1983. Schiller, P.W. Conformational analysis of enkephalin and conformation-activity relationships. In: Udenfriend, S., and Meienhofer, Joy eds. The Peptides: Analysis, Synthesis, Biology. Vol. 6. Orlando: Academic Press, 1984. pp. 219-268. Schiller, P.W., and DiMaio, J. Opiate receptor subclasses differ in their conformational requirements. Nature (London) 297:74- 76, "1982. Schiller, P.W., and DiMaio, J. Aspects of conformational restriction in biologically active peptides. In: Hruby, V.J., and Rich, D.H., eds. Peptides: Structure and Function. Rockford, Ill.: Pierce Chemical Company, 1983. pp. 269-278. Schiller, P.W., and Nguyen, T.M.-D. Activity profiles of novel side chain-to-side chain cyclized opioid peptide analogs. Neuropeptides 5:165-168, 1984. Schiller, P.W.; Eggimann, B.; DiMaio, J.; Lemieux, C.; and Nguyen, T.M.-D. Cyclic enkephalin analogs containing a cystine bridge. Biochem Biophys Res Commun 101:337-343, 1981. Schiller, P.W.; DiMaio, J.; and Nguyen, T.M.-D. Activity profiles of conformationally restricted opioid peptide analogs. In: Ovchinnikov, Y.A., ed. Proc 16th FEBS Meeting. Utrecht, The Netherlands: VNU Science Press, 1985a. pp. 457-462. Schiller, P.W.; Nguyen, T.M.-D.; Lemieux, C.; and Maziak, L.A. Synthesis and activity profiles of novel cyclic opioid peptide monomers and dimers. J Med Chem 28:1766-1771, 1985b. Schiller, P.W.; Nguyen, T.M.-D.; Maziak, L.A.; Wilkes, B.C.; and Lemieux, C. Structure-activity relationships of cyclic opioid peptide analogues containing a phenylalanine residue in the 3- position. J Med Chem 30:2094-2099, 1987. Wilkes, B.C., and Schiller, P.W. Theoretical conformational analysis of a u-selective cyclic opioid peptide analog. Biopolymers 26:1431-1444, 1987. Wilkes, B.C., and Schiller, P.W. Theoretical conformational analysis of p-selective cyclic opioid peptide analogs. In: Marshall, G.R., ed. Peptides: Chemistry and Biology. Leiden, The Netherlands: ESCOM Science Publishers, 1988. pp. 619-620. 72 ACKNOWLEDGMENTS The authors' work described in this chapter was supported by operating grants from the Medical Research Council of Canada (MT- 5655), the Quebec Heart Foundation, and the U.S. National Institute on Drug Abuse (DA-04443-01). AUTHORS Peter W. Schiller, Ph.D., Director Brian C. Wilkes, Ph.D. Laboratory of Chemical Biology and Peptide Research Clinical Research Institute of Montreal 110 Pine Avenue West Montreal, Quebec, Canada H2W 1R7 73 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D., eds. National Institute on Drug Abuse, 1988 Conformational Studies of Dermorphin V. Renugopalakrishnan, Ph.D., and Rao S. Rapaka, Ph.D. Dermorphin, H-Tyr-D-Ala-Phe-Gly-Tyr-Pro-Ser-NH,, a D-Ala- containing amidated heptapeptide, is a potent p-receptor agonist. It was originally isolated from the skin of a South American frog of the genus Phyllomedusae by Broccardo et al. (1981) (for a review, see Feuerstein 1986), and it was subsequently synthesized (de Castiglione et al. 1981; Montecucchi et al. 1981). Its occurrence in mammalian tissue has not been demonstrated to date (Negri et al. 1981). Dermorphin is similar to the other opioid peptides, especially the enkephalin and dynorphin family of peptides, in having Tyr residue in the first position of the sequence. The presence of D-Ala residue in the second position and the occurrence of Phe and Tyr residues in the third and fifth positions should be expected to confer unique conformational preferences and thus dermorphin serves as an excellent model system for investigating conformation-receptor site selectivity relationships. MWe have investigated the conformations of dermorphin using vibrational spectroscopic studies (which are ideal for peptides with chromophoric residues possessing unique electronic transitions), 1D and 2D NMR studies (both at room temperature and at elevated temperatures), molecular mechanics-dynamics approach, and CD studies. CD studies of dermorphin in Hp0, trifluroethanol (TFE) and methanol, and the temperature effects in the above solvents provide insight into the conformation of dermorphin, although chromophoric residues present in dermorphin complicate the observed CD spectra. The studies reported here represent our continuing investigations (Bhatnagar et al. 1985; Pattabiraman et al. 1986), and similar studies from other laboratories are also discussed. Aqueous solutions of dermorphin were used in all the spectroscopic studies, whereas CD studies were performed in Hy0, trifluroethanol (TFE), and methanol. While the earlier 1D and 2D NMR studies had utilized dimethyl sulfoxide (DMSO) (Salvadori et al. 1983; Arlandini et al. 1985; Pastore et al. 1985; Toma et al. 1985) as the solvent, we employed 90 per cent Hy0-10 per cent D0 in our 1D and 2D NMR studies, as we believe aqueous solutions are more relevant than organic solvents to deduce physiologically relevant conformation(s). 74 Modern spectroscopic techniques utilized here offer the advantage of suppression of HoO signals, a problem that plagued especially IR and NMR studies in the 1960s and 1970s. EXPERIMENTAL STUDIES CD, FT-IR, and Raman studies were performed as described earlier (Renugopalakrishnan et al. 1985, 1986; Prescott et al. 1986; Rapaka et al. 1987). 1D and 2D TH NMR studies of polypeptides were performed in 90 per cent Hy0-10 per cent D0 on a 500 MHz Bruker AM-500 spectrometer (Renugopalakrishnan et al. 1987, 1988; Huang et al. 1988). Typical concentrations were in the range of 10-12.4 mM. Proton resonances were assigned based on homonuclear decoupling experiments and chemical shift data (Wuthrich 1986). Chemical shifts are reported in ppm relative to the shift of HDO at 4.8 ppm as an internal reference. In 2D NOESY experiments, Hp0 resonance was irradiated at all times except during the data acquisition (Huang et al. 1988). THEORETICAL STUDIES Molecular mechanics studies employed the program AMBER developed in the laboratory of Peter Kollman, and the conformations were displayed visually using the program MIDAS (Weiner and Kollman 1981). The details of the calculations have been reported previously (Pattabiraman et al. 1986). Recently, we have begun a reinvestigation of the conformation of dermorphin using the program CHARMM developed in the laboratory of Martin Karplus (Karplus and McCammon 1981). The molecular dynamics calculations have been recently extended up to 15 picoseconds, and the results will be reported elsewhere (Prabhakaran et al. submitted for publication). In the molecular mechanics calculations, we considered two B-turn conformations and an extended conformation to restrict the search in conformational space. A distance-dependent dielectric constant, e, simulated qualitatively the effect of solvent, but we did not explicitly include solvation shells in the computations. GENERAL DISCUSSION OF THE CONFORMATIONAL MODEL OF DERMORPHIN DERIVED FROM EXPERIMENTAL AND THEORETICAL STUDIES An energetically stable conformation of dermorphin derived from molecular mechanics calculations is shown in figure 1. Dermorphin assumes a type III' B-turn conformation at the N-terminal segment, Tyr-D-Alap-Phe3-Glyg, and a type I B-turn conformation at the C-terminal segment, Tyrg-Prog-Sery-NH,. Total energies of the B-turn conformations, (III'-I), (II'-III), and (II'-I), and a fully extended conformation are presented in table 1. The fully extended conformation is less stable than the folded conformations. The three folded conformations, however, differ by 1 kcal/mole from one another and therefore can interconvert on 75 FIGURE 1 Conformation of dermorphin from molecular mechanics calculations conventional spectroscopic time scale, although time-resolved FT-IR and Raman may be able to detect them. The Tyr residues, which stack with a skew and therefore are not superimposable, probably provide the major driving force for the stabilization of the folded conformations. The stability of the folded conformation is, however, not surprising, considering the presence of D-Alay and Prog residues, which are compulsive B-turn promoting residues (Chou and Fasman 1978). The stacking of Tyrj-Tyrg side chains can be observed from figure 1. The folded conformation is consistent with the bulk of the experimental spectroscopic data in aqueous solution. Temperature dependence of CD spectra of dermorphin in TFE solution (not shown here) manifests an unusual CD pattern with a broad positive band at A=226nm (band II) and somewhat less broad positive band at A=198nm (band I). As the temperature is increased to 45° C, a dramatic shift in the CD bands occurs. A broad negative band begins to appear at A=218nm, which persists at 60° C with a shift of the negative trough toward lower wave length region. The above observation qualitatively indicates that the chromophore responsible for band II is disrupted by heating. The CD spectra of dermorphin in TFE, Hy0, and methanol, representing solvents of varying polarity, suggest that dermorphin manifests discrete conformational states in solution phase. The observed CD spectra are difficult to interpret in terms of the secondary structure but probably are the composite of two B-turns (Renugopalakrishnan et al. submitted for publication). Raman spectrum of dermorphin in HO shows an amide I band at 1681 em! and a doublet amide III band at 1253 cm-! and 1265 cm-1. Raman amide I bands beyond the 1668-1678 em! are 76 TABLE I Conformational Energies of the seven models of dermorphine Model B-Turn-1 B-Turn-II Total Energy in kcal/mol r-1 ur 1 -70.7 1-111 I 11 -69.9 1-1 I 1 -69.8 nr-11 I 11 -57.2 V'-1 Vv 1 -56.9 V-111 Vv 111 -46.4 Extended Trans Trans -46.3 believed to originate from B-turns (Bandekar and Krimm 1979; Tu 1986). The doublet amide III band at 1253 cm-! and 1265 cm-! is at best representative of extended/"random"/B-turn structures. The alternative explanation for the amide III doublet can be advanced from the side chain Raman vibrations of the aromatic residues. To decide between the alternatives, deuterium exchange studies have been carried out to observe the shift of amide III bands resulting from exchange of labile hydrogen atoms. After the dissolution and equilibration of the sample in D0 solution, one of the amide III bands, the band at 1253 cm-1, is lost, whereas the 1265 cm~! band shifts toward lower wave numbers to 1261 cm-1. Therefore the 1253 cm~! band is assigned to the peptide backbone vibrations, and the above frequency is probably a mixed mode originating from B-turn and probably extended structures. The amide I' band occurs at 1661 cm-!. Although Raman results are largely indicative of B-turn or folded conformation, an admixture of extended structure cannot be ruled out. 500 MHz 1D TH NMR spectrum of dermorphin in Hy0 is shown in figure 2. Ramachandran angles, ¢, for Tyr;, D-Alap, Phes, Gly 4, Tyrg and Sery were derived from a Karplus-Tike equation, using the values of the coefficients A, B, and C derived by Bystrov et al. (1973). From the ¢ angles derived, it is concluded that a fully extended conformation is not compatible with the observed spin coupling constants, J. From the calculated Ramachandran angles, ¢, one is led to conclude that either type II' or III' B-turn occurs at the N-terminal segment, whereas the C-terminal B-turn may contain any one of three types of B-turns--types I, II, and III. It is difficult to discriminate between them based only on spin coupling constant data. The variation of aromatic proton resonances as the temperature is increased is indicative of the unfolding of the dermorphin from a folded conformation to an unfolded state in which Tyr residues are no longer stacked. From the combined results, one cannot but conclude that dermorphin probably assumes a manifold of folded conformations, which interconvert in the spectroscopic time scale. It is possible the heptapeptide contains a partially extended 77 "i J MUL 2 3 2 i 0 PPM FIGURE 2 500 MHz 'H NMR spectrum of dermorphin in Hy0 segment at the N-terminal end, but, in any event, such a conformational state has a low probability of occurrence in the aqueous solution. Most of the previous spectroscopic studies of dermorphin were exclusively performed in dimethyl sulfoxide (Salvadori et al. 1983; Arlandini et al. 1985; Pastore et al. 1985; Toma et al. 1985), and NMR studies were utilized to derive the secondary structure of dermorphin. Toma et al. (1985) investigated the solution conformation of a series of [Alan] substituted dermorphin analogs by 500 MHz TH NMR spectroscopy. Preferred conformations were calculated using a semi-empirical method. They reached the conclusion that none of the calculated conformations were able to satisfy the experimental data. In contrast, both experimental and theoretical studies could at best be reconciled with a type I B-turn at the C-terminus. Nevertheless, no consensus could be reached at the N-terminus, and the question of any preferred conformation at the N-terminus could not be resolved. However, Pastore et al. (1985) have reported 1D and 2D-NMR study of dermorphin in DMSO and reached the conclusion that the heptapeptide assumes an essentially extended structure. The above investigators assumed corrections for ring current effects in dermorphin. The question of interaction between amide protons and DMSO was thought to be a major factor in the observed conformation in DMSO. An extended structure of dermorphin in DMSO may be a special 78 situation that is probably not valid in aqueous solutions of dermorphin. We believe that dermorphin assumes a manifold of folded conformations in aqueous solution, although an extended conformation at the N-terminus should also be considered. Nevertheless, in a lipophilic environment, it is likely that dermorphin assumes a folded conformation, which is probably the most relevant at the up-receptor site (Alford et al. in preparation). Therefore, two different perspectives of dermorphin conformation relevant to DMSO and aqueous solution exist in the literature currently. Due to the relatively small size of dermorphin, which exhibits rapid molecular tumbling, it is difficult to provide a clear-cut resolution of the existing conformational populations. Numerous u- and 8-receptor selective opioid peptide analogs have been synthesized, and conformational studies have been conducted on a number of analogs. B-turns, B-sheets, and extended structures have been hypothesized as some of the recognition features for the opioid receptor types (see Rapaka 1986 for a review). However, conformation-receptor selectivity relationships have not yet been established. It is expected that with the multifaceted research techniques employed, the large number of analogs available, and a greater understanding of the biochemistry of the opioid receptors, the critical factors for conformation- receptor selectivity relationships will be better understood, paving the way for design of highly receptor selective analogs and safe and potent analogs devoid of undesirable side effects. REFERENCES Alford, D.; Duzgunes, N.; Renugopalakrishnan, V.; and Rapaka, R.S. Circular dichroism study of dermorphin encapsulated in liposomes. Submitted. Arlandini, E.; Ballabio, M.; de Castiglione, R.; Gioia, B.; Malnati, M.L.; Perseo, G.; and Rizzo, V. Spactroscapie investigations on dermorphin and its (L-Ala¢) analog. Int J Peptide Protein Res 25:33-46, 1985. Bandekar, J., and Krimm, S. Vibrational analysis of peptides, polypeptides, and proteins. 4. Characteristic amide bands of B-turns. Proc Natl Acad Sci USA 76:774-777, 1979. 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Negri, L.; Melchiorri, P.; Falconierri-Erspamer, G.; and Erspamer, G. Radioimmunoassay of dermorphin-like peptides in mammalian and non-mammalian tissue. Peptides (suppl) 2:45-49, 1981. Pastore, A.; Temussi, P.A.; Salvadori, S.; Tomatis, R.; and Mascagni, P. A conformational study of the opioid peptide dermorphin by one-dimensional and two-dimensional nuclear magnetic resonance spectroscopy. Biophys J 48:195-200, 1985. Pattibiraman, N.; Sorensen, K.R.; Langridge, R.; Bhatnagar, R.S.; Renugopalakrishnan, V.; and Rapaka, R.S. Molecular mechanics studies of dermorphin. Biochem Biophys Res Commun 140:342-349, 1986. Prabhakaran, M.; Renugopalakrishnan, V.; and Rapaka, R.S. Molecular dynamics simulation of secondary structure of dermorphin. Submitted. Prescott, B.; Renugopalakrishnan, V.; Glimcher, M.J.; Bhushan, A.; and Thomas, G.J., Jr. A Raman spectroscopic study of hen egg yolk phosvitin. Biochemistry 25:279-298, 1986. Rapaka, R.S. Research topics in the medicinal chemistry and molecular pharmacology of opioid peptides--present and future. Life Sci 39:1825-1843, 1986. Rapaka, R.S.; Renugopalakrishnan, V.; Collette, T.W.; Dobbs, J.C.; Carreira, L.A.; and Bhatnagar, R.S. Conformational features of dynorphin A(1-13): Laser Raman spectroscopic studies. Int J Peptide Protein Res 30:284-287, 1987. Renugopalakrishnan, V.; Horowitz, P.M.; and Glimcher, M.J. Structural studies of phosvitin in solution and in the solid state. J Biol Chem 254:11406-11413, 1985. 80 Renugopalakrishnan, V.; Strawich, E.S.; Horowitz, P.M.; and Glimcher, M.J. Studies of the secondary structure of amelogenin from bovine tooth enamel. Biochemistry 25:4879-4887, 1986. Renugopalakrishnan, V.; Huang, S.-G.; and Rapaka, R.S. A 500 MHz TH NMR spectroscopic study of Met5-enkephalinamide in aqueous solution: Ethanol induced conformational changes. Biochem Biophy Res Commun 143:126-132, 1987. Renugopalakrishnan, V.; Rapaka, R.S.; Huang, S.-G.; Moore, S.; and Hutson, T.B. Dynorphin A(1-13) peptide NH groups are solvent exposed: FT-IR and 500 MHz TH NMR spectroscopic evidence. Biochem Biophys Res Commun 151:1220-1225, 1988. Renugopalakrishnan, V.; Rapaka, R.S.; Balschi, J.A.; Collette, T.W.; Dobbs, J.C.; Carreira, L.A.; Pattabiraman, N.; Langridge, R.; Sorensen, K.R.; Bhatnagar, R.S.; Huang, S.-G.; and MacElroy, R.D. Molecular conformations of dermorphin. Submitted. Salvadori, S.; Tomatis, R.; Gibbons, W.A.; Tancredi, T.; and Temussi, P. NMR studies of neutral dermorphin and its synthetic analogs. In: Hruby, V.J., and Rich, D.H., eds. Peptides: Structure and Function. Rockford, Illinois: Pierce Chemical Company, 1983. pp. 785-788. Toma, F.; Dive, V.; Fermandijian, S.; Darlak, K.; and Grzonka, Z. Preferred solution and calculated conformations of dermorphin and analysis of structure-conformation-activity relationships in the series [AlaNl-dermorphin. Biopolymers 24:2417-2431, 1985. Tu, A.T. Peptide backbone conformation and microenvironment of side chains. In: Clark, R.J.H., and Hester, R.E., eds. Spectroscopy of Biological Systems New York: John Wiley and Sons, 1986. pp. 47-112. Wuthrich, K. NMR Spectroscopy of Proteins and Nucleic Acids. New York: John Wiley and Sons, 1986. 292 pp. Weiner, P.K., and Kollman, P.A. Assisted model building with energy refinement. A general program for modeling molecules and their interactions. J Computational Physics 2:287-303, 1981. ACKNOWLEDGMENT Dr. R. L. Hawks and Mrs. Rani S. Rapka provided helpful discussions to the authors during the preparation of the manuscript. 81 AUTHORS V. Renugopalakrishnan, Ph. D. Laboratory for the Study of Skeletal Disorders and Rehabilitation Department of Orthopaedic Surgery Harvard Medical School and Children's Hospital Enders-1220 300 Longwood Avenue Boston, Machusetts 02115, USA Rao S. Rapaka, Ph. D. 10A-13, National Institute on Drug Abuse 5600 Fishers Lane Rockville, Maryland 20857, USA 82 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D., eds. National Institute on Drug Abuse, 1988 Use of Molecular Biological Methods to Study Neuropeptides Michael J. Brownstein, M.D., Ph.D. INTRODUCTION Armed with molecular biological techniques, neurobiologists interested in biologically active peptides have begun to work on problems that they could only dream of attacking 10 years ago. The structures of several peptide precursors have been determined by isolating and sequencing DNAs complementary to their respective mRNAs, and similarities among peptide precursors have been cataloged. Based on the structures of the precursors, inferences about their processing were generated and a number of processing enzymes have been identified. Two of these have been purified, and one has itself been cloned. The availability of cDNA probes that specifically hybridize to mRNAs that encode peptide precursors and processing enzymes allows the levels of these mRNAs to be measured and—by means of in situ hybridization histochemistry—to be visualized in discrete cells. In addition, cDNA probes can be used to screen genomic libraries to isolate genes that encode peptide mRNAs (or to determine the cause of genetic defects in peptide production). The regulatory elements of the genes can ultimately be identified and the transactivating molecules that mediate tissue-specific expression of gene products and regulate mRNA levels can be identified. Examples of the latter include the recently characterized intracellular receptors for steroids and thyroid hormones. To date only two neuropeptide receptors have been purified and sequenced. Advances in expression cloning technology may soon contribute to pushing aside our ignorance of this class of binding protein. 83 CLONING PEPTIDE PRECURSORS: THE CASE OF GALANIN Galanin, a 29 amino acid peptide, was isolated from the upper small intestine of pigs by Tatemoto, Mutt, and their colleagues (1983). Like so many other peptides, it has a C-terminal amide. This structural feature led to its discovery. Afterwards, galanin was found to be present in the enteric nervous system of the gastrointestinal tract (Melander et al. 1985; Rokaeus et al. 1984), the urogenital tract (Bauer et al. 1986a), the pancreas (Dunning et al. 1986), the adrenal medulla (Bauer et al. 1986b), and the brain (Melander et al. 1986). It has several actions, including inhibition of phasic activity of the small intestine (Fox et al. 1986), production of hypoglycemia (McDonald et al. 1985), suppression of insulin release, and central stimulation of growth hormone (Ottlecz et al. 1986). With few exceptions, DNAs encoding peptide precursors have been isolated from cDNA libraries by screening them with mixtures of synthetic oligonucleotides, the compositions of which were based on the amino acid sequence of the peptides. It was in this way that we isolated cDNA, encoding the galanin precursor from a pig adrenal medullary library (Rokaeus and Brownstein 1986). The precursor (preprogalanin, preproGAL) is rather typical of this class of proteins. Itis 123 amino acids long and is comprised of a leader (signal) sequence, the 29 amino acids of galanin, and a 59 amino acid sequence (galanin message associated protein, GMAP) (see figure 1). Unlike proopiomelanocortin, for example, preproGAL may encode only one active peptide, galanin itself. The galanin sequence is flanked on both sides by pairs of lysine and arginine residues. The C-terminal lysine and arginine are separated from the final alanine in galanin by a glycine, the donor of the amide moiety. 84 Met Pro Arg Gly Cys Ala Leu Leu leu Ala Ser Leu Leu Leu Ala Ser Ala Leu Ser Ala Thr Leu Gly Leu Gly Ser Pro Val Lys Glu Lys Arg Gly Trp Thr Leu Asn Ser Ala Gly Tyr Leu Leu Gly Pro His Als lle Asp Asn His Arg Ser Phe His Asp Lys Tyr Gly Leu Ala Gly Lys Arg... Ser FIGURE 1. Partial sequence of preprogalanin. A very hydrophobic N- terminal signal sequence (beginning with residue 1, Met) precedes the (underlined) sequence of galanin (residues 33-61). Pairs of basic amino acids (Lys-Arg) bracket the galanin sequence. A glycine residue, the donor of the C-terminal amide, is found in position 62. The 59-residue sequence of as yet unknown function comprises the amino-terminal half of the precursor. It is clear that precursors like preproGAL are cleaved to yield their active products by a series of enzymes. The first of these, located in the cisternum of the rough endoplasmic reticulum, removes the signal peptide from the prepropeptide converting it to a propeptide. Subsequent processing seems to occur principally in the secretory granule after the propeptide has traversed the Golgi apparatus. First the propeptide is split by an endopeptidase. More than one such endopeptidase may exist. A 70,000 dalton paired basic residue specific aspartyl protease (Chang and Loh 1984; Loh et al. 1985) has been shown to be involved in the processing of proopiomelanocortin and provasopressin. The pH optimum of this enzyme is low (four-five) allowing it to function in the acid milieu of the secretory vesicle. It cleaves precursors between their paired bases or C-terminal to them. In addition to the paired basic residue specific cleavage enzyme, there are single basic residue cleaving enzymes. Such an enzyme has been found associated with rat brain membranes (Devi and Goldstein 1984). It cleaves 85 dynorphin Bj.29 between Thrj3 and Arg to yield dynorphin By.j3. It seems to be a neutral thiol protease. Peptides liberated from their precursors by the action of one of the above endopeptidases may have basic residues attached to their C- or N-termini. These need to be trimmed off. The first trimming enzyme to be discovered (Hook et al. 1982) and purified (Fricker and Snyder 1983) was a carboxypeptidase. Complementary DNA encoding this enzyme has recently been isolated. There is also an aminopeptidase that removes basic residues from peptides’ N-termini when cleavage by the paired base specific endopeptidase occurs between two basic residues leaving one behind (Gainer et al. 1984). This enzyme appears to be a metalloprotease stimulated by Cot*2 and Zn+2. The enzyme responsible for carboxyl-amidation of peptides was first described by Bradbury et al. (1982). This copper dependent enzyme uses a C-terminal glycine as the donor of the amide group. Other functional groups are physically added to peptides by enzymes, notably N- acetyltransferases, kinases, and sulfate transferases. CLONING PEPTIDE "PRECURSORS": THE CASE OF VALOSIN The major structural features of a typical peptide precursor and its mode of processing were outlined above. Comparison of the structure of a protein containing the sequence of valosin to other precursors illustrates the power of cDNA cloning to help in identifying peptides as strong or weak candidates for biological functions. Valosin is a 25 amino acid peptide purified from side fractions of an earlier preparation of porcine peptide HI and secretin (Schmidt et al. 1984). Following its isolation, valosin was found to release gastrin, to augment pentagastrin-induced gastric secretion, to stimulate pancreatic protein secretion, and to suppress migrating myoelectric complexes of the small bowel (Schmidt et al. 1985). On screening a porcine adrenal medullary cDNA library with an oligonucleotide pool constructed on the basis of the amino acid sequence of 86 valosin, we detected several cDNAs (Koller and Brownstein 1987). The longest of these had a 2,466 base pair open reading frame that encoded a ~ 88,660 dalton protein containing the amino acid sequence of valosin (see figure 2). This protein is unlike other peptide precursors characterized to date: (1) It has no obvious N-terminal or internal signal sequences and seems, in fact, to reside in the cytoplasm of cells. (2) Its message is found in many tissues, neuronal and nonneuronal ones alike. (3) The valosin sequence is not bracketed by single or paired basic residues. In fact, it appears to have been released from the valosin-containing protein by the action of a chymotrypsin-like enzyme. It seems likely, then, that valosin is not a physiologically active molecule but rather an artifactual product of a (hitherto unknown) and rather ubiquitous cytoplasmic protein. 481 ..Gly Leu Glu Asp Val Lys Arg Glu Leu Gin Glu Leu Val Gin Iyr Pro Val Glu His Pro Asp Lys Phe Leu Lys Phe Gly Met Thr Pro Ser Lys Gly Val Leu Phe Iyr Gly Pro Pro Gly Cys Gly Lys Thr Leu Leu Ala ... FIGURE 2. The portion of the valosin-containing protein (VCP) that contains the valosin sequence (underlined). Note that valosin is not neighbored by canonical processing signals. While VCP does have pairs of basic residues scattered throughout it, many other proteins that are not peptide precursors do too. Furthermore, analysis of its entire sequence shows that VCP has no obvious N-terminal or internal signal sequences. 87 PUTTING CLONING TO WORK Cloning a cDNA and sequencing it are not ends in themselves. A cDNA and the structural information derived from it should be used to forge tools that can be used for biological studies (see table 1). TABLE 1. Examples of uses to which cloning data can be put. A. Uses of cDNAs 1. Screening genomic libraries allows specific genes or gene families to be isolated and sequenced. Putative regulatory elements can be fused to marker genes for studies of gene expression. New genes can be introduced into the cells of transgenic animals. Genes from animals with genetic defects can be analyzed. 2. Full-length cDNAs inserted into appropriate vectors can be used to manufacture large amounts of proteins for biochemical studies. (In the case of peptide precursors, substrates for processing enzyme assays can be prepared this way.) 3. cDNAs, cRNAs, or synthetic oligonucleotides can be used to measure specific mRNAs in tissues or to visualize mRNAs in discrete cells by means of Northern blotting and in situ hybridization histochemistry, respectively. 4. Mutant cDNAs can be expressed in cells in order to determine the function of the altered protein domains. B. Uses of peptides synthesized on the basis of cDNA sequences 1. Novel candidates for roles as neuropeptide transmitters can be synthesized and their biological activities explored. 2. Antibodies against peptides can be used for immuno- cytochemistry or immunoprecipitation (following pulse-chase experiments, for example). 88 A WORD ABOUT RECEPTOR CHARACTERIZATION In principle, there are three ways to clone cDNAs that encode receptors. One might isolate the receptor, partially sequence it, and screen a cDNA library with oligonucleotide probes based on the amino acid sequence. To purify enough of a protein to sequence—S50-100 pmoles perhaps—is nontrivial, and receptors are frequently N-terminally blocked. Consequently close to a nmole of material might be required; the pure receptor has to be fragmented and the fragments themselves purified and sequenced. Antireceptor antibodies can be used to screen bacterial expression libraries. Raising such antibodies and proving that they are specific for a particular receptor is difficult, however, and if one employs an antibody that does not recognize the receptor of interest or one that is promiscuous, one's work will be for naught. Finally, it should be possible to transfect a negative mammalian cell line with a eucaryotic expression library and to identify clones of cells that begin to make surface receptors. This method has not yet been employed successfully for neurotransmitter receptors, but recent advances in vector design and transfection procedures should lead to its wider adoption. CONCLUDING REMARKS Numerous biologically active peptides have been discovered in the past decade. Unfortunately, more is often known about the anatomy and neurochemistry of peptidergic neurons than about their function. It is to be hoped that use of molecular biological methods will contribute to overcoming this problem. 89 REFERENCES Bauer, F.E.; Christofides, N.D.; Hacker, G.W.; Blank, M.A; Polak, J.M.; and Bloom, S.R. Distribution of galanin immuno- reactivity in the genitourinary tract of man and rat. Peptides 7:5-10, 1986a. Bauer, F.E.; Hacker, G.W.; Terenghi, G.; Adrian, T.E.; Polak, J.M.; and Bloom, S.R. Localization and molecular forms of galanin in human adrenals: Elevated levels in pheochromocytomas. J Clin Endocrinol Metab 63:1372-1378, 1986b. Bradbury, A F.; Finnie, M.D.A.; and Smyth, D.F. Mechanism of C- terminal amide formation by pituitary enzymes. Nature 298:686-688, 1982. Chang, T.L., and Loh, Y.P. In vitro processing of proopiocortin by membrane-associated and soluble converting enzyme activities from rat intermediate lobe secretory granules. Endocrinology 114:2092-2099, 1984. Devi, L., and Goldstein, A. Dynorphin converting enzyme with unusual specificity from rat brain. Proc Natl Acad Sci. USA 81:1892-1896, 1984. Dunning, B.E.; Ahren, B.; Veith, R.C.; Béttcher, G.; Sundler, F.; and Téborsky, G.J., Jr. Galanin: A novel pancreatic neuropeptide. Am J Physiol 251:E127-E133, 1986. Fox, J.E.T.; McDonald, T.J.; Kostolanska, F.; and Tatemoto, K. Galanin: An inhibitory neural peptide of the canine small intestine. Life Sci 39:103-110, 1986. Fricker, L.D., and Snyder, S.H. Purification and characterization of enkephalin convertase, an enkephalin synthesizing carboxypeptidase. J Biol Chem 258:10950-10955, 1983. Gainer, H.; Russell, J.T.; and Loh, Y.P. An aminopeptidase activity in bovine pituitary secretory vesicles that cleaves the N-terminal arginine from B-lipotropingg_gs. FEBS Lett 175:135-139, 1984. Hook, V.Y.H.; Eiden, L.E.; and Brownstein, M.J. A carboxy- peptidase processing enzyme for enkephalin precursors. Nature 295:341-342, 1982. 90 Koller, K.J., and Brownstein, M.J. Use of a cDNA clone to identify a supposed precursor protein containing valosin. Nature 325:542-545, 1987. Loh, Y.P.; Parish, D.C; and Tuteja, R. Purification and characterization of a paired basic residue-specific pro- opiomelanocortin converting enzyme from bovine pituitary intermediate lobe secretory vesicles. J Biol Chem 260:7194-7205, 1985. McDonald, T.J.; Dupre, J.; Tatemoto, K.; Greenburg, G.R.; Radziuk, J.; and Mutt, V. Galanin inhibits insulin secretion and induces hyperglycemia in dogs. Diabetes 34:192-196, 1985. Melander, T.; Hokfelt, T.; and Rokaeus, A. Distribution of galanin-like immunoreactivity in the rat central nervous system. J Comp Neurol 248:475-517, 1986. Melander, T.; Hokfelt, T.; Rokaeus, A.; Fahrenkrug, J.; Tatemoto, K.; and Mutt, V. Distribution of galanin-like immuno- reactivity in the gastro-intestinal tract of several mammalian species. Cell Tissue Res 239:253-270, 1985. Ottlecz, A.; Samson, W.K.; and McCann, S.M. Galanin: Evidence for a hypothalamic site of action to release growth hormone. Peptides 7:51-53, 1986. Rokaeus, A., and Brownstein, M.J. Construction of a porcine adrenal medullary cDNA library and nucleotide sequence analysis of two clones encoding a galanin precursor. Proc Natl Acad Sci USA 83:6287-6291, 1986. Rokaeus, A.; Melander, T.; Hokfelt, T.; Lundberg, J.M.; Tatemoto, K.; Carlquist, M.; and Mutt, V. A galanin-like peptide in the central nervous system and intestine of the rat. Neurosci Lett 47:161-166, 1984. Schmidt, W.E.; Mutt, V.; Carlquist, M.; Kratzin, H.; Conlon, J.M.; and Creutzfeldt, W. Valosin: Isolation and characteri- zation of a novel peptide from porcine intestine. FEBS Lett 191:264-268, 1985. Schmidt, W.E.; Mutt, V.; Konturek, S.J.; and Creutzfeldt, W. Peptide VQY: Isolation and characterization of a new biologically active gastrointestinal peptide. Dig Dis Sci 29:75S, 1984. 