Tyr-W-MIF-1 Attenuates Down-Regulation of Opiate Receptors in SH-SY5Y Human Neuroblastoma Cells

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MORPHINE
NALOXONE

Vol. 284, Issue 2, 611-617, February 1998

Tyr-W-MIF-1 Attenuates Down-Regulation of Opiate Receptors in SH-SY5Y Human Neuroblastoma Cells¹

Laura M. Harrison, Abba J. Kastin and James E. Zadina

Tulane University School of Medicine and Veterans Affairs Medical Center, New Orleans, Louisiana

	Abstract

Top Abstract Introduction Methods Results Discussion References

Down-regulation of opiate receptors is demonstrated more easily in vitro than in vivo. The possible role of endogenous opiate-modulatingpeptides in preventing such down-regulation was investigated byaddition of Tyr-W-MIF-1 to an in vitro preparation, the humanneuroblastoma cell line SH-SY5Y, in which down-regulation of opiatereceptors has been demonstrated previously. Although both morphineand Met-enkephalin down-regulated mu and delta receptors afterchronic (24 h) exposure in serum-free medium, Tyr-W-MIF-1, atdoses of up to 100 µM, did not affect receptor number when administeredalone. This lack of effect could not be attributed to degradationof the peptide during chronic treatment because high-performanceliquid chromatography showed that 79% of the peptide remainedintact after a 24-h incubation. When coadministered with 3 µMmorphine, Tyr-W-MIF-1 dose-dependently attenuated morphine-induceddown-regulation of both mu and delta receptors. Down-regulationof mu receptors by the selective agonist PL017 was also attenuatedby Tyr-W-MIF-1, but down-regulation of delta receptors by theselective agonist DPDPE was not. These studies indicate that endogenousopiate modulators may play a role in opiate tolerance at the levelof receptor down-regulation.

	Introduction

Top Abstract Introduction Methods Results Discussion References

Differences between in vivo and in vitro preparations in studies of receptor down-regulation may help explain some mechanismsof opiate tolerance. Down-regulation has been easier to demonstratein vitro than in vivo (Zadina et al., 1995). For example, deltaagonists down-regulate receptors in cell lines containing onlydelta receptors (Chang et al., 1982; Law et al., 1982, 1983),and morphine and mu agonists down-regulate receptors in cell linescontaining mu receptors (Werling et al., 1989). Down-regulationof both mu and delta receptors has been demonstrated in the humanneuroblastoma cell lines SH-SY5Y and SK-N-SH in response to chronicmorphine and selective agonists (Carter and Medzhiradsky, 1993;Baumhaker et al., 1993; Zadina et al., 1990, 1993a, 1994a).

Early in vivo studies showed no change in receptor number after exposure to chronic agonists (Klee and Streaty, 1974; Holltet al., 1975). More recent studies have shown down-regulationin response to chronic etorphine (Tao et al., 1987), PL017 (Taoet al., 1990) and DPDPE (Tao et al., 1991). A major differenceexists, however, between in vitro and in vivo studies, becausedown-regulation in response to morphine has been observed onlyrarely in vivo (Bhargava and Gulati, 1990). Indeed, under thesame conditions in which etorphine down-regulates receptors, morphineincreases receptor number (Tao et al., 1987). The only preparationin which down-regulation in response to morphine is observed consistentlyin vivo is the prenatal or early neonatal rat (Tempel et al.,1988).

These studies highlight two of the important features of opiate receptor down-regulation: a) in vitro preparations, whichexhibit down-regulation to many different agonists, may lack oneor more components of the adaptation response to chronic drugexposure that is present in mature animals; b) the manner in whichcells adapt to chronic morphine seems to depend on the characteristicsof the specific cells studied. Different brain regions and celllines, for example, may have different complements of G-proteinsor efficiencies of coupling to intracellular signaling pathways.

