Delta Opioid Modulation of the Binding of Guanosine-5'-O-(3-[35S]thio)triphosphate to NG108-15 Cell Membranes: Characterization of Agonist and Inverse Agonist Effects

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Vol. 283, Issue 3, 1276-1284, 1997

Delta Opioid Modulation of the Binding of Guanosine-5 $'$ -O-(3-[³⁵S]thio)triphosphate to NG108-15 Cell Membranes: Characterization of Agonist and Inverse Agonist Effects¹

Philip G. Szekeres and John R. Traynor

Department of Chemistry, Loughborough University, Leicester, LE11 3TU, UK (P.G.S., J.R.T.), and Department of Pharmacology, University of Michigan Medical School, Ann Arbor, Michigan (J.R.T.)

	Abstract

Abstract Introduction Materials & Methods Results Discussion References

The ability of the delta opioid agonist DPDPE ([D-Pen²,D-Pen⁴]enkephalin) to stimulate binding of the GTP analog guanosine-5 $'$ -O-(3-[³⁵S]thio)triphosphate ([³⁵S]GTP $gamma$ S) to pertussis toxin-sensitive G proteins has been characterizedin membranes from NG108-15 mouse neuroblastoma X rat glioma cells.The presence of GDP, or its hydrolysis-resistant analog GDP $beta$ S,and Mg⁺⁺ ions was essential to observe agonist-mediated stimulation of[³⁵S]GTP $gamma$ S binding, although the guanine dinucleotides alone hadcomplex inhibitory and stimulatory effects on [³⁵S]GTP $gamma$ S binding. The relative ability of the delta antagonistsbenzylidenenaltrexone and naltriben to inhibit DPDPE-stimulated[³⁵S]GTP $gamma$ S binding suggested the opioid receptor involved was ofthe delta-2 subtype. Ligand binding assays demonstrated biphasicbinding of these antagonists to this single receptor type. [³⁵S]GTP $gamma$ S binding was also stimulated by [D-Ser²,Leu⁵,Thr⁶]enkephalin > deltorphin II = DPDPE = etorphine > levallorphan= diprenorphine = nalorphine = naltrindole. The delta antagonistsbenzylidenenaltrexone, TIPP (Tyr-Tic-Phe-Phe) and naltriben hadno effect, but ICI 174864 (N,N-diallyl-Tyr-Aib-Phe-Leu-OH) actedas an inverse agonist and inhibited [³⁵S]GTP $gamma$ S binding. Pertussis toxin pretreatment blocked agoniststimulation of [³⁵S]GTP $gamma$ S binding and also reduced basal binding, thus confirmingthe presence of constitutively active delta receptors. Replacementof Na⁺ in the assay buffer with K⁺ afforded an increased level of basal [³⁵S]GTP $gamma$ S binding and an apparent increase in both the inverse agonistactivity of ICI 174864 and the agonist activity of the partialagonist diprenorphine relative to the full agonist [D-Ser²,Leu⁵,Thr⁶]enkephalin. The stimulation of [³⁵S]GTP $gamma$ S binding to NG108-15 cell membranes allows a functionalmeasure of delta opioid activity that can provide systems of differingrelative efficacy.