91 Tatemoto, K.; Rokaeus, A.; Jornvall, H.; McDonald, T.J.; and Mutt, V. Galanin—a novel biologically active peptide from porcine intestine. FEBS Lett 164:124-128, 1983. AUTHOR Michael J. Brownstein, M.D., Ph.D. Laboratory of Cell Biology National Institute of Mental Health Bethesda, Maryland 20892 U.S.A. 92 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D., eds. National Institute on Drug Abuse, 1988 Three Technical Approaches for Cloning Opioid Receptors Curtis A. Machida, Ph.D.; John Salon, Ph.D.; David Grandy, Ph.D.; James Bunzow, M.S.; Paul Albert, Ph.D.; Eric Hanneman, Ph.D.; and Olivier Civelli, Ph.D. INTRODUCTION A basic tenet of modern pharmacology is that the biological activity of a drug is the result of chemical events triggered by the drug's interaction with specific receptors on responsive cells. Although the chemical structures of drugs have been extensively studied, very little information has been obtained about the molecular structures of drug receptors. The structural analysis of receptors is fraught with difficulties, which are in part due to limitations of the techniques used to manipulate integral membrane proteins. Most membrane proteins are hydrophobic, and the removal of the lipid moiety severely limits or abolishes the solubility of the protein in aqueous media. Although the techniques of nonaqueous protein chemistry have advanced over the past few years, certain experimental constraints often make a direct attack on a protein’s structure difficult to manage. In addition, the removal of the membrane lipid can disrupt the oligomeric structure of the membrane proteins and can obscure the involvement of associated receptor subunits. Limiting receptor abundance presents an additional problem. Depending on the nature of the signal transduction, a specific receptor can constitute from less than 0.01 percent to as much as 0.5 percent of the plasma membrane protein mass. Pharmacologically important receptors generally fall into the lower end of the abundance spectrum. Thus, attempts to purify receptors are compromised by the need for large amounts of starting material. This problem is often exacerbated by the need to use a tissue that is scarce or difficult to obtain. In addition, receptor preparations are often very unstable. Both native and purified receptor preparations can be sensitive to assorted cations, oxidizing or reducing agents, and a variety of other materials and methods commonly used for their preparation and storage. The loss of receptor activity compromises the ability to assess the integrity and purity of the receptor preparation. For these reasons, it is likely that the determination of the primary amino acid structure of many low 93 abundance neuroreceptors will be inferred from the analysis of their cloned nucleic acid sequences. This review will discuss the strategies that can be applied to the molecular cloning of one specific family of neuroreceptors, the opioid receptors. THE OPIOID RECEPTORS The analgesic and euphoric responses to opiates are the result of a cascade of biochemical events that are triggered by the interaction of the opiates with specific receptors found on the cell membranes of nervous system tissues (West and Miller 1983; Paterson et al. 1984; Holaday 1985). These opioid receptors not only recognize exogeneous alkaloids such as morphine, but moreover interact with their endogeneous ligands, the opioid peptides. The opioid receptors are clearly involved in physiological phenomena such as pain perception, addiction, and withdrawal, and are implicated in hormone secretion, response to injury, and gastrointestinal motility (Holaday 1985). The molecular basis of the participation of opioid receptors in these phenomena is unknown. Martin and coworkers (Martin et al. 1976; Gilbert and Martin 1976) were the first to postulate the existence of different types of opioid receptors based on differences in the pharmacological profiles of the different opiates. Although the precise number of opioid receptor types is still a matter of conjecture, it is generally accepted that the opioid receptors can be subdivided into three major types, u, §, and x (Pasternak et al. 1983; Paterson et al. 1984). These three receptor types are distinguished on the basis of four criteria: (1) patterns in ligand selectivity, (2) anatomical distribution, (3) physiological and behavioral profiles, and (4) differences in the cellular response to activation (Dole et al. 1975; Paterson et al. 1984; Holaday 1985). Three models can account for the heterogeneity of the opioid receptors. First, the three opioid receptors are structurally different and are encoded by different genes; second, the opioid receptors are encoded by different but homologous genes; or third, the opioid receptors are encoded by identical genes but differ in posttranslational modifications or in their interactions with second messengers. At the present time, there is no definitive evidence to favor one model over the others. Using Schwyzer’s concept (Schwyzer et al. 1980), one can formulate the existence of at least two domains in the active site of the opioid receptor: the message domain, which recognizes the common amino terminal sequence of the enkephalins, Tyr-Gly- Gly-Phe, and the address domain recognizing the remainder of the opioid peptide sequence. This model suggests that at least one region of the opioid receptor is common to the different receptor types and that the opioid receptors must therefore be homologous. 94 Furthermore, in view of the recently discovered homology between the B-adrenergic receptor, muscarinic acetylcholine receptor, and opsin genes (Kubo et al. 1986; Dixon et al. 1986; Bonner et al. 1987; Hall 1987), the possibility that the opioid receptors may also be encoded by homologous if not identical genes is very attractive. Knowledge about the physical characteristics of the opioid receptor has been obtained directly from receptor purification experiments. Attempts at opioid receptor purification have been hampered by the receptor’s sensitivity to denaturation and low abundance (Zukin and Maneckjee 1986). These receptors constitute less than 0.005 percent of the total rat brain membrane proteins. In spite of the extreme difficulties in purifying opioid receptors, several laboratory groups (Bidlack et al. 1981; Newman and Barnard 1984; Gioannini et al. 1985; Simonds et al. 1985; Cho et al. 1986) have succeeded in purifying opioid receptor proteins to homogeneity. The two common characteristics established for the ligand binding subunit of the opioid receptor are (1) an apparent Mr range of 55,000-65,000 and (2) its glycosylated nature. These two properties, plus ligand selectivity, represent the important criteria for judging the authenticity of a cloned opioid receptor. APPROACHES TO THE MOLECULAR CLONING OF THE OPIOID RECEPTOR Our hope in understanding the molecular structure and activation of the opioid receptors lies with the use of recombinant DNA technology. The cloning of the opioid receptors will allow detailed examination of receptor structure-function relationships and receptor gene expression. This approach will therefore help explain the molecular mechanisms of receptor activation and its resulting cellular responses. The opioid receptors are macromolecular components of plasma membranes, which specifically bind opioid ligands according to three criteria: (1) high affinity for opioids and opiates, (2) saturable binding, and (3) binding that is stereospecific and naloxone reversible (Dole et al. 1975). These three criteria constitute the accepted functional definition of the opioid receptor. Therefore, an authentic molecular clone of the opioid receptor must be able to code for a product that fulfills all three criteria. In addition, an opioid receptor clone must encode a product with the expected characteristics of a membrane protein. Two structural characteristics of membrane proteins are the presence of a signal sequence that facilitates the insertion of the receptor in the membrane, and the presence of hydrophobic sequences that correspond to potential transmembrane domains of the receptor. The signal peptide is not an absolute requirement, since some membrane proteins do not have signal sequences. Since the distribution of the opioid receptor in the central nervous system and in peripheral organs is well documented (Pert 95 and Synder 1973; Pfeiffer et al. 1982; Atweh and Kuhar 1983; Paterson et al. 1984; Mansour et al. 1987), in situ hybridization analysis using an opioid receptor clone as probe should correlate sites of receptor mRNA synthesis with sites of receptor protein localization. However, the distinction between sites of mRNA synthesis and receptor protein localization may be difficult to evaluate precisely because of differences in assay sensitivity. Alternatively, an opioid receptor clone may be used to express receptor protein in sufficient quantity to serve as an antigen in the preparation of antibodies. These antibodies can then be used in immunocytochemical analyses to precisely correlate the distribution of the receptor encoded by the molecular clone to the known distribution of the opioid receptor. Finally, based on physical criteria obtained during receptor purification experiments, the opioid receptor clone should encode a glycoprotein with an apparent Mr range of 55,000-65,000. Three different strategies can be employed in the molecular cloning of the opioid receptor. The first approach begins with the isolation of the receptor in sufficient quantity to permit amino acid sequencing. This sequence would be reverse translated into a DNA oligonucleotide probe and this probe would then be used in the isolation of an opioid receptor cDNA or gene clone. The second strategy proposes to clone the opioid receptor through gene expression without prior purification of the receptor protein. The third strategy assumes some sequence similarity between opioid receptors and other neuroreceptors and exploits this feature in hybridization experiments designed to identify potential opioid receptor clones. CLONING THE OPIOID RECEPTOR WITH THE USE OF RECEPTOR AMINO ACID SEQUENCE INFORMATION The traditional cloning strategy consists of purifying and sequencing the opioid receptor protein. The amino acid sequence information would then be used to identify a corresponding receptor cDNA clone. This approach requires large-scale protein purification in order to prepare a sufficient quantity of homogeneous opioid receptor to permit partial amino acid sequencing. Several laboratories have succeeded in purifying the opioid receptor to homogeneity (Bidlack et al. 1981; Newman and Barnard 1984; Gioannini et al. 1985; Simonds et al. 1985; Cho et al. 1986). The objectives of these laboratories were to purify the ligand binding domain of the opioid receptor. Two approaches have been employed to purify opioid receptors: the labeled ligand binding approach and the affinity chromatography approach. In the labeled ligand binding approach, radioactive opioid ligands are bound and covalently cross-linked to opioid receptors in the membrane; the label serves as a marker in subsequent purification steps. Since binding of the ligand is performed with native receptor-membrane complexes, artifacts due to 96 aberrant protein interactions are minimized. One drawback, however, is that the ligand binding site is irreversibly occupied, making binding assays or reconstitution experiments impossible. The purification of solubilized opioid receptors by affinity chromatography is dependent on the receptor’s ability to recognize immobilized opioid ligands. The receptor population isolated by this technique can be tested for binding ability and can be obtained in sufficient quantity to sequence. The major drawback to this approach is the difficulty in preserving biological activity during subsequent purification steps. Pure receptors are subjected to partial proteolytic digestion. Peptide fragments are separated by high-performance liquid chromatography and analyzed using automated high-sensitivity gas phase amino acid sequencing. Currently, automated peptide sequencing requires as little as 10 picomoles of purified peptide. The sequences of at least two peptide fragments are then reverse translated into their corresponding DNA sequences and oligonucleotides complementary to these sequences are then chemically synthesized. The choice of oligonucleotide length and sequence is critical for successful cloning and has been discussed (Anderson and Young 1987). In general, oligomers of at least 17 bases in length containing the least amount of degeneracy are synthesized. The radiolabeled synthetic oligomers then serve as hybridization probes to identify receptor cDNAs (or genes) in appropriate libraries. This isolated clone is then used as a template for determining the entire sequence of the opioid receptor. CLONING THE OPIOID RECEPTOR BY GENE TRANSFER IN EUKARYOTIC CELLS Gene transfer systems have been used successfully in the molecular cloning of eukaryotic genes, including receptor genes (Kuhn et al. 1984; Chao et al. 1986). This approach is based on the expression of cell surface receptors on eukaryotic cells and does not rely on the availability of receptor amino acid sequence information. In this approach, a large population of cDNAs (or large fragments of genomic DNA) from tissues known to express opioid receptors are transfected into receptor-deficient eukaryotic cells. Transfectants that have incorporated exogeneous DNA are selected according to traditional techniques (Southern and Berg 1982) and are tested for their ability to express opioid receptor by binding analyses. In transfections using genomic DNA fragments, the fragments are purified by conducting secondary transfections. This step consists of repeating the transfection procedure using the DNA of the primary transfectant as the donor. If pools of cDNAs are transfected into cells, the opioid receptor cDNA can be isolated by gradually decreasing the size of the analyzed pool to unity. Several different variations of this procedure can be envisioned; in particular, cDNA libraries enriched in opioid receptor sequences can be constructed through mRNA subtraction (Hedrick 1984). 97 There is also the possibility of expressing an opioid receptor cDNA in prokaryotic cells. However, in view of the requirements necessary to maintain the biological activity of the receptor, it seems unlikely that such an expression system would be successful. The gene transfer and expression approach was adapted by our laboratory as one strategy to attempt to clone the human opioid receptor gene. This strategy is shown in figure 1. Large fragments of human genomic DNA are cotransfected with plasmid DNA (pRSVneo), which confers neomycin resistance to opioid receptor-deficient mouse L cells. Drug resistant colonies are selected by growth in neomycin analogue G418 and receptor-bearing colonies are identified using an opioid receptor detection assay. If receptor antibodies are available, these would be used in fluorescent-activated cell sorting or in situ rosetting assays to identify receptor-bearing transfectants. The unavailability of opioid receptor antibodies that recognize extracellular antigenic determinants has precluded the use of these conventional detection assays and prompted the development of new techniques that allow screening of transfectants with radioactive ligands (see next section for details). Once receptor-bearing transfectants have been identified, DNA from these cells is transferred into new recipient mouse L cells. DNA from secondary transfectants containing the opioid receptor gene is then used to prepare a genomic library in either a lambda or cosmid cloning vector. The genomic library is then screened by filter hybridization using nick-translated human repetitive sequence DNA to detect sequences contained in the original human donor, but not recipient, mouse cell lines. Positive clones containing human donor DNA are mapped with restriction endonucleases, and then reintroduced by transfection into recipient L cells to assay for opioid receptor gene expression. Development of Tools for the Detection of Neuroreceptor Expression in Eukaryotic Cells Eukaryotic cells are ideal gene transfer recipients for the expression of neurohormone and neurotransmitter receptors. The eukaryotic cell membrane environment and posttranslational machinery are necessary for correct neuroreceptor conformation and are critical determinants in the successful detection of the receptor by ligand binding. In spite of the ideal host environment, eukaryotic expression libraries have not been widely used for the isolation of clones expressing neuroreceptors. One major obstacle that has hindered the use of eukaryotic expression libraries has been the lack of rapid and reliable screening procedures. To facilitate the screening of large numbers of transfectant colonies, our laboratory has recently adapted a replica copy technique originally used for identifying somatic cell mutants (Raetz et al. 1982). The transfer membrane is a polyester nylon cloth that permits colony replication with high fidelity and 98 Gene Transfer and Molecular Cloning of the Human Opioid Receptor Gene Human brain DNA Ca PO, + neo or gpt plasmids transfection Dish of mouse cells (lacks receptor) neo or gpt resistant colonies Drug Selection (10-14 days) Screening Assays Using Receptor ntibodies or Ligands In situ In_situ replica filter Rosette binding assay Assay FACS Isolation of Primary Transfectant Expressing Receptor Gene S y Tr fect: Cons Library Screen Using Human Repetitive Sequence Probe Analyze Positive W by Transfection FIGURE 1 Molecular cloning of the human opioid receptor by gene transfer and expression in eukaryotic cells. 99 superior resolution (see fig. 2). Following drug selection of stable transfectants, one or more sheets of sterilized polyester nylon are placed on top of the cell colonies and overlaid with a monolayer of glass beads. The beads retain the filter uniformly against the bottom of the dish and permit the exchange of growth medium to the cells without changing the colony pattern. After 5-7 days of growth, the medium is aspirated, the beads are discarded, and the nylon membranes are removed with sterile tweezers. Up to five multiple copies of the transfectant population have been made from a single dish. The multiple copies allow simultaneous screening of transfectant colonies with different radioiodinated neurohormone ligands in either the presence or the absence of nonradioactive blockers (see fig. 3). Positive signals that appear in duplicate using the radioactive ligand alone are identified by autoradiography. The specificity of the binding can be determined with the use of nonradioactive blockers. If desired, cell colonies that express neuroreceptors can then be purified from the master plate of transfectants. To test the level of sensitivity of the in situ binding assay in detecting opioid receptors, the assay was standardized by using the mouse neuroblastoma N4TGl, a cell line that expresses approximately 50,000 § opioid receptors per cell (Amano et al. 1972). As shown in fig. 4, 105,10°, and 10* N4TGl or opioid receptor-negative mouse L cells were mechanically spotted on nylon cloth; the filters were then subjected to binding with (3- [*25I]iodotyrosyl?’)R-endorphin (0.15 nM in 50 mM Tris-HCl pH 7.4, 1 percent BSA, 0.05 percent poly-L-lysine, 50 ug/ml bacitracin, 10 ug/ml leupeptin, and 10 ug/ml trypsin inhibitor, for 1 hr at room temperature) in the absence or presence of opioid receptor antagonist, naloxone (100uM). The filters were then washed with ice cold buffer, dried briefly, and placed under X-ray film. Figure 4 shows the results of an 18 hr autoradiographic exposure of a typical experiment. Clear signals emanating from as few as 10,000 opioid receptor-positive N4TGl cells were observed; very little signal was observed for mouse L cells or for N4TGl cells whose receptor sites were blocked with naloxone. Other experiments have shown that a signal from as few as 1,000 N4TGL cells can be observed. This represents a detection limit of as few as 5 X 107 opioid receptors for this assay. Screening Expression Libraries for Opioid Receptor Expression Eukaryotic expression libraries were constructed using high molecular weight human genomic DNA [from the human neuroblastoma SKN-SH cell line, which expresses 50,000 opioid receptors per cell (Yu et al. 1986)] as the donor DNA for transfections. This DNA was cotransfected with neomycin resistance plasmids into opioid receptor-deficient mouse L cells and stable transfectants isolated by selection with G418. Assuming that the human genome contains approximately 3 X 10° bases and that each stable transfectant incorporates 10° bp of DNA, the entire human genome 100 Bn-EP BX18 10-19 1-19(9)* 25-28 10-19, 1-19 (0X9) $ —-N wl = N | oS N . ies, i) 10 20 10 20 Retention Time (min) FIGURE 2 Transfectant colonies were grown on polyester nylon filters for 7 days. Replica filters were carefully removed from the master dish and colonies fixed with 10 percent trichloroacetic acid (10 minutes) and stained with 0.05 percent Coomassie blue in methanol :water:acetic acid (45:45:10; 10 minutes). Excess stain was removed by washing with methanol:water:acetic acid. WITH AVIDIN 180. se. 0 By,-tP 80. A BXla 70. 60. $8. cs OMoL NX 40. 30. 20. 10. AMO» OZCOW Ad 2 213333 42 4 aa33ay id aaa} . T T _— +1 1. 10. 100. 1000. COMPETITOR CONCENTRATION [NMJ FIGURE 3 In situ replica filter binding assay for detection of transfectants expressing neuroreceptors. 101 DOT ASSAY FOR OPIOID RECEPTOR EXPRESSION N4TG1 CELL # N4TG1 +Blocker L . @ 10° # 2 10* &% » FIGURE 4 N4TGl or L cells were spotted on nylon cloth and subjected to binding with (3-[!?°I]iodotyrosyl?’)R-endorphin (0.15 nM, room temperature, 1 hr.) in the absence or presence of the opioid antagonist, naloxone (100 uM). The filters were then washed with ice cold buffer, dried briefly, and placed under X-ray film. Clear signals emanating from as few as 10,000 opioid receptor- expressing N4TGl cells are observed; very little signal is observed for L cells or for N4TGl cells whose receptor sites are blocked with naloxone. The aberrant signal emanating from 10,000 N4TGl cells in the presence of blocker is not reproducible and is believed to be an artifact. 102 can be easily represented by approximately 3,000 independent transfectant colonies (Kuhn et al. 1984). We have prepared several transfection libraries and screened these libraries with (3-[**3I]iodotyrosyl?’)R-endorphin using the detection technique described in the previous section. Thus far, we have been unsuccessful in detecting opioid receptor-positive clones. Our results with the opioid receptor-rich N4TGl cell line indicate that an opioid receptor-bearing transfectant colony (1,000-5,000 cells per colony) can be detected if the receptor gene is expressed at a level of at least 10,000 receptors per cell. If the human opioid receptor promoter is weak in the heterologous mouse cell system, our screening assay may not be sensitive enough to detect transfectants expressing receptor at low levels. CLONING THE OPIOID RECEPTOR BY THE HOMOLOGY APPROACH An emerging concept in the field of molecular neurobiology is that transmembrane signalling neuroreceptors involve three distinct components. First, there is a specific receptor exposed on the external surface of cell membranes that recognizes and interacts with ligands, such as hormones or drugs, or responds to a sensory stimulus such as light. Second, exposed at the cytoplasmic surface are effector enzymes such as adenylate cyclase that either generate the second messenger cAMP or in some other way effect an intracellular response. Third, interposed both functionally and physically between the receptor and its effectors are transducing or coupling proteins that bind GTP (so- called G-proteins). The available evidence suggests that signalling systems of this type demonstrate a high degree of structural, functional, and regulatory homology (Dolhman et al. 1987). To date, seven pharmacologically or functionally related G- protein receptors have been cloned and their primary sequences shown to be similar. These are the f-adrenergic receptor from human (Kobilka et al. 1987), hamster (Dixon et al. 1986), and turkey (Yarden et al. 1986), the muscarinic acetylcholine receptor from porcine brain and heart (Kubo et al. 1986a, b), the human and bovine opsin protein (Nathans and Hogness 1984, 1983), as well as the visual pigments from drosophila (Zuker et al. 1985), the human mas-oncogene (Young et al. 1986), and the yeast mating factor receptor (Burkholder and Hartwell 1985). All these proteins display a certain degree of sequence similarity at the amino acid level, display similar hydropathic profiles, and have conserved functionally important amino acids or glycosylation sites. The opioid receptor interacts with the same regulatory G- proteins as these other receptors. It is therefore postulated that the opioid receptor will possess an amino acid structure similar to the above mentioned G-protein related receptors. This postulated relationship is the premise upon which the approach to cloning the opioid receptor by homology is based. 103 Probe Design The most often used probes are full-length double-stranded cDNAs, short synthetic oligonucleotides, or mRNA riboprobes that are labeled with %2P, 33S, or biotin. The selection of the probe will depend on the screening strategy. Full-length cDNAs for a related receptor or short oligonucleotides for a consensus region are the most appropriate probes for the screening of recombinant DNA libraries. We shall focus our discussion on these methods. If two nucleic acid sequences are related, the use of a cDNA probe complementary to one should identify the other if the probe is labeled by nick-translation and the regions of similarity are a significant fraction of the nick-translated lengths. An alternative to using double-stranded cDNAs is to use single- stranded synthetic oligonucleotides, which are complementary to putative consensus regions of the receptor. Oligomers, which typically can range from 14 to 60 or more bases, are easily end- labeled with T4 polynucleotide kinase and [v-32P)ATP. Since the probe is labeled at either its free 5'-phosphate or hydroxyl group, only one radiophosphate is incorporated per strand. Therefore, this type of probe has a lower specific activity than nick-translated cDNAs. Screening of the Library Screening of recombinant libraries involves the hybridization of radioactive probes to filter bound nucleic acid targets that constitute the elements of the library. Duplex formation in terms of both the number of positives and the intensity of signals is a function of both the stability of the duplex formed and the rate of hybridization. Nucleic acid hybridization depends on the random collision of two complementary sequences. The time course of the reaction is thus determined by the concentration of the reassociating species and by a second-order rate equation. While the quantitative hybridization of two perfectly matched sequences in solution can be rigorously described mathematically, the hybridization of a nucleic acid strand in solution to a filter-immobilized complementary sequence can only be qualitatively approximated. An important consideration when identifying new proteins by cross-hybridization involves the discrimination of homologous from heterologous matches... When probing with both single-strand oligomers and denatured double-strand cDNAs, the ratio of the extent of hybridization of homologous sequences to heterologous sequences is not constant but varies with time. Hybridization to similar sequences is maximal early in the reaction and decreases with increasing time of incubation. Therefore, although the homologous reaction is faster and will reach completion earlier, the heterologous reaction will eventually catch up. The discrimination of related sequences is therefore maximal early in the reaction but deteriorates very quickly. Thus, for most cases, maximal discrimination between homologous and heterologous 104 sequences is best accomplished by keeping the incubation time short. Nucleic acids hybridize very slowly at low ionic strength. As the ionic strength of the hybridization solution increases, so does the rate of duplex formation. This effect is most dramatic at low salt concentrations (0.15 M Na‘), but remains marked up to 1.5 M Na*. High salt concentration stabilizes mismatched duplexes; so to detect cross-hybridizing species, the salt concentration of both the hybridization and wash solution must be kept fairly high, generally at 2-6xSSC (1xSSC is 0.15M NaCl, 0.015 NaCitrate, pH 7.0). The stability of a nucleic acid duplex can be described by its melting temperature, T,. In general, the rate of reassociation as well as the stability of the duplex is maximal at 20-30°C below the T,. The optimal temperature for nucleic acid reassociation in aqueous salt solution lies in the range from 60- 75°C. However, extended incubation at such temperatures can lead to a considerable amount of thermal strand scission. Hence, it is desirable to reduce the temperature while maintaining the stringency of the nucleic acid interaction. The effective incubation temperature can be lowered by including formamide in the hybridization solution. Formamide acts to destabilize hydrogen-bonding between double-strand nucleic acids (McConoughy et al. 1969). In addition to affecting the T,, formamide also affects the rates of hybridization. This effect is minimal at formamide concentrations of 30-50 percent; however at concentrations of 20 percent formamide, the rate is decreased by one-third, while at 80 percent the rate can drop as much as threefold for DNA-DNA and as much as twelvefold for DNA-RNA duplexes. Thus, in practice, the inclusion of formamide in the hybridization solution can be used to alter the stringency of the incubation by holding the incubation temperature constant and varying the formamide concentration. The effective incubation temperature can be reduced to as much as 50°C below the T, for perfect matches. The effects of temperature, base composition, and formamide can be approximated by an equation that estimates the T, of the duplex; Ty, = 69.3 + 0.41(G+C) percent - 650/L where (G+C) percent is the percentage of G and C residues in the duplex and L is the average length of the probe (Marmur and Doty 1962; Wetmur and Davidson 1968). Furthermore, taking into consideration possible mismatches, the T, of the duplex decreases 1°C with every 1 percent increase in the number of mismatches (Bonner et al. 1973), and the T, at differing ionic strengths (ul and u2) can be related by (T,)y; - (Tp)y: = 18.5 log(u2/ul) (Dove and Davidson 1962). After hybridization, washing is carried out to remove unhybridized probe and to dissociate unstable hybrids. The temperature and salt concentration of the washing solution determine which hybrids will be detected. In general, washing should be done under stringent conditions: at 5-20°C below the 105 T, for a well-matched hybrids (65-70°C), and at 12-20°C below the T, for cross-reacting species (50-60°C). No absolute rule exists for the duration of the washing period. In general, several short (5-10 minutes) nonstringent washes are conducted, prior to the final stringent washes (15-30 minutes). During the washes, filter-bound background radioactivity can be monitored with the use of a hand-held monitor. In principle, this strategy can lead to the molecular cloning of any G-protein related receptor. Since the extent of the similarity between opioid receptor sequences and other G-protein related sequences can only be approximated, the successful use of this strategy in the cloning of the opioid receptor will require the careful determination of the appropriate hybridization conditions. This determination, although based on theoretical considerations discussed above, will be primarily empirical. The molecular clone obtained by the homology approach will then be expressed in eukaryotic cells to confirm the expression of authentic opioid receptors. CONCLUSION Three different strategies can be employed in the molecular cloning of the opioid receptor. The first strategy consists of purifying and sequencing the opioid receptor and utilizing the amino acid sequence in the isolation of a cDNA clone. This traditional cloning approach has proven to be difficult in the cloning of the opioid receptor because of the receptor’'s low abundance and high sensitivity to denaturation. The second strategy proposes to clone the opioid receptor through gene expression in eukaryotic cells without prior purification of the receptor protein. The cloning of the opioid receptor by this approach has remained elusive. The third strategy utilizes the possible homology between opioid receptors and other G-protein neuroreceptors as a hybridization tool in identifying potential opioid receptor clones. This approach, while extremely attractive in light of the growing number of G-protein related receptors that have found to be homologous, requires the analyses of many full-length cDNA clones. 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Zuker, C.S.; Cowman, A.F.; and Rubin, G.M. Isolation and structure of a rhodopsin gene from Drosophila melanogaster. Cell 40:851-858, 1985. Zukin, R.S., and Maneckjee, R. Solubilization and characterization of opiate receptors. Methods Enzymol 124:172-190, 1986. 109 AUTHORS Curtis A. Machida, Ph.D. John Salon, Ph.D. David Grandy, Ph.D. James Bunzow, M.S. Paul Albert, Ph.D. Eric Hanneman, Ph.D. Olivier Civelli, Ph.D. Vollum Institute for Advanced Biomedical Research Oregon Health Sciences University Portland, Oregon 97201, U.S.A. 110 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D., eds. National Institute on Drug Abuse, 1988 Effects of Opioid Peptides on Human Neuroblastoma Cells Wolfgang Sadee, Dr. rer. nat.; Victor C. Yu, Ph.D.; and Gunther Hochhaus, Ph.D. The discovery of multiple opioid receptor types (e.g., UL, J, xk) makes it necessary to study the molecular mechanisms of opioid action in transformed cell lines that yield homogenous cell populations under well-defined conditions in vitro. Much has been learned from the use of such cell lines, which include the mouse neuroblastoma x rat glioma hybrid NG 108-15 (Gilbert and Richelson 1983). However, this line, as well as other neuroblastomas tested, expresses only the 3 receptor. Therefore, we have screened a series of human neuroblastoma cell lines for the presence of different opioid receptor types. Of three lines with 10,000 opioid sites or more per cell, all displayed 8 receptor sites (Hochhaus et al. 1986); however, one of these human neuroblastomas also expressed abundant pu receptor sites (SK-N-SH, ~ 50,000 sites per cell) in a ratio of Wd = 4.5 (Yu et al. 1986). This cell line has potential as an excellent in vitro model for studying the effects of opiates and opioid peptides. However, in this cell line we found only a 20 percent inhibition of PGE{—stimulated adenylate cyclase activity following treatment with opioid agonists (Yu et al. 1986). An additional problem is that there are several interconverting phenotypes of SK-N-SH, which include both a strongly substrate adherent nonneuronal form and a neuroblast form that grows more slowly to higher saturation cell densities. Only the latter appears to express opioid receptors. AN IN VITRO MODEL TO STUDY OPIOID EFFECT In order to provide more reproducible cell culture conditions, we selected a phenotypically stable neuroblast subclone of SK-N-SH, designated SH-SY5Y (Ross and Biedler 1985). The SH-SY5Y clone carries a similar number of opioid receptors as the parent line, yet opioid inhibition of adenylate cyclase remains slight. In order to increase the opioid response, we tested the effects of neuronal differentiation on receptor-adenylate cyclase coupling. Three differentiating agents, retinoic acid, nerve growth factor, and dibutyryl 111 ¢ll FIGURE 1. Human neuroblastoma cells, clone SH-SY5Y, grown in culture in either the absence (left) or the presence (right) of 10 uM retinoic acid. cAMP, caused neurite extensions that are characteristic of neuronal maturation (fig. 1). Of these three, only retinoic acid (10 pM maintained over 5-6 days) produced differentiated cells that yield a 10- to 50—fold increase in PGE4—stimulated adenylate cyclase activity. Moreover, the ability of opioids to inhibit the PGE response was also enhanced by retinoic acid (45 percent inhibition), while nerve growth factor was less effective (~ 35 percent inhibition). We also tested the ability of opioids to inhibit stimulation of adenylate cyclase by forskolin (100 uM), which directly acts on the enzyme rather than a stimulatory receptor. Opioids were even more effective in inhibiting the forskolin response (65 percent inhibition in retinoic acid treated cells). This opioid effect was inhibited by naloxone and pretreatment with pertussis toxin, suggesting the involvement of opioid receptors via an N; coupling protein (fig. 2). Hence, the SH-SYS5Y subclone, when differentiated with retinoic acid, represents a system for quantitative studies of pu and possibly & receptor mechanisms that include tolerance and opioid dependence. % MAXIMAL INHIBITION so 5 8 ¢s 883888 MORPHINE MORPHICEPTIN DAGO DADLE DPDPE MORPHINE + NALOXONE MORPHINE + PERTUSSIS TOXIN FIGURE 2. Inhibition of stimulated cAMP production in intact cells by opioids. The morphine response was defined as maximum inhibition (i.e., 100 percent). Both PGE4 (1 uM) and forskolin (100 uM) were employed as the stimulating agents. 