One possibility contributing to the tolerance response and to the lack of receptor down-regulation in mature animals is thepresence of an endogenous "opiate-modulating system," such asthe Tyr-MIF-1 family of peptides. Tyr-MIF-1 (Tyr-Pro-Leu-Gly-NH₂)and Tyr-W-MIF-1 (Tyr-Pro-Trp-Gly-NH₂) have been isolated fromhuman and bovine brain (Hackler et al., 1993; Erchegyi et al.,1992; Horvath and Kastin, 1989, 1990), and they both bind selectivelyto the mu receptor (K_i = 1 µM for Tyr-MIF-1 and K_i = 70 nM forTyr-W-MIF-1) (Zadina et al., 1994c). They exhibit opiate agonistand antagonist properties in the guinea pig ileum, with antagonismmost easily observed in tolerant tissue (Erchegyi et al., 1992,1993; Zadina et al., 1992). Tyr-MIF-1 has a significantly longerhalf-life in neonatal versus adult plasma, a finding that suggeststhe possible postnatal appearance of its degradative enzymes (Kastinet al., 1994).

In this study, we used an in vitro preparation, the human neuroblastoma cell line SH-SY5Y, in which opiate receptor down-regulationby morphine and selective agonists has already been demonstrated(Zadina et al., 1990, 1993a, 1994a), to test whether Tyr-W-MIF-1can block this agonist-induced decrease in receptor number. Wechose Tyr-W-MIF-1 instead of Tyr-MIF-1 because of its higher affinityfor the mu receptor. Serum-free medium was used to avoid degradationof the peptide, and therefore we characterized the suitabilityof this culture condition for the study of receptor regulationin SH-SY5Y cells.

	Methods

Top Abstract Introduction Methods Results Discussion References

Materials. All trans-retinoic acid was obtained from Sigma Chemical Co. (St. Louis, MO), [³H]DAMGO (60 Ci/mmol) from Amersham (Arlington Heights, IL), [³H]pCl-DPDPE (40 Ci/mmol) from Dupont New England Nuclear (Wilmington,DE) and fetal bovine serum from Intergen (Purchase, NY). Tyr-W-MIF-1was synthesized in our laboratory by solution-phase methods. PL017and DPDPE were obtained from Multiple Peptide Systems throughthe National Institute on Drug Abuse.

Cell culture conditions. SH-SY5Y human neuroblastoma cells were cultured, harvested and prepared for binding assays as described previously (Zadinaet al., 1993a, 1994a). Cells of passage 24-31 were cultured ina medium (EFF) containing a 1:1 ratio of Eagle's Minimum EssentialMedium and F12 (Gibco no. 41500-034 and no. 21700-075; Grand Island,NY) with 10% fetal bovine serum, 100 µg/ml streptomycin and 100IU/ml penicillin (Gibco). They were grown at 37°C in a humidifiedatmosphere containing 5% CO₂. At about 90% confluence, cells weredifferentiated into a neuronal phenotype with RA (10 µM). RA wasadministered, with the media change, every 2 days for the last6 days of culture, for a total of three treatments. To avoid metabolismof administered peptides, cells were switched to a serum-freemedium (EFN), with the medium supplement N2 [containing insulin(bovine, 5 µg/ml), transferrin (human, 100 µg/ml), progesterone(20 nM), putrescine (100 µM), and Na selenite (30 nM)], with thelast RA treatment. Drugs were administered for the last 24 h ofculture.

Plasma membrane preparation. Cells were rinsed three times with serum-free medium (EF) and then dissociated with Ca⁺⁺/Mg⁺⁺-free phosphate-buffered saline containing 0.04% EDTA. After centrifugation(183 × g for 7 min at 4°C) for removal of the phosphate-bufferedsaline and EDTA, cells were reconstituted in 50 mM TRIS, vortexedand homogenized with a polytron at setting 6 (23,000 rpm) for20 sec. The homogenate was centrifuged at 30,000 × g for 20 min,and the pellet was incubated for 1 h at room temperature in 50mM TRIS/100 mM NaCl to remove endogenous ligands. After anothercentrifugation at 30,000 × g for 20 min, the pellet was reconstitutedin STEM (0.25 M sucrose, 5 mM TRIS, 0.5 mM EDTA and 1 mM MgSO₄),and protein samples were taken. The sample was divided into equalaliquots and, after a final centrifugation, resuspended in 2 mlSTEM for freezing. Protein was measured by the method of Lowryet al. (1951) with bovine serum albumin as standard.