	Introduction

Abstract Introduction Materials & Methods Results Discussion References

There is considerable interest in the development of delta opioid-selective, nonpeptide compounds as analgesic agents thatmay show an improved side effect profile over morphine and othercurrently available mu agonist therapies (Porreca et al., 1995).To expedite this process, a full understanding of the action ofdelta opioid agonists at the cellular level is essential, particularlybecause compounds active at this receptor may show agonist, antagonistand inverse agonist properties (Costa and Herz, 1989). Opioidreceptors are members of the family of seven-transmembrane domainreceptors and couple to inhibitory G proteins, such that opioidagonists stimulate the exchange of bound GDP for GTP, which canbe measured as an increase in the binding of the stable GTP analog[³⁵S]GTP $gamma$ S to cell membranes (Sim et al., 1995; Traynor and Nahorski,1995). Such opioid agonist-mediated stimulation of [³⁵S]GTP $gamma$ S binding has an absolute requirement for GDP (Traynor andNahorski, 1995). In addition, µM levels of GDP are needed foroptimum agonist-stimulation of [³⁵S]GTP $gamma$ S binding at several receptor systems (Gierschik et al.,1991; Lazareno et al., 1993; Lorenzen et al., 1993; Offermannset al., 1994). However, the level of GDP required varies acrosssystems. Thus, to observe agonist responses at m1 and m3 receptorsexpressed in CHO or human embryonic kidney cells, only low levels(0.1 µM) of GDP are required, whereas for m2- and m4-mediatedincreases in the same cells, 10-fold higher levels of GDP areneeded (Lazareno et al., 1993; Offermanns et al., 1994). In contrast,the alpha-2 adrenergic-mediated stimulation of [³⁵S]GTP $gamma$ S binding in PC-12 cells requires no GDP (Tian et al., 1994).

The mu opioid receptors in SH-SY5Y cells couple to G_i and G_o proteins, including G_alphai3, G_alphai2, G_alphai1,G_alphao1 and G_alphao2, but have a preferencefor G_alphai3 (Laugwitz et al., 1993). In contrast, deltaopioid receptors in NG108-15 cells couple especially to G_alphai2(McKenzie and Milligan, 1990). However, when expressed in CHOcells, both mu and delta receptors couple to similar populationsof G protein subtypes (Chakrabarti et al., 1995). Such differencesor similarities in the coupling of opioid receptors to G proteinsubtypes may define the specific requirements for GDP and certainions to obtain an optimum agonist-stimulated [³⁵S]GTP $gamma$ S response and contribute to the properties of the receptor.

We report on the characterization of delta opioid modulation of [³⁵S]GTP $gamma$ S binding response in NG108-15 cells. A complex relationshipexists between the concentration of GDP and its effect on [³⁵S]GTP $gamma$ S binding, but opioid agonist-mediated stimulation of thisresponse follows a simple relationship, increasing with increasingGDP. Changes in [³⁵S]GTP $gamma$ S binding provide a functional method for investigatingdelta opioid activity and allow for study of the action of agonistsand inverse agonists, as exemplified by ICI 174864. A preliminaryaccount of some of the results has been presented (Szekeres andTraynor, 1995).

	Materials and Methods

Abstract Introduction Materials & Methods Results Discussion References

Chemicals and drugs. [³H]Diprenorphine (1.11 TBq/mmol) was purchased from Amersham (Aylesbury, UK),and [³⁵S]GTP $gamma$ S (46.1 TBq/mmol) was purchased from Dupont New EnglandNuclear Research Products (Boston, MA). DAMGO, DPDPE, DSLET, pertussistoxin and all other chemicals were of analytical grade and purchasedfrom Sigma Chemical (St. Louis, MO). [D-Ala²,Glu⁴]Deltorphin II (Tyr-D-Ala-Phe-Glu-Val-Val-Gly-NH₂) was obtainedfrom Peninsula (St. Helens, UK), and BNTX, NTB and ICI 174864[N,N-diallyl-Tyr-Aib-Phe-Leu-OH (Aib = $alpha$ -aminoisobutyric acid)]were purchased from RBI (St. Albans, UK). The following compoundswere kindly donated as indicated: CI977 [5R-(5 $alpha$ ,7 $alpha$ ,8 $beta$ )-N-methyl-N-[7-(1-pyrrolidinyl)-1-oxaspiro[4,5]dec-8-yl]-4-benzofuranacetamide-HCl;Parke-Davis, Cambridge, UK], etorphine and diprenorphine (Reckitt& Colman, Hull, UK); nalorphine and levallorphan (Zeneca Pharmaceuticals,Alderley Park, UK) and TIPP (Tyr-Tic-Phe-Phe; Tic = tetrahydroisoquinoline-3-carboxylicacid) (Dr. S. J. Paterson, St. Thomas's Hospital, London, UK).Ecoscint scintillation fluid was purchased from National Diagnostics.DMEM (without sodium pyruvate; with 4500 mg/l glucose), DMEM/NutrientMix F-12, fetal calf serum, new born calf serum, fungizone (amphotericinB), L-glutamine, penicillin/streptomycin solution and hypoxanthine(13.6 µg/ml)/aminopterin (0.176 µg/ml)/thymidine (3.88 µg/ml)supplement were all purchased from GIBCO Laboratories (Paisley,UK).