113 EFFECT OF un AND 8 RECEPTOR SELECTIVE OPIOID PEPTIDES In order to determine which opioid receptor type is responsible for inhibition of the PGE 1— or forskolin—cAMP response, we tested a series of opioids for their efficacy. Both morphine and the potent general agonist etorphine gave similar maximal responses (45 percent of the PGE1 response and 65 percent of the forskolin response). Since these agonists are not highly selective for either pu or 8 sites, we then chose several opioid peptides of high selectivity (fig. 2). It should be noted that the efficacy of any of these ligands at the pu sites has not been previously established. Both the p specific agonist morphiceptin and the highly p selective agonist DAGO gave the same maximal inhibitory effects as morphine and etorphine. This result strongly suggests that these peptides are full agonists and that the inhibitory response is mediated by the pu sites. Indeed, we confirmed earlier findings that morphiceptin is inactive at the 6 sites in NG 108-15 cells. In contrast, the potent and highly 3 selective DPDPE gave only a small partial response at 30 nM, at which concentration one might expect near maximal activation of 3 sites. Maximal response of DPDPE at 10 uM was only ~ 65 percent of that obtained by the other agonists, and it is likely that this partial response is largely mediated by cross—reaction with the pu sites. The pu and 8 agonist DADLE, on the other hand, gave full inhibitory effects at rather low concentrations (< 1 uM). These results support the view that the opioid receptor inhibition of adenylate cyclase in SH-SY5Y cells is largely mediated by the pu site. Therefore, this subclone is ideally suited for studying the efficacy, tolerance, and dependence of the narcotic analgesics in vitro. It should be noted that all of the above results were obtained in the presence of the phosphodiesterase inhibitor IBMX. Therefore, the conclusions from these studies are limited to the activity of adenylate cyclase. However, initial experiments in the absence of IBMX suggest that the opioid agonists may also increase the activity of phosphodiesterase. This would indicate a second mechanism by which cellular cAMP levels could be regulated. We are currently investigating this possibility. BIOTINYLATED B-ENDORPHIN A better understanding of the molecular events involved in the opioid response in neuroblastoma cells can be attained through the study of opioid receptors on single cells. Such studies would clarify both the distribution of opioid receptors throughout a cell population and their location on the cell. A method for rapid isolation and quantitation of receptors is desirable. Therefore, we intend to utilize the avidin-biotin system for opioid receptor analysis (Korpela 1984). Typically, a suitable ligand is labelled with biotin and allowed to bind to the receptor site. Next, the biotinyl-tracer receptor complex is incubated with avidin. 114 Avidin has an extremely high binding affinity for biotin Kg= 107" Su). The avidin molecule is then labelled with fluorescent ayes, colloidal gold, or enzymes. It is important to employ a biotinylated tracer that retains high receptor affinity in the presence of avidin. pp—(1-31)—endorphin reacting with biotinyl N-hydroxysuccinamide, with or without an intervening e—aminocaproyl spacer arm, yields a series of biotinylated products with one or more substitutions per molecule. Tyr-1 and Lys 9, 19, 24, 28, 29 represent possible reaction sites, as shown in figure 3. Tyr-Gly—-Gly-Phe-~Met-Thr-Ser-Glu-Lys-Ser- 1 10 GIn-Thr—Pro-Leu-Val-Thr-Leu-Phe-Lys—Asn— 11 20 Ala—-lle-lle-Lys—Asn-Ala-Tyr-Lys-Lys-Gly-Glu 21 30 FIGURE 3. Human B—endorphin. These derivatives were purified by HPLC and characterized by FAB- mass spectrometry and trypsin digestion followed by HPLC (fig. 4) and again FAB-MS. Biotinylation of a lysine residue eliminates one tryptic cleavage site, which allows one to determine the site of biotinylation. The Tyr-1 terminal NH2 group was not affected in any of the products isolated, perhaps because, in the tertiary structure, it could have an internal location and/or it could be involved in hydrogen binding. Monobiotinylated fractions with substitution at either Lys—9 (fig. 4), Lys— 19, or Lys—24, 28, 29 (Bx1 a) were analyzed for binding to the pn and & opioid receptors in rat brain homogenates and neuroblastomas. All derivatives retained significant opioid receptor affinity, even in the presence of avidin. The highest affinity among the derivatives was found with Bx1a, which was equally potent to native Br—endorphin, even in the presence of avidin (fig. 5). Therefore, this derivative fulfills all criteria for application of the biotin—avidin system to the analysis of the opioid receptor. The biotinylated Br—endorphin derivative Bx1a also displayed high affinity to a Bn—endorphin specific antibody (Peninsula Labs). We therefore developed an ELISA method for the quantitation of Bh— endorphin, using Bx1a as the tracer and an avidin—alkaline phosphatase complex as the enzyme indicator. Optimal incubation conditions yielded a sensitivity of 0.5 femtomole Br—endorphin per sample, equivalent to the most sensitive 1251-RIA currently available. Current applications of the biotin—avidin system to opioid molecular pharmacology are in progress. 115 Replica Transfer of Transfectant Colonies Replica Filter 1 Replica Filter 2 Replica Filter 3 0. o - 09". o 99" o # ‘oo . ‘eq . te ‘ag . 5... Yt © ® ® - . > A 2 ° . — a a * ole F FIGURE 4. HPLC records (reverse phase) of tryptic digests of Bh— endorphin and Bx1B with biotinylation predominantly at Lys—-19. Screening Eukaryotic Expression Libraries For Neuropeptide Receptor Genes Using Novel In _Situ Replica Filter Binding Assays Human neural Ca PO, Drug selection DNA + transfection 10 days neo plasmid Dish of mouse cells neo resistant (lacks receptor) colonies Overlay with polyester sheets (up to 5 copies) Grow 5-7 days Oo Replica Copy Replica Copy Replica Copy Replica Copy Master Dish Preblock with In situ binding Stain with Maintain colonies excess cold with '25[-labeled bromphenol at reduced peptide tid blue temperature n_situ binding fleuropentios with labeled peptide Autoradiography Autoradiography Remove neuropeptide —————— receptor positive colony from master dish Identification of Receptor Positive Colony FIGURE 5. Equilibrium binding competition curves between 3H-DAGO (1 nM) and Br—endorphin or Bx1a in rat brain homogenates in the presence of avidin. 116 REFERENCES Gilbert, J.A., and Richelson, E. Function of delta opioid receptors in cultured cells. Mol Cell Biochem 55:83-91, 1983. Hochhaus, G., Yu, V.C., and Sadée, W. Delta opioid receptors in human neuroblastoma cell lines. Brain Res 382:327-331, 1986. Korpela, J. Avidin, a high affinity biotin—binding protein, as a tool and subject of biological research. Med Biol 62:5-26, 1984. Ross, R.A. and Biedler, J.C. Presence and regulation of tyrosinase activity in human neuroblastoma cells. Cancer Res 45:1628—-1632, 1985. Yu, V.C., Richards, M.L., and Sadée, W. A human neuroblastoma cell line expresses pu and d opioid receptors. J Biol Chem. 261:1065- 1070, 1986. ACKNOWLEDGMENT Supported by Public Health Research Grant #DA 01095 and DA 01466 from the National Institute on Drug Abuse. AUTHORS Wolfgang Sadée, Dr. rer. nat. Victor C. Yu, Ph.D. Guinther Hochhaus, Ph.D. School of Pharmacy University of California San Francisco, California 94143, USA 117 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D., eds. National Institute on Drug Abuse, 1988 Analgesia and Neuropeptides David J. Mayer, Ph.D. INTRODUCTION Until iy recently, virtually nothing was known about the neurochemical basis of pain. The past few years have seen an unprecedented explosion of information in the neurosciences, neurochemistry, the role of peptides in behavior, and, most important here, the neurobiology of pain and pain modulation. As statistics about the epidemiology of pain have surfaced, the biomedical importance of pain research has become apparent. Thus pain research in general and research on the involvement of opioid and other peptides in pain in particular have undergone an impressive expansion in the past decade. This chapter will review the extensive literature on the mechanisms of pain modulation by opioid and other neuropeptides. Commensurate with this increase in knowledge about endogenous peptide involvement in pain modulation has come a search for the environmental stimuli that might normally activate these systems. Much interest has focused on the role of painful and stressful environmental events. This chapter will examine the involvement of these types of events in the activation of endogenous peptide pain modulatory systems. THE ROLE OF OPIATES AND OPIOID PEPTIDES IN PAIN MODULATION The discovery of the enkephalins (Hughes 1975) and the subsequent discovery of related opioid peptides has led to a great interest in the role of these substances in pain modulation. This research has elucidated an important role for these substances in pain modulation. This section will review both animal and human studies of the role of endogenous opioids in pain modulation. Historical Perspective A number of critical discoveries about the neurobiology of opiate action have occurred in the past few years: (1) The demonstration of stereospecific 118 and saturable binding sites for opiates in the central nervous system (Hiller et al. 1973; Pert and Snyder 1973; Terenius 1973). (2) The associated demonstration of multiple binding sites for opiates [See Martin, (Martin 1983) for an excellent review of this topic]. Q The discovery of endogen- ous ligands for opiate receptors (Hughes 1975). (4) The concept of using opiate antagonists to antagonize endogenous behavioral repertoires (Akil ef or 1972). These findings, along with the extensive utilization of the intracerebral microinjection technique to localize the site of action of neurochemicals within the central nervous system (Tsou and Jang 1964), have, in turn, had an important impact on theoretical and methodological research strategies utilized for the study of the effects of opiates on behavior. Methodological Considerations Before these discoveries, the study of the analgesic effects of opiates (as well as other peptides) was primarily phenomenological. The analgesic effects of opiates were catalogued and seen in the light of designing drugs with more therapeutically desirable and fewer therapeutically undesirable effects for application to clinical pathology. Although clinical utility certainly remains an important concern of opiate research, the discoveries described above have resulted in research that is conceptually broader. The current overall view is that opiates often act on endogenous biological substrates for beha- viors. Hence the behavioral pharmacology of opiates now addresses the organization of the neurobiological substrates of behavior. Much of the research in this area now proceeds in the following pattern: (1) Can a behavior elicited by opiates be elicited by exogenous environmental mani- pulations? For example, can analgesia be elicited by transcutaneous nerve stimulation? (2) If so, can the behavior, when initiated by nonpharmacolog- ical means, be shown to utilize SHdgsnons opiates? This question is gener) approached by examining whether the behavior can be antagonized y opiate antagonists and reduced by the induction of tolerance to opiates (that is, does cross-tolerance occur?). Additional support for a role of endogenous opiates is provided by the demonstration of a correlation between release of endogenous opiates and the occurrence of the behavior under study. (3) If the behavior is shown to involve endogenous opiates, the precise neuroanatomical foci underlying the behavior are examined utilizing the microinjection of opiate agonists and antagonists into restricted central nervous system loci. (4) The opiate receptor type involved in the behavior is examined by administering opiate agonists and antagonists at least partially selective for particular receptor subtypes (mu, kappa, delta, etc.). (5) Ideally, steps (3) and (4) are combined to determine the anatomical locus of specific receptor types involved in the behavior being studied. (6) An attempt is made to determine the precise endogenous ligand (beta-endorphin, Met-enkephalin, dynorphin, etc.) involved in a particular behavior. Again, an attempt is made to determine the anatomical locus of action of the parti- cular ligand. This is, of course, an idealized outline of the path followed to investigate opioid involvement in a behavior. More often than not the actual course of research is less direct than this, and the final conclusions are not usually simple. Nevertheless, keeping in mind the general approach described above will aid the reader to see the overall progression the field. Until the early 1970s, in spite of evidence to the contrary (Tsou and Jang 119 1964; Dewey et al. 1969), the generally accepted theory of opiate analgesic action (Lim 1966) considered opiates to iis analgesia by a central ner- vous system mechanism analogous to the action of local anesthetics on a peripheral nerve. That is, it was thought that opiates acted by directly Inactivating the afferent transmission of pain in the central nervous system. Since then, a fio advance in our conception of the neural processing of pain has occurred. It has become clear that information about tissue damage 1s not passively received by the nervous system. Rather, it is filtered, even at the first synapse, by complex modulatory systems. The discovery of these systems has fostered, and has in turn been fostered by, the notion that the central nervous system contains endogenous substances, endorphins, that possess analgesic properties virtually identical to opiates of plant and syn- thetic origin. In this section, the development of these concepts is examined. The existence of opiate and nonopiate central nervous system pain modula- tory Meciantems activated by environmental stimuli such as stress is then dis- cussed. Development of the Concept of Endogenous Pain Control It has long been recognized that a simple invariant relationship between stimulus intensity and the magnitude of pain perception is often not present. Two general classes of observations support the complexity of this relation- ship. The first is the clinical observation that pain is often present without any apparent precipitating pathology. This situation represents the clinical problem of pain treatment. More important for the topic of this section is the common observation that pain may not be experienced in the presence of factors that should produce it; that is, under a variety of circumstances, total or Piru analgesia is seen. These observations were explicitly recognized in earlier models of pain perception in spite of the lack of direct evidence supporting the theoretical models (Noordenbos 1959; Melzack and Wall 1965). Thus, the concept that the nervous system possesses intrinsic pay iry mechanisms was recognized when only indirect evidence was available. The earliest work indicating that opiates produce analgesia, at least in part, by activation of endogenous pain inhibitory systems was done by Irwin ef al. (1951). They demonstrated that morphine was not effective in inhibiting the spinally mediated tail flick response in spinalized rats. They reasoned based on this result, that morphine must activate supraspinal neural circuitry which has an output to the spinal cord and modulates the processing of nociceptive information at spinal level. ' This work was largely Jonorsg until the early 1970s, even though it was replicated in the mouse (Dewey ef al. 1969). The first impetus for the detailed study of pain-modulatory circuitry resulted from the observation that electrical stimulation of the brain could powerfully suppress the perception of pain (Reynolds 1969; Mayer et al. 1971). Further investigation of stimulation-produced analgesia provided considerable detail about the neural circuitry involved [see Mayer and Watkins (1984) for a detailed review of this topic]. Significantly, at that time, several similarities were recognized between these observations and information emerging from a concomitant resurgence of interest in the mechanisms of Opias analgesia (Mayer ef al. 197 D e most important parallel facts revealed by these studies were the following: (1) 120 Effective loci for both opiate microinjection analgesia (Tsou and Jang 1964) and stimulation-produced analgesia (Mayer et al. 1971) lie within the periaqueductal and periventricular gray matter of the brain stem. (2) Opiate analgesia and stimulation-produced analgesia are both mediated in part by the activation of a centrifugal control system that exits from the brain and modulates pain transmission at the level of the spinal cord (Dewey ef al 1969; Irwin ef al. 1951). (3) The ultimate inhibition of the transmission of nociceptive information occurs, at least in part, at the initial processing stages in the spinal cord dorsal horn and homologous trigeminal nucleus caudalis by selective inhibition of nociceptive neurons (Satoh and Takagi 1971). In addition to these correlative observations, studies of stimulation-produced analgesia provided direct evidence indicating that there were mechanisms in the central nervous system that depend upon endogenous opiates: (1) Subanalgesic doses of morphine were shown to synergize with subanalgesic levels of brain stimulation to produce behavioral analgesia (Samanin and Valzelli 1971). (2) Tolerance, a phenomenon invariably associated with repeated administration of opiates, was observed to the analgesic effects of brain stimulation (Mayer and Hayes 1975), (3) Cross-tolerance between the Sl oesie effects of brain stimulation and opiates was demonstrated (Mayer and Hayes 1975). (4 a analgesia could be Spiotonized by naloxone, a specific narcotic antagonist (Akil ef al. 1972, 1976a). This last observation, in particular, could be most parsimoniously explained if electrical stimulation resulted in the release of an endogenous opiate-like factor. Indeed, naloxone antagonism of stimulation-produced analgesia was ical impetus leading to the eventual discovery of such a factor (Hughes Coincidental with work on stimulation-produced analgesia, another discovery of critical importance for our current concepts of endogenous analgesia sys- tems was made. Several laboratories, almost simultaneously, reported the existence of stereospecific binding sites for opiates in the central nervous system (Hiller et al. 1973; Pert and Snyder 1973; Terenius 1973). These "receptor" sites were subsequently shown to be localized to neuronal synaptic regions (Pert et al. 1974) and to overlap anatomically with loci involved in the neural processing of pain (Pert ef al. 1975). The existence of an opiate receptor again suggested the likelihood of an endogenous compound with opiate properties to occupy it. In 1974, Hughes (1975) and Kosterlitz reported the isolation from neural tissue of a factor (enkephalin) with such properties. An immense amount of subsequent work has characterized this and other neural and extraneural compounds with opiate Piopeties As with the opiate receptor, the anatomical distribution of endogenous opiate ligands shows overlap with sites involved in pain processing [see Akil ef al. (1984) for a recent review of these studies]. To summarize these important historical developments, the existence of an endogenous opiate analgesia system is suggested by several lines of evidence. Electrical stimulation of the brain produces analgesia. The anatomical structures and neural mechanisms involved in stimulation-pro- duced analgesia parallel those involved in opiate analgesia. The central nervous system contains opiate binding sites and endogenous ligands capa- ble of interacting with those sites. These binding sites and ligands are found 121 at anatomical loci consistent with sites at which stimulation-produced analgesia and opiate microinjection analgesia are elicited. Neural Circuitry Involved in Analgesia Resulting from the Administration of Exogenous Opiates This section will review the current data available on the sites and mechan- isms involved in the modulation of pain by the administration of exogenous opiates. Primarily, two lines of experimentation will be examined: (1) The. locations in the central nervous system of sites at which administration of Shicjes results in analgesia and the administration of opiate antagonists blocks analgesia. (2) The locations in the nervous system where lesions block the action of exogenously administered opiates. Following the work of Tsou and Jang (1964), it wasn’t until the early 1970's, with one exception (Lotti ef al 1965), that opiate microinjection mapping studies began. Initially these studies concentrated on the periaqueduc- Jal perivemaioular regions of the merencapasion and diencephalon (Jacquet and Lajtha 1973; Pert and Yaksh 1974; Yaksh ef al. 1976). Overall, these and other studies confirmed the importance of the periaqueductal-peri- ventricular region in opiate analgesia and provided an impetus for the examination of other brain areas. A second brain area that has proved to be of considerable importance for opiate action is the anatomically complex region of the ventromedial medulla. This region consists of at least three distinct nuclei: the medially located nucleus raphe magnus (NRM), the more laterally situated nucleus reticularis paragigantocellularis (NRP), and the dorsolaterally located nucleus reticularis gigantocellularis (NRG). Based on retrograde ein a, Watkins ef al. (1980) have proposed the term nucleus raphe alatus (NRA) for the combined cell groups in NRM and NRP. Takagi ef al. {979 were the first group to map this region for analgesia resulting from morphine microinjection. Overall (Takagi 1980), this group found the NRP to be approximately 20 times more sensitive to Myiphipe than the NRG. They found microinjection of morphine into the NRM to be ineffective in the production of analgesia. This point is controversial, since other groups (Azami et al. 1982; Zorman et al. 1982) have reported analgesia from microinjection into NRM. Azami ef al. (1982) did find, however, that the NRM was less sensitive than the NRPG. A number of other brain areas including the amygdala (Rodgers 1977, 1978), the medial lemniscus (VanRee 1977), nucleus medialis dorsalis of the thalamus (VanRee 1977), the mesencephalic reticular formation (Haigler and Mittleman 1978; Pert and Yaksh 1974), and the nucleus of the solitary tract (Oley et al. 1982) have been reported to produce analgesia when injected with opiates. However, the work on these areas is scant compared with those discussed above, and the relative potency of injections into these areas has not been explored. A final but crucial point to be made in this section concerns the analgesic effects of microinjections of opiates directly into the intrathecal space of the nial cord. Although Tsou and Jang (1964) reported no analgesia from irect spinal appiisation of morphine, subsequent work has consistently demonstrated relatively potent effects of intrathecal morphine microinjection 122 (Yaksh and Rudy 1976, 1977). From this line of evidence it appears, then, that at least three general areas of the central nervous system are involved in opiate analgesia: the peria- queductal-periventricular gray matter, the ventromedial medulla, and the spinal cord. This observation indicates that the analgesic effects of a systemi- cally administered Opiate may produce analgesia by acting at any, all, or some combination of these distinct regions. The utilization of the microinjection of narcotic antagonists has provided at least a partial answer to this question. A number of early studies concluded that supraspinal sites of opiate action are the effective ones, since analgesia from a administered opioies was antagonized by either in- tracranioventricular or intracerebral microinjection of narcotic antagonists (Albus et al. 1970; Jacquet and Lajtha 1974; Tsou, 1963; Vigouret et al 1973). Later work, however, demonstrated that naloxone administered intrathecally could antagonize the analgesia resulting from even relatively high doses of s AME administered opiates (Yaksh and Rudy 1977). Thus, these studies lead to the paradoxical conclusion that both supraspinal sites and spinal sites of opiate action are the critical ones involved in analgesia. This seeming paradox was resolved in a series of complex but unusually important studies by Yeung and Rudy (1980a,b). They demonstrated that by simultaneously administering various doses of morphine intrathecally (into the spinal cord) and intraventricularly (into the brain) a multiplicative dose response function was observed. That is, simultaneous spinal and supraspinal morphine resulted in greater analgesia than the same total dose administered at either location alone. The effect is quite large, with the multiplicative factor being as much as 45 under certain circumstances (Yeung and Rudy 1980a). This type of multiplicative interaction, as will be seen below, may turn out to be a confounding factor in many pharmacological and physio- logical analyses of the involvement of opiates in various behaviors. Thus, the reader should keep in mind, when evaluating the literature on this and other topics, the potential for complex interactions between the same or various neurotransmitters and/or neuromodulators. Although the experiments just described elucidate the contribution of spinal vs. supraspinal sites to opiate analgesia, the relative contribution of the various supraspinal sites at which opiates act to produce analgesia is less clear. The only work to examine this issue utilizing microinjection of nar- cotic antagonists was done by Azami ef al. (1982). They found, as did the work of Takagi’s group, that the NRP was more sensitive to morphine than the NRM for the elicitation of analgesia. Surprisingly, however, they found, when analgesia was produced by systemically administered morphine, naloxone injection into the NRM antagonized analgesia more effectively than injection into more lateral medullary regions including the NRP. They concluded that NRP does not make a significant contribution to the analge- sia resulting from systemic administration of morphine. The relative contribution of medullary vs. more rostral mesencephalic sites has not been examined. An approach similar to the one just described for dissecting the neural circuitry participating in opiate analgesia utilizes the selective destruction of 123 nuclei and pathways suspected of being involved in opiate analgesia. Opiates are administered systemically or at discrete sites in the nervous system and the effects of particular lesions are examined. An overview of this work supports the conclusion reached above utilizing injection of antagonists. It appgery that several brain areas including the periaqueductal gray matter, M, and NRP need to be intact for the full expression of opiate analgesia. Environmental Activation of Endogenous Analgesia Systems The demonstration that opiates activate well-defined neural systems capable of potently blocking pain transmission suggests, but by no means proves, that the function of this system is to dynamically modulate the perceived intensity of noxious stimuli. If, in fact, this system : such a physiological role, then one might expect that the level of activity within the system would be influenced by impinging environmental stimuli. If environmental situations that produce analgesia could be identified, it would give credibility to the idea that invasive procedures, such as brain stimulation or narcotic drugs, inhibit pain by mimicking the natural activity within these pathways. TABLE 1 SYSTEMIC OR |DYNOR- |ENKE- CROSS |CNS IT NALOXONE |PHIN PHALIN |TOLER- EN DORPHIN ANTI- ANTI- ANCE EVEL SERUM |SERUM ACUPUNCTURE 12,1317 REFERENCES FOR TABLE 1 1. Akil and Liebeskind 1975 2. Akil et al. 1976b 124 3. Akil et al. 1972 4. Akil et al. 1978b . Kajander ef al. 1984 . Kayser and Guilbaud 1981 5. Augustinsson et al. 1977 48. Kraus et al. 1981 6. Belenky ef al. 1983 49. Kulkarni SK 1980 7. Bodnar et al. 1978 50. Lewis et al. 1981 8. Bodnar ef al. 1978 51. Madden et al. 1977 9. Cannon ef al. 1982 52. Mah et al. 1980 10. Cannon et al. 1984 53. Maier et al. 1980 11. Chance et al. 1978 54. Mayer and Hayes 1975 12. Chapman et al. 1980 55. Mayer and Murfin 1976 13. Chapman ef al. 1976 56. Mayer et al 1976 14. Chesher and Chan 1977 57. Mcgivern et al. 1979 15. Cobelli et al. 1980 58. Meyerson ef al. 1978 16. Coderre and Rollman 1984 59. Miczek and Thomson 1984 17. Das et al. 1984 60. Miczek et al. 1982 18. Drugan ef al. 1981 61. O’Conner and Chipkin 1984 19. Fanselow 1979 62. Panerai ef al. 1984 20. Faris et al. 1983 63. Pertovaara ef al. 1982b 21. Freeman et al. 1983 64. Richardson and Akil 1977 22. Frenk and Yitzhaky 1981 65. Ross and Randich 1984 23. Galligan ef al. 1983 66. Rossier ef al. 1977 24. Geller 1970 67. Rossier et al. 1978 25. Gintzler 1980 68. Saavedra 1981 26. Girardot and Holloway 1984 69. Schlen and Bentley 1980 27. Girardot and Holloway 1984 70. Sessle et al. 1981 28. Grau et al. 1981 71. Shimizu ef al. 1981 29. Grevert et al. 1983 72. Shyu et al. 1982 30. Griffiths ef al. 1983 73. Snow and Dewey 1983 31. Hall and Stewart 1983b 74. Szechtman ef al. 1981 32. Hall and Stewart 1983a 75. Terman et al. 1983 33. Han and Xie 1984 76. Teskey and Kavaliers 1984 34. Han et al. 1984 77. Teskey et al. 1984 35. Han et al. 1983 78. Urca ef al. 1982 36. Hart ef al. 1983 79. Urca et al. 1981 37. Hayes et al. 1978 80. Watkins ef al. 1982d 38. Hill and Ayliffe 1981 81. Watkins Cobelli ef al. 1982 39. Holaday ef al. 1986 82. Watkins Young ef al. 1983 40. Hosobuchi et al. 1977 83. Willer et al. 1982b 41. Hosobuchi ef al. 1979 84. Willer and Albe-Fessard 1980 42. Hyson et al. 1982 85. Willer et al. 1981 43. Janal et al. 1984 86. Willer et al. 1982b 44. Jorgensen et al. 1984 87. Woolf and Wall 1983 45. Jurna 1980 88. Zamir et al. 1980 89. Zorman et al. 1982 TABLE 1 - Summary of representative studies on endogenous opiate analgesia systems. Each number in each cell of the matrix indicates a study utilizing a particular opiate manipulation to implicate endogenous opiates in various forms of environmentally produced analgesia. Citation numbers are matched with authors at the bottom of the table. The various opiate manipulations studied are indicated in the vertical columns and the environmental manipulations in the horizontal rows. Abbreviations: CCA = classically conditioned analgesia; COND = conditioned; CNS = central nervous system; DEP = deprivation; 125 DNIC = diffuse noxious inhibitory controls; ECS = electroconvulsive shock; FREQ = frequency; FPFS = front paw footshock; INT = intensity; INTER = intermittent; IT = intrathecal; LO = low; MIN = minutes; NRM = region of the nucleus raphe magnus; PAG = periaqueductal gray matter; SPA = stimula- tion produced analgesia; SPON = spontaneous; TNS = transcutaneous nerve stimulation; TS = tail shock; 4PFS = four paw footshock A systematic search for environmental stimuli that activate pain inhibitory systems was begun by Hayes et al. (1978ab). They observed that potent analgesia could be produced by such diverse stimuli as brief footshock, centrifugal rotation, and injection of intraperitoneal saline. These effects appeared to be specific to pain perception insofar as normal motor behavior, Lo and corneal reflexes, vocalization, startle responses, and response to touch remain unimpaired (Hayes ef al. 1978b). Two important additional concepts emerged from this work. First was the conclusion that exposure to stress” was not sufficient to produce analgesia. Although almost all envi- ronmental stimuli studied to date that produce analgesia are stressors (cf. table 1), the failure of classical stressors, such as ether vapors and horizontal oscillation, to produce pain inhibition indicated that "stress" was not the critical variable responsible. Second was the rather unexpected finding that the opiate antagonist, naloxone, did not block all environmentally induced analgesias (Hayes et al. 1978b). Therefore, it appeared that non-opiate Puioms must exist in addition to the system activated by opiates described earlier. Although the stimuli studied by Hayes et al. (1978a,b) did not appear to activate an opiate system, subsequent investigations found clues that endogenous opioids might be involved in at least some types of environmen- tally induced analgesias. Akil ef al. (1976b) studied the analgesic effects of prolonged footshock. In contrast to the results of Hayes ef al. (1978a,b), naloxone did partially antagonize the analgesia. This initial indication of opiate involvement led Akil and coworkers to look for biochemical evidence that footshock caused brain opiates to be released. They found that changes in brain opiate levels did indeed parallel the development of footshock- induced analgesia (Akil ef al., 1976b). When tolerance developed to the analgesic effects of footshock, brain opiate levels returned to control values. The controversy over the involvement of opiates in footshock induced analgesia was resolved, in part, by Lewis ef al. (1980). They noted that the duration of footshock used by Hayes et al. (1978b; 1978a) and Akil ef al. (e795) differed greatly and examined whether this variable might explain the difference in their results. By comparing the effects of naloxone on analgesia produced by brief (3 Ae VS. prolonged (30 min) footshock, Lewis et al. (1980) showed that only the latter could be blocked by naloxone. This suggested that different analgesia systems become active as the duration of footshock increases. Concurrent with this work of Lewis et al. (1980), Watkins et al.