Opiate receptor assays. Saturation binding assays were performed in 50 mM TRIS with 0.1% bovine serum albumin at a final volume of 600 µl. For mureceptor assays, aliquots (200 µl, containing 100 µg protein)of membranes were incubated for 90 min at 23°C with varying concentrations(0.08-5 nM) of [³H]DAMGO. Nonspecific binding was measured in the presence of 1µM DAMGO. For delta receptor assays, membranes were incubatedfor 4 h at 23°C in the presence of varying concentrations (0.08-5nM) of [³H]pClDPDPE, with nonspecific binding measured in the presenceof 10 µM naltrexone. Bound and free ligands were separated byfiltration. Specific binding at low concentrations of isotopewere 70 to 85% for [³H]DAMGO and 50 to 65% for [³H]pCl-DPDPE.

HPLC. Tyr-W-MIF-1 was iodinated by the chloramine T method, and the monoiodinated fraction was isolated by HPLC. The specific activity(2100 Ci/mmol) was diluted with nonradioactive Tyr-W-MIF-1 toa final concentration of 200,000 cpm/30 µM Tyr-W-MIF-1 in 7.5ml EFN/10 µM RA. SH-SY5Y cells were incubated at 37°C in thismedium in T-25 flasks for 1 min or 2, 5 or 24 h. At the end ofthe incubation, 3.5 ml of medium was transferred to 3.5 ml ice-coldethanol for 30 min, centrifuged at 3500 rpm for 30 min and thesupernatant dried down (Speed-Vac, Savant Instruments, Hicksville,NY). The extract was reconstituted in 400 µl of 0.1% trifluoroaceticacid/water (HPLC buffer A) and fractionated by HPLC on a VydacC18 no. 201HS54 (46 × 250 mm) column. The gradient for bufferB (methanol in 0.1% trifluoroacetic acid) increased from 20 to45% during 20 min, then remained at 45% for 30 min, increasedto 65% in 0.5 min, remained at 65% for 20 min, then increasedto 80%. Retention times of synthetic standards for Tyr-W-MIF-1and its fragments were determined with the same column and gradient.

Statistical analyses. Values (mean ± S.E.M.) are represented as percent of control to normalize differences in B_max from one assay to the next.Percent attenuation was calculated as follows: [(% decrease inB_max induced by 3 µM MS) $-$ (% decrease in B_max induced by 3 µMMS + Tyr-W-MIF-1)]/% decrease in B_max induced by 3 µM MS. Multipleexperiments were analyzed by analysis of variance followed byDuncan's range test.

	Results

Top Abstract Introduction Methods Results Discussion References

Suitability of serum-free culture conditions for study of receptor regulation. To study the role of a peptide in receptor regulation, it was necessary to culture the cells in a serum-free medium to avoiddegradation of the peptide. However, because the presence of serumwas required for initial seeding and growth of the cells, theywere cultured in a serum-containing medium (EFF) until 48 h beforeharvest. At this point, they were transferred to a medium (EFN)containing the supplement N2 and were allowed to adjust to thesenew conditions for 24 h before drug treatment. The switch to serum-freeconditions caused a significant change in the mu:delta ratio from1.9:1 in EFF to 1.3:1 in EFN [F(1,12) = 7.90, P < .05]. The serummay contain opiate-like substances, as demonstrated in both bindingand guinea pig ileum assays (Zadina et al., 1994a). Therefore,the removal of the serum, rather than the addition of N2, wouldappear to be the more likely explanation for the change in receptors.

The stability of Tyr-W-MIF-1 in the serum-free medium was tested directly by incubation of a radiolabeled form of the peptidewith the cultured cells for various time points; samples of themedium were tested by HPLC. The percent of intact Tyr-W-MIF-1remaining after 2, 5 and 24 h of incubation was 95, 92.1 and 79.2,which indicates that the peptide was quite stable in the EFN mediumfor the duration of the experiments described in this study. Figure1 shows the HPLC profile from the 24-h sample (solid line) comparedwith that exposed for only 1 min (dashed lines). There was a smallpeak at the position of free Tyr, which indicates some cleavageof this N-terminal residue.