Cell culture. NG108-15 cells (kindly provided by Dr. M. Keen, Department of Pharmacology, University of Birmingham, UK) were grown in 175-cm² tissue culture flasks in DMEM supplemented with 5% fetal calfserum and hypoxanthine (13.6 µg/ml)/aminopterin (0.176 µg/ml)/thymidine(3.88 µg/ml) at 37°C in a 5% CO₂ atmosphere. CHO cells transfectedwith the mouse delta opioid receptor were a kind gift from Dr.C. J. Evans (Department of Psychiatry, University of Californiaat Los Angeles). Cells were grown in 175-cm² tissue culture flasks in DMEM/Nutrient Mix F-12 supplementedwith 5% fetal calf serum, 2.5 µg/ml amphotericin B, 50 units/mlpenicillin, 50 µg/ml streptomycin and 258 µg/ml L-glutamine at37°C in a 5% CO₂ atmosphere.

Membrane preparation. Confluent monolayers of NG108-15 cells or CHO cells were rinsed once and harvested by gentle agitation in DMEM, followed bycentrifugation (250 × g, 2 min). The cell pellet was resuspendedin a buffer of 20 mM HEPES, pH 7.4, 100 mM NaCl and 4 mM MgCl₂(buffer A) and homogenized using a tissue tearer (twice at 5 sec,30,000 rpm). The resultant crude membrane fraction was collectedby centrifugation (50,000 × g, 15 min), washed in buffer A andrecentrifuged as before. The pellet was finally resuspended inbuffer A to give a protein concentration of $approx$ 0.25 mg/ml (Lowryet al., 1951). All procedures were performed at 0° to 4°C. Inexperiments to determine opioid binding, buffer A was replacedwith 50 mM Tris·HCl, pH 7.4, in all procedures.

Opioid binding assays. Binding was performed in Tris·HCl buffer to afford parameters for high-affinity binding of the ligands (Rodriguez et al.,1992) as follows: membrane protein ( $approx$ 250 µg) was incubated inTris·HCl, pH 7.4, with [³H]diprenorphine (0.04-10 nM) or [³H]DPDPE (0.04-20 nM) in a final volume of 1 ml. After allowingthe system to reach equilibrium for 1 hr at 25°C (Cotton et al.,1985; Ho et al., 1997), the mixture was rapidly vacuum-filteredthrough GF/B filters to separate bound from free ligand, and thefilters were rinsed three times in 3 ml of ice-cold buffer (Tris·HCl,pH 7.4). Radioactivity retained on the filters was determinedby liquid scintillation counting. Nonspecific binding was definedas the binding remaining in the presence of 10 µM naloxone. Specificbinding was typically >80% of total binding at the radioligandK_d.