(1982d) made the observation that brief shock restricted to the front paws produced analgesia that was antagonized by low doses (0.1 mg/kg) of naloxone. In contrast, even high doses (20 m, yo of naloxone failed to reduce analgesia produced by hind paw shock. In addition, they showed that animals made tolerant to morphine showed cross-tolerance to front paw but not hind paw 126 footshock analgesia. Thus it appears that front paw shock activates an endogenous opiate analgesia system while hind paw shock activates an inde- pendent nonopiate analgesia system. In addition, this work showed again that stress is not a sufficient factor to activate opiate analgesia systems, since identical shock parameters were used for hind paw and front paw shock (Watkins et al. 19824). Additional work has revealed the following important facts about front paw and hind paw footshock-induced analgesias (FSIA): (1) Front paw FSIA is mediated by central nervous system opioids, since elimination of extraneural opiates by Bypophysecion adrenalectomy, or sympathetic blockade does not block the effects (Watkins et al. 1982c). (2) Front paw FSIA involves a neural circuit that ascends to the brain and then descends by way of the dorsolateral funiculus (DLF) to block pain transmission at the spinal level (Watkins et al. 1982a). This descending DLF ng originates in the nucleus raphe alatus (NRA) (Watkins ef al 1983a). (3) The complete circuitry for the effect is caudal to the Sse phn since decerebration does not affect the analgesia (Watkins ef al. 1983b). (4) The critical opiate synapse for the system is situated in the spinal cord (see figure 1) at the segment of nociceptive input, since intrathecal injection of naloxone in the lumbosacral but not thoracic spinal cord blocks the effect (Watkins and Mayer 1982). (5) Once the system is activated, continued opiate release is not needed, since naloxone only blocks the effect when given before footshock but not after (Watkins and Mayer 1982). (6) The integrity of a cord serotonin is critical for the expression of front paw FSIA (Watkins et al. 1984a). (7) Front paw FSIA is blocked by small systemic or intrathecal doses of the peptide CCK-8 (Faris ef al. 1983) and potentiated by the putative CCK antagonists, fofimiide and benzotript (Watkins et al. Im (see section below on CCK for a more detailed discussion of this point). Hind paw FSIA is also a CNS-mediated phenomenon (Watkins ef al. 1982c). However, this manipulation activates both intraspinal and supraspinal pain inhibitory systems (Watkins ef al. 1982a). The brain centers for hind paw FSIA differ from those for front paw FSIA since NRA lesions do not eliminate the analgesia (Warns et al. 1983a). The neurochemical bases of hind paw FSIA also differ from front paw FSIA: (1) CCK, serotonin, and norepinephrine do not appear to be involved in hind paw FSIA (Watkins et al. 1984a). (2) Brain, but not spinal cord, acetylcholine is necessary for the expression of hind paw FSIA but does not appear to be involved in front paw FSIA (Watkins ef al. 1984c). Of considerable interest is that both hind paw and front paw FSIA can be classically conditioned by repeated pairings of a CS with footshock (Watkins et al. 1982b). Regardless of whether on or front paw shock is used as the UCS, an opiate analgesia system in many ways similar to the one involved in front paw FSIA is activated, since conditioned analgesia is eliminated by (1) systemic and intrathecal naloxone, (2) morphine tolerance, (3) DLF lesions, and (4) NRA lesions and is unaffected by hypophysectomy, adrenalectomy, and sympathetic blockade (Watkins ef al. 1982c¢). In addition, as would be expected, higher structures are involved in the conditioned analgesia since it is eliminated by decerebration and reduced by periaqueduc- tal gray (PAG) lesions (Watkins ef al. 1983b). 127 & ROSTRAL 3 [cenvEns [yn A PBA — MEDULLA MEDULLA L_¢| (NRA) (NRA, other | P—1 nuclei) DLE DLF NONDLF | SO DORSAL HORN — Figure 1. Neural circuitry 9 opiate and nonopiate analgesia induced by front paw and hind paw shock. Front paw shock activates the nucleus raphe alatus (NRA) within the ventral medulla. This nucleus sends a descending projection through the DLF to the dorsal horn of the spinal cord. A serotonergic pathway lying outside of the DLF (non-DLF) is recruited as well. In turn, endogenous opioids are released, inhibiting pain transmission neurons (PTN). Activation of endogenous opiates stimulates a negative feedback loop, which utilizes CCK to reduce activity of endogenous ns systems. Hind paw shock inhibits PTN via two nonopioid pathways: an intraspinal pathway and a descending DLF pathway. The latter originates from the NRA and from some other yet unidentified medullary area(s). Classically conditioned (opioid) analgesia seems to result from activation of the same DLF output pathway as front paw (opioid) FSIA. After conditioning trials in which the conditioned stimulus is paired with either front paw or hind paw shock (the unconditioned stimulus), the condi- tioned stimulus becomes capable of activating rostral centers in the brain which, in turn, activate the periaqueductal gray (PAG) and subsequently the nucleus raphe alatus. This results, via a descending DLF pathway, in the release of endogenous opioids within the dorsal horn, producing analgesia. 128 A circuit diagram of these systems is shown in figure 1. A point that should be emphasized is that the involvement of other neurotransmitters or neuromodulators at the spinal cord level may be quite complex. For ex- ample, as shown in figure 1 and discussed in detail below, cholecystokinin cE appears to modulate endogenous opioid systems. Intrathecal application of CCK antagonizes an festa from application of exogenous opigles as well as analgesia elicited by activation of endogenous opiates (Faris et al. 1983). Also, CCK antagonists applied intrathecally potentiate these analgesias as well as reversing opiate tolerance { Wats et al. 1984b). These findings suggest that other transmitters and/or modulators may interact with opiates to form complex circuits. In addition to the work done by Liebeskind’s group [see Terman ef al. (1984) for a review] and our own, a number of other laboratories have now demonstrated that numerous environmental variables can be critical in determining the particular pain modulatory circuitry activated. Table 1 summarizes the environmental events now known to influence the transmis- sion of pain utilizing endogenous opioid peptides. It is clear that numerous environmental manipulations result in modulation of pain transmission. The involvement of 2 opioids in pain modulation is now beyond question. On the other hand, many questions remain unanswered. For example, it is generally not known where a particular endogenous opioid is released by a particular environmental manipulation nor is the endogenous ligand or the receptor type involved usually known. Nevertheless, the techniques and general strategies for answering these questions are available, and progress in this area should be forthcoming. It should also be pointed out that, in addition to systems that modulated nociceptive information utilizing endogenous opioids, there are nonopiate systems as well. For example, Maier’s group has shown that inescapable tail shock results in opiate analgesia, but analgesia resulting from tail shocks with identical temporal and intensity characteristics is nonopiate if the shocks are escapable (Maier ef al. 1982). In sum, a review of the animal data provides strong evidence for the existence of multiple pain modulatory systems. Our knowledge of endogenous Opiate analgesia systems probably represents the most detailed description of any opioid behavioral system available. It is, however, less clear what the critical characteristics of the environmental stimuli activating these systems are. Although many of the events activating the systems are clearly stressful, not all are. Also, a number of known stressors are ineffective. Evidence for Endogenous Opiate Analgesia in Man At this point, some parallels will be made between the work described above and experimental and clinical studies in humans. This will be done in order to highlight the potential relevance of this work to the very difficult problem of treating pain syndromes in man. Throughout this discussion, it will be important to bear in mind that a number of distinct modulatory systems have been identified under controlled laboratory conditions. In the more naturalistic circumstances of clinical research, it is likely that more than one of these systems may be active at any given time, which may account for the variability and controversy in the clinical literature. Research on the involvement of endogenous opioids in pain modulation in 129 man has examined a number of environmental manipulations known to have some degree of efficacy for the reduction of clinical and experimental pain. Most of these procedures were developed before the recent explosion of information about endogenous pain control systems. Indeed, many of them evolved from theoretical approaches that are now outdated or incorrect. Nevertheless, the procedures are efficacious and have inspired a considerable body of research aimed at determining the involvement of endogenous opioids in pain modulation. There are at least two situations available for study in which endogenous pain modulatory systems may be active in man. The first involves the basal, tonic activity within these systems and allows the experimenter to assess whether pain inhibition occurs continuously, at least to some degree. The second involves clinical manipulations that attempt to activate pain inhibitory systems. Attempts have been made to determine whether pain modulatory systems are tonically active. The assumption made by these studies has been that administration of opiate antagonists should alter the perception of pain if opiate systems are tonically active. This change in pain perception would be recorded either as a decreased pain threshold or an increased level of ongoing pain. In general, naloxone has failed to affect pain thresholds of normal human volunteers (Grevert ef al. 1978; El-Sobky et al. 1976). On the other hand, Buchsbaum et al. (1977) found that naloxone lowered the thresholds of fiblects with naturally high pain thresholds, yet had no effect in subjects with low pain thresholds. This observation is consistent with reports that the high pain thresholds seen in some cases of congenital insensitivity to pain can be lowered by naloxone (Cesselin ef al. 1984; Dehan et al. 1977; Dehen et al. 1978). It should be pointed out that demonstrating analgesic or hyperalgesic effects of drugs in human subjects is difficult. These studies, taken together, suggest that endogenous opjcte pain modula- tory circuits may not always be tonically active in people. Such a conclusion is supported by the report that naloxone decreases the higher pain thresholds seen in man in the morning as compared with those in the afternoon (Davis et al. 1978). Naloxone appears to be more consistently effective when delivered to experimental subjects who are experiencing some level of clinical puis In this regard, these results are consistent with the animal studies described above in which pain was observed to be a powerful activator of endogenous analgesia systems. Thus, Lasagna (1965), Levine ef al. (1979), and Gracely et al. (1983) report that naloxone can increase the reported intensity of Dosionariive pain. It is important to note that two of these studies reported complex dose-response interactions between naloxone and pain. Levine et al. found that while naloxone produced hyperalgesia at high doses, low doses produced analgesia. The Lasagna study is somewhat more difficult to interpret because no placebo control group was included, but the results are consistent with a conclusion that naloxone has both analgesic and hyperal- Josie effects. These reports, in turn, are consistent with reports in the animal iterature (Girardot and Holloway 1984a; Grau 1984; Mcgivern et al. 1983) indicating that certain environmental manipulations produce hyperalgesia as well as analgesia, and some of these "hyperalgesia systems" may be opiate in nature since the hyperalgesia can sometimes be antagonized by naloxone. This is a complex but important observation because it indicates that studies 130 of the effects of naloxone on pain levels must be interpreted with extreme caution. In conclusion, it appears that, under normal circumstances, endo- genous opiate pain inhibitory systems have little spontaneous activity. owever, when some level of pain is present, these systems seem to be activated. A second line of research on the involvement of endogenous opioids in pain modulation in man has examined a number of environmental manipulations known to have some degree of efficacy for the reduction of clinical and experimental pain. This research has utilized two primary experimental strat- egies. The first reasons that if a particular environmental manipulation induces analgesia by utilizing endogenous opioids, that analgesia should be antagonized by a narcotic antagonist (usually naloxone). The second strate reasons that if endogenous opioids are involved in an environmentally elicited analgesia, then changes should be observed in the levels of these compounds in plasma or the central nervous system. Stimulation-produced analgesia in man Perhaps the most dramatic outcome of the basic science research on endogenous opioids has been the rapid and effective clinical application to the treatment of chronic pain syndromes in man. As early as 1973, Richardson and Akil (1977) reported the use of periventricular gray stimulation to treat pain syndromes. Since then there have been more than 20 reports in the literature describing various studies of this technique. In a recent review of this literature Young et al. (1984) conclude that "the 7sthiod is reasonably effective in properly selected patients and, importantly, safe." Several lines of evidence indicate a likely but not unequivocal role for endogenous opiates in stimulation produced analgesia (SPA) in man. Table 2 summarizes the evidence for the involvement of endogenous opioids in SPA in man. Opiate antagonists are Fopored to reduce SPA, tolerance develops to SPA, and dependence upon SPA has been reported. A more controversial literature exists with regard to the release of endogenous opi- oids, primarily Beta-endorphin, by electrical stimulation of the periaqueduc- tal gray matter in man. It can be seen from table 2 that generally increased levels of endogenous opioids have been found to result from this stimula- tion. However, the possibility that these results are due to an artifact of using a contrast medium for electrode placement has been raised (Dionne et al. 1984; Fessler et al. 1984). This criticism has been convincingly disputed for at least for some circumstances (Akil and Richardson 1985), At this point, it seems likely that endogenous opioids mediate, at least in part, the analgesia elicited by periaqueductal gray stimulation in man. The particular sad icy opioid and its site wr mechanism of action have not been established. Counter-irritation analgesia in man The belief that an acute painful stimulus can be used to alleviate ongoing pain has been held since antiquity and is known as counter- irritation. This procedure has a great deal in common with acupuncture and TNS. All use the 2PDliganion of somatic stimuli, either noxious or innocuous, to obtain relief from pain. The site of treatment in relation to the painful area is 131 highly variable, ranging from the painful dermatome itself to a theoretically unpredictable constellation of points in classical Chinese acupuncture. Lastly, the duration of treatment varies from less than a minute to hours. All of these factors, as we have seen, are important determinants of the effects produced by footshock in animals. Thus, the highly variable effects observed in the clinic would be predicted from animal research. Nevertheless, human data suggest the involvement of the same systems described above. TABLE 2 EVIDENCE FOR THE INVOLVEMENT OF OPIOID PEPTIDES IN STIMULATION-PRODUCED ANALGESIA IN MAN NALOXONE TOL/DEP ENDORPHIN LEVELS B-ENDORPHIN ENKEPHALIN PLASMA CSF PLASMA CSF 4< 15 2> 5> 4> 10< 14 6= 3> 13< 8 7= 11> 1< 12 9> 15< REFERENCES FOR TABLE 2 1. Adams 1976 9. Hosobuchi 1981 2. Akil and Richardson 1985 10. Hosobuchi et al. 1977 3. AKkil ef al. 1978a 11. Hosobuchi et al. 1979 4. Akil et al. 1978b 12. Hosobuchi and Wemmer 1977 5. Amano ef al. 1980 13. Richardson and Akil 1977 6. Dionne et al. 1984 14. Schmidt et al. 1981 7. Fessler et al. 1984 15. Tsubokawa et al. 1984 8. Hosobuchi 1978 TABLE 2 - The effect of various opiate manipulations on analgesia and endorphin levels resulting from electrical stimulation of the brain. Symbols: "<" = attenuates analgesia; "=" = no effect on endorphin level; ">" = increases endorphin levels. Numbers in the table refer to numbered citations listed alphabetically below the table. Abbreviation: CSF = cerebrospinal fluid; TOL/DEP = tolerance or dependence. Twelve studies have measured the effect of naloxone on clinical or ex- perimental analgesia produced by pounce, Of these, eight reported that naloxone reduced the analgesia while four found no effect. In two of the studies failing to find a naloxone effect (Chapman et al. 1980, 1983) the negative erprgiarion of the results has been called into question (Miglecz and Szekely 1985; Mayer and Price 1981). The third of the four negative studies examined long-term effects of acupuncture on migraine headache (Lenhard and Waite 1983) and thus does not fit into the general paradigm of the other studies addressed here. The final pegaiive study (Kenyon ef al. 1983) utilized a dose of naloxone (0.4 mg.), which is on the low end of the 132 TABLE 3 EVIDENCE FOR THE INVOLVEMENT OF OPIOID PEPTIDES IN COUNTERIRRITATION ANALGESIA IN MAN A ACUPUNCTURE ANALGESIA NALOXONE ENDORPHIN LEVELS B-ENDORPHIN ENKEPHALIN PLASMA CSF PLASMA CSF 9)< < 24) = 6)> 13)> ©9)> - (x 2° &> © 12)= )< = 2 De 13)= )< (18)< 26)= 5= (@A7)< 16)> B TRANSCUTANEOUS NERVE STIMULATION NALOXONE B-ENDORPHIN LEVELS HI FREQ LOW FREQ HIGH FREQ LOW FREQ PLASMA CSF PLASMA = < 19 (D= 19)= 19: % a to)> 3 3: 20 2 22)< 22) = REFERENCES FOR TABLE 3 1. Boureau et al. 1979 16. Masala ef al. 1983 2. Casale et al. 1983 17. Mayer et al. 1977 3. Chapman 1978 18. Mayer et al. 1976 4. Chapman et al. 1983 19. O’Brien et al. 1984 . Pertovaara and Kemppainen 1981 Pertovaara ef al. 1 Sjolund and Eriksson 1979 . Sjolund et al. 1977 Szczudlik and Kwasucki 1984 Szczudlik and Lypka 1983 Szczudlik and Lypka 1983 5. Chapman ef al. 1980 6. Clement-Jones et al. 1980 7. Facchinetti ef al. 1984 8. Freeman et al. 1983 9. He and Dong 1983 10. Hughes et al. 1984 11. Johansson et al. 1980 12. Kenyon et al. 1983 Tsunoda ef al. 1 13. Kiser et al. 1983 . Umimo et al. 1984 14. Lenhard and Waite 1983 29. Willer et al. 1982b 15. Lundberg et al. 1985 TABLE 3 - The effect of various opiate manipulations on analgesia and endorphin levels resulting from transcutaneous nerve stimulation and acupunc- ture. Symbols: "<" = attenuates analgesia or endorphin level; "=" = no effect on analgesia or endorphin level; ">" = increases endorphin levels. Numbers in the table refer to numbered references. Abbreviation: CSF = cerebrospinal fluid. BIRRRBRREE range of effective doses. Thus, it seems clear that naloxone, at least under most circumstances, appears to antagonize acupuncture analgesia. 133 Table 3-A summarizes the studies that have examined the effect of naloxone on "acupuncture" analgesia as well as those studies which have measured "acupuncture-induced changes in plasma or CSF Beta-endorphin or enkephalin levels. It is important to note that "acupuncture" is not a well-defined procedure. The only criterion for including a study in this table was that the authors call the procedure "acupuncture." Many of the procedures discussed below under transcutaneous electrical nerve stimula- tion (TNS) are similar or identical to those defined as "acupuncture" here. The effects of acupuncture on CSF and plasma endorphin levels present a somewhat less consistent picture, but this is not surprising considering the complexities of these Byes of data. Considering that one could question the entire concept of plasma endorphin levels, since they are indicative of CNS level in only very indirect ways, a nevertheless somewhat consistent picture emerges. As can be seen in table 3-A, five studies have reported endorphin increases while six have reported no effects. Such results should be interpreted with extreme caution since (1) the meaning of increases in lasma endorphin levels are entirely unclear, and (2) even CSF endorphin evels are likely to be ambiguous since the site of endorphin release probably varies with the particular type of acupuncture stimulation. Nevertheless, an overview of these data is consistent with an involvement of endogenous opioids in at least some forms of acupuncture analgesia. The literature concerning the involvement of endogenous opioids in TNS analgesia is considerably more complex than that associated with acupunc- ture analgesia. This is likely to result from a JEroqer variability in the intensity, frequency, duration, location, and other parameters of TNS. Despite this diversity in experimental paradigm, some general consistencies are apparent in the literature. While only 4 of 13 studies of TNS analgesia have reported naloxone antagonism, all 4 studies utilized lows {Fequiney TNS. On the other hand, none of 6 studies utilizing high-frequency TN found a naloxone antagonism (see table 3-B for references). The effects of TNS on endorphin levels have been less well studied. As seen in table 3-B, 3 of the 6 reported studies have found an increase in endorphin levels, while the remainder have found no effects. Such results should be interpreted with the caveats discussed above in mind. Overall, these results are strikingly consistent with Feposis in the animal literature (e.g., Han et al. 1984) and suggest the possibility that certain types of sensory stimulation either inactivate opiate systems or activate opiate hyperalgesia systems as discussed above. Nevertheless, these results are consistent with an emerging picture that low-frequency, high-intensity acupuncture-like TNS (cf. Sjolund and Eriksson 197) invokes endogenous opioid mechanisms. Such studies, taken together, probably provide the most convincing evidence available that endogenous opioids can function to modulate pain transmission in man. In conclusion, acupuncture and transcutaneous nerve stimulation appear to be forms of counterirritation that activate both opiate and nonopiate systems. The variable clinical outcomes observed following these treatments probably result from differential recruitment of segmental, extrasegmental, opiate, and nonopiate pain inhibitory systems, all of which are now known to be activated by these types of stimulation in animals. Stress analgesia in man A manipulation related to, but not identical with, counterirritation analgesia is a phenomenon most generally referred to as "stress analgesia." This issue 134 was discussed above in relation to animal studies, and similar caveats should be taken under consideration in human studies. These studies have utilized environmental manipulations tht are either severe physical or psychological stressors. The stressors catalogued in this section include surgery, labor and childbirth, application of overtly painful stimuli such as cold pressor pain or ischemic pain, chronic pain, anticipation of pain, and chronic stressful states such as life threatening disease. TABLE 4 EVIDENCE FOR THE INVOLVEMENT OF OPIOID PEPTIDES IN STRESS ANALGESIA IN MAN NALOXONE ENDORPHIN LEVELS B-ENDORPHIN ENKEPHALIN PLASMA CSF PLASMA CSF 6) < 8) > D> (11) = 12) < 3 < 3 > @) 11 13 < 15) < 1) > 5. =< 1) > 14) < 2) > 13) < 4) < REFERENCES FOR TABLE 4 1. Atkinson et al 1983 9. Pertovaara ef al. 1982a 2. Cohen et al. 1982 10. Puig et al. 1982 3. Delke et al. 1985 11. Smith et al. 1985 4. Frid and Singer 1979 12. Szczudlik and Lypka 1983 S. Frid et al. 1981 13. Willer and Albe-Fessard 1980 6. Jungkinz ef al. 1983 14. Willer ef al. 1981 7. Katz et al. 1982 15. Willer et al. 1982a 8. Pancheri et al. 1985 TABLE 4 - The effect of various opiate manipulations on analgesia and endorphin levels resulting from stress. Symbols: "<" = attenuates analgesia or endorphin level; "=" = no effect on analgesia or endorphin level; ">" = increases endorphin levels. Numbers in the table refer to numbered citations listed alphabetically below the table. Abbreviation: CSF = cerebrospinal fluid. Examination of table 4 reveals a strikingly consistent outcome for studies of this sort. It can be seen that in eight of eight studies in which a "stressful" manipulation increased nociceptive thresholds, naloxone at least partially reversed this increase. Another study (Janal er al. 1984) utilized vigorous exercise, at least a possible stressor, to increase pain threshold and also showed naloxone reversibility. In addition, and not surprisingly, since beta-endorphin is coreleased with ACTH, stress resulted in an increase in plasma beta-endorphin levels in five of five studies. Although such a result is not convincing alone, it is certainly consistent with the notion that endogenous opioids may underlie changes in pain threshold produced by stress. In addition, such results are consistent with the results of counterir- ritation studies discussed above with respect to the observation that naloxone 135 peversiiiny is more likely to occur with high intensity peripheral stimulation (see table 3). In conclusion, considering the diversify of procedures used in counterirritation studies and stress studies, a generally convincing picture of opioid involvement in pain modulation in man emerges. Many important questions about the nature of this involvement remain RnB The most important of these are the particular endogenous opiate involved and its site of action. Answers to such questions are unlikely to come from human studies, since invasive procedures are probably necessary to acquire such information. The consistency of the animal and human studies, however, indicates the likelihood that such questions may be studied with animal models and verified in man. Placebo analgesia in man A placebo manipulation may well be considered a form of stress, at least under some circumstances. Naloxone has also been used to examine whether endogenous opiates are involved in placebo analgesia. Levine and coworkers ( 1978) reported that naloxone antagonized placebo analgesia in postsurgical atients. Although this conclusion has been questioned on technical grounds {Goldstein and Grevert 1978; Kor 978; Skrabanek 1978), little conflicting data have been published. Gracely et al. (1983) have reported that naloxone results in an increase in pain levels experienced by post surgical patients that is independent of placebo effects. On the other hand, Levine and Gordon (1984), in a study that rectified the technical problems of their earlier one (Levine et al. 1978), found convincing evidence for at least a partial reversal of placebo analgesia by naloxone. A difficulty with all of these studies is that surgical stress itself is a powerful activator of endogenous opioid systems (see Bo0ve) and may influence the experimental results. A carefully controlled study utilizing experimentally induced ischemic pain (Grevert et al. 1983) indicates that a partial antagonism of placebo analgesia can occur in the absence of any effects of naloxone on baseline pain responsivity. At this point, it seems most likely that endogenous opioids mediate at least some components of Ploesha analgesia. It should be kept in mind, however, that placebos, like other analgesic manipulations discussed above, are multidimensional manipulations likely to activate multiple pain inhibitory and possibly pain facilitatory systems. Thus, i a manipula- tion that has at least a superficial resemblance to placebo procedures, consistently has failed to be antagonized by naloxone (Barber and Mayer 1977; Goldstein and Hilgard 1975; Mayer et al. 1976; Spiegel and Albert 1983). The possibility that opiates are involved in some aspect of placebo analgesia appears particularly reasonable considering the fact that footshock analgesia can be classically conditioned in rats. Placebo analgesia can easily be conceived of as a classical conditioning paradigm wherein the placebo manipulation (e.g., injections, pills) serves as the conditioned stimulus and prior medication or treatment serves as the unconditioned stimulus. The observation by Grevert et al. (1983) that placebo effects tend to extinguish with repeated trials supports such a conceptualization. Although explanations of this sort are clearly speculative, they are indicative of the wealth of concepts from rial ain research now available for clinical evaluation. Our increasing knowledge of pain modulatory systems has the potential not only of providing explanations of current therapies but of suggesting new approaches for the control of pain. The preponderance of current pain therapies involve either the surgical destruction of neural tissue or the use of addictive drugs. Such procedures offer great difficulties for the prolonged treatment of chronic pain. If multiple pain inhibitory systems 136 could be activated pharmacologically or otherwise in an alternating sequence, the problems of tissue destruction and addiction could be circumvented. OTHER PEPTIDES In addition to the endogenous opioids. other peptides have been reported to be involved in endogenous analgesia-producing mechanisms in various ways. Thus, neurotensin and substance P produce analgesia upon central ad- ministration by themselves; CCK, on the other hand, has been demonstrated to modulate analgesia produced by other manipulations. Substance P In addition to the numerous papers that have proposed substance P (SP) as a transmitter of primary afferent neurons in the spinal cord and medulla, it has been demonstrated that SP possesses analgesic properties, as well. Systemic and intracerebroventricular (ICV) administration of SP produce analgesia in mice (Stewart ef al. 1976; Starr et al. 1978; Hall and Stewart 1983a; Meszaros ef al. 1981; Oehme ef al. 1980) and in rats following both systemic (Mohrland and Gebhart 1979) and ICV (Malick and Goldstein 1978; Meszaros ef al. 1981) injections. It should be noted that this analgesic effect when compared with that produced by opiates is very small (Frederickson et al. 1978; Frederickson — Gesellchen 1980) and has failed to be observed at all, perenay following systemic administration, by others (Goldstein and 550 1979; Growcott and Shaw 1979; Hayes and Tyers 1979; Inoki et al. The analgesic action of SP is antagonized oy naloxone (Frederickson ef al. 1978; Frederickson and Gesellchen 1980; Malick and Goldstein 1978; Stewart et al. 1976). Since SP does not bind to opiate receptors (Terenius 1975; Szreniawsky et al. 1980) SP Appareil releases opioid peptides. Both the eriaqueductal central gray (PAG) and the spinal cord are likely substrates or this SP effect because (1) SP has been demonstrated to produce analgesia both after administration into the PAG (Mohrland and Gebhart 1979 and following intrathecal administration (Doi and Jurna 1981, 1953 (2) SP causes a release of opioid peptides in both the PAG (del Rio ef al. 1983) and the spinal cord (Tang ef al. 1983), and (3) tolerance to and opiate cross-toler- ance with the analgesic action of SP has been demonstrated following intraventricular injections (Naranjo et al. 1984). The apparent paradox that intrathecal injection of SP may induce both analgesia and "hyperalgesia" (Akerman et al 1982; Lembeck ef al 1981; Matsumura ef al. 1985; Yoshpel and Henry 1983; Yasphal ef al. 1982) [but see Piercey et al. (1981) for absence of any change in nociceptive threshold] has been partially resolved by Yashpal and coworkers. They showed that the SP-induced analgesia occurs after 10-15 min, when "hyperalgesia" disappears. Although these findings are consistent with results of others, they are in conflict with those obtained by Han ef al. (1984). The latter administered SP antibodies into the PAG and intrathecally prior to inducing electroacupunc- ture analgesia. Whereas the SP antibodies reduced electroacupuncture analgesia following intracerebral administration, confirming the importance of the analgesic effects of SP at this site in this behavior, they potentiated SlsquoumNAcHITS analgesia upon intrathecal administration. In view of the fact that the hyperalgesic effects of SP have been shown to be generall short-lived [up to 10 minutes (Yashpal and Henry 1983; Yasphal et al. 1982)], 137 while the analgesic effect has lasted in some studies for over 30 minutes (e.g. Doi and Jurna 1981, 1982b; Yashpal and Henry, 1983), the predominant hyperalgesic action of spinal SP on electroacupuncture is surprising. Although the analgesic effect of SP has been reliably observed and its mechanism understood, the very existence of SP-induced analgesia remains enigmatic. First, it seems to pagale a role for SP as a transmitter of pain, as the analgesic effects clearly abolish its presumably algesic ones. Second, since it has been proposed that the presumed hyperalgesia results from spinal convulsive-like excitation (Bossut ef al. 1986), the physiological relevance of the analgesic action is to be doubted. Neurotensin NT has been administered to mouse and rat via three different routes: intracerebroventricularly (ICV), intracisternally (IC), and intrathecally (IT). As NT affected the pain threshold in a different way depending on the route of administration, - literature is reviewed accordingly. IC administration. The analgesic effect of NT has been observed in mice (Clneschpiys and McGuffin 1977) and rats {Ouneschiids et al. 1979). ereas NT analgesia in mice was dose-related and could be observed on the hot plate test, writhing test (Clineschmidt and McGuffin 1977; Davis et al. 1983; Osbahr ef al. 1981), and tail immersion test (Nemeroff et al. 1979), it could be demonstrated only on the hot plate test and not on the tail-flick test in rats (Clineschmidt et al. 1979). Naloxone (1-5 mg/kg) failed to antagonize NT-induced analgesia in both species (Clineschmidt and McGuffin 1977; Clineschmidt et al. 1979; Osbahr et al. 1981); however, the observation that repeated pretreatment with morphine reduced the analgesic effect of NT (Luttinger et al. 1983) could be viewed as cross-tolerance, thus suggesting some involvement of opiate mechanisms. NT analgesia is reduced by thyrotropin releasing hormone (Osbahr et al 1981) and its structural analogs (Hernandez ef al. 1984). The mechanism of this antagonism is, as yet, not fully understood. IT administration. The behavioral effects of a drug injected IC may be caused at both spinal and supraspinal sites of action. One way to test heifer spinal sites are involved in NT-induced analgesia is administering the drug IT. The results of IT administration of NT are somewhat confusing. In rats NT in doses up to 90 micrograms [3,000 times the dose producing hot plate analgesia in this species following IC administration rh et al 1979)], failed to produce hot plate analgesia when administered IT (Clineschmidt et al. 1982; Martin and Naruse 1982). These results seem to indicate that the site of action for NT-induced gesia is supraspinal. However, Yaksh et al. (1982) reported that doses of 1-100 micrograms of neurotensin injected IT produced analgesia on the hot plate, and even some analgesia on the tail flick test. Moreover, this group reported that this analgesia was fully reversible by naloxone (10 or 15 mg/kg). Consistent with this report are the finding that IT-administered NT produced naloxone (2 mg/kg) reversible analgesia in the mouse Hylgen and Wilcox 1983). However, this analgesia was not observed on the tail flick reflex but rather on aversive behavior following intraperitoneal administration of acetic acid. 138 ICV administration. When NT is administered ICV to mice, it readily roduces analgesia on the writhing test, and this analgesia is not reversible Ph naloxone (5 mg/kg) (Nicolaides et al. 1985). However, results obtained in the rat are more equivocal. Thus, while 20 micrograms of NT ICV in the latter species induced analgesia in one study (Martin ef al. 1981), 5 micro- grams did not in others (Kalivas et al. 1982; Parolaro et al. 1983). Although these observations seem consistent with the view that these negative findings result from an insufficient dose of NT, hot plate analgesia from the cisterna Jogha was reported following 25 ng of NT (Clineschmidt and McGuffin 1977). It seems, therefore, hardly likely that the anatomical substrate for NT analgesia is located in the immediate vicinity of the lateral ventricles; structures in the brainstem in the immediate proximity of the cisterna seem better candidates. This conclusion was not confirmed by a mapping study, in which both periventricular structures (medial preoptic area, amygdala), mesencephalic (rostral periventricular gray), and rhombencephalic (medial ars of the reticular formation) were equally effective injection sites for inducing hot plate analgesia with NT in rats ore et al. 1982). Conclusion. NT undoubtedly has analgesic properties, but neither its mechanism nor its site of action are understood. Thus, it is possible that NT induces analgesia upon IT administration by releasing endogenous opioids. This would Sola some of the results using this Jrasien (Hylden and Wilcox 1983; Yaksh ef al. 1982) but not the lack of analgesia obtained by others (Clineschmidt ef al. 1982; Martin and Naruse 1982) The increase in latency to response 2pgned from discrete injection of NT into supraspinal areas (Kalivas ef al. 1982) may well reflect true analgesia in some cases, but not all. Thus, although it is not known whether NT excites neurons in pala or PAG upon iontophoretic application, in view of its effects in spinal cord and cortex this is a likely possibility. If NT causes general neuronal excitation, it could well cause analgesia in the PAG, as do electrical stimulation (Mayer et al 1971) and injection of glutamate Behbehani and Fields 1978; Urca et al. 1980). Also, electrical stimulation Abbott and Melzack 1978) and morphine (Rodgers 1977, 1978; VanRee 977) in forebrain produce analgesia. Further work is needed in order to decide these issues. CCK The earliest experiments with CCK in systemic doses of over 50 micro- grams/kg in the mouse (Zetler 1980, 1983) and intracerebral or intrathecal doses of 10-40 ng in the rat (Jurna and Zetler 1981) demonstrated the analgesic potential of this peptide. The observation that this analgesia was reversible by naloxone made these authors Suggest that it was mediated by gudopsnons opioids. However, at these and higher doses it failed, unlike morphine, to depress ascending A-delta and C fiber activation (Doi and Jurna 1982a), suggesting a different mode or site of action. More recent experiments indicate that lower doses of CCK, although playing a role in opiate analgesia, have effects opposite to the one initially de- scribed. Thus, 3 micrograms/kg of systemic and 3.6 ng of intrathecal CCK Smagonies the analgesia produced by morphine and opiate mediated foot shock analgesia (aris et al. 1983). Similar effects were observed by others (Itoh ef al. 1985; Han et al. 1985). The antagonistic effect of CCK follows an inverted "U" dose response curve with doses lower and higher than the aforementioned producing less effect. 