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Fig. 1. HPLC chromatogram of ¹²⁵I-Tyr-W-MIF-1 after 1 min (dashed line) and 24 h (solid line). At 24 h, 79% of the cpm eluted at theposition of the intact peptide.

Because Tyr-W-MIF-1 remained mostly intact in our culture conditions, we next tested whether the peptide affected mu or deltareceptor number when administered alone for 24 h. The peptidehad no effect on mu or delta receptor number at a dose of 30 µM(data not shown) or 100 µM (fig. 2). This lack of effect couldnot be attributed to degradation of the peptide or to an inabilityof agonists to down-regulate receptors in serum-free medium. Asshown in figure 2, under the same experimental conditions, thepeptide Met-enkephalin at a dose of 10 µM down-regulated bothmu (67 ± 1% of control) and delta (31 ± 5% of control) receptors.Thus, chronic Tyr-W-MIF-1 does not down-regulate receptors underconditions in which a known peptide agonist is capable of down-regulatingreceptors.

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Fig. 2. Mu receptor and delta receptor number expressed as percent of control B_max after 24 h incubation with Tyr-W-MIF-1 or Met-enkephalinin serum-free medium. Neither mu nor delta receptor number wasdecreased by Tyr-W-MIF-1 under the same conditions in which Met-enkephalin(Met-enk) reduced mu receptors to 67 ± 1% of control and deltareceptors to 31 ± 5% of control (n = 2).

In addition to Met-enkephalin, chronic morphine also down-regulates receptors under conditions in which Tyr-W-MIF-1 does notchange receptor number. Down-regulation of mu and delta receptorswas dose-dependent, with 1, 3 and 10 µM doses of morphine reducingthe B_max of mu receptors to 73 ± 7, 57 ± 11 and 52 ± 6% of controland the B_max of delta receptors to 99 ± 2, 60 ± 4 and 46 ± 12%of control (data not shown). This agrees with our earlier findingof dose-responsive down-regulation of opiate receptors in EFFmedium (Zadina et al., 1993a

The ability of an antagonist to up-regulate receptors in serum-free medium was also tested. Naloxone previously has been shownto up-regulate mu and delta receptors after chronic treatmentin SH-SY5Y cells (Zadina et al., 1993a

, 1994a

). Here we comparedthe ability of naloxone to up-regulate receptors in EFF versusEFN. Figure 3 shows that naloxone retains its ability to up-regulatereceptors in serum-free medium. Mu and delta receptors were up-regulatedabout equally in the two culture conditions (24 ± 5% in EFF vs.28 ± 11% in EFN for mu and 31 ± 9% in EFF vs. 43 ± 19% in EFNfor delta). This finding confirms our earlier preliminary results(Zadina et al., 1994a

) with a supplement (B27, Gibco) that ismore complex than the N2 supplement used here. Together, theseresults argue that mechanisms other than, or in addition to, displacementof opiates in the serum account for the ability of naloxone toup-regulate receptors.

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Fig. 3. Up-regulation of mu and delta receptors in serum-containing medium (EFF) and serum-free medium (EFN), expressed as percentincrease in B_max, after 24 h incubation with 10 µM naloxone (Nlx).Values are means ± S.E.M. for three to five experiments.