[³⁵S]GTP $gamma$ S binding assay. Unless otherwise stated, cell membranes ( $approx$ 250 µg of protein) were incubated in buffer A containing [³⁵S]GTP $gamma$ S (100 pM) and GDP (100 µM) for 1 hr at 30°C in a totalvolume of 1 ml and in the presence of varying concentrations ofopioids. Samples were then rapidly vacuum-filtered through GF/Bfilters and washed three times with 3 ml of ice-cold buffer A.Bound radioactivity was quantified by liquid scintillation counting.Nonspecific binding was defined using 10 µM unlabeled GTP $gamma$ S. Specificbinding was typically 90% to 95% of total binding. To examinethe stability of [³⁵S]GTP $gamma$ S at the end of the incubation assay, 100 µl samples ofthe incubation mixture were taken, centrifuged and applied tocellulose-PEI thin-layer liquid chromatography plates that weredeveloped using a solvent system of 0.5 M K₂HPO₄, containing 0.01M $beta$ -mercaptoethanol. After drying, the plates were cut into 1-cmstrips and counted for radioactivity as above. The purity of the[³⁵S]GTP $gamma$ S used in the assays, as determined by thin-layer liquidchromatography, was > 90%.

Data analysis. Binding data were analyzed with the program LIGAND (Munson and Rodbard, 1980) to provided estimates for the total receptornumber (B_max), binding affinity (K_d or K_i) and slope of the bindingisotherms. The data was fitted to both one- and two-site models.To determine whether the two-site model produced a statisticallybetter fit of the data than the one-site model, the variance ratiotest (F test) facility of LIGAND was used, where P < .05 was consideredsignificant. The EC₅₀ for stimulation of [³⁵S]GTP $gamma$ S binding obtained at various drug concentrations was determinedfrom nonlinear curve fitting of the data fitted, using GraphPADPrism (GraphPAD, San Diego, CA). Apparent antagonist affinityconstants (K_e) were calculated from [³⁵S]GTP $gamma$ S binding assay concentration-effect curves in the absenceor presence of a single concentration of antagonist using theequation K_e = [antagonist]/(DR $-$ 1), where DR = (EC₅₀ in the presenceof antagonist)/(EC₅₀ in the absence of antagonist) (Kosterlitzand Watt, 1968). Statistical comparisons between groups of datawere made by Student's t test, where P < .05 was considered significant.

	Results

Abstract Introduction Materials & Methods Results Discussion References

Characterization of basal and agonist-stimulated [³⁵S]GTP $gamma$ S binding. The NG108-15 cells used in this study expressed a homogeneous delta opioid receptor population. This was demonstrated by theability of the selective delta opioid agonist DPDPE (K_i = 1.64± 0.07 nM; Hill coefficient, 0.95 ± 0.06; n = 3) but not the muand kappa opioids DAMGO and CI977 (K_i = >1000 nM) to displacebinding of the nonselective antagonist [³H]diprenorphine. In addition, the number of receptors labeledby [³H]diprenorphine (559 ± 61 fmol/mg/protein, K_d = 0.32 ± 0.01 nM,n = 3) was the same as the number labeled by [³H]DPDPE (501 ± 94 fmol/mg/protein, K_d = 1.68 ± 0.51 nM). The CHOcells used expressed delta receptors at a density of 404 ± 23fmol/mg of protein (n = 3) determined with [³H]diprenorphine (K_d = 0.2 ± 0.01 nM).

Preliminary data (not shown) indicated that DPDPE (1 µM) maximally stimulated the binding of the labeled GTP analog [³⁵S]GTP $gamma$ S to membranes from NG108-15 cells. Optimum stimulationof [³⁵S]GTP $gamma$ S binding was achieved at 30°C in the presence of 100 µMGDP. Agonist-stimulated binding of the labeled nucleotide waslinear up to $approx$ 150 µg of membrane protein, reaching maximal effectat 250 µg of protein, and increased linearly with time up to 90min at 30°C, at which time a 2.2-fold stimulation over basal bindingwas observed. Higher temperatures resulted in a decreased effectivenessof the agonist response (1.6-fold stimulation at 37°C), whereasat 20°C, a 2.5-fold stimulation was observed but over 180 min.