139 Subsequent work with proglumide, a CCK antagonist, showed that this compound, after both systemic and intrathecal administration, significantly porated analgesia induced by morphine, endogenous opioids, and various ehavioral manipulations that release endogenous opioids in rats (Watkins et al. 1984b, 1985; Tang et al. 1984). Another CCK antagonist, benzotript, has similar effects. Also, morphine analgesia in rats immunized against CCK is potentiated (Faris 1985). Proglumide (Suberg et al 1984) or CCK antibodies (Suberg ef al. 1985) potentiate the morphine induced, naloxone reversible suppression of nociceptive spinal cord dorsal horn neurons indicating that the interaction between CCK and morphine occurs at the same site. The antagonist action of CCK on opiate action and proglumide’s potentia- tion seems not to be limited to analgesia. Itoh and Katsuura (1981) found that CCK significantly reduced the duration of catalepsy following in- traventricularly injected beta-endorphin in rats, whereas proglumide poten- tiated it (Itoh et al. 1985; Katsuura and Itoh 1985). Similarly, proglumide was found to potentiate morphine’s effect on open field motility in the rat (Ben-Horin ef al. 1984). The interaction between CCK and opiate action has some very interesting clinical implications. Thus, it has been demonstrated in rats that proglum- ide prevents or reduces tolerance induced by repeated morphine administra- tion (Watkins et al. 1984b; Tang et al. 1984). Together with the recent demonstration that proglumide potentiates morphine analgesia in humans as well (Price et 21.1985), these findings promise new perspectives both for the use of opiates in treating pain and for treating opiate addicts. 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Zamir, N.; Simantov, R.; and Segal, M. Pain sensitivity and opioid activity in genetically and experimentally hypertensive rats. Brain Res 184:299- 310, 1980. Zetler, G. Analgesia and ptosis caused by caerulein and cholecystokinin octapeptide (CCK-8). Neuropharmacology 19:415-422, 1980. Zetler, G. Cholecystokinin (CCK): Ascension from gut to brain - behavioral pharmacology of CCK and analogs. Psychopharmacol Bull 19:347-351, 1983. Zorman, G.; Belcher, G.; Adams, J.E.; and Fields, HL. Lumbar intrathecal naloxone blocks analgesia produced by microstimulation of the ventromedial medulla in the rat. Brain Res 236:77-89, 1982. ACKNOWLEDGMENT Portions of the work reported in this chapter were supported by P.H.S. Grant DA-00576. AUTHOR David J. Mayer, Ph.D. Department of Physiology Medical College of Virginia Virginia Commonwealth University Richmond, Virginia 23298, U.S.A. 156 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D., eds. National Institute on Drug Abuse, 1988 Mechanism of Development of Tolerance and Dependence to Opioids in Neuroblastoma x Glioma Hybrid Cells and Mice Shail K. Sharma, Ph.D.; Madhav Bhatia, M.Sc.; and Ranju Ralhan, Ph.D. Neuroblastoma x glioma (NG108-15) hybrid cells are enriched with opioid receptors (Klee and Nirenberg 1974; Chang and Cuatrecasas 1979). In these cells opiates and opioid peptides regulate the synthesis of cyclic AMP at two different levels. A rapid receptor- mediated inhibition of adenylate cyclase is followed by a delayed and long-lived compensatory increase in its activity. It has been suggested that the latter effect may be responsible for narcotic dependence and tolerance (Sharma et al. 1975a,b 1977; Traber et al. 1975; Lampert et al. 1976). Ascorbic acid suppresses the etorphine-induced compensatory increase in the levels of cAMP with Tittle or no effect on the short- term response of NG108-15 hybrid cells to the effector agents (Sharma and Khanna 1982). These studies suggest that ascorbic acid may play a role in the prevention of the development of tolerance in therapeutic applications of narcotics as analgesics, The mechanism by which ascorbic acid prevents the development of tolerance to opiates is still obscure, Effect of Ascorbate on Etor hine-Induced z in Cyclic AMP Levels p ed Alterations Results reported earlier from this laboratory show that ascorbic acid suppresses the etorphi i y phine-induced compensatory increase in the levels of cAMP in NG108- 15 hybrid cells (Sharma and Khanna 1982) interest to study the i ascorbate concentration on etorphine-induced 157 compensatory increase in basal and PGE;-stimulated cAMP levels. Results in tl show that in the absence of ascorbate, etorphine led to a compensatory increase of 80 percent in the basal and 65 percent in the PGE;-stimulated cAMP levels. A progressive decrease in the compensatory response is seen as the concentration of ascorbate is raised to 10mM. Initially, at lower concentrations of ascorbate the decrease is more pronounced for PGE;-stimulated cAMP levels. Preexposure of NG108-15 hybrid cells to ascorbate did not abolish stimulatory or inhibitory effects of drugs on cAMP levels (Sharma and Khanna 1982), indicating that receptors for opiates and PGE; were functionally coupled to adenylate cyclase. The effect of preincubation of NG108-15 hybrid cells with ascorbate on etorphine-induced compensatory increase in the levels of cAMP was studied. In this experiment cells were preexposed to ascorbate for 4 hours. After washing, the second incubation was with and without etorphine for an additional 4 hours. The monolayer cultures were washed free of ascorbate and used to determine basal and PGE;-stimulated cAMP levels as in tl. Results in t2 show lnat etorphine-induced basal and PGE,-stimulated compensatory increase in cAMP levels observed is of the same order of magnitude in the cells preincubated with or without ascorbate. The data from tl and t2 clearly show that simultaneous presence of ascorbate and etorphine is necessary to suppress the etorphine-induced compensatory increase in basal and PGE,-stimulated cAMP levels. These studies have been carried out in a cultured cell line of neuronal origin. Therefore, we studied the effect of ascorbic acid on development of tolerance and dependence in vivo in mice. The in vivo effects of ascorbate on morphine-induced analgesia, physical dependence, and tolerance were studied, In mice ascorbate, when administered along with morphine, suppresses the development of tolerance and physical dependence on the drug, without significantly affecting its analgesic properties. Mice receiving morphine along with ascorbate became less tolerant to and dependent on the drug. The duration of ‘morphine-induced analgesia, however, is progressively reduced with an increase in the amount of ascorbate. However, ascorbate does not alter the intensity of morphine-induced analgesia (Khanna and Sharma 1983). Ascorbate at 1g/kg body weight did not alter the pH of blood and did not have an effect on the levels of lipid-peroxides in blood and brain, These results suggest that action of ascorbate is not mediated by its oxidation and lipid peroxide formation. 158 TABLE 1 Suppression of opiate-induced compensatory increase in c-AMP levels by ascorbate NG108-15 hybrid cells (1.2 x 106, passage 20) were plated in (Medium A) DMEM (Flow Labs U.K.) supplemented with 0.1 mM-hypoxanthine, 1yM- aminopterin, 16 uM-thymidine, and 10 percent of fetal bovine serum (Flow Labs) in 60 mm Falcon petri- dishes. When 60-80 percent confluent, the culture plates were divided in five groups: (i) control with no effector agents; (ii) etorphine (1.6 yM); (iii) etorphine 1.6 yM and sodium ascorbate (1 mM); (iv) etorphine 1.6 yM and sodium ascorbate (5 mM); (v) etorphine 1.6 4M and sodium ascorbate (10 mM). The cells were incubated for 4 hours at 37°C, washed with medium B [DMEM with 25 mM Hepes (4-(2-hydroxyethyl)- l-piperazine-ethanesul fonic acid)]. Incubations were carried out in 3 ml of medium B with 0.5 mM Ro20-1724 [4-(3-butoxy-4-methoxybenzyl) imidazolidine-2-one]. Amounts of intracellular levels of c-AMP were determined over a period of 15 minutes with and without PGE; (10 4M), by the method of Gilman (1970). Protein in each petri dish was estimated by the method of Lowry et al. (1951). Values are the average of three individual experiments (each experiment had four plates in a group). Additions during cell cAMP (Pmole/mg protein) growth for 4 h Basal PGE, - 328 3800 Etorphine 584 6263 Etorphine + ascorbate 1 mM 535 3954 Etorphine + ascorbate 5 mM 308 4400 Etorphine + ascorbate 10mM 192 3542 159 TABLE 2 Compensatory increase in cAMP levels after preincubation of cells with ascorbate NG108-15 hybrid cells (1.4x10%, passage 20) were plated in medium A in 60 mm petri dishes. When 60-80 percent confluent the culture plates were divided in two groups (eight plates in each group): (i) control with no effector agents; (ii) sodium-ascorbate (5mM). The cells were incubated for 4 hours at 37°C, washed with 4 x 3 ml medium A, and each set of culture plates was divided into two groups: (ia) control with no effector agents; (ib) etorphine 1.6 YM; (iia) control with no effector agents; (iib) etorphine 1.6 HM. Incubations were carried out in 4 ml medium A for 4 hours at 37°C and washed with medium B, 3m] medium B with 0.5 mM Ro20-1724 was added, and the plates were incubated in presence of naloxone with and without PGE; (10 yM) for 15 min. Intracellular cAMP levels were determined as in tl. Each value is the average of three individual experiments (each experiment had four plates in a group). Additions during cell growth cAMP (pmole/mg protein Preincubation 1 Preincubation 2 (4 h) (4 h) Basal PGE, - - 433+49 5821+254 - Etorphine 782436 8063+422 Ascorbate - 371419 52164397 Ascorbate Etorphine 679+42 7976+510 160 Mechanism of Ascorbate Action Ascorbic acid may exert its effect at the level either of binding of opiates to the receptor or of coupling of the receptor to other components of the adenylate cyclase system, i.e., inhibitory guanine nucleotide regulatory protein (Ni) and catalytic unit of adenylate cyclase. Effect of Ascorbate on (3H) Etorphine and (3H) DADLE Binding Effect of ascorbate on binding of (15,16-3H) etorphine to intact NG108-15 hybrid cells was studied as a function of ascorbate concentration. Ascorbate at 1 and 5 mM concentration inhibited the specific binding of etorphine by 28 percent and 56 percent (t3). Similar_effect of sodium ascorbate on D-Ala‘- (tyrosyl-3,5-3H) enkephalin (5-D-leucine) binding was observed. Specific binding was inhibited by 24 percent, 56 percent, and 68 percent, respectively, in the presence of 1 mM, 5 mM, and 10 mM ascorbate (t4). These studies are compatible with those of Dunlap et al. (1979). In order to ascertain that ascorbate does not destroy opiate receptors, NG108-15 hybrid cells in monolayer were preincubated yith 1 and 5 mM ascorbate, washed and assayed for (°H) etorphine binding. There was no significant change in specific (°H) etorphine binding in the cells preincubated with ascorbate as compared to that in controls (t5). These results show that ascorbic acid does not destroy opiate receptors. Effect of Ascorbate on GTPase Activity Klee et al. (1984) proposed that opiate inhibition of adenylate cyclase in NG108-15 hybrid cells is the direct result of stimulation of a low Km GTPase component associated with Ni protein of the adenylate cyclase complex. Adenylate cyclase shuttles between two states, an active one with bound GTP and an inactive one with bound GDP. Stimulatory receptors facilitate exchange of GTP for bound GDP, whereas inhibitory receptors (including opiate receptors) stimulate low Km GTPase activity, which converts GTP bound to the Ni complex to GDP (Ross and Gilman 1980; Katada and Ui 1979, 1982a,b; Koski et al. 1982). We have studied the short- and long-term effects of sodium ascorbate and etorphine on low Km GTPase activity and thus Ni in NG108-15 hybrid cells. Etorphine stimulates low Km GTPase activity of NG108- 15 hybrid cells by 54 percent. This acute stimulatory 161 effect of etorphine is reversed by opiate antagonist naloxone (t6). TABLE 3 Effect of sodium ascorbate on binding of (3H) etorphine to monolayer cultures of NG108-15 hybrid cells NG108-15 hybrid cells (2x10%, passage 20) were plated in medium A in 24 well Falcon culture plates. When 80 percent confluent, the wells were washed with medium B. Incubations wore carried out in 2 m1 of medium B containing 2 nM (15,16-°H) etorphine at 37°C in a water bath. Specific binding was determined by subtracting the nonspecific binding measured in the presence of 2.5 yM naloxone from total binding at each concentration of sodium ascorbate. Each value is the average of four individual determinations and is expressed as Mean + S.D. Addition (3H) etorphine binding CPM/mg protein None 750 + 101 Sodium ascorbate 0.1 mM 770 + 58 Sodium ascorbate 0.5 mM 697% 47 Sodium ascorbate 1.0 mM 537 + 56 Sodium ascorbate 5.0 mM 327 + = 20 162 TABLE 4 Effect of sodium ascorbate on binding of (3H) DADLE to monolayer cultures of NG108-15 hybrid cells Conditions of the experiment were the same ag in t3. Specific binding of 5nM D-Ala‘-(tyrosyl-3,5-"H) enkephalin (5-D-leucine) was measured. Addition (3H) DADLE binding CPM/mg protein None 295 + 14 Sodium ascorbate 1 mM 225 + 18 Sodium ascorbate 5 mM 131 + 11 Sodium ascorbate 10 mM 92 + 5 TABLE 5 Binding of (3H) etorphine to NG108-15 hybrid cells, preincubated with ascorbate NG108-15 hybrid cells were plated in 60 mm Falcon petri dishes as described in tl. When 60-80 percent confluent, the monolayer of cells was washed with 5 x 3 ml of medium B, and plates were divided in three sets: (i) control with no effector agents; (ii) sodium ascorbate (1 mM); (iii) sodium ascorbate 5mM. Incubations were carried out in3 ml of medium B, for 60 min at 37°C, washed with 5 x 3 ml of medium B, and jncubated in 3 m1 of medium B containing 2 nM (15,16- H) etorphine at 37°C in a water bath. Specific binding was determined as described in t3. Preincubation (3H) etorphine binding 60 min CPM/mg protein None 1085 + 134 Sodium ascorbate 1 mM 1243 + 78 Sodium ascorbate 5 mM 1153 + 133 163 TABLE 6 Effect of etorphine and sodium ascorbate on GTPase activity in membranes prepared from NG108-15 hybrid cells Membranes were prepared and used for GTPase assay as described by Koski and Klee (1981). All experimental conditions were the same except that membranes were collected by centrifugation at 48,000 g for 50 min. Concentration of effector agents were naloxone, 2.5 mM; etorphine, 1 uM; sodium ascorbate, 5 mM; PGE, 10 uM. Each value is the difference of GTPase activity obtained in the absence and presence of 50 yM GTP determined in triplicates and is expressed as Mean + S.D. Additions GTPase activity (+ PGE.) pmole of Pi formed/min)ng protein - 35.3 + 1.3 Naloxone 35.5 + 3.8 Etorphine 54.6 + 0.89 Etorphine + naloxone 33.5 + 1.1) These results are consistent with the earlier observations of Koski and Klee (1981) on opiate stimulation of low Km GTPase activity. Recently we have shown that NG108-15 hybrid cells grown with etorphine or ascorbic acid for 4 hours had decreased low Km GTPase activity. Inhibition of the low Km GTPase by ascorbic acid may be the mechanism by which ascorbic acid inhibits the etorphine-induced compensatory increase in cAMP formation (manuscript under preparation). 164 References Chang, K.J., and Cuatrecasas, P. Multiple opiate receptors-enkephalins and morphine bind to receptors of different specificity. J Biol Chem 254:2610-2618, 1979, Dunlap, C.E.; Leslie, F.M.; Rado, M.; and Cox, B.M. Ascorbate destruction of opiate stereospecific binding in guinea pig brain homogenate. Mol Pharmacol 16:105-119, 1979. Gilman, A.G. A protein binding assay for adenosine 3':5'-cyclic monophosphate. Proc Natl Acad Sci USA 67:305-312, 1970. Katada, T., and Ui, M, Islet-activating protein: Enhanced insulin secretion and cyclic AMP accumulation in pancreatic islets due to activation of native calcium ionophores. J Biol Chem 254:469- 479, 1979. Katada, T., and Ui, M. ADP-ribosylation of the specific membrane protein of C. cells by islet- activating protein associated with modification of adenylate cyclase activity. J Biol Chem 257:7210- 7216, 1982a. Katada, T., and Ui, M. Direct modification of the membrane adenylate cyclase system by islet- activating protein due to ADP-ribosylation of a membrane protein. Proc Natl Acad Sci USA 79:3129- 3133, 1982b, Khanna, N.C., and Sharma, S.K. Megadoses of vitamin C prevent the development of tolerance and physical dependence on morphine in mice. Life Sci 33:401-404, 1983. Klee, W.A., and Nirenberg, M. A neuroblastoma X glioma hybrid cell Tine with morphine receptors. 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Biochemical properties of hormone-sensitive adenylate cyclase. Annu Rev Biochem 49:533-564, 1980. Sharma, S.K.; Nirenberg, M.; and Klee, W.A. Morphine receptors as regulators of adenylate cyclase activity. Proc Natl Acad Sci USA 72:590-594, 1975a. Sharma, S.K.; Klee, W.A.; and Nirenberg, M. Dual regulation of adenylate cyclase accounts for narcotic dependence and tolerance. Proc Natl Acad Sci USA 72: 3092-3096, 1975b. Sharma, S.K.; Klee, W.A.; and Nirenberg, M. Opiate- dependent modulation of adenylate cyclase. Proc Natl Acad Sci USA 74:3365-3369, 1977. Sharma, S.K., and Khanna, N.C. Ascorbate suppresses the opiate-induced compensatory increase in cyclic AMP in neuroblastoma X glioma hybrid cells. Biochem J 208: 43-46, 1982. Traber, G.; Gullis, R.; and Hamprecht, B. Influence of opiates on the levels of adenosine 3':5' cyclic monophosphate in neuroblastoma X glioma hybrid cells, Life Sci 16:1863-1868, 1975. Acknowledgments This work is supported by grant No. 5/3-1 (8)-BMSII from Indian Council of Medical Research to Dr. Sharma. Mr. Bhatia is a recepient of the K.D. Birla Smarak Kosh Scholarship. Dr. Ralhan is a Lecturer in the Department of Biochemistry. Authors shail kr. Sharma, Ph.D. Madhav Bhatia, M.Sc. Ranju Ralhan, Ph.D. Department of Biochemistry All-India Institute of Medical Sciences New Delhi-110 029, India 166 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D., eds. National Institute on Drug Abuse, 1988 Development of Spinal Substrate for Nociception in Man Veena Bijlani, Ph.D.; Tilat A. Rizvi, M.Sc.; and S. Wadhwa, M.S. The dorsal horn of the spinal cord is the first site of interaction between primary afferents and intrinsic neurons. There is considerable evidence in literature about the existence of a variety of descending fibers taking part in the spinal neuronal circuitry. The small diameter nociceptive fibers have been shown to establish synaptic contacts with the neurons of lamina I, II, and 1II(Kerr 1975; Bishop 1980; Christensen and Perl 1970; Willis and Coggeshall 1978). Spino- thalamic tract neurons are dispersed in lamina I, IV, V, and VI (Trevino et al. 1978; Kerr 1975; Carsten and Trevino 1978). The small neurons of lamina II and III do not appear to project for long distances (Trevino and Carsten 1975). Kerr (1975) has suggested these to be inhibitory neurons. The precise under- standing of function of neuronal circuitry requires that the afferent and efferent synaptic connections and the transmitters of its constituent be identified. Studies were done on the dorsal gray of human fetal spinal cord ranging in age from 8 to 37 weeks of intrauterine life with a view to identify neuronal circuits that modify/modulate the afferent inputs. MATERIAL AND METHODS Present study was conducted on 30 human embryos and fetuses ranging in age from 8 to 37 weeks of intra- uterine life obtained by hysterotomy and still birth autopsies. The fetal age was calculated on the basis of last menstrual period, crown rump length, biparietal diameter, and external features of the fetuses, while that of premature infant was assessed on the basis of crown heel and biparietal length. Lower cervical segments of spinal cord were processed for various techniques. The neurons and afferent fibers were identified in the 167 Golgi preparation (100 up thick celloidin sections), and circuitry was reconstructed using camera lucida. One Golgi impregnated neuron was processed for electron microscopy using the method of Fairen et al. (1977). 1 ym semithin sections were cut to identify different zones for ultrastructural studies, and electron microscopy was done to study synaptogenesis. Immunohistochemical localization of substance P, enkephalin, and serotonin at different age periods was carried out with the help of avidin biotin peroxidase complex technique using monoclonal anti- body (Sera Lab). GABA was localized using polyclonal antibody (Sera Lab) with PAP technique of Sternberger (1974). RESULTS Morphologically, on the basis of axonal projections and dendritic arborization, different types of neurons could be identified in different zones of dorsal horn. Interneurons (encased of Lima and Coimbra 1983) and projection neurons in marginal zone (Bijlani et al. 1986), islet, stalked, bipolar and multipolar neurons in substantia gelatinosa, and multipolar and antenna neurons in deeper zone were typed in Golgi preparation at all age periods (unpublished observation). One interneuron at 13 weeks (encased) after Golgi impregnation was processed for electron microscopy. Different types of axodendritic and axosomatic synapses with clear spherical, dense core and pleomorphic vesicles were found on the dendrite and soma of this neuron (figs. 1lc,l1d). Mild substance P immunoreactivity was localized at the age of 8 weeks in the tangential plexus of fibers in superficial dorsal horn and in laterally curving fibers. Immunostained ventrally curving fibers could also be seen in the region of substantia gelatinosa (figs. 2a,2d). Intensity of immunoreactivity increased with the age (fig.3). Serotonin immunoreactivity was also found to be of the same pattern as that of substance P at 12 weeks in the superficial dorsal horn. Both medially and laterally curving fibers picked up intense reaction. Inter- mediate horn was found to have network of immunostained fibers (fig. 2b). Immunoreactivity again intensifies with the increasing age. Enkephalin was localized at the age of 12 weeks of gestation in the laterally curving fibers and in intermediate gray. At 14 weeks onward mild immuno- reactive positive cells were found in marginal zone and substantia gelatinosa. At the same age superficial dorsal gray, i.e., the region capping the dorsal horn, 168 FIGURE 1 Electron micrographs bl (1a) 2 an renal rn synapse (arrow) with clear spherical and dense core vesicles at 18 weeks of intrauterine life in marginal zone. X 35640. (1b) serial types of synapses from deeper zone at 25 weeks of age. X 35640. (1c) Golgi impregnated neuron from marginal zone after gold toning at 13 weeks of age. X 6385. (1d) asymmetric synapse (arrow) on the soma of gold toned neuron(c) with clear spherical vesicles. X 46827. 169 FIGURE 2 Photomicrographs showing immunoreactivity in the dorsal horn of spinal cord at the age of 16 weeks of gestation. 2a - Substance P X 75. 2b - Serotonin X 75. 2c - Enkephalin X 75. 2d - Substance P immunoreactive fibres under high power X 750. 170 ILT FIGURE 3 8 WK 12 WK 14WK 16 WK 18 WK 22WK 26WK 37 WK 1 T T T T 1 T SUBSTANCE MILD IMMUNOREACTIVE |INCREASING IMMUNOREACTIVITY P FIBRES GABA IMMUNO POSITIVE] IMMUNO POSITIVE TERMINALS NEURONS SUPRASPINAL ENKEPHALIN INCREASING IMMUNO REACTIVITY IN FIBRES SEROTONIN INCREASING IMMUNO REACTIVITY IN FIBRES Comprehensive chart illustrates the appearance of various neurotransmitters in the dorsal gray at different age periods. and laterally curving fibers were also immunopositive (fig. 2¢). GABA was first localized in terminals on dorsal side of superficial dorsal gray at 8 weeks, while at 10 and 12 weeks immunostained cells were seen in the marginal zone, substantia gelatinosa, and intermediate gray (unpublished observation). At ultrastructural level dense core vesicles were seen in axonal terminals at 8 weeks. From 12 weeks onward axosomatic synapses with plemorphic vesicles were identified (Rizvi et al. 1986). These vesicles could contain either GABA or serotonin or even enkephalin. Asymmetric synapses were seen at 18 weeks (fig. la), while axoaxonic synapse was visible at 20 weeks (Rizvi et al. 1986). Serial types of synapses could be visualized at 25 weeks (fig.1lb). DISCUSSION Gobel (1978a) stated that all neurons in the marginal zone are projection neurons. Our studies are not in agreement with Gobel, as we have identified both projection (Waldeyer 1888) and interneurons at 13 weeks in the marginal zone on the basis of cell size, location, and dendritic morphology (Bijlani et al. 1986). We could also identify "encased neuron", specifically described by Lima and Coimbra (1983) in rat spinal cord as having a prominent dorsally directed dendrite situated dorsolaterally. Encased neuron picked up from Golgi section reembedded in araldite, was sectioned for electron microscopy (fig. lc) and was found to have axosomatic (fig.1ld) as well as axodendritic synapses. This neuron appears to be contacted by descending supraspinal fibers and could thus be involved in modulation mechanisms (Lima and Coimbra 1983). We also found this neuron situated in close proximity of GABAergic terminals at 8 weeks. No GABA positive cells were seen in dorsal horn at this age period (unpublished observations). The punctate appearance of GABA positive terminals in the region of Lissauer tract suggests the presence of GABA in the bulbospinal fibers. Cajal (1909) and Gobel (1978b) have reported central and limiting cells, islet, arboreal, and lamina II-III border cells in substantia gelatinosa, respectively. In our Golgi studies at 13 to 14 weeks we could find primitive stalk cell with axon projecting to lamina I. According to Gobel (1978b), these neurons are equivalent to the limiting cells of Cajal (1909) and may be excitatory interneurons, but according to Bennett et al. (1982) they contain enkephalin, an inhibitory neurotransmitter. 172 We could also find islet cell with axon in its vicinity in the same lamina (Bijlani et al. 1985). According to Gobel (1978b), these neurons may be inhibitory interneuron of Golgi type II class and central cells of Cajal (1909). In deeper zone we could find antenna neurons with dendrites directed toward substantia gelatinosa. According to Willis et al. (1979), some spinothalamic tract cells in monkey do send dorsally directed dendrites through lamina II to lamina I so it may correspond to spinothalamic tract cell. Substance P is putative neurotransmitter for dorsal sensory neurons (Otsuka and Konishi 1977; Nicoll et al. 1980). Recently Bossut et al. (1986) stated that substance P does not appear to be a primary afferent transmitter for pain in the spinal cord. Present investigations have suggested that substance P appears very early in ontogeny, as it was visible at 8 weeks embryonic spinal cord in our study (Mehra and Bijlani 1986). The neuropeptide has earlier been reported in the dorsal horn of human spinal cord at 12 weeks (Charnay et al. 1983) with immunofluorescent technique. Our immunohistochemical studies corroborate with Charnay et al. (1983) but with earlier ontogenic appearance (figs. 2a,2d). The role of descending fibers in the modulation of sensory pathways at spinal level is well illustrated (Fields and Basbaum 1978; Mayer and Price 1976). Activation of serotoninergic pathways has been described to inhibit nociceptive responses of spinothalamic neurons (Messing and Lytle 1977). In dorsal horn serotoninergic axons have been described by Dahlstrom and Fuxe (1965) that originate from brain stem cells containing 5 HT. In our study serotonin positive immunoreactivity was localized at the age of 12 weeks using monoclonal antibodies. Serotonin positive neurons could not be identified in the spinal cord, thus supporting supraspinal origin of these fibers. Serotoninergic terminals gave an appearance of honey comb network around unstained neurons in substantia gelatinosa, supporting close proximity of gelatinosa neurons to supraspinal serotoninergic terminals. At ultrastructural level visualization of axosomatic and axodendritic synapses with pleomorphic vesicles may correspond to serotoninergic terminals (Rizvi et al. 1986). Ruda and Gobel (1980) have described in detail the mode of action of descending serotoninergic fibers on islet, stalked, and projection neurons and 173 have stressed the modulatory role in nociception. Our observations indicate the existence of a morphological substrate corroborating Ruda and Gobel's (1980) findings. Neuromodulatory role of enkephalin in the pain sensory system was supported by physiological (Basbaum and Fields 1978; Mountcastle 1980) and anatomical (Eokfelt et al. 1977; Glazer and Basbaum 1981) findings. Enkephalin has been localized immuno- histochemically in the spinal cord of man (DeLanerolle and LaMotte 1983) and monkey (Aronin et al. 1981) and in human fetuses and infants (Charnay et al. 1984) by immunofluorescent technique. Enkephalin immunoreactive fibers in these studies were predominant in the marginal layer and substantia gelatinosa (Elde et al. 1976; Sar et al. 1978), while enkephalin containing cell bodies were located in the substantia gelatinosa (Ditirro and Ho 1980). Opiate receptors have. been described to be located in the superficial dorsal horn on primary afferent fibers (Atweh and Kuhar 1977), thereby indicating the formation of axoaxonic synapses (Jesselet al. 1979) and causing presynaptic inhibition by enkephalinergic neurons of substantia gelatinosa (Mudge et al. 1979). In contrast, physiological studies have shown that enkephalin acts at postsynaptic sites in dorsal horn (Henry et al. 1980). At electron microscopic levels in rat dorsal horn enkephalin has been localized in axon terminals (Pelletier and Leclere 1979) and found to form synapses with dendrites and soma (Hunt et al.. (1980). For the first time, enkephalin positive neurons were found in lamina I,II, III, and V at ultra- structural level (Aronin et al. 1981). According to these authors, enkephalin binds mostly to opioid receptors contained on dendrites and soma within the spinal cord, while direct synapses by enkephalinergic axons with primary afferent fibers form a secondary and not so common site of interaction. Therefore, earlier concept that opiate receptors are on primary afferent terminals and form axoaxonic synapses for presynaptic inhibition appears to be contradicted. In present investigation on developing dorsal gray, enkephalin immunoreactivity was localized in the dorsal gray at the age of 12 weeks in fibers entering to intermediate dorsal horn through lateral funiculus. From 14 weeks, immunoreactive fibers were found in superficial dorsal gray, i.e., marginal zone and substantia gelatinosa (fig.2c). Laterally curving fibers also were found to show immunoreactivity. Our immunohistochemical findings corroborate with the immunofluorescent finding of Charnay et al. (1984). 