Attenuation of morphine-induced down-regulation of both mu and delta receptors by Tyr-W-MIF-1. Of the doses of morphine tested for down-regulation of opiate receptors in EFN (1, 3 and 10 µM), the intermediate dose waschosen for the interaction studies because it afforded enoughdown-regulation to detect enhanced or attenuated down-regulationbut avoided the possibility that a supramaximal dose of morphinecould prevent detection of attenuation. The dose of Tyr-W-MIF-1was varied (10, 30, 100 µM) so that it represented 3 times, 10times or 33 times the dose of morphine, and the two drugs wereadministered to the cells simultaneously for 24 h. Down-regulationof mu receptors by morphine was attenuated by Tyr-W-MIF-1 in adose-dependent manner. Figure 4 shows the percent attenuationof morphine-induced down-regulation of mu receptors by increasingdoses of Tyr-W-MIF-1. The 10 µM dose of Tyr-W-MIF-1 had no effect,but down-regulation was significantly attenuated by 30 µM (28± 9%, P < .05) and 100 µM (49 ± 8%, P < .01) doses of Tyr-W-MIF-1.

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Fig. 4. Attenuation of mu receptor down-regulation by Tyr-W-MIF-1. The main figure illustrates increasing percent attenuation withincreasing doses of Tyr-W-MIF-1 (*P < .05; **P < .01 comparedwith control cells given morphine but no Tyr-W-MIF-1). Inset showsthe results expressed as percent of control B_max. Coincubationwith increasing doses of Tyr-W-MIF-1 (+ WI0, + W30 and + W100)resulted in smaller decreases from control B_max. Values are mean± S.E.M. for two to three experiments.

In addition to its effect on mu receptor down-regulation, Tyr-W-MIF-1 also attenuated morphine-induced down-regulation ofdelta receptors, as shown in figure 5. The attenuation (54 ± 9%)of morphine-induced down-regulation by 30 µM Tyr-W-MIF-1 was significant(P < .05), but the higher dose (100 µM) was less effective (39± 8%, P > .1).

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Fig. 5. Attenuation of delta receptor down-regulation by Tyr-W-MIF-1. The main figure illustrates percent attenuation with increasingdoses of Tyr-W-MIF-1 (*P < .05 compared with control cells givenmorphine but no Tyr-W-MIF-1). Inset shows the results expressedas percent of control B_max. Coincubation with 30 µM and 100 µM(+ W30 and + W100) but not 10 µM (+ W10) Tyr-W-MIF-1 resultedin smaller decreases from control B_max. Values are mean ± S.E.M.for two to three experiments.

Effects of Tyr-W-MIF-1 on selective agonist-induced down-regulation of opiate receptors. In addition to morphine, selective agonists also have been shown to down-regulate opiate receptors in SH-SY5Y cells (Zadinaet al., 1994a). We therefore tested the ability of Tyr-W-MIF-1to attenuate this down-regulation by selective agonists. Figure6 shows the dose-responsive attenuation by Tyr-W-MIF-1 of mu receptordown-regulation induced by PL017, a mu selective agonist. PL017alone (1 µM) decreased mu receptor B_max by 52%, in agreement withour earlier work (Zadina et al., 1994a). Tyr-W-MIF-1 attenuatedthis effect at 30 µM (29 ± 1%) and 100 µM (68 ± 2%) doses. Thispattern parallels that seen with morphine-induced down-regulationof mu receptors.

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Fig. 6. Attenuation by Tyr-W-MIF-1 of PL017-induced down-regulation of mu receptors. Results are expressed as percent attenuation(mean ± S.E.M. for two separate experiments) with increasing dosesof Tyr-W-MIF-1.

The delta selective agonist DPDPE (5 nM) caused a large (80%) reduction in delta receptors, in agreement with our previousfindings (Zadina et al., 1994a

). However, Tyr-W-MIF-1 caused onlya small attenuation of the down-regulation, and this effect wasnot dose-responsive (18, 20 and 17% attenuation with 10, 30 and100 µM Tyr-W-MIF-1, respectively; data not shown). Thus, the effectof Tyr-W-MIF-1 on selective agonist-induced down-regulation ofdelta receptors was different from its effect on morphine-induceddown-regulation of delta receptors.