DPDPE (1 µM) stimulation of [³⁵S]GTP $gamma$ S binding to crude membranes from NG108-15 cells was critically dependent on the presenceof GDP. The role of this nucleotide was complex because both basaland delta opioid-stimulated [³⁵S]GTP $gamma$ S binding showed a triphasic response to GDP (fig. 1a).GDP concentrations over the range of 0.1 to 3 µM inhibited [³⁵S]GTP $gamma$ S binding, but at >3 µM GDP, [³⁵S]GTP $gamma$ S binding was increased, followed by a reversal at higherconcentrations (>30 µM) of GDP. With concentrations of GDP of $>=$ 3 µM, differences were seen in the effects on the binding of[³⁵S]GTP $gamma$ S in the presence and absence of DPDPE (1 µM), resultingin a separation of basal and agonist-stimulated binding and thusa measurable agonist response. At 100 µM GDP, a stimulation of[³⁵S]GTP $gamma$ S binding over basal representing an agonist-mediated increasein [³⁵S]GTP $gamma$ S of 55.7 ± 2.2 (n = 3) fmol/mg of protein was obtained(fig.1a, inset). The poorly hydrolyzable guanine nucleotide analogGDP $beta$ S mimicked the effect of GDP in all aspects, including theability to facilitate agonist-mediated [³⁵S]GTP $gamma$ S binding (fig. 1b). However, neither of the dinucleotidesADP and UDP nor the mononucleotide GMP could substitute for GDPin affording delta agonist-mediated stimulation of [³⁵S]GTP $gamma$ S binding. Moreover, none of these nucleotides inhibitedbasal [³⁵S]GTP $gamma$ S binding, but all three produced a concentration-dependentincrease in [³⁵S]GTP $gamma$ S binding in the absence of delta opioid agonist, resultingin a >300% increase in binding over basal values (fig. 2). Preliminarymetabolism studies suggested that the presence of unlabeled nucleotidesstabilized the [³⁵S]GTP $gamma$ S against degradation. After 60 min at 30°C, only 25 ± 5%of the added radioactivity was recovered as [³⁵S]GTP $gamma$ S. However, in the presence of 100 µM GDP or ADP, recoveryincreased to 49 ± 4% and 74 ± 7%, respectively (n = 3).

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Fig. 1. Effect of (a) GDP and (b) GDP $beta$ S on the binding of [³⁵S]GTP $gamma$ S (100 pM) to membranes of NG108-15 cells in the absence ( $open circle$ ) andpresence ( $bullet$ ) of DPDPE (1 µM), where 100% represents the levelof [³⁵S]GTP $gamma$ S binding in the absence of guanine dinucleotide, whichwas 75.7 ± 3.3 fmol/mg of protein (a) and 123.8 ± 15.3fmol/mgof protein (b). Insets, degree of stimulation of [³⁵S]GTP $gamma$ S binding by 1 µM DPDPE. Assays were performed as describedin Materials and Methods for 60 min at 30°C. Points representmean ± S.E.M. from three separate determinations performed induplicate. **P < .01 and *P < .05 compared with control. $dagger$ P <.05 compared with no dinucleotide.

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Fig. 2. Effect of the nucleotides ADP ( $bullet$ ), GMP ( $black-square$ ) and UDP ( $black-triangle$ ) on [³⁵S]GTP $gamma$ S (100 pM) binding to membranes from NG108-15 cells. Assayswere performed as described in Materials and Methods for 60 minat 30°C. Points represent mean ± S.E.M. from three separate determinationsperformed in duplicate.

DPDPE (1 µM) also stimulated the binding of [³⁵S]GTP $gamma$ S to membranes from CHO cells expressing the recombinant mouse delta receptor.In contrast to the response in NG108-15 cells, the level of GDPneeded to achieve a separation of basal and agonist-stimulatedbinding was much lower, with an optimum concentration at 3 µM,and the effects of GDP on [³⁵S]GTP $gamma$ S binding were only inhibitory (fig. 3).