174 At 17 weeks, in addition to immunoreactive fibers, some cells positive for enkephalin could also be visualized, suggesting the presence of enkephalin in substantia gelatinosa neurons. The intensity of reaction in fibers and cells increased from 12 weeks to 25 weeks (the specimen used for immunohistochemical localization). Curtis and Johnston (1974) and Levy (1977) have described GABA as a major neurotransmitter involved in mediation of presynaptic and postsynaptic inhibition and presynaptic felicitation. Wolf (1981) has described relationship between GABA positive neurons and development of excitatory synapses in developing visual cortex and has specified that in prenatal phase GABA has extra synaptic function. Light et al. (1979) and Kumazawa and Perl (1978) have stressed the roles of GABAergic synapses in the integration of afferent information. In the present investigations on human fetal material, GABA was localized using polyclonal antibodies. At 8 weeks of intrauterine life, immunopositive terminals were identified in dorsal most-regions of the spinal cord. These appear to be in the region of Lissauer tract and could be the terminals of bulbospinal pathways. At 12 weeks of intrauterine life, GABA positive cells were found in the marginal zone, substantia gelatinosa, as well as in the deeper zones. These findings support the results of Barber et al. (1982) in the rat spinal cord. These authors, however, identified GAD positive cell bodies. At ultrastructural level presence of various types of synapses with morphologically different types of vesicles, namely, clear spherical (fig. 1b), dense core (fig. la), and pleomorphic vesicles (Rizvi et al. 1986), suggest the presence of different transmitter, e.g., substance P, serotonin, GABA, and enkephalin, CONCLUSIONS In conclusion, present investigations suggest that among various neurotransmitters that have been described in the literature to play a role of mechanism of nociception, substance P of dorsal root origin appears at 8 weeks and at the same age GABA in the bulbospinal fibers is present. Serotonin and enkephalin neurotransmitters are present at 12 weeks in the fibers while enkephalinergic cell bodies are visualized at 14 weeks onward. The presence of these transmitters indicates the possibility of the existence of various components of morphological 175 substrate for nociception in spinal cord at very early stages of human ontogeny. 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Trevino, D.L.; Maunz, R.A.; Bryan, R.N.; and Willis, W.D. Location of cells of origin of the spinothalamic tract in the lumbar enlargement of cat. Exp Neurol 34:64-77, 1972. Trevino, D.L., and Carsten, E. Confirmation of the location of spinothalamic neurons in the cat and monkey by retrograde transport of horseradish peroxidase. Brain Res 98:177-182, 1975. Waldeyer, W. Dass Gorilla-Ruckenmark. Abhandlungen der Konighlichen Akademie der Wissen chaften. 1888. pp. 1-147 (quoted by Willis and Coggeshall 1978). Willis, W.D.; Kenshalo, D.R. Jr.; and leonard, R.B, The cells of origin of the primate spinothalamic tract. J Comp Neurol 188:534-574, 1979. Wolf, J.R. Some morphogenetic aspects of the development of the central nervous system. In: Immelmann, K.; Barolow, G.W.; Petrinovitch, L.; and Main, M. eds. The Bielefeld Interdisciplinary Project. New York: Cambridge University Press, 1981. pp. 164- 190. AUTHORS Professor Veena Bijlani, M.B.B.S., M.S., Ph.D., F.A.M.S. Tilat A. Rizvi, M.Sc. S.Wadhwa, M.B.B.S., M.S., M.A.M.S. Department of Anatomy All-India Institute of Medical Sciences New Delhi-110 029, India 179 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D., eds. National Institute on Drug Abuse, 1988 Differential Effects of Opioid Peptides Administered Intracerebrally in Loci of Self- Stimulation Reward of Lateral Hypothalamus and Ventral Tegmental Area—Substantia Nigra Jitendra Singh, Ph.D., and T. Desiraju, Ph.D. INTRODUCTION In recent years the knowledge on the wide distributions of the opioid neurons, fibre terminals, and their receptors has been growing (Atweh and Kuhar 1983; Akil et al. 1984; Snyder 1984, 1986). The opioid peptide neuronal and receptor mechanisms are considered to participate in a range of homeostatic integrations in the different subsystems of the brain, including the stress response and coping, pain control, anal- gesia, neuro-endocrine, cardiovascular, and other visceral regulations, and the mechanisms of reward, mood, and psyche. The present state of knowledge generally indicates that the beta-endorphin neurons and the epsilon, mu, and delta receptor mechanisms might be pre- dominantly involved in the visceral and neuro-endocrine regulations, the enkephalins and the delta receptors involved primarily in the psychic and other limbic neuronal mechanisms, the dynorphins and the kappa receptors primarily involved in the analgesic and sedative neuronal mechanisms, and with several overlapping roles also in the functioning of these neurons and receptors in different subsystems. The enkephalins were shown to have the reward properties in intra- ventricular self-administration experiments (Stein and Belluzzi 1979), the leu-enkephalin was more self-administered than the met- -enkephalin or the morphine. The self-administration of morphine and of D-ala®- met®-enkephalinamide (and its blockade by naloxone) into the self- stimulation sites of lateral hypothalamus was also reported (Olds 1979; Olds and Williams 1980), but these results were argued to be artifacts by Bozarth (1983), who stated that the morphine self- administration property was not present in lateral hypothalamus, but present only in the ventral tegmental area (Bozarth and Wise 1981). Shaw et al. (1984) reported that while the intra-ventricularly injected morphine caused a reduction of spontaneous motor activity, the elec- trical self-stimulation (SS) of medial prefrontal cortex (MPC) was facilitated. Similar results were also observed by them with the intra- ventricular injection of the enkephalin analogue BW 180 (tyr-D-ala- gly-phe-D-leu), but these effects were indirect according to them as direct injections of morphine or naloxone into MPC caused no change 180 in the SS of MPC. Naloxone (intraperitoneal) has also been shown to cause a small but significant reduction in the SS of lateral hypo- thalamus (Ichitani et al. 1985). Broekkamp et al. (1976) reported that the SS of LH was inhibited by injecting morphine into central grey. In contrast, microinjections of morphine or of D- ala®-met®-enkephalin- amide administered into ventral tegmental area facilitated the SS of lateral hypothalamus and the effect of morphine was antagonized by systemic naloxone (Phillips et al. 1983). They also reported rewarding effects "in the conditioned place preference paradigm and that such a facilitatory effect was attenuated by haloperidol or by lesions of dopamine pathways (Phillips et al. 1983). The above studies indicate the need for investigations of the role of the opioid peptides administered into the different regions of SS to understand the intrinsic and interlinked components in the mechanisms of the brain reward neuronal systems. The present study was designed to investigate the effects of enkephalins and dynorphins administered directly into the loci of self-stimulation of ventral tegmental area- substantia nigra (SN-VTA) and of lateral hypothalamus (MFB-LH) on the self-stimulation operant rates of the same loci. Such studies have not appeared in the literature so far. METHODS Wistar rats weighing 260-320 g were implanted with bipolar SS elec- trodes made up of 28 g stainless steel wire, and bipolar cannula-cum- wire electrode made up of the same type of wire joining to 22 g cannula needle. The cannula-wire electrode (both insulated except for tips) served either as bipolar SS electrode or for microinjections of chemicals through the cannula into the SS site. In each rat one bipolar wire electrode and one bipolar cannula electrode were implanted, one in MFB-LH and the second in ipsilateral SN-VTA . In different rats the placement of the two types of electrodes was interchanged between the regions. After a few days of post-operative recovery, the self- stimulation rates of each of these sites were shaped and stabilized reproduceably in a few sessions. The stimuli used were sine waves of 50 Hz, 0.25 sec train duration for each pedal press, and current intensities ranging between 75 pA and 200 uA as required to get the maximum possible SS without apparent side effects. The duration of a control or a test session was 15 min. At least three test sessions (with drug) and three control sessions (with vehicle) were made for each dose, and all repeated in at least three rats. 33 rats were used in the present study. All intra-cerebral injections (drug or vehicle solutions) were made through the cannula slowly in about 60 seconds in a constant volume of 1 pl. At the end of the experiment, the place- ments of the electrodes were noted from frozen sections cut at 60 u stained with cresyl violet, and marked on the charts of atlas of Paxinos and Watson (1982). Data were processed by using the F test (Anova) to test the homogeneity of variance and by Student's 't' test to know the levels of significance of the effects. The chemicals used were: leu®-enkephalin; met®-enkephalin; leu’- enkephalinamide; dynorphin-A[1-13] (all these of Sigma, USA); D-ala’- D-leu®-enkephalin (BW 180C of Wellcome Research Laboratories, 181 UK); naloxone-HCI (Endo Laboratories, USA). RESULTS The leu®-enkephalin (leu-enk) was administered (500 ng) into SN-VTA and one hour and two hours later, the SS operants were recorded. It was observed that the SS of the site was reduced by 48% at 1 hr and by 70% at 2 hrs from the level of the control value obtained under the vehicle injection (Fig.l), the SS of the other site (MFB-LH) was not changed. In the reverse experiment, administration of the leu-enk in MFB-LH has not changed the SS of the same site but has caused a facilitation of the SS of the SN-VTA (Fig.l). A similar pattern of response was obtained with the leu’-enkephalinamide also (Fig.2). The D-ala?-D-leu’-enkephalin (ala-leu-enk or BW 180c) caused, contrary to the above opioids, a facilitatory effect on the SS of SN-VTA when it was administered either in the SN-VTA or in the MFB-LH (Fig.3). This opioid also has not influenced the SS of the MFB-LH. Naloxone hydrochloride (30 mg/kg ip) has brought down the facilitated effect of SN-VTA back to about the normal level (Fig.3). The met®-enkephalin (met-enk) administered in doses of 500 ng or 2 ug either into SN-VTA or into the MFB-LH has not been found to influence the SS of either region (Fig.4). Dynorphin-A[1-13](dyn) administered in doses of 500 ng or lug into SN-VTA has caused facilitation of its SS. Administration of the same into the MFB-LH has not influenced either its SS or that of the SN-VTA (Fig.5). In summary, the leu-enk or its amide have caused reduction in the SS of SN-VTA when administered into the same site. When these opioids were administered into the MFB-LH its own SS was not influenced, but caused indirect facilitatory effects on the SS of SN-VTA. Met-enk caused no changes of SS in both these regions. Contrary to leu-enk, dynorphin-A[1-13] caused facilitatory effect in the SN-VTA, and also no effect through MFB-LH. Ala-leu-enk caused both types of faci- litatory effects on the SS of SN-VTA, when it was administered into it and also into the MFB-LH, without changing the SS of the MFB-LH. DISCUSSION There seems to be no study made previously to find the effects of the above cited opioid peptides on the SS of SN-VTA and of MFB-LH, after administering them into the same SS sites. It was previously reported (Shaw et al. 1984) that only the intra- ventricular administrations of BW 180 (ala-leu-enk) up to 40 ug doses, or morphine up to 20 ug, caused facilitation of the SS of the medial prefrontal cortex (MPC), but no effects were observed when morphine or naloxone was administered into the MPC. As the ventricular drug could act at many sites in the brain, the authors interpreted the effects as indirect ones on the MPC. These authors have also reported that 182 ( Leu’) ENKEPHALIN - intracerebral SN - VTA MFB - LH 2000 1 A & .e (n=5x3 ) 1500 1000 - Zz 3 « 500 - ~~ Ww - < @ | tA B 8 WJ & 2500 1 WEB LH 500ng i, 2 Oe [r= ater hr Beater ane W.. 2000 1 (n=3x3) TT ———— 1600 - 1000 - 500 FIGURE 1 Effects of slow microinjection (1 pl in 60 sec) of leuenkephalin either into SN-VTA (A) or into MFB-LH (B) on the electrical self-stimulation of the injected site and of the other site. Cannula site is open circle, filled circle is wire. Typical placement sites of histology indicated in the atlas drawings of hypothalamus and midbrain. A', one hour or two hours (A" after the drug is administered in other site; B, before the drug is administered in the other site; D', one hour or two hours (D") after the drug is administered in the same site; V, after the vehicle (saline) is administered in the same site. 'n' indicates the data of number of rats and the number of sessions conducted on each of them. * = P < 0.005; ** = P < 0.001. 183 (Leu’) ENKEPHALINAMIDE =intracerebral SN-VTA MFB - LH O° eo 2000 + mT ~~ 7 A (n=3x3) i astro | h H] iM So SE : ~s- lateral hypothalamus under naloxone (5mg/kg ip). The effects of naloxone hydrochloride on the SS could depend on the regional differen- ces and on the conditions of reinforcement, the FR-30 schedules being most affected and the CR schedules least affected. Schaefer and Michael (1985) observed the SS (FR-30) of the periventricular grey to decrease in a dose-dependent manner, by about 70% at a naloxone dose of 30 mg/kg given sub-cutaneously. At this dose, they have also observed a slight reduction (about 15%) in the ambulatory activity. Phillips et al. (1983) reviewed the observations to show that morphine or ala-met-enk administration into SN-VTA caused facilitation of the SS of lateral hypothalamus, whereas our results with the ala-leu-enk administration into the SN-VTA have not caused any change in the SS of MFB-LH. Probably the difference in the opioids used and the receptors upon which they act could be the reason for the opposite patterns of the results. Our present study with the leu-enk, met-enk, ala-leu-enk, and dyn has also disclosed such differences in the pat- terns of the effects on SS of the SN-VTA and the MFB-LH. In the studies of Phillips et al. (1983) the effect of morphine or of ala-met- enk on the SS of the injected site (SN-VTA) was not studied, whereas we have found that with the ala-leu-enk the SS of the injected site (SN-VTA) was facilitated. We have also observed the converse, i.e., administration of the ala-leu-enk into the MFB-LH has not changed the SS of the injected site and yet led to a change of the SS of the SN-VTA. This could imply that at the MFB-LH the ala-leu-enk could have acted on an additional interlinked substrate besides on the SS substrate (intrinsic) of MFB-LH and that the additional substrate could have been linked to the SN-VTA intrinsic substrate of SS. In other words, the opioid effects probably differentiated in the MFB-LH the intrinsic SS substrate from a separate substrate present there and interlinked to the SN-VTA mechanism of SS. The mode of synaptic transmission actions of opioids and the details about differences in the proportions of the opioid receptor types present on the neurons of the MFB-LH and the SN-VTA are not adequately available to enable to infer the possible mechanisms underlying the effects seen in the present study. A review of the previous studies (North and Williams 1983) indicates that morphine would enhance K* conductance and cause inhibition of noradrenergic neuronal firing. These effects could widely differ according to the types of the neurons and the sites in the brain. There was also an opposite type of observa- tion that morphine when administered iontophoretically led probably indirectly to an increase in the firing of dopaminergic neurons at SN-VTA and that iontophoressed naloxone had not reversed this effect, 188 whereas the non-DA neurons in the vicinity were suppressed, which could be reversed by naloxone (Gysling and Wang 1983). It has been reported that the leu-enk has primarily the delta receptor activity (Akil et al. 1984). Dynorphin-A [1-13] is known to be very potent at both mu and kappa receptors, and its fibre terminals are present only in SN and not in LH, which has the cell bodies (Akil et al. 1984). Ala-leu-enk also labels preferentially the delta sites. Hence, the opioid peptides used in the present study would be primarily acting upon the delta, mu, and kappa receptors of the non-opioid and the opioid neurons and axon terminals in the MFB-LH and SN-VTA. However, the differences in the proportions of these receptor types present in the two regions, and the organization of the types of neurons and terminals in the linkages of circuits in which these receptors are located in the two regions, are unknown. The mu receptors are pro- bably more predominant in the MFB-LH (Akil et al. 1984), whereas the delta and kappa may be relatively more in the SN-VTA substrates of SS. It is hypothesized from the present results that the leu-enk in the MFB-LH could be inhibiting a projection mechanism inhibitory to the SS system of SN-VTA, thereby releasing the facilitation of the SN-VTA. The opposite type of effects of the leu-enk and the ala-leu-enk on the SS of SN-VTA, when these are administered in the SN-VTA, is probably due to their differences in actions on the recep- tor types present in the SN-VTA. The dynorphin-A actions suggest that the kappa receptors seem to be involved in the SS mechanism of SN-VTA and not in that of MFB-LH. The differential effects of the above opioids on the SS of the SN-VTA and the MFB-LH emphasize the differences in the neural mechanisms of the SS of the two regions. Our previous study (Singh and Desiraju 1986) of the SS of the two regions with local administrations of halo- peridol and apomorphine also disclosed that the two regions have separate synaptic types of intrinsic mechanisms of SS, besides having an inter-linkage mechanism. As the opioids have shown either inhibitory or facilitatory effects on the SN-VTA, and little such effects on the MFB-LH, the possibility arises whether this striking difference could be due to the dopaminergic neurons and receptors present in the SN-VTA. This difference in effects could also as well be due to the opiate receptors present on non-dopaminergic neurons and terminals located in the SN-VTA. SUMMARY Leu-enkephalin, leu-enkephalinamide, ala-leu-enkephalin, met-enkephalin and dynorphin-A[l1-13] were administered in microinjection into one of the self-stimulation sites of SN-VTA or MFB-LH and the electrical self-stimulation (SS) of the injected site and of the second site was recorded. The study revealed that the leu-enkephalin and the leu- enkephalinamide inhibited the SS of SN-VTA and produced no effect on the SS of MFB-LH, when administered into these sites. The MFB-LH injection, however, facilitated the SS of SN-VTA. The effect of ala- leu-enkephalin injection in MFB-LH was similar to the above, but the effect of the injection in SN-VTA was different in that it caused 189 the facilitation of its SS and not the depression as seen with leu- enkephalin. Met-enkephalin injections in the two regions caused no direct or indirect changes of the SS of the regions. Dynorphin injection in SN-VTA facilitated its SS, like the injection of ala-leu-enk, but dynorphin injections in MFB-LH produced no effects. The results essen- tially demonstrate the differences in the effects of the different opioids in the reward system of the SN-VTA, and it is discussed that these differences are probably due to the preferences in the types of the receptors upon which these opioids act in the SN-VTA neuronal organisation. The results also demonstrate the major difference in the organisation of the reward substrate of the MFB-LH from that of the SN-VTA, as the effects of the opioids in the MFB-LH are mar- kedly different or none compared to the effects in the SN-VTA. REFERENCES Akil, H.; Watson, S.J.; Young, E.; Lewis, M.E.; Khachaturian, H.; and Walker, J.M. Endogenous opioids: biology and function. Ann Rev Neuro- sci 7: 223-255, 1984. Atweh, S.D., and Kuhar, M.J. Distribution and physiological significance of opioid receptors in the brain. Br Med Bull 39: 47-52, 1983. Bozarth, M.A. Opiate reward mechanisms mapped by intracranial self- administration. In: Smith, J.E., and Lane, J.D., eds. The Neurobiology of Opiate Reward Processes. Amsterdam: Elsevier Biomedical, 1983. pp.331-359. Bozarth, M.A., and Wise, R.A. Intracranial self-administration of morphine into the ventral tegmental area in rats. Life Sci 28: 551- 555, 1981. Broekkamp, C.L.; Van Den Bogaard, J.H.; Heynen, H.J.; Rops, H. 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Ann Rev Physiol 48: 461-471, 1986. Stein, L., and Belluzzi, J.D. Brain endorphins: possible role in reward and memory formation. Federation Proc 38: 2468-2472, 1979. ACKNOWLEDGEMENT The general support of the Indian Council of Medical “Research, New Delhi, to this Department research. AUTHORS Jitendra Singh Research Scholar Department of Neurophysiology National Institute of Mental Health and Neuro Sciences Bangalore 560 029, INDIA T. Desiraju Professor & Head Department of Neurophysiology National Institute of Mental Health and Neuro Sciences Bangalore 560 029, INDIA 191 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D., eds. National Institute on Drug Abuse, 1988 Peptides and Thermoregulation Rakesh Shukla, Ph.D., and Bhola N. Dhawan, M.D. Many neurotransmitters are involved in the central regulation of body temperature under normal conditions, in fever, and during exercise and heat and cold stress. Emphasis on amines and prostaglandins has declined to some extent, and a major focus in recent years has been on the peptides that might participate in central nervous system (CNS) mediation of temperature control. Interest in the neurobiology of peptides has developed coincident with their identification and chemical characterization in mammalian brain. Several of these peptides were originally isolated from pituitary tissue or the alimentary canal, but they also occur in various regions of the CNS. Although the central roles of most of the peptides are still not adequately understood, many neuropeptides are known to have profound effects on regulation of body temperature, and the available data on the neuropeptides will be briefly reviewed. 1. OPIOIDS The endogenous opioids are unique in that their ability to alter thermoregulatory mechanisms is shared by nonpeptide opioids. While evidence is accumulating that opioid ligands and opioid receptors play a functional role in thermoregulation, an exhaustive study in different species has not yet been undertaken for opioid peptides. Much less information is available on the opioid peptides than on morphine. A. Morphine Most studies have been conducted with morphine, although some investigations have also been carried out with other opioids. Several reviews have appeared on the effects of morphine on body temperature, the most comprehensive being those by Clark (1979), Clark and Lipton (1983, 1985), and a recent review by Adler et al. (1988). The effects of morphine are species-dependent. A hypothermic response is predominant in the dog, rabbit, and pigeon; a hyperthermic response in cat, cattle, goat, and horse; and a dual response (low-dose hyperthermia and high-dose hypothermia) in rat, mouse, and primates (Clark and Lipton 1985). A biphasic response, 197 hypothermia followed by hyperthermia, in rat and mouse is also reported (Rosow et al. 1980). All these responses to morphine are blocked and antagonized by naloxone. There is also some interaction with calcium channel antagonists (Pillai and Ross 1986b). Morphine responses are dependent on ambient temperature: a hypothermic response is predominant at ambient temperature below thermoneutrality; biphasic responses appear as the ambient temperature increases, and ultimately hyperthermia predominates at the highest ambient temperatures (Adler et al. 1988). Recent studies have demonstrated that morphine responses are also dependent on the route of administration (Adler et al. 1984; Geller et al. 1986), and route is a critical determinant not only of quantitative effects but of qualitative effects as well. The exact mechanisms involved in the body temperature changes produced by morphine are still not known with certainty. The effects may result primarily from the actions on oxygen consumption, however. Morphine-induced hypothermia is associated with decrease in oxygen consumption and metabolic heat production in a variety of species (Lotti et al. 1966; Lin et al. 1980). Recent studies by Adler and his colleagues (1986, 1988) suggest that body temperature responses to morphine are due to the change in thermal set point in hypothalamus. In dog, an increased heat loss after morphine administration has been demonstrated (see Clark and Lipton 1985 for a review and references). Some interaction of morphine with dopaminergic and cholinergic systems in thermoregulation has been shown by Cox et al. (1975) and Adler et al. (1986). B. Naloxone Naloxone has been used by several investigators to establish evidence for involvement of opioid receptors. Naloxone, per se, however, does not have an effect on thermoregulation in rat (Pillai and Ross 1986a) or man (Fuenmayor and Cubeddu 1986) though in morphine-dependent rats naloxone and related compounds reduced rectal temperature by a central action since quarternary derivatives were inactive (Katovich et al. 1986). The drug interactions are not always well defined. Thus naloxone only partially blocked ethanol hypothermia, which was completely blocked by kappa antagonist MR 2266 (Pillai and Ross 1986a), whereas it completely antagonized microwave blockade of amphetamine hyperthermia (Lai et al. 1986). The biphasic temperature changes with phencyclidine are antagonized by naloxone, by the £ and « antagonist SKF 10,007 as well as by the pure kx antagonist MR2266 (Hiramatsu et al. 1986). C. Endogenous Opioids Identification of endogenous peptides and their precursor molecules in the brain encouraged intense research efforts to determine both the in vivo and the in vitro effects of these substances and the possible functional roles played by the u, «x, and § opioid receptors. Recent data utilizing more selective ligands in rat suggest that u opioid receptors play a role in hyperthermic response. Morphine, a prototypic p ligand, and DAGO, a pu selective receptor agonist, produce hyperthermia in several species 193 of animals (Adler et al. 1988) and prompt rats to seek warmer temperatures. On the other hand, « receptors seem to be involved in hypothermia, as U50488H, a « receptor agonist, produces dose-related hypothermia. A role for § receptors in thermoregulation cannot be ruled out completely. a. B-Endorphin. If nonpeptide opioids act at receptors that are stimulated by opioid peptides, the thermoregulatory effects of endogenous opioids and of morphine and related agonists ought to be alike. When B-endorphin is injected centrally to a variety of species, it induces patterns of temperature change that closely resemble those associated with central or peripheral administration of morphine (Clark and Lipton 1985). Relatively low doses of morphine and B-endorphin raise the level at which temperature is regulated in the cat, rat, mouse, and rabbit (Rezvani et al. 1982), primate (Murphy and Lipton 1983), and fish (Kavaliers 1982). Evidence from studies on rabbits indicates that this change in regulation may be due to impaired input from peripheral warmth sensors (Rezvani and Heath 1984). Such an effect would be of greater significance in a warmer environment and could account for the greater increase in body temperature at usual ambient temperatures than in a cold environment after injection of a given dose of B-endorphin to cats, rabbits, etc. In contrast to the above species, which have been used most often for the study of opioid-induced temperature changes, B-endorphin lowers the temperature of chickens and hamsters (Clark and Lipton 1983). In those species in which small doses of B-endorphin induce hyperthermia, naloxone and similar antagonists ought to lower temperature if B-endorphin contributes to maintenance or elevation of body temperature. Both naloxone and naltrexone prevented a rise in the temperature of rats secondary to restraint or handling, or lowered temperature when stress was minimized by habituation of the animals to the experimental procedures (Clark and Lipton 1983; Pae et al. 1985). Except for such reports, evidence is not available to indicate that reasonable doses of opioid antagonists appreciably affect temperature. So it is unlikely that B-endorphin, which has been readily antagonized in most studies, plays a major role in normal thermoregulation, even in hot or cold environments (Clark et al. 1983). Likewise, naloxone has not altered responses to pyrogen in the cat, rat (Clark and Lipton 1983), guinea pig (Kandasamy and Williams 1983), and sheep (Duranton and Bueno 1984). So a role for B-endorphin in fever is unlikely. This view is also supported by the fact that antipyretics failed to antagonize the hyperthermic action of opioid peptides in the cat, mouse (Clark and Lipton 1983), guinea pig (Kandasamy and Williams 1983), and rabbit (Kandasamy and Williams 1983; Rezvani and Heath 1984). It is likely that the endorphin effects are mediated via a mechanism independent of the arachidonic acid cascade. 194 b. Enkephalins. Very little information is available on the potential thermoregulatory actions of enkephalins. Met-enkephalin is a relatively weak agonist in altering body temperature (Clark and Lipton 1985), probably because of its rapid inactivation (Miller 1981). To obtain measurable temperature changes, larger doses (0.1 mg to 10 mg centrally) of the enkephalins (as compared to B-endorphin) have been required. The usual response at room temperature has been hyperthermia (Clark and Lipton 1985), although there have been exceptions (Sakurada et al. 1983). Shukla et al. (1982) have demonstrated that Met-enkephalin induced hyperthermia varied inversely with ambient temperature over a temperature range of 100 to 33°C in the desert rat Mastomys natalensis. A major difference between Met-enkephalin and B-endorphin is that the hyperthermic response to the former is less readily antagonized by naloxone (Clark and Lipton 1983). Hence the lack of appreciable effect of naloxone on temperature does not rule out the mediation of thermoregulation by enkephalins. Assessment of this possibility has been hampered by the lack of a selective enkephalin antagonist. A number of relatively stable and more potent enkephalin analogs have been tested (see 1985 review by Clark and Lipton). Unfortunately, these have generally been more readily antagonized by naloxone, and act more like B-endorphin than like the parent enkephalins, probably because the structural modifications that increase stability tend to shift sensitivity away from naloxone-insensitive types of receptors. Recently Shukla et al. (1988) suggested an enkephalinergic and serotonergic interaction in the thermoregulation of the desert rat. c. Other Opioid Peptides. Dermorphin produces a naloxone-reversible hypothermia which is unaffected by antagonists of other putative neurotransmitters such as serotonin, catecholamines, GABA, acetylcholine, etc. (Tatara et al. 1986). Currently available data do not permit a definitive statement regarding the role of opioid peptides in thermoregulation. It is, however, abundantly clear from data reviewed above that multiple opioid receptors are involved. It appears likely that several types of transmitters/modulators are involved in regulation of body temperature in health and disease and that their relative importance varies in various situations. It is necessary to study the effect of specific agonists and antagonists at various opioid receptors in several species, not only at different ambient temperatures but also during pyrexia induced by different agents to assess their roles. It is also necessary to study their interaction with other putative neurotransmitters and to analyze in depth their effect on heat production and heat loss mechanisms. There is evidence to indicate that some of the peptides may be acting at sites such as the septum (see below). Such sites have not been investigated for the effect of opioid peptides. 