	Discussion

Top Abstract Introduction Methods Results Discussion References

In this study, we established the suitability of serum-free culture conditions for the study of opiate receptor regulationand used this preparation to examine the effects of the opiate-modulatingpeptide Tyr-W-MIF-1 on agonist-induced decreases in receptor number.Tyr-W-MIF-1 remained largely intact during 24 h of culture inserum-free medium, but did not affect receptor number when administeredalone. However, Tyr-W-MIF-1 dose-dependently attenuated morphine-induceddown-regulation of both mu and delta receptors. The effect ofTyr-W-MIF-1 on selective agonist-induced down-regulation revealeddifferences between mu and delta receptors; the PL017-induceddown-regulation of mu receptors was attenuated by Tyr-W-MIF-1,but the DPDPE-induced down-regulation of delta receptors was not.These studies represent the first demonstration of attenuationby an endogenous ligand of morphine-induced changes in receptornumber and suggest a mechanism whereby endogenous antiopiatescan counteract the effects of chronic morphine.

Several peptides have been proposed to play a role in opiate tolerance and dependence by acting as "antiopiates." Accordingto the proposed model, administration of exogenous opiates, suchas morphine, causes the release of endogenous antiopiate peptides.These peptides counteract the effects of morphine, thereby causinga need for increased doses of the drug to achieve a given effect(tolerance). When the drug is removed, the continued presenceof the antiopiate peptide in the absence of opiate drug causesthe symptoms of withdrawal (Rothman, 1992; Zadina et al., 1994b).When we introduced the antiopiate concept with MIF-1 (Pro-Leu-Gly-NH₂)in 1979, we predicted that other types of antiopiates would befound (Kastin et al., 1979). Among the proposed antiopiates isneuropeptide FF, whose actions in opiate tolerance and dependencehave been relatively well characterized. The level of this peptidein the cerebrospinal fluid is increased after chronic morphine(Malin et al., 1990b), and it can attenuate morphine antinociception(Yang et al., 1985) and precipitate withdrawal (Malin et al.,1990a). Antibodies to this peptide can attenuate naloxone-inducedwithdrawal (Malin et al., 1990b) and reverse morphine tolerance(Lake et al., 1991). It does not, however, bind to opiate receptorsand therefore must exert its antiopiate actions through a homeostaticprocess (Allard et al., 1989; Raffa et al., 1994).

The Tyr-MIF-1 peptides display antiopiate activity and can be described as "opiate modulating," because the peptides exhibitboth agonist and antagonist properties, depending on the preparation.As an example of an opiate agonist property, Tyr-W-MIF-1 inducesnaloxone-reversible analgesia after either intracerebroventricularor intrathecal routes of administration (Gergen et al., 1996a;Zadina et al., 1993b). Also, in SH-SY5Y cells, Tyr-MIF-1 inhibitscAMP in a naloxone-reversible manner (Zadina et al., 1991). Examplesof antagonist properties are the ability of Tyr-MIF-1 to precipitatewithdrawal (Malin et al., 1993) and to antagonize stress-induced(Galina and Kastin, 1987) as well as morphine-induced analgesia(Kastin et al., 1984).

The opiate modulating nature of the peptides is best demonstrated within a single preparation in which the peptides can exhibiteither agonism or antagonism, depending on the conditions of testing.This was first demonstrated with the guinea pig ileum. In ileafrom naive animals, the peptides inhibit electrically inducedcontractions, but in ilea from animals made tolerant to morphineor with "receptor reserve" reduced by alkylating agents, theyantagonize opiate-induced contractions (Erchegyi et al., 1992,1993; Zadina et al., 1992). Tyr-W-MIF-1 can bind to both mu₁ andmu₂ receptors (Zadina et al., 1996) and can induce analgesia inthe mouse through a mu₂ mechanism but antagonize mu₁ analgesiainduced by morphine and DAMGO (Gergen et al., 1996b).