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Fig. 3. Effect of varying the concentration of GDP in the absence ( $open circle$ ) or presence ( $bullet$ ) of DPDPE (1 µM) on [³⁵S]GTP $gamma$ S (100 pM) binding to membranes from CHO cells expressingthe delta receptor. Assays were performed as described in Materialsand Methods for 60 min at 30°C. Points represent mean ± S.E.M.from three separate determinations performed in duplicate. *P< .05. Inset, degree of stimulation by 1 µM DPDPE.

The presence of Na⁺ ions was not necessary to observe agonist-stimulated [³⁵S]GTP $gamma$ S binding, but this cation inhibited control binding preferentiallyover DPDPE-stimulated binding, resulting in an optimal windowfor stimulation over the concentration range of 10 to 100 mM Na⁺ (fig. 4). In comparison, agonist-stimulated binding of [³⁵S]GTP $gamma$ S cells had an absolute requirement for Mg⁺⁺, although this ion had a biphasic action on both control andDPDPE-stimulated [³⁵S]GTP $gamma$ S binding (fig. 5). Optimum agonist-stimulated binding [³⁵S]GTP $gamma$ S was observed at 4 mM Mg⁺⁺ .

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Fig. 4. Effect of Na⁺ concentration on basal ( $open circle$ ) and DPDPE (1 µM)-stimulated ( $bullet$ ) [³⁵S]GTP $gamma$ S (100 pM) binding to NG108-15 membranes. Assays were performedin the presence of 4 mM MgCl₂ as described in Materials and Methodsfor 60 min at 30°C. Points represent mean ± S.E.M. from threeseparate determinations performed in duplicate.

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Fig. 5. Effect of Mg⁺⁺ concentration on basal ( $open circle$ ) and DPDPE (1 µM)-stimulated ( $bullet$ ) [³⁵S]GTP $gamma$ S (100 pM) binding to NG108-15 membranes. Assays were performedin the presence of 100 mM NaCl as described in Materials and Methodsfor 60 min at 30°C. Points represent mean ± S.E.M. from threeseparate determinations performed in duplicate.

Conditions used in all subsequent experiments were 80 to 150 µg of membrane protein in the presence of 100 µM GDP, 100 mMNaCl and 4 mM MgCl₂ at 30°C for 1 hr.

Effects of agonists and antagonists on [³⁵S]GTP $gamma$ S binding. DPDPE caused a concentration-dependent increase in the binding of [³⁵S]GTP $gamma$ S over control, affording an EC₅₀ value of 31.2 ± 3.1 nM(n = 12) and reaching maximal stimulation at 1 µM of the opioid(figs. 6 and 7). This stimulation was completely blocked afterincubation of the cells with pertussis toxin (100 ng/ml) for 24hr before preparation of the membranes (fig. 7), confirming theinvolvement of G proteins of the G_o/G_i class. Pertussis toxintreatment also lowered basal binding of [³⁵S]GTP $gamma$ S in these cells by 56.0 ± 2.2%, to 18.7 ± 0.8 fmol/mg proteinfrom a basal level of 41.2 ± 1.2 fmol/mg protein (P < .01; n =3).

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Fig. 6. Stimulation of [³⁵S]GTP $gamma$ S (100 pM) binding to membranes of NG108-15 cells by DPDPE alone ( $bullet$ ) or in the presence of 300 nM naloxone( $open circle$ ), 10 nM BNTX ( $black-square$ ) or 0.2 nM NTB ( $black-triangle$ ). Assays were performed asdescribed in Materials and Methods for 60 min at 30°C, and valuesrepresent mean ± S.E.M. from three separate determinations performedin duplicate. Binding of [³⁵S]GTP $gamma$ S was 39.1 ± 5.3 fmol/mg protein in the absence of DPDPEand 107.9 ± 9.2 fmol/mg of protein in the presence of DPDPE (10µM).