195 II. ANTIPYRETIC PEPTIDES A. ACTH/MSH ACTH and MSH, which were first isolated from pituitary tissue, are widely distributed within the brain (Krieger and Martin 1981). They were first shown to reduce temperature when given centrally to rabbits (Lipton et al. 1984). Subsequently, ACTH and MSH were found to be antipyretic when administered centrally or peripherally in doses that had no effect on normal temperature (Murphy et al. 1983). The parent molecule ACTH (1-39) was actually the first peptide with documented antipyretic activity. Most of the recent research, however, has been focused on MSH. This peptide is about 25,000 times more potent than acetaminophen as an antipyretic (Murphy et al. 1983). MSH reduces fever whether administered j.c.v., i.v., or into the stomach of rabbits (Murphy and Lipton 1982). Its central site of action may be the septum, as injections of MSH into the septum are also antipyretic. ICV administration of ACTH reduces endotoxin-induced fever in squirrel monkeys, and MSH is likewise antipyretic when given i.v. to these primates (Lipton and Shih 1985). Corticotropin-releasing factor (CRF), which releases ACTH/MSH from the pituitary, also reduces fever in a dose-related fashion when given i.c.v. to rabbits. The precise mechanism of action of MSH in reducing fever has not been determined. However, it is unlikely that antipyretic doses directly inhibit central heat production and conservation pathways, since MSH has no effect on the temperature of a febrile rabbit exposed to cold (Richards and Lipton 1984). The doses required to induce the antipyretic and hypothermic effects of peptides differ. These effects appear to represent distinct actions within the CNS. Studies on hyperthermic responses to arachidonates suggest that central release of MSH could mediate the antipyretic effect of acetaminophen. B. Arginine Vasopressin (AVP) The role in thermoregulation of arginine vasopressin, the antidiuretic hormone in man, has been studied in the past. Most of the supportive data have been obtained recently, however. Studies of temperature-induced changes in plasma vasopressin levels or diuresis have produced conflicting data. Concentration of AVP did not change in the pig during exposure to warm, neutral, or cold environments (Forsling et al. 1976). Cooling of the rostral hypothalamus in cold and thermoneutral environments, or heating in thermoneutral and warm environments, likewise did not affect vasopressin levels. However, increasing core temperature to 420C caused a rise in plasma vasopressin that could be completely suppressed by reducing preoptic/anterior hypothalamic temperature. Brisk water diuresis was observed with preoptic/anterior 196 hypothalamic cooling in rhesus macaques, presumably due to inhibition of vasopressin release (Hayward and Baker 1968). These findings suggest a relation between vasopressin and central temperature control mechanisms. They give no indication, however, that this relationship is important under normal circumstances. The evidence for arginine vasopressin as an endogenous antipyretic is strong but not yet conclusive. It includes direct suppression of fever by the application of AVP in a sensitive, dose-dependent manner by push pull perfusion into the region of the septum in animals given intravenous pyrogens, and the appearance of AVP in the perfusate after perfusion of the septal region with an artificial interstitial fluid during fever. The vasopressin concentration is inversely related to the magnitude of fever. Hemorrhage, a well-known stimulus for the release of vasopressin into the circulation, was found to be without effect on normal body temperature but to suppress the fever elicited from intravenous pyrogen. The application of an antibody to AVP in the septal region led to a markedly greater rise in body temperature than would normally occur from a fixed dose of endotoxin given intravenously (Cooper 1987). AVP itself is without effect on normal body temperature in the sheep when perfused through the ventral septal area. Zeisberger et al. (1980) and Merker et al. (1983) have demonstrated that the pregnant guinea pig close to term and several hours post partum is refractory to endotoxin. In the nonpregnant guinea pig during fever, AVP reactivity was increased in fibers projecting from the hypothalamus to the septum and amygdala (Zeisberger et al. 1983). Arginine vasopressin suppressed pyrexia caused by intraventricular injection of PGE when the AVP was perfused through the rostral diencephalic loci at which PGs caused fever (Ruwe et al. 1985). Evidence of the endogenous antipyretic action of AVP has been found in rats (Kovacs and De Wied 1983). Banet and Wieland (1985) found that AVP infused into the lateral septum of the rat suppressed the heat production caused by hypothalamic cooling but did not affect vasomotor tone in the skin. The reduction in thermoregulatory increase in heat production that led to a fall of body temperature during cold exposure might explain the antipyretic action of AVP. Wilkinson and Kasting (1986) presented evidence to indicate that vasopressin reduces the set point for body temperature in febrile rats. Only one study (Lee et al. 1985) has evaluated the role of AVP in a subhuman primate, macaque monkeys, where intraventricular AVP had no effect on the normal body temperature or fever, except at a dose of 65 ng, where the mean fall of body temperature of 0.50C appeared to be due to a larger response in one animal. AVP has also been shown to cause hyperthermia in rabbit (Lipton and Glyn-Ballinger 1980) but is without effect in cats and causes hypothermia or hyperthermia when microinjected into the preoptic area in the rat (Naylor et al. 1986). 197 Arginine vasopressin might be a mediator of fever within the anterior hypothalamus/preoptic anterior hypothalamus and an antipyretic within the ventral septal area. Such a dual function would be consistent with a negative feedback system to modulate the magnitude of fever, a useful function if fever is a beneficial accompaniment of disease. A role for AVP as a fever mediator as well as an endogenous antipyretic is, however, far from conclusive. III. OTHER PEPTIDES A. Thyrotropin-Releasing Hormone (TRH) TRH is the most extensively studied peptide, and it usually induces a brief increase in temperature (Clark 1979). Cats respond with hypothermia (Metcalf 1974; Myers et al. 1977), however, as do rats (Lin et al. 1980) and nonhibernating ground squirrels (Stanton et al. 1981). TRH-induced temperature changes are independent of its action on the thyroid. Effects of TRH on body temperature were determined over a range of ambient temperatures, but the pattern of body temperature change in the majority of reports is consistent with increase in the level of regulation. TRH has frequently been observed to have a general excitatory action that would tend to raise temperature by increasing heat production. It can enhance locomotor and other behavioral activities alone and can reverse behavioral depression, hypnosis, and anesthesia induced by other agents (Clark and Lipton 1983). The hyperthermic effect of TRH administered into the preoptic/anterior hypothalamus of rats was unaffected by pretreatment with aspirin, but was reduced by adrenergic antagonists (Chi and Lin 1983). However, based on resistance to inhibition by adrenergic antagonists, other investigators have concluded that the noradrenergic system is not essential for this response in mice given TRH by intraperitoneal injection (Pawlowski and Kwiatek 1983). In another study, TRH given intraperitoneally to mice caused hyperthermia that was associated with increased plasma norepinephrine and epinephrine concentration (Boschi et al. 1983). Simultaneous injection of these catecholamines increased hyperthermia. Adrenal demedullation suppressed both the increase in plasma catecholamines and TRH-induced hyperthermia, but not the hyperthermic response to TRH plus catecholamines. Hypophysectomy also reduced TRH hyperthermia, in contrast to earlier reports, but not the increase of plasma catecholamines or the effect of combinations with exogenous catecholamines. These authors concluded that both the adrenal and pituitary have essential roles in TRH-induced hyperthermia. When injected into the hypothalamus of pigeons, TRH induced hyperthermia, shivering, and vasodilation that was probably compensatory (Lathi et al. 1983). Evidence that TRH might be involved in the maintenance of body temperature has been presented by Prasad et al. (1978, 1980). In this study, a 198 dose-related decrease in temperature occurred when rabbit TRH antiserum was injected into the lateral ventricle of rats, and this response was prevented if the antiserum was neutralized with TRH. B. Neurotensin (NT) Neurotensin was initially isolated from bovine hypothalamus (Carraway and Leeman 1973). The primary temperature response to central administration of NT in a variety of species is hypothermia, which is enhanced in cold environments. Neurotensin has been reported to have less than one-thousandth the potency of bombesin in rats exposed to cold (Brown et al. 1977), whereas under similar conditions in mice both of these peptides were equipotent (Mason et al. 1980). Injections of NT into 223 brain sites in rat (Kalivas et al. 1982) indicated that regions responsive to its hypothermic action are distinct from sites at which it inhibits nociception. Administration of NT into the periaqueductal gray had no clear effect on normal body temperature (Kalivas et al. 1982). The N-terminal fragments of NT were inactive, but a C-terminal fragment (8-13) did lower temperature (Widdowson et al. 1983). Neurotensin also lowered the temperature of guinea pigs and hamsters only in a cold environment and did not change the temperature of fish, frogs, lizards, pigeons, ground squirrels, woodchucks, and rabbits (Prange et al. 1979). The research on the mechanism of action of NT has been limited to studies on interactions with other substances. Intracisternally administered NT potentiated the hypothermic response of ethanol (Luttinger et al. 1981) and of dopamine agonists (Jolicoeur et al. 1983), but inconsistent effects were obtained with pentobarbital- induced hypothermia (Nemeroff et al. 1977). The hypothermic response to NT in rat was antagonized by i.c.v. administration of prostaglandin E2 and by calcium chelator EGTA (Lee et al. 1983) but not by TRH, somatostatin, or naloxone. The hypothermic response was also antagonized by amine and cholinergic antagonists (Morley et al. 1982) and was enhanced by thyroidectomy (Nemeroff et al. 1980). Since central administration of EGTA and PGE2 alone causes hyperthermia, a nonspecific antagonism may be responsible for preventing the hypothermic effect of NT at thermoneutral environment. Mason et al. (1982) suggested that release of central prostaglandins may oppose the hypothermic response of NT in cold environment. Lee and Myers (1983) concluded that NT renders the animals poikilothermic, because NT caused hypothermia in rats in thermoneutral and cold environments but not in hot (349-400C) environment. C. Bombesin Bombesin was originally isolated from frog skin (Anastasi et al. 1972, 1975). The central administration of bombesin caused hypothermia in rat and mouse at normal laboratory temperatures. The magnitude of the fall in the temperature has generally been dose 199 related. However, systemically given bombesin did not affect the temperature of rats in the cold (Brown et al. 1977; Brown and Vale 1980). It was subsequently found that injections of bombesin into the PO/AH of rats increased locomotor activity and enhanced both heat reinforcement and heat escape behavior (Hawkins and Avery 1983). It was concluded that the effects on behavior are secondary to the change in activity and do not demonstrate that bombesin lowers the regulated temperature. Avery and Calisher (1982) showed that in a thermoneutral environment i.c.v. bombesin caused dose-related decrease in body temperature and food intake of food-deprived rats. D. Somatostatin Nemeroff et al. (1979) found that intracisternal administration of somatostatin in mice caused hyperthermia at normal laboratory temperature. Brown et al. (1981) did not find any change in body temperature of rat after intracisternal administration of somatostatin in cold environment. Lateral ventricular administration of somatostatin also did not alter the temperature of rabbits (Lipton and Glyn 1980). In only one study somatostatin caused hyperthermia at high ambient temperature and hypothermia at low ambient temperature (Chandra et al. 1981). The pattern of associated effector changes was unusual in that the hyperthermic response at ambient temperature was associated with vasoconstriction and an increase in metabolic rate, whereas the hypothermic response at lower ambient temperature was associated with vasodilation and decreased metabolism. Morley et al. (1982) elicited a small decrease in temperature of rats with i.c.v. injection of somatostatin (10 pg), which was even less if given with TRH. Somatostatin did not appreciably affect changes in temperature induced by bombesin or neurotensin. Intracisternal administration of somatostatin 10 min after pentobarbital did not alter the hypothermic response to the barbiturate (Breese et al. 1975). However, a slight enhancement by i.p. somatostatin of pentobarbital-induced hypothermia has been reported in the mouse (Prange et al. 1975). E. Angiotensin II The major response to central administration of angiotensin in most of the species has been a fall in temperature; the monkey, when experiments were conducted in a hot environment, was an exception (Clark 1979). Later, Lin and coworkers (1980) reported that central injection of angiotensin to rats did not alter body temperature when the ambient temperature was 30°C but caused comparable dose-related hypothermia at lower ambient temperatures. The hypothermic response was inhibited by pretreatment with propranolol or by depletion of whole brain catecholamines with 6-hydroxydopamine. Depletion of brain serotonin by 5,6-dihydroxytyptamine did not inhibit the response to angiotensin, nor did prior administration of atropine or phentolamine. They 200 concluded that the hypothermic action of angiotensin II is due to jts effects on the mechanisms that promote reduced metabolism and increased heat loss. The heat loss effectors vary in different species. IV. KININS Small hyperthermic responses, which were associated with increased muscle tone, ear vessel vasodilation, and piloerection were inhibited by pretreatment with indomethacin and acetaminophen. These responses were recorded after lateral ventricular administration of bradykinin to rabbit (Almeida et al. 1978). However, i.c.v. administration of bradykinin to rat (Francesconi and Mager 1981) and to mouse (Nemeroff et al. 1979) did not alter body temperature. Similarly, substance P caused a small rise in temperature of rabbit when given in the third ventricle. This hyperthermic response was reduced by pretreatment with indomethacin, phenobarbital, or phentolamine but not by acetazolamide, atropine, capsaicin, or propranolol (Krupin et al. 1982). In the rat, substance P was consistently ineffective in altering temperature whether given i.c.v., i.v., or intracisternally at any ambient temperature. V. CONCLUDING REMARKS Attention has been focused on the role of neuropeptides in thermoregulation, because many of them are found within neuroanatomical sites important to temperature control and exert profound effects on body temperature. As with several other classes of putative neurotransmitters, the effect seen is dependent on species, ambient temperature, degree of restraint imposed on the subject, route of drug administration, and several other factors. For neuropeptides also the effect observed is dependent on several factors. A limiting factor has been the unavailability of selective pharmacological antagonists in many classes. Specific antisera to many peptides have, however, become available in recent years. The physiological relevance of a peptide to temperature control could be studied by inactivation of the endogenous peptide through local treatment with specific antibodies. There is evidence that certain peptides such as bombesin, which disrupt thermoregulation, have no physiological significance in temperature control (Clark and Lipton 1983). For many of the peptides, the data available are not yet adequate to determine their roles as mediators in central thermoregulation. As noted above, however, convincing data exist to support an antipyretic role for certain peptides, such as ACTH/MSH. To understand the physiological role of central peptides in thermoregulation, several methodological factors should be considered in future studies. The effect of peptides should be tested in animals exposed to cold, hot, and thermoneutral environments. This will make it possible to assess the functional nature of the peptide effect. Past research clearly reveals that 201 species differences do exist for the temperature responses obtained by the central administration of peptides. These may reflect either real differences in the utilization of specific peptides in temperature control or artifactual differences due to physical factors such as variation in spread of peptide to active sites after intracerebral injections. Many systems of the brain are involved in thermoregulation, and multiple contributions of a given neuropeptide to thermoregulatory control may lead to conflicting results when the peptide is injected into different brain regions. It is already known that endogenous peptide levels are affected by stress, and it has been shown that opiate-induced temperature responses are reversed by restraint stress. Stress may be reduced by avoiding restraint; in all studies, of course, appropriate use of control animals is essential to minimize misinterpretation of data, since stress can never be eliminated from the experiments with conscious animals. The route of administration also plays an important role. Thus it has been shown that intracerebroventricular administration of most agonists, including pu, x, and ¢ agonists, produced hyperthermia, possibly because mostly pu receptors are reached by that route (Geller et al. 1986). It is also important to recall that the thermoregulatory apparatus utilizes other major body systems (respiratory, cardiovascular, and others). Thus, for example, a centrally acting peptide that primarily affects the distribution of peripheral blood flow could secondarily alter body temperature and be thought erroneously to act directly on thermoregulatory controls. Direct actions on thermoeffector pathways can generally be discovered in experiments carried out in disparate thermal environments. These considerations underline one obvious conclusion: only through triangulation of information from experiments using different methods can the importance of a neuropeptide to thermoregulation be established. Techniques that are relatively new in this field, such as assay of peptides in brain samples taken from febrile, hypothermic, and hyperthermic animals, and immunoneutralization coupled with pyrogen administration or direct thermal challenge, can provide convincing evidence about the role of specific peptides in physiological control of body temperature. There are technical difficulties and other problems with these approaches, but there is little doubt about the advantages they provide. A second major question in research on neuropeptides is whether they may eventually have some clinical application. In the case of thermoregulation, as with several other functions, it is too early to predict. There is considerable hope, however, that applications will be found once the roles of central neuropeptides are understood. MWe speculate that the mechanism of action of temperature-altering agents such as pyrogens may be explainable in terms of alterations in central peptides. 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Effects of mammalian and avian neurotensins and neurotensin fragments on wet-dog shaking and body temperature in the rat. Regulatory Peptides 7:357-365, 1983. Wilkinson, M.F., and Kasting, N.W. Centrally applied vasopressin is antipyretic due to its effects on febrile set point. Proc IUPS 30th Congr 16(119.07):60, 1986. Zeisberger, E.; Merker, G.; and Blahser, S. Fever response in the guinea pig before and after parturition and its relationship to the antipyretic reaction of the pregnant sheep. Brain Res 212:379-392, 1980. Zeisberger, E.; Merker, G.; Blahser, S.; and Krannig, M. Changes in activity of vasopressin neurons during fever in the guinea pig. Neurosci Lett (suppl.)14:S414, 1983. AUTHORS Rakesh Shukla, Ph.D., Scientist Bhola N. Dhawan, M.D, F.N.A, F.A.M.S., Director Central Drug Research Institute Lucknow 226001, India 208 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D., eds. National Institute on Drug Abuse, 1988 Endogenous Opioids and Immune Responses: An Experimental Study P. K. Mediratta, M.D.; N. Das, Ph.D.; V. S. Gupta, B.Sc; and P. Sen, M.D., Ph.D. ABSTRACT Possible involvement of endogenous opioids in humoral immune responses has been explored in the experimental animals. Opioid agonists like morphine and leu-enkephalin significantly enhanced antigen-induced histamine release from the peritoneal mast cells of sensitised rats in vitro; this was effectively antagonised by naloxone. Naloxone itself inhibited antigen-induced histamine release. Animals were effectively protected against anaphylactic shock by naloxone which also antagonised morphine-induced increase in anaphylactic mortality. Naloxone reduced haemagglutination titre to sheep red blood cells and IgE antibody titre as measured by passive cutaneous anaphylaxis. Thus, endogenous opioids appear to be involved in the mediation of humoral immune responses. They seem to act at various steps in the immune mechanism viz (i) antibody production and (ii) release of mediators of hypersensitivity reactions. INTRODUCTION In the cities we live in, we are surrounded all over by a polluted atmosphere containing billions of heterogenous substances which are foreign to our system. Although most of us can withstand an onslaught by these agents, a considerable number of individuals respond violently and develop various types of immunological disorders. It is, however, not known why only some and not all persons respond violently to these offending substances. It has been reported that many psychosocial situations and stressful conditions can modify host resistance to a variety of illnesses including allergic and infectious disorders and influence the immune processes of an individual (Solomon and Amkraut 1981). Hypothalamus is known to be a centre for correlation and co- ordination of the autonomic and endocrinal activities with the emotions of an individual. Stein et al. (1976) observed that in sensitised animals lesion of the anterior hypothalamus produced significant protection against anaphylaxis, lowered the titre of the circulating antibodies, and also depressed the delayed type of 209 hypersensitivity reactions. Hypothalamus is rich in neurohormones and neurotransmitters, which may affect immune functions. Opioid peptides are one such group of hypothalamic neuropeptides. A num- ber of reports indicate that administration of opioids or opioid antagonists can modulate the immune competence (Lancet 1984). Hence, it was considered worthwhile to explore the possible role of endogenous opioids in immune responses. MATERIALS AND METHODS The experiments were carried out mainly on Wistar rats (100-150 gms) and Swiss mice (20-30 gms) of either sex. They were obtained from the local source and fed on Hind Lever Laboratory animal feed with water available ad 1ib. Animals were sensitised using egg albumin (EA) or sheep red blood cells (SRBC) as antigens. Freund's complete adjuvant and B. -pertussis yere used as adjuvants. The results were statistically analysed by Chi“ test or t test as appropriate. Acute Systemic Anaphylaxis In Mice Four groups of mice (15- > in each td were sensitised by injecting subcutaneously 0.2m] EA ( 25mg/m1) along with 0.5 m1 of triple antigen (containing 20,000 x 10°B. pertussis organisms) and 0.2 m1 of Freund's complete adjuvant. On the 12th day following sensitisation, control group received 0.2 m1 of normal saline; one group was given naloxone 10mg/kg i.p., second group received morphine in a dose of 10mg/kg i.p and third group was administered naloxone (10mg/kg) along with morphine (10mg/kg). Thirty minutes after the drug pretreatments all the groups were challenged with 0.2 ml EA i.v., and mortality was recorded after two hours. Histamine Release From The Peritoneal Mast Cells Of Sensitised Rats In Vitro Histamine release from the peritoneal mast cells was studied by the method of Chakravarty et al. (1973). Rats were sensitised by injecting subcutaneously 0.5 ml ER ( (25 mg/m1) along with 0.5 ml triple antigen (containing 20,000 x 10°B. pertussis organisms) and 0.5 m1 Freund's complete adjuvant. Rats were sacrificed by exsanguination on the 14th day; peritoneal cell suspensions were prepared and divided into 10-12 samples. Cells were usually pooled from two sensitised rats. Samples were treated with various drugs under olnvestigation (opioid agonists and antagonist) and incubated at 37°C under gentle shaking for 10 minutes. The antigen (0.5 mg/ml EA) was added to the cell suspension and the incubation, thereafter, continued for another tenminutes. The reaction was terminated by placing the samples in ice cold water. Adequate controls using agonists or antagonist alone were included. Histamine content of different samples was estimated by biological assay using isolated guinea pig ileum. Control histamine release as well as spontaneous release values were detected from the results. 210 Haemagglutination Titre To Sheep Red Blood Cells (SRBC) Two groups of 6 mice were immunized by injecting 1 x 109sRBC i.p. One group was given naloxone 5 mg/kg twice daily from day 1 to 5 and the control group received normal saline in the same schedule. Animals were bled on the 8th day and sera separated. Two fold dilutins (0.025m1) of the sera were made in the microtitre plates with normal saline. To each well 0.025 m1 of 1% (V/V) SRBC was added. The plates were incubated at 379C for one hour and then observed for haemagglutination. Passive Cutaneous Anaphylaxis This was studied in two groups of 6 rats sensitised with 0.5 m1_EA (25mg/m1) with 0.5 ml triple antigen (containing 20,000 x 10%8. pertussis organisms) and 0.5 ml of Freund's complete adjuvant subcutaneously. The test group received naloxone 5 mg/kg twice daily from day 1 to 5 while the control group received normal saline. Animals were bled on the 6th day and sera collected. Serial dilutions of the sera were made,and 0.1 m1 of different dilutions was injected into the shaven dorsal skin of normal rats. 72 hours later i.v. challenge was givenwith EA (0.5m1) and Evan's blue (1%,0.2m1) and blueing reaction at test site was observed after one hour. RESULTS Effect On Acute Systemic Anaphylaxis Pretreatment with naloxone (10mg/kg) significantly protected animals against anaphylactic shock; mortality was reduced from 56% in the control group to 32% «in the naloxone pretreated group (p£0.01). Morphine pretreatment (10mg/kg) enhanced anaphylactic mortality which was effectively antagonised by naloxone (p<0.001; Table 1). Effect On Antigen Induced Histamine Release Opioid agonists like morphine (100 uM) and leu-enkephalin (10 uM) significantly enhanced antigen induced histamine release from the peritoneal mast cells of sensitised rats in vitro; this enhancement was effectively antagonised by naloxone (Table 2(i) and 2(ii)). Naloxone (1 uM) pretreatment itself significantly inhibited antigen induced histamine release (p{0.01, Table 3). Effect On Haemagglutination Titre To SRBC In the control group in all the 6 i.e., 100% animals the detectable level of haemagglutination titre was between 1/128 and 1/2048. Pretreatment with naloxone reduced the detectable level of Dasmazgiuiination titreto1/2-1/161inall the 6 (100%) animals (Table 4). 211 TABLE 1. Effect of Naloxone and Morphine on Acute Systemic Anaphylactic Mortality in Mice Group No. of Sensitization (Day 12) % Animals (Day 0) Drug Pre- Chal- Mortality p treatment lenge 1 25 EA+DPT+FA Normal Saline EA 56.00 2 25 EA+DPT+FA Naloxone EA- 32.00 <0.01 10mg/kg I.P. 3 23 EA+DPT+FA Morphine EA 78.26 {0.01 10mg/kg I.P. 4 15 EA+DPT+FA Morphine 10mg/kg I.P. + EA 33.33 ¢0.001 Naloxone 10mg/kg I.P. EA- Egg albumin 0.2 m1(25mg/m1) DPT- Triple antigen 0.5 ml (containing 20,000,X 10%. pertussis organisms) FA- Freund's complete adjuvant 0.2 ml TABLE 2(i) Effect of Morphine and its Modification by Naloxone on the Antigen Induced Histamine Release from Peritoneal Mast Cells of Sensitized Rats in Vitro Expt. % Histamine Release No. Egg Albumin(EA) EA+Morphine EA+Morphine+Naloxone (0.5mg/m1) (100 uM) (1 uM) A B C 1. 16.0 31.6 4.4 2. 10.5 27-7 12.4 3 17.4 32.4 Z+3 A 31.7 39.4 21.7 The differences between columns Aand B (p €0.01) andBandC (p £0.01 are significant by t test for paired comparison. 212 TABLE 2(ii) Effect of Leu-enkephalin and its Modification by Naloxone on the Antigen Induced Histamine Release from Peritoneal Mast Cells of Sensitized Rats in Vitro Expt. % Histamine Release No. Egg Albumin(EA) EA+Leu-enkephalin EA+Leu-enkephalin+ (0.5mg/m1) (10 uM) Naloxone (1 uM) A B ¢ 1. 17.4 34.1 5.5 2. 10.5 24.0 12.0 3. 16.0 34.0 4.0 4. 31.7 49.6 6.7 The differences between columns A and B (p«0.001) and B and C (p<0.05) are significant by t test for paired comparison. TABLE 3. Effect of Naloxone on the Antigen Induced Histamine Release from the Peritoneal Mast Cells of Sensitized Rats in Vitro Expt. % Histamine Release No Egg Albumin (EA) EA+Naloxone (0.5 mg/ml) (1 uM) A B 1 11.9 4.3 2 33:3 3.7 3 16.0 5.0 4 10.5 0:5 5 17.4 6.7 6 31.7 10.6 The difference between columns A and B is significant (p<0.01) by t test for paired comparison. 213 Table 4. Effect of Naloxone on Haemagglutination Titre to Sheep Red Blood Cells (SRBC) in Mice Group Pretreatment No. of Antibody Detectable Level of Hae- Animals Not Det- magglutination titre ectable 1/2-1/64 1/128-1/2048 5 SRBC 6 0 0 6 (1x1071.P.) (100%) + Normal Saline (from day 1 to 5) 2; SRBC + Naloxone 6 0 6 0 (5mg/kg BD- (100%) from day 1 to 5) Animals were bled on 8th day after the sensitization with SRBC. Effect on Passive Cutaneous Anaphylaxis The detectable Tevel of IgE antibody in the control animals was between 1/1 - 1/10 in 33.33% and up to 1/100 in 66.67% of the animals. In the naloxone treated group, on the other hand, in 50% of the animals the antibodies could not be detected,while in 16.67% cases it ranged between 1/1 - 1/10 and up to 1/100 in 33.33% cases (Table 5). Discussion Hypothalamus and other areas of the brain have several neurotransmitters including endogenous opioids. Recently it has been reported that hypothalamus is activated by the immune system which by a feed back mechanismmay modulate the immune responses (Besedovsky and Sorkin 1977; Stein et al.1976). Opioid agonists and antagonists have been shown to modulate the immune competence (Lancet 1984). An agent may affect the immune system by acting at one or more than one step in the immune mechanism. Our experimental studies were confined to finding out the role of endogenous opioids in humoral immune responses inalbino rats and mice using egg albumin and sheep red blood cells as antigens and Freund's complete adjuvant and B. pertussis as adjuvants. In the initial experiments, role of opioids in acute systemic anaphylaxis was studied. Naloxone, an opioid antagonist when given in a dose of 10mg/kg i.p., significantly protected animals against anaphylactic shock. This corroborates the findings of Amir (1982) who showed that administration of naloxone and naltrexone provided a 214 TABLE 5. Effect of Naloxone on Passive Cutaneous Anaphylaxis in Rats Group Pretreatment No. of Antibody Detectable Level of IgE Animals Not Det- Antibody ectable 1/1-1/10 1/100 i. EA+DPT+FA 6 0 2 6 + (33.33%) (66.67%) Normal Saline (from day 1 to 5) 2. EA+DPT+FA + Naloxone 6 3 1 2 (5mg/kg BD- (50%) (16.67%) (33.33%) from day 1 to 5) EA- Egg albumin 0.5 m1 (25mg/m1) DPT- Triple antigen 0.5 ml (containing 20,000 x 10%. pertussis organisms) FA- Freund's complete adjuvant 0.5 ml significant protection against anaphylactic shock. Morphine, an opioid agonist, however, enhanced anaphylactic mortality which was effectively antagonised by naloxone (Table 1). The present findings that apparent blockade of opioid receptors protects against anaphylactic shock suggest a role for endogenous opioids in the pathophysiology of systemic anaphylaxis, a condition associated with antigen antibody interaction. To further elucidate the involvement of endogenous opioids in immune mechanisms, experiments were done to study the effect of opioids on histamine release, the latter being an important mediator of antigen- antibody reaction. Opioid agonists like morphine (a um receptor agonist) and leu-enkephalin (a delta receptor agonist) produced a significant increase in the antigen induced histamine release from the peritoneal mast cells of sensitised rats in vitro. This increase was effectively antagonised by naloxone (Table 2(i) and 2(i1)) suggesting thereby that the potentiating effect of opioid agonists on antigen induced histamine release is mediated by opioid receptors and both u and delta receptors appear to be involved. Involvement of u and delta opioid receptors has also been reported for IgE mediated serotonin release from rat mast cells (Yamasaki et al. 1982). Naloxone 'perse' also significantly inhibited antigen induced histamine release from peritoneal mast cells of sensitised rats in vitro (Table 3) indicating a role of endogenous opioids in the mediation of antigen induced histamine release. The protective effect of naloxone against anaphylactic shock observed in the present study (Table 1) could be because of its inhibitory effect on the mediator release. 