A key characteristic of Tyr-MIF-1 peptides is their ability to bind to opiate receptors. For an antiopiate to account forthe high degree of opiate tolerance that can be attained, it mustbe able to bind to the opiate receptor (Smith et al., 1988). Tyr-MIF-1peptides are the only proposed antiopiates (excluding forms ofopioids themselves) that have the ability to bind to opiate receptors.Both Tyr-MIF-1 and Tyr-W-MIF-1 bind selectively to mu over deltaand kappa receptors (Zadina et al., 1994c). According to the antiopiatepeptide model of tolerance and dependence, such peptides counteractthe actions of administered opiates. However, the mechanism ofthis counteraction is unknown and has not been studied at thecellular level. The use of a preparation in which morphine-induceddown-regulation has been demonstrated (SH-SY5Y cells) and of apeptide (Tyr-W-MIF-1) which binds to the mu opiate receptor affordsa unique opportunity to study this endogenous peptide's abilityto counteract the actions of morphine at the cellular and receptorlevel during chronic administration.

Tyr-W-MIF-1 attenuated morphine-induced down-regulation of the mu receptor in a dose-dependent manner, but it did not affectreceptor number when administered alone. These results suggestthat it may be working as a partial agonist. Although it bindsto the mu receptor, the affinity of Tyr-W-MIF-1 (70 nM) is farless than the affinity of morphine for this receptor (Zadina etal., 1994c). However, at the two higher doses used here, whenit is present in a 10-fold or 33-fold excess over morphine, itmay be able to compete with morphine for binding to the receptor.If Tyr-W-MIF-1 has lower efficacy at this receptor, it could preventmorphine's agonist activity without having appreciable activityof its own. Thus, by acting as a partial agonist, it could attenuatemorphine's actions at the mu receptor and the subsequent down-regulationof this site. This would be in agreement with studies involvingthe guinea pig ileum, in which Tyr-MIF-1 and Tyr-W-MIF-1 increasetheir antagonist activity when the receptor reserve is low, suchas in tolerant tissue (Erchegyi et al., 1992,1993; Zadina et al.,1992). Met-enkephalin has been shown to negatively modulate morphineanalgesia, but this action is blocked by the delta antagonistICI 174864 and thus does not result from partial agonism at themu receptor (Jiang et al., 1990). The partial agonism by an endogenousligand suggested by the present studies therefore is an unusualphenomenon at the opiate receptor.

The attenuation of morphine-induced down-regulation of the delta receptor was unexpected and suggests that the mechanism ofaction of Tyr-W-MIF-1 at this receptor may not be simple partialagonism. The affinity of Tyr-W-MIF-1 for the delta receptor (15µM) is 200-fold lower than its affinity for the mu receptor (Zadinaet al., 1994c). Even in a 10- and 33-fold excess over morphine,it seems unlikely that the peptide could compete for binding atthe delta receptor. It has been suggested that down-regulationof the delta receptor by morphine in SK-N-SH cells occurs throughthe mu receptor (Baumhaker et al., 1993), which might accountfor the ability of a mu-acting peptide to attenuate delta down-regulation.However, we have shown previously that in SH-SY5Y cells morphinedown-regulates delta receptors even when the mu receptor is blockedby the selective antagonist CTAP (Zadina et al., 1994a). Thus,attenuation of delta receptor down-regulation in this preparationseems unlikely to occur through the mu receptor.

Alternatively, Tyr-W-MIF-1 could be acting through a nonopiate, high-affinity binding site which it shares with Tyr-MIF-1and which is present in SH-SY5Y cells (Zadina et al., 1990, 1993a).However, Tyr-MIF-1 inhibits cAMP in SH-SY5Y cells in a naloxone-reversiblemanner, which suggests activity at opiate receptors rather thanat this nonopiate site (Zadina et al., 1991). Tests of other signalingpathways and development of antagonists for this site will benecessary to define its role, if any, in the modulation of down-regulationobserved in the present studies.