215 Experiments were also done to find out the role of endogenous opioids on antibody production. Naloxone administration effectively reduced haemagglutination titre to SRBC inmice (Table 4),suggesting an effect on IgG and/IgM antibodies. Naloxone pretreatment also suppressed IgE antibody production as measured by passive cutaneous anaphylaxis in the present study. In the naloxone treated group antibody production was completely inhibited in 50% of the animals (Table 5). Thus, it is observed that apparent blockade of opioid receptors by naloxone suppressed formation of anti SRBC and IgE antibodies,i.e., endogenous opioids, appear to be involved in the synthesis of these immunoglobulins. In conclusion, the present findings suggest that endogenous opioids appear to be involved in the mediation of humoral immune responses. They seem to act at various steps in the immune mechanism viz(i) antibody productionand (ii) release of mediator s of hypersensitivity reactions. REFERENCES Amir, S. Opiate antagonists improve survival in anaphylactic shock. Eur J Pharmacol 80:161-162, 1982. Besedovsky, H.0., and Sorkin, E. Network of immune-neuroendocrine interactions. Clin Exp Immunol 27:1-12, 1977. Chakravarty, N.; Goth, A.; and Sen, P. Potentiation of dextran- induced histamine release from rat mast cells by phophotidyl serine. Acta Physiol Scand 88:469-480, 1973. Opiates, opioid peptides and immunity. Lancet 1:774-775, 1934. Solomon, G.F., and Amkraut, A.A. Psychoneuroendocrinological effects on the immune response. Annu Rev Microbiol 35:155- 184, 1981. Stein, M.; Schiavi, R.C.; and Camerino, M. Influence of brain and hepriaty on the Monae system. Science 191:435-440, 1976. Yamasaki, Y.; Sh} amura, 0.; Kizu, A.; Nakagawa, M.; and Ijichi,H IgE-mediated *“C-serotonin release from rat mast cells modula- ted by morphine and endorphins. Life Sci 31:471-478, 1982. AUTHORS P. K. Mediratta, M.D. N. Das, Ph.D. V. S$. Gupta, B.Sc. P. Sen, M.D., Ph.D. Department of Pharmacology University College of Medical Sciences New Delhi - 110 029, India 216 Opioid Peptides: An Update; NIDA Research Monograph 87 Rao S. Rapaka, Ph.D., and Bhola N. Dhawan, M.D., eds. National Institute on Drug Abuse, 1988 An Update of Selected Topics in the Biology and Chemistry of Opioid Peptides Rao S. Rapaka, Ph.D.; Bhola N. Dhawan, M.D.; and V. Renugopalakrishnan, Ph.D. The discovery of enkephalins by Kosterlitz and colleagues (Hughes et al. 1975) was immediately followed by an era of synthesis of a large number of opioid peptides. At present, a great deal of attention is being paid to conformational analysis, receptor biochemistry, mechanism(s) of action, addiction mechanisms, and physiological actions of opioids. The chemistry and biology of opioids have been extensively reviewed (Udenfriend and Meienhofer 1984; Rapaka 1986; Rapaka and Hawks 1986; Rapaka et al. 1986; Olson et al. 1987; Dhawan and Rapaka 1988). This article is intended to focus on selected topics only and is not a thorough review. More detailed information is available from the above reviews. In this article, the importance of using pure peptides and the need for extensive characterization of these peptides is emphasized. In addition, some of the recent advances in synthetic methodology, rationales for some of the newly synthesized p-, §-, and «- specific ligands, conformational properties of opioids, the role of lipids in conformational induction of ligands, and a few selected biological aspects (such as immunomodulation by opioids) are briefly discussed. Numerous opioid peptides have recently been synthesized and evaluated for various biological activities. In order to obtain dependable data, a pure compound is essential and purity of the compound cannot be overemphasized. Much more rigorous analytical testing should be undertaken for commercial samples and for those compounds that are synthesized by solid phase peptide synthesis. As there is no way of establishing absolute purity, as many criteria as possible should be employed to establish the purity of the product. If the peptide is synthesized in-house, the material is likely to be checked for purity at each stage and the end product is therefore likely to be pure. Due to the ready availability of new products from several commercial suppliers, and the facilities for custom synthesis, a large number of studies now utilize commercial samples. Recently, Brown et al. (1986) reported on the problems associated with commercial peptides. Samples of the tachykinin-related peptides were analyzed from several commercial sources. Some of the problems encountered were 217 these: (1) peptides had incorrect sequences; peptides might have an incorrect residue, or material supplied might be a mixture of the peptides; (2) peptide content varied as much as three- to sixfold; (3) for radiolabeled compounds, radioactivity might not be associated with the authentic substance. These findings indicate that results obtained with these compounds will make the data worthless and adequate quality control checks must be made for these compounds prior to their use. Amino acid analysis, sequencing data, TLC data in several systems, HPLC analysis in at least two solvent systems, elemental analysis, and any other pertinent physicochemical data should be obtained prior to their use. In addition, optical purity and radiochemical purity (in the case of using labeled products) of the peptides is also critical. A measure of optical rotation alone will not guarantee an optically pure product. Enzyme digestions (Rapaka et al. 1976, 1977) to establish the optical purity, along with utilization of synthetic methods that yield optically pure products, might be helpful. Radiochemical purity of the labeled product should be determined, and since some of the labeled products are unstable, chemical purity should also be determined prior to use. Batch-to-batch variation should always be monitored. This problem may be much more important with solid phase peptide synthesis than with synthetic material obtained from conventional methods. All batches should be compared with a reference standard batch. Recently, Taylor et al. (1986) reported that anomalous binding of DPDPE resulted due to batch variability, and the results from the impure batch indicated a two receptor model instead of a single receptor model. HPLC purification of the material yielded chromatographically pure compound and gave the predicted results. Hence, even a minor component can potentially lead to erroneous conclusions. The chemical complexity of peptides makes the analysis of peptides very difficult and demands utilization of innovative, extremely specific, and sensitive methods. In spite of the recent advances (Desiderio et al. 1986; Fridland and Desiderio 1987; Sternson 1987) in analytical techniques for the analysis of peptides, adequate methodology for the analysis of extremely small amounts of opioid peptides, their precursors and metabolites, is not currently available. FAB-MS and LC analysis is increasingly being utilized successfully in the area of peptide analysis (Canova-Davis et al. 1988). The development of solid phase peptide synthesis (SPPS) was instrumental in providing a large number of peptides for structure-activity studies. Following the development of solid phase peptide synthesis by Merrifield (1963), many other methods have been explored to simplify and to automate the synthesis. None of them have really been widely accepted. Recently, Houghten and colleagues have reported a modified solid phase method that is simple (Houghten 1985; Houghten et al. 1986a,b, 1988). This method permits simultaneous synthesis of up to 100 or more peptides 218 of up to 15 residues in length. The synthesis is fast, and these analogs can be synthesized within a month. No special equipment is needed, and the procedure is not labor-intensive. This method is referred to as the simultaneous multiple peptide synthesis (SMPS), and it involves placing the solid phase resin in a porous polypropylene packet. Several such packets (up to 100 or so) containing the protected amino acid resin can be deprotected together in a Nalgene bottle. Coupling steps are performed in different containers. After the coupling step, the resin packets are returned to the common reaction bottle and the synthesis is continued. At the end of the desired synthesis, the peptide can be cleaved utilizing an apparatus that permits simultaneous cleavage of several samples (up to 24). After the peptides are liberated from the resin, they are purified by routine methods. Thus SMPS permits the synthesis of a large number of peptides with reduced time and cost, and it appears to be suitable for the synthesis and evaluation of a large number of analogs for structure-activity studies. Another interesting approach to obtain complex and difficult-to- synthesize peptides for structure-activity studies is through the expression of synthetic genes (for a review, see Taylor, this volume). Standard methods of peptide synthesis, either conventional or solid phase methods, are too cumbersome for the preparation of large numbers of peptides, their deletion analogs, and analogs incorporating natural and unnatural amino acid residues. The approach of utilizing synthetic genes and recombinant DNA technology is an attractive alternative to conventional peptide synthesis. This involves synthesis of the desired oligonucleotide sequence and preparation of mutant gene coding for the desired analogs followed by expression. Mutagenesis of the synthetic gene code of the natural structure is the critical step in the generation of the analogs. Mutagenesis may be induced in either a random or a more controlled fashion. Chemicals such as hydrazine, nitrous acid, and sodium bisulfite have been used, as well as physical methods, such as UV irradiation. Other methods include purposeful introduction of one or more restriction enzyme recognition sites to achieve chosen mutations and oligonucleotide directed mutagenesis. Oligotide directed mutagenesis appears to be the most commonly used, and the phosphorothiate DNA method for mutagenesis is one of the most efficient methods to achieve an oligonucleotide directed mutagenesis. Methodologies for the expression of the synthetic gene and purification of the product have been reviewed extensively (see Marston 1986). Numerous p-, 8§-, and k- selective opioid analogs have been synthesized, and several reviews have already appeared (Morley 1980; Hansen and Morgan 1984; Morley and Dutta 1986; Udenfriend and Meienhofer 1984). Here, some of the recently synthesized analogs are discussed briefly. One of the usual approaches was "conformational restriction" by cyclization. Synthetic analogs, H-Tyr-Cyclo [-D-Apbu-Gly-Phe-Leu-1 (DiMaio and Schiller 1980; DiMaio et al. 1982), homologs containing amino acid residues of 219 varying chain lengths in position 2 (Schiller et al. 1985; Schiller 1986), and related retro-inverso homologs (Berman et alN 1983) were p-selective compounds. Later, a cyclic tetrapeptide H-Tyr-D-Orn-Phe-Asp-NH» rE EER was designed by Schiller et al. (1985), and pharmacological characterization revealed that it was one of the most u-selective compounds. Another approach to the development of p-receptor specific peptides was utilized by Hruby and colleagues (1988). In this approach, a synthetic analog related to the somatostatin fragment, D-Phe-Cys-Phe-D-Trp-Lys-Thr-Cys-Thr(ol), which interacts weakly with opioid receptors as well, was utilized as a template to the development of opioid ligands of high receptor affinity. Following a detailed structure-activity study, a number of p-receptor selective analogs, such as H-D-Phe-Cys-Tyr-D-Trp-Lys-Thr-Pen-Thr-NH, (CTP), ed were developed. Some of these analogs exhibited decreased affinity for somatostatin binding and a high u/§ specificity. This template was further extended to analogs containing tetrahydroisoquinoline moieties. This represents a successful manipulation for modulation of one major physiological activity into another activity. Conformational studies on these analogs might shed light on conformation-receptor selectivity relationships. Recently, novel u-selective analogs with antagonist activity were reported by Judd et al. (1987). The analogs were obtained by modifications of the Tyr] residues of D-AlaZ-Metd- enkephalinamide, and the modified tyrosine residues were m-Tyr, B-methyl-m-Tyr, oa, B-dimethyl-Tyr and N-phenethyl-m-Tyr. Biological evaluation of these analogs revealed that (1) shifting of phenolic-OH from the ortho to meta position enhanced relative antagonist activity, (2) addition of B-CH3 to m-Tyr enhanced p-selectivity, (3) analogs with u-selectivity had a common energy accessible 2-3 B 11' turn, (4) a, B-dimethyl-m-OH, Tyr!-analog had a low affinity and an N-phenylethyl analog was a pure antagonist. A rationale for design of peptides based on structural comparison to an opiate compound [3-(m-OH phenyl)-piperidine] was presented. One of the earliest successful syntheses of receptor-selective ligands was that of a s-receptor specific compound, D-PenZ, D-Pend-enkephalin. Two other examples of §-selective analogs are linear hexapeptides, DTLET and DSLET, and these analogs have been extensively used as §-receptor probes. Recently, Roques and colleagues reported the synthesis of analogs of 220 H-Tyr-Ser-Gly-Phe-Leu-Thr-OH and H-Tyr-Thr-Gly-Phe-Leu-Thr-OH (Delays Goyet et al. 19857. The three analogs reported are [D- Ser? (O-t-butyl), Leu? 1 enkephalinyl-Thrb, DSTBULET; [D-Ser2(0-t- buLyls, Leud] Snkephainyl- Thrb (o-t-butyl), BUBU; and [D-Thr2(0-t-butyl), Leu3l-enkephalinyl-Thr DTTBULET. DSTBULET displays a higher affinity Far rat brain membrane preparation than DSLET and [D-PenZ, Pen3] enkephalin. DSTBULET has a high specific binding, and it is resistant to degradation by peptidases present in the crude rat brain membrane preparation (a typ of 1 hr, compared to t 1,2 of 10 min for Met-enkephalin). BUBU is an even more selective §-receptor ligand. However, DTTBULET is an inactive ligand. These ligands are apparently influenced by the large conformational changes induced by the bulky t-butyl groups. It was suggested that these analogs are better probes, as the other two §-selective analogs, DPDPE and DPLPE, although highly §-receptor specific, have variable affinity depending on the preparation, toxic effects are exhibited at higher concentrations, and more important, have comparatively lower affinity for the receptor site. Although a large number of p- and &-selective peptides have already been reported, very few k-receptor selective peptide ligands have been reported to date. Recently, Schiller et al. (1988) i GL conformationally restricted dynorphin analogs such as [D-Orn Asp? l-dynorphin A-(1-8). However, these peptides are no long k-receptor selective, but u-receptor selective. This led the authors to hypothesize that these cyclizations resulted in overall folded conformations, which are incompatible with the conformational requirements of the k-receptor. Conformational aspects of the peptides are being actively investigated to help design potent and receptor specific compounds, and to understand conformation-receptor selectivity relationships. TH NMR studies were performed on a number of §-selective penicillamine-containing enkephalin analogs by Mosberg and colleagues (Mosberg 1987; Mosberg et al. 1987). Discrepancies of conformation-dependent NMR parameters between DPDPE and DPLPE (which have similar &-selectivities) were observed. It appears that the Gly residue is flexible and as such plays a crucial role, altering its local conformation to allow similar spatial relationships between key groups in different analogs leading to §-affinity. From NMR data, conformational features of DPDPE and DCDPE appear very similar. However, DPDPE is much more §-selective and less potent as compared yith DCDPE. This suggests that gem-dimethyl groups of Pen in DPDPE lead to adverse reaction. The adverse steric reaction may be much greater at p-sites than at &-receptor sites. Studies on the ring expanded analogs of DPDPE and DPLDPE revealed that increasing the ring size led to a reduction in &-receptor selectivity and that expanded conformations favored p-receptor binding, whereas compact conformations are favorable for &-receptor binding. Analogs containing bulky t-Leu residue(s) revealed that bulky substituents at residue 2 decrease affinity to §-receptors and even more so to p-receptors. 221 In a related study by Belleney et al. (1987), conformational properties of DTLET, (H-Tyr-D-Thr-Gly-Phe-Leu-Thr-OH), and D-Pen2, L-PenS-enkephalin (DPLPE) were determined by 'H NMR spectroscopy. The results, surprisingly, indicated similarities in the overall structure for the two-folded backbone conformations for the constrained DPLPE and the flexible peptide DTLET. Relative orientations of the Tyr and Phe residues were found to be similar. Interestingly, the Tyr-Phe distance was 10 AO for both the peptides, which reflects a quasilinear backbone orientation. This extended conformation may be associated with §-receptor selectivity. From these studies it was hypothesized that incorporation of sterically bulky residues at positions 2 and/or 6 in DSLET and DTLET would reinforce structural analogy to DPDPE-1ike peptides, thus leading to inhibition of u-receptor binding. However, this should still permit §-receptor affinity due to the inherent flexibility of the linear hexapeptide. The above hypothesized analogs have been recently synthesized and were shown to have high affinity as well as high selectivity for the §-receptor (Delay-Goyet et al. 1988). In spite of a large number of studies, conformation-receptor selectivity relationships are not adequately understood. The role of the lipid phase of the membrane for the facilitation of ligand-receptor interaction has been addressed earlier (Schwyzer et al. 1982; Gysin and Schwyzer 1983; Erne et al. 1985; Sargent and Schwyzer 1986; Schwyzer 1986). Erne et al. (1985) demonstrated that interaction of dynorphin A-(1-13) with the lipid membrane results in the formation of an a-helix at the N-terminal (from 1-9, and helix formation beyond the 9th residue is inhibited by Pro 10). The N-terminal message portion is perpendicularly inserted into the hydrophilic membrane. Recently conformational features of dynorphin A-(1-13) and interaction of dynorphin A-(1-13) with lipids were investigated by Renugopalakrishnan and colleagues (Rapaka et al. 1987; Huang et al. 1988; Renugopalakrishnan et al. 1988a,b; Renugopalakrishnan and Rapaka 1988) utilizing NMR, CD, FT-IR and Raman spectroscopy. These studies indicated that in aqueous solution dynorphin has an open structure, and the segment Argg-Arg7-Ile-Argg- manifests considerable side chain mobility on the NMR time scale and N-terminal segment may be disordered. In the presence of lipid, a steep increase in molar ellipticity value starting at Apgonm indicated a large conformational change. This is consistent with the observations of Erne et al. (1985). Recently, Schwyzer (1986) estimated the conformation, orientation, and accumulation of dynorphin A-(1-13) on the surface of lipid membrane. Schwyzer used a-helical conformation of dynorphin as the most stable conformation interacting with the hydrophilic phase. He calculated the Gibbs free energy, AG for the transfer of increasing number, m, of n-terminal residues from "random" coil conformation in water to a-helical conformation in the hydrophobic phase to predict the preferred conformation of dynorphin and its orientation and accumulation on the surface of neutral lipid membrane. A model of dynorphin was derived in which the hydrophobic segments of the 222 lipid were in contact with the a-helical segment and the "random" coil segment was protruding into the aqueous phase. This ingenious study presents a plausible explanation of the events leading to the observed interaction of dynorphin A-(1-13). The role of neuropeptides in general, and of opioid peptides in particular, is being increasingly studied in the regulation of the immune system, as the neuropeptides appear to be agents of communication between the immune system and the brain (for reviews, see Morley et al. 1987; Plotnikoff et al. 1986a). ACTH suppresses y-interferon production (Johnson et al. 1984), VIP inhibits the egress of small lymphocytes (Moore 1984), substance P is chemotactic and cross-reacts with the chemotactic receptor of rabbit neutrophils (Marasco et al. 1981; Ruff et al. 1985; Payan et al. 1983), and somatostatin inhibits the proliferation of T-lymphocytes (Payan et al. 1984). Thus, the studies to date indicate that the neuropeptides may play an important role in immunomodulation and that such modulation may involve the central nervous system, the endocrine system, and the autonomic nervous system (Plotnikoff et al. 1985; Morley et al. 1987; Wybran 1985; Donohoe et al. 1985; Blalock and Smith 1985). Two interesting and independent observations, one by Wybran et al. (1979) demonstrating the presence of morphine-like and MetS-enkephalin-like receptors on blood lymphocytes, and the other by Hazum et al. (1979) demonstrating the presence of B-endorphin receptors on lymphoblastoid cells, generated a great deal of interest on the role of opioid peptides in immunoregulation. Human blood T cells have receptors for morphine and enkephalins, whereas B cells have receptors for B-endorphin, and T and B cell involvement may be a critical factor in generating an immune response. For researchers in the drug abuse area, study of the role of morphine and other opiates might yield clues to the higher incidence of bacterial and viral infections in opiate addicts. It has been shown that morphine decreases the ability to eradicate infections (Tubaro et al. 1983; for a minireview, see Yahya and Watson 1987). Morphine injections into lateral ventricles suppress natural killer cell activity (Shavit et al. 1986), and heroin addicts have decreased T-lymphocyte activity (Singh et al. 1980), thus suggesting that prolonged abuse of opiates impairs the immune system. On the other hand, enkephalins have been shown to prolong the survival time of tumor-bearing mice, enhance lymphocyte blastogenesis in mice, increase size of thymus in mice, and, in humans, to show significant increase in active T cell rosettes and increase natural killer (NK) cell activity (Plotnikoff et al. 1985). Similarly, B-endorphin enhances NK activity and active T cell rosettes. The enhancement of NK cell activity is important for defense against bacterial and viral infections. Here it is interesting to note that the NK cell stimulating ability appears to be associated with the N-terminal sequence of B-endorphin (Kay et al. 1983). In addition, both MetS-enkephalin and B-endorphin enhance interferon production (Mandler et al. 1986). 223 Morphine depresses T cell E-rosetting (Donohoe et al. 1985), and it was shown by Tubaro et al. (1983) that polymorphonuclear cell activity for phagocytosis and superoxide radical production by polymorphonuclear cells are depressed. In contrast, B-endorphin and dynorphin enhance superoxide radical formation (Sharp et al. 1985). It is very interesting that the opiates and opioid peptides act similarly at the analgesic receptors, where they appear to mediate different immunologic responses. It is worthwhile that a large number of opiates and opioid peptide analogs be tested for their actions on the immune system and to develop SAR relationships that will lead to the design of therapeutically useful peptide drugs. This is particularly interesting in terms of initial encouraging results obtained with methionine enkephalin in the treatment of AIDS patients (Plotnikoff et al. 1986b). It appears that there is an exciting possibility of obtaining new leads for management of this condition from centrally acting peptides. Awareness of the important role opioid peptides may be playing in regulation/modulation of physiological activities/behavior has been increasing. There also appears to be a close interaction between the enkephalins and other naturally occurring peptides and other putative neurotransmitters like dopamine (Radhakishun et al. 1988) and 5-HT (Foster and Roberts 1988). It should be rewarding to study the interaction with other neurotransmitters, particularly the biogenic amines, in greater detail. Among the central autonomic activities possibly regulated by the opioid peptides, the effects on cardiovascular regulation (Said 1987) and thermoregulation (Shukla and Dhawan, this volume) appear to be particularly significant. The role in reaction to stress has been extensively studied, the initial studies having been undertaken with morphine. The recent work has been reviewed by Olson et al. (1987). There is evidence that some of the central effects of clonidine and central antihypertensives like centhaquin may be mediated via the opioid receptors (Srimal et al. 1988). Phencyclidine may be exerting some of its effects via pu- or x-receptors, particularly its effects on body temperature (Hiramatsu et al. 1986) . In the past few years, considerable data have been generated on the role of opioid peptides in the control of eating, which is stimulated by opioid agonists (Majeed et al. 1986) in several species (Kavaliers and Hirst 1986; Yirmiya et al. 1986), as well as that of fluid intake, perhaps through a homeostatic control of water balance (Spencer et al. 1986). It is interesting to note that their effects may depend on the taste. Thus agonists were reported to enhance eating of palatable foods (Jackson and Cooper 1986). This behavior could be suppressed by naltrexone (Kirkham et al. 1986), which also lowered pleasure rating for sweet food and selected odors (Fantino et al. 1986). The possible role of opioids in pathogenesis of several functional disorders of gut has been reviewed by Dhawan et al. (1988). 224 Recent evidence indicates an important role of opioid systems in the regulation of sexual behavior in both sexes. Initial reports suggest an inhibitory effect of opioid peptides on male sexual behavior via the medial preoptic area (Band et al. 1986), but if the male sex drive is low they may mediate rewards of sex (Miller and Baum 1986). They also mediate sexual behavior in the female, particularly the proceptive behavior (Wiesner et al. 1986), and interaction with 5 HT in such regulatory effects has been suggested (Allen et al. 1986). There are several neurological disorders in whose etiology opioid peptides may be involved (Dhawan et al. 1988). More definitive data need to be generated in these disorders, but a major limiting factor is the nonavailability of suitable animal models for conditions such as Alzheimer's disease. There is an urgent need also to develop suitable models for neurodegenerative disorders, nerve injury, and other neurological conditions (Taylor et al. 1987). It will be useful to develop sensitive in vitro bioassay systems involving critical biochemical parameters having predictive capabilities. With the increased availability of data in species other than the rat and mouse, it has become abundantly clear that significant species differences do exist in the effects of opioid agonists, and these help in better understanding of their possible physiological roles. Several investigators have in recent years included multiple species in their studies (Davis et al. 1986; Fanselow and Sigmundi 1986) to assess the central roles of peptides. Recently, studies have been extended, not only to other species of laboratory animals and nonhuman primates, but also to insects, fish, and some unnatural ones like the bat, deer mice, and ground squirrel (Shukla et al. 1988; see Olson et al. 1987 for additional references). It is difficult to explain some of the results obtained with the opioids based on the currently available data, but more comparative studies are indicated. It is also necessary to extend studies to different age groups of animals, since age-related changes in modification of stress responses (Iny et al. 1986) as well as analgesia (Hoskins et al. 1986) have been reported. It is therefore important to carry out carefully controlled studies before drawing firm conclusions regarding various regulatory roles being assigned to opioid peptides. A great deal of research work has been carried out during the past decade on opioids, and yet the mechanisms of their various biological actions are far from clear. 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Opioid Peptides: Biology, Chemistry and Genetics. Orlando, FL: Academic Press, 1984. pp. 410. Wiesner, J.B.; Dudley, C.A.; and Moss, R.L. Effect of B-endorphin on sociosexual proclivity in a choice paradigm. Pharmacol Biochem Behav 24:507-511, 1986. Wybran, J.; Appelboom, T.; and Famaey, J.P. Suggestive evidence for receptors for morphine methionine-enkephalin on normal and human blood T lymphocytes. J Immunol 123:1068-1070, 1979. Wybran, J. Enkephalins and endorphins as modifiers of the immune system : Present and future. Fed Proc 44:92-94, 1985. Yahya, M.D., and Watson, R.R. Minireview: Immunomodulation by morphine and marijuana. Life Sci 41:2503-2510, 1987. Yirmiya, R.; Holder, M.D.; and Garcia, J. Effects of naloxone and cholecystokinin on food and water intake in the Brattleboro rat. Soc Neurosci Abstr 12:1491, 1986. AUTHORS Rao S. Rapaka, Ph.D. 10A-13, National Institute on Drug Abuse 5600 Fishers Lane Rockville, Maryland 20857 U.S.A. Bhola N. Dhawan, M.D. Director, Central Drug Research Institute Chattar Manzil P.0. Box 173 Lucknow 226001, India V. Renugopalakrishnan, Ph.D. Laboratory for the Study of Skeletal Disorders and Rehabilitation Department of Orthopaedic Surgery Harvard Medical School and Children's Hospital ENDERS-1220 300 Longwood Avenue Boston, Massachusetts 02115 U.S.A. 232 National Institute on Drug Abuse 2arch MONOGRAPH SERIES While limited supplies last, single copies of the monographs may be obtained free of charge from the National Clearinghouse for Alcohol and Drug Information (NCADI). Please contact NCADI also for information about availability of coming issues and other publications of the National Institute on Drug Abuse relevant to drug abuse research. Additional copies may be purchased from the U.S. Government Printing Office (GPO) and/or the National Technical Information Service (NTIS) as indicated. NTIS prices are for paper copy. Add $3.00 handling charge for each order. 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Ludford, M.S., eds. A RAUS Review Report. GPO out of stock NCADI out of stock NTIS PB #82-148198/AS $21.95 40 ADOLESCENT MARIJUANA ABUSERS AND THEIR FAMILIES. Herbert Hendin, M.D., Ann Pollinger, Ph.D., Richard Ulman, Ph.D., and Arthur Carr, Ph.D. NCADI out of stock GPO out of stock NTIS PB #82-133117/AS $21.95 42 THE ANALYSIS OF CANNABINOIDS IN BIOLOGICAL FLUIDS. Richard L. Hawks, Ph.D., ed. GPO out of stock NTIS PB #83-136044/AS $21.95 44 MARIJUANA EFFECTS ON THE ENDOCRINE AND REPRODUCTIVE SYSTEMS. Monique C. Braude, Ph.D., and Jacqueline P. Ludford, M.S., eds. A RAUS Review Report. NCADI out of stock GPO out of stock NTIS PB #85-150563/AS $21.95 45 CONTEMPORARY RESEARCH IN PAIN AND ANALGESIA, 1983. Roger M. Brown, Ph.D.; Theodore M. Pinkert, M.D., J.D.; and Jacqueline P. Ludford, M.S., eds. A RAUS Review Report. NCADI out of stock GPO out of stock NTIS PB #84-184670/AS $15.95 46 BEHAVIORAL INTERVENTION TECHNIQUES IN DRUG ABUSE TREATMENT. John Grabowski, Ph.D.; Maxine L. Stitzer, Ph.D., and Jack E. Henningfield, Ph.D., eds. NCADI out of stock GPO out of stock NTIS PB #84-184688/AS $21.95 47 PREVENTING ADOLESCENT DRUG ABUSE: INTERVENTION STRATEGIES. Thomas J. Glynn, Ph.D.; Carl G. Leukefeld, D.S.W.; and Jacqueline P. Ludford, M.S., eds. A RAUS Review Report. GPO Stock #017-024-01180-1 $5.50 NTIS PB #85-159663/AS $28.95 234 48 MEASUREMENT IN THE ANALYSIS AND TREATMENT OF SMOKING BEHAVIOR. John Grabowski, Ph.D., and Catherine S. Bell, M.S., eds. GPO Stock #017-024-01181-9 $4.50 NCADI out of stock NTIS PB #84-145184/AS $21.95 50 COCAINE: PHARMACOLOGY, EFFECTS, AND TREATMENT OF ABUSE. John Grabowski, Ph.D., ed. GPO Stock #017-024-01214-9 $4 NTIS PB #85-150381/AS $21.95 51 DRUG ABUSE TREATMENT EVALUATION: STRATEGIES, PROGRESS, AND PROSPECTS. Frank M. Tims, Ph.D., ed. GPO Stock #017-024-01218-1 $4.50 NTIS PB #85-150365/AS $21.95 52 TESTING DRUGS FOR PHYSICAL DEPENDENCE POTENTIAL AND ABUSE LIABILITY. Joseph V. Brady, Ph.D., and Scott E. Lukas, Ph.D., eds. GPO Stock #017-024-01204-1 $4.25 NTIS PB #85-150373/AS $21.95 53 PHARMACOLOGICAL ADJUNCTS IN SMOKING CESSATION. John Grabowski, Ph.D., and Sharon M. Hall, Ph.D., eds. NCADI out of stock GPO Stock #017-024-01266-1 $3.50 NTIS PB #89-123186/AS $21.95 54 MECHANISMS OF TOLERANCE AND DEPENDENCE. Charles Wm. Sharp, Ph.D., ed. GPO out of stock NTIS PB #89-103279/AS $36.95 55 PROBLEMS OF DRUG DEPENDENCE, 1984: PROCEEDINGS OF THE 46TH ANNUAL SCIENTIFIC MEETING, THE COMMITTEE ON PROBLEMS OF DRUG DEPENDENCE, INC. Louis S. Harris, Ph.D., ed. NCADI out of stock GPO out of stock NTIS PB #89-123194/AS $42.95 56 ETIOLOGY OF DRUG ABUSE: IMPLICATIONS FOR PREVENTION. Coryl LaRue Jones, Ph.D., and Robert J. Battjes, D.S.W., eds. GPO Stock #017-024-01250-5 $6.50 NTIS PB #89-123160/AS $28.95 57 SELF-REPORT METHODS OF ESTIMATING DRUG USE: MEETING CURRENT CHALLENGES TO VALIDITY. Beatrice A. Rouse, Ph.D., Nicholas J. Kozel, M.S., and Louise G. Richards, Ph.D., eds. GPO Stock #017-024-01246-7 $4.25 NTIS PB #88-248083/AS $21.95 58 PROGRESS IN THE DEVELOPMENT OF COST-EFFECTIVE TREATMENT FOR DRUG ABUSERS. Rebecca S. Ashery, D.S.W., ed. GPO Stock #017-024-01247-5 $4.25 NTIS PB # to be assigned 59 CURRENT RESEARCH ON THE CONSEQUENCES OF MATERNAL DRUG ABUSE. Theodore M. Pinkert, M.D., J.D., ed. GPO Stock #017-024-01249-1 $2.50 NTIS PB # to be assigned 60 PRENATAL DRUG EXPOSURE: KINETICS AND DYNAMICS. C. Nora Chiang, Ph.D., and Charles C. Lee, Ph.D., eds. GPO Stock #017-024-01257-2 $3.50 NTIS PB # to be assigned 61 COCAINE USE IN AMERICA: EPIDEMIOLOGIC AND CLINICAL PERSPECTIVES. Nicholas J. Kozel, M.S., and Edgar H. Adams, M.S., eds. GPO Stock #017-024-01258-1 $5 NTIS PB #131866/AS $28.95 235 62 NEUROSCIENCE METHODS IN DRUG ABUSE RESEARCH. Roger M. Brown, Ph.D., and David P. Friedman, Ph.D., eds. GPO Stock #017-024-01260-2 $3.50 NTIS PB #130660/AS $21.95 63 PREVENTION RESEARCH: DETERRING DRUG ABUSE AMONG CHILDREN AND ADOLESCENTS. Catherine S. Bell, M.S., and Robert J. Battjes, D.S.W., eds. GPO Stock #017-024-01263-7 $5.50 NTIS PB #89-103287/AS $28.95 64 PHENCYCLIDINE: AN UPDATE. Doris H. Clouet, Ph.D., ed. GPO Stock #017-024-01281-5 $6.50 NTIS PB #89-131858/AS $28.95 65 WOMEN AND DRUGS: A NEW ERA FOR RESEARCH. Barbara A. Ray, Ph.D., and Monique C. Braude, Ph.D., eds. GPO Stock #017-024-01283-1 $3.25 NTIS PB #89-130637/AS $21.95 66 GENETIC AND BIOLOGICAL MARKERS IN DRUG ABUSE AND ALCOHOLISM. Monique C. Braude, Ph.D., and Helen M. Chao, Ph.D. eds. GPO Stock #017-024-01291-2 $3.50 NCADI out of stock NTIS PB # to be assigned 68 STRATEGIES FOR RESEARCH ON THE INTERACTIONS OF DRUGS OF ABUSE. Monique C. Braude, Ph.D., and Harold M. Ginzburg, M.D.,J.D., eds. GPO Stock #017-024-01296-3 $6.50 NTIS PB # to be assigned 69 OPIOID PEPTIDES: MEDICINAL CHEMISTRY. Rao S. Rapaka, Ph.D.; Gene Barnett, Ph.D.; and Richard L. Hawks, Ph.D., eds. GPO Stock #017-024-1297-1 $11 NTIS PB # to be assigned 70 OPIOID PEPTIDES: MOLECULAR PHARMACOLOGY, BIOSYNTHESIS, AND ANALYSIS. Rao S. Rapaka, Ph.D., and Richard L. Hawks, Ph.D., eds. GPO Stock #017-024-1298-0 $12 NTIS PB # to be assigned 71 OPIATE RECEPTOR SUBTYPES AND BRAIN FUNCTION. Roger M. Brown, Ph.D.; Doris H. Clouet, Ph.D.; and David P. Friedman, Ph.D., eds. GPO Stock #017-024-01303-0 $6 NTIS PB # to be assigned 72 RELAPSE AND RECOVERY IN DRUG ABUSE. Frank M. Tims, Ph.D., and Carl G. Leukefeld, D.S.W., eds. GPO Stock #017-024-01302-1 $6 NTIS PB # to be assigned 73 URINE TESTING FOR DRUGS OF ABUSE. Richard L. Hawks, Ph.D., and C. Nora Chiang, Ph.D., eds. GPO Stock #017-024-1313-7 $3.75 NTIS PB # to be assigned 74 NEUROBIOLOGY OF BEHAVIORAL CONTROL IN DRUG ABUSE. Stephen I. Szara, M.D., D.Sc., ed. GPO Stock #017-024-1314-5 $3.75 NTIS PB # to be assigned 75 PROGRESS IN OPIOID RESEARCH. PROCEEDINGS OF THE 1986 INTER- NATIONAL NARCOTICS RESEARCH CONFERENCE. John W. Holaday, Ph.D.; Ping-Yee Law, Ph.D.; and Albert Herz, M.D., eds. GPO Stock #017-024-01315-3 $21 Not available from NTIS 236 76 PROBLEMS OF DRUG DEPENDENCE, 1986. PROCEEDINGS OF THE 48TH ANNUAL SCIENTIFIC MEETING, THE COMMITTEE ON PROBLEMS OF DRUG DEPENDENCE, INC. Louis S. Harris, Ph.D., ed. GPO Stock #017-024-1316-1 $16 NTIS PB #88-208111/AS $44.95 77 ADOLESCENT DRUG ABUSE: ANALYSES OF TREATMENT RESEARCH. Elizabeth R. Rahdert, Ph.D., and John Grabowski, Ph.D., eds. GPO Stock #017-024-1348-0 $4 NTIS PB #89-125488/AS $21.95 78 THE ROLE OF NEUROPLASTICITY IN THE RESPONSE TO DRUGS David P. Friedman, Ph.D., and Doris H. Clouet, Ph.D., eds. GPO Stock #017-024-01330-7 $6 NTIS PB #88-245683/AS $25.95 79 STRUCTURE-ACTIVITY RELATIONSHIPS OF THE CANNABINOIDS Rao S. Rapaka, Ph.D., and Alexandros Makriyannis, Ph.D., eds. GPO Stock #017-024-01331-5 $6 NTIS PB #89 109201/AS. $25.95 80 NEEDLE SHARING AMONG INTRAVENOUS DRUG ABUSERS: NATIONAL AND INTERNATIONAL PERSPECTIVES. Robert J. Battjes, D.S.W., and Roy W. Pickens, Ph.D., eds. GPO Stock #017-024-01345-5 $5.50 NTIS PB #88-236138/AS $25.95 81 PROBLEMS OF DRUG DEPENDENCE, 1987. PROCEEDINGS OF THE 49TH ANNUAL SCIENTIFIC MEETING, THE COMMITTEE ON PROBLEMS OF DRUG DEPENDENCE, INC. Louis S. Harris, Ph.D., ed. GPO Stock #017-024-01354-4 $17 NTIS PB $89 109227/AS $50.95 82 OPIOIDS IN THE HIPPOCAMPUS. Jacqueline F. McGinty, Ph.D., and David P. Friedman, Ph.D. eds. GPO Stock #017-024-01344-7 $4.25 NTIS PB #88-245691/AS $19.95 83 HEALTH HAZARDS OF NITRITE INHALANTS. Harry W. Haverkos, M.D., and John A. Dougherty, Ph.D., eds. GPO Stock #017-024-01351-0 $3.25 NTIS PB #89-125496/AS $21.95 84 LEARNING FACTORS IN SUBSTANCE ABUSE. Barbara A. Ray, Ph.D., ed. GPO Stock #017-024-01353-6 $6 NTIS PB #89-125504/AS $28.95 85 EPIDEMIOLOGY OF INHALANT ABUSE: AN UPDATE. Raquel A. Crider, Ph.D., and Beatrice A. Rouse, Ph.D., eds. GPO Stock #017-024-01360-9 $5.50 NTIS PB #89-123178/AS $28.95 86 COMPULSORY TREATMENT OF DRUG ABUSE: RESEARCH AND CLINICAL PRACTICE. Carl G. Leukefeld, D.S.W., and Frank M. Tims, Ph.D., eds. GPO Stock #017-024-01352-8 $7.50 NTIS PB # to be assigned 88 MECHANISMS OF COCAINE ABUSE AND TOXICITY. Doris H. Clouet, Ph.D., Khursheed Asghar, Ph.D., and Roger M. Brown, Ph.D., eds. GPO Stock #017-024-01359-5 $11 NTIS PB #89-125512/AS $36.95 89 BIOLOGICAL VULNERABILITY TO DRUG ABUSE. Roy W. Pickens, Ph.D., and Dace S. Svikis, B.A., eds. GPO Stock #017-022-01054-4 $5 NTIS PB #89-125520/AS $21.95 237 (39 U. C. BERKELEY LIBRARIES CO041kL43900 TT | 3 h® ra ils a ' . . Fr | Ee . . a) . Es FY wo: mph sf E. BE SERN