The effects of Tyr-W-MIF-1 on selective agonist-induced down-regulation reveal differences between mu and delta receptors,as well as between morphine and other ligands. The PL017-induceddown-regulation of mu receptors was attenuated by Tyr-W-MIF-1,but the DPDPE-induced down-regulation of delta receptors was not.The lack of attenuation at delta receptors could be caused bythe high affinity of DPDPE for these receptors (Akiyama et al.,1985) or by its high efficacy in down-regulating delta receptors.We have shown that in SH-SY5Y cells DPDPE down-regulates deltareceptors with an IC₅₀ of 0.5 nM and a maximal effect of about80% reduction of B_max, compared with an IC₅₀ of 179 nM and maximaleffect of 62% reduction for PL017 (Zadina et al., 1994a). It couldbe argued that the inability of Tyr-W-MIF-1 to attenuate DPDPE-induceddown-regulation of delta receptors is caused by the high degreeof down-regulation achieved by the dose (5 nM) used here. However,this dose is just enough to produce maximal down-regulation, whereasthe dose of PL017 chosen (1 µM) is well above that required toachieve maximal down-regulation of mu receptors (Zadina et al.,1994a).

The ability to modulate actions of morphine but not of other ligands, including peptides, has been demonstrated previouslyfor the enkephalin analog DPDPE (Heyman et al., 1989). Such findings,as well as those presented here, suggest differences in the wayscells respond to morphine as compared with other opiate ligands.As mentioned, in vivo studies have demonstrated down-regulationof opiate receptors in response to many ligands, but rarely tomorphine. More recently, it has been demonstrated that clonedmu and delta receptors expressed in HEK 293 cells internalizein response to enkephalins and etorphine but not in response tomorphine under the same conditions (Keith et al., 1996; Ardenet al., 1995). Thus, morphine may induce unique changes in a cell'sresponsiveness, and the type of cell and presence of modulatorscan affect the responsiveness.

In summary, we have demonstrated that under appropriate culture conditions an endogenous peptide can attenuate morphine-induceddown-regulation. In addition, these findings demonstrate anotherexample of different responses of cells to morphine and otheropiate ligands, illustrated by the failure of Tyr-W-MIF-1 to attenuateDPDPE-induced down-regulation even though it can attenuate morphine-induceddown-regulation of delta receptors. The in vitro condition, withthe addition of this endogenous peptide, may help clarify thein vivo condition, in which significant down-regulation in responseto morphine is not easily demonstrated. These findings, therefore,indicate a role for endogenous opiate modulators in the mechanismof tolerance and dependence and suggest a specific cellular mechanism,down-regulation of receptors, that is altered by these peptides.

	Acknowledgments

The authors thank Dr. Laszlo Hackler for synthesis of Tyr-W-MIF-1 and NIDA for the PL017 and DPDPE.

	Footnotes

Accepted for publication October 27, 1997.

Received for publication July 21, 1997.

¹ This work was supported by the VA and National Institute on Drug Abuse Predoctoral Training Grant DA05645 to L.M.H. Preliminaryreports of these results were presented at the International NarcoticsResearch Conference in Long Beach, CA in July 1996, and at theSociety for Neuroscience Meeting, Washington, DC, November 1996.

Send reprint requests to: James E. Zadina, Ph.D., Research Service (151), VA Medical Center, 1601 Perdido Street, New Orleans, LA 70146.

	Abbreviations

DAMGO, Tyr-D-Ala-Gly-N-MePhe-Gly-ol; CTAP, D-Phe-Cys-Tyr-D-Trp-Arg-Thr-Pen-Thr-NH₂; ICI 174, 864, N,N-diallyl-Tyr-Aib-Aib-Phe-Leu-OH([N,N-diallyl-Tyr¹,Aib^2,3]Leu-enkephalin); DPDPE, Tyr-D-Pen-Gly-Phe-Pen ([D-Pen²,D-Pen⁵]-enkephalin); PL017, Tyr-Pro-N-MePhe-D-Pro-NH₂; EDTA, ethylenediaminetetraacetic acid; MS, morphine sulfate; RA, retinoic acid; HPLC, high-performance liquid chromatography; EF, Eagle's Minimum Essential Medium + F12; EFN, EF + N2 supplement; EFF, EF + fetal bovine serum.

	References

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MORPHINE
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Tyr-W-MIF-1 Attenuates Down-Regulation of Opiate Receptors in SH-SY5Y Human Neuroblastoma Cells1

Tyr-W-MIF-1 Attenuates Down-Regulation of Opiate Receptors in SH-SY5Y Human Neuroblastoma Cells¹