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Fig. 7. DPDPE-mediated stimulation of [³⁵S]GTP $gamma$ S (100 pM) binding to NG108-15 membranes prepared from control ( $bullet$ ) and pertussis toxin(100 ng/ml, 24 hr)-treated ( $black-triangle$ ) cells. Assays were performed asdescribed in Materials and Methods for 60 min at 30°C. Pointsrepresent mean ± S.E.M. from three separate determinations performedin duplicate. All pertussis toxin-treated values were significantly(P < .01) lower than the basal value.

The stimulatory effect of DPDPE was antagonized by naloxone (300 nM), which shifted the concentration-effect curve to theright by $approx$ 13-fold to give an apparent K_e value for naloxone of19.6 ± 3.6 nM, which is indicative of delta opioid receptor involvement(Leslie, 1987

). The putative delta-1 opioid receptor antagonistBNTX (Portoghese et al., 1992

) and putative delta-2 opioid receptorantagonist NTB (Sofuoglu et al., 1991

) shifted the dose-effectcurve of DPDPE to the left in a parallel fashion, allowing calculationof apparent K_e values of 1.5 ± 0.1 and 0.078 ± 0.01 nM, respectively(fig. 6).

DPDPE is a putative delta-1 agonist (Mattia et al., 1992

). The putative delta-2 agonists [D-Ala²,Glu⁴]deltorphin II and DSLET (Mattia et al., 1992

) also stimulatedthe binding of [³⁵S]GTP $gamma$ S to membranes from NG108-15 cells. [D-Ala²,Glu⁴]Deltorphin II afforded a similar maximal response to DPDPE (102.6± 1.1% of the DPDPE response), but DSLET afforded a higher maximum,representing 119.4 ± 2.7% of the DPDPE response (P < .05) (fig.8). The EC₅₀ values for these compounds were 19.2 ± 5.8 and 5.3± 0.6 nM, respectively (data not shown). Etorphine had a similarmaximum to DPDPE, whereas levallorphan, diprenorphine and nalorphinewere all weaker, partial agonists. Of the delta opioid antagonists,naltrindole showed a small degree of agonist activity, whereasTIPP, BNTX and NTB did not significantly alter the basal levelof [³⁵S]GTP $gamma$ S binding (fig. 8). In contrast, ICI 174864 inhibited [³⁵S]GTP $gamma$ S binding by 17.0 ± 6.3%. Replacement of the Na⁺ ions in the assay medium with K⁺ ions resulted in an increased level of basal [³⁵S]GTP $gamma$ S binding and a consequently much greater inhibition of[³⁵S]GTP $gamma$ S binding by ICI 174864 such that an EC₅₀ value of 77.2± 27 nM could be determined (fig. 9). This inhibitory effect ofICI 174864 was blocked when the assay was performed in the presenceof naloxone (fig. 9). Replacement of Na⁺ ions with K⁺ ions also resulted in an increased efficacy of the partial agonistdiprenorphine relative to the full agonist DSLET (fig. 10).

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Fig. 8. Relative activity of various ligands to stimulate [³⁵S]GTP $gamma$ S (100 pM) binding to NG108-15 cell membranes. Concentrations usedwere DSLET, [D-Ala²,Glu⁴]deltorphin II (DELT II) and DPDPE (3 µM); etorphine, levallorphan,diprenorphine, nalorphine, naltrindole, NTB and ICI 174864 (10µM); BNTX (1 µM); and TIPP (5 µM). Points represent mean ± S.E.M.from at least three separate determinations performed in duplicateand are normalized to the maximal effect produced by DSLET thatrepresented 37.6 ± 2.9 fmol [³⁵S]GTP $gamma$ S bound/mg of protein. Assays were performed as describedin Materials and Methods for 60 min at 30°C. $dagger$ Significantly greaterthan the DPDPE response (P < .05). *Significantly below basalvalue (P < .05).

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Fig. 9. Effect of ICI 174864 on [³⁵S]GTP $gamma$ S (100 pM) binding to NG108-15 membranes in Na⁺ (100 mM; open columns)- or K⁺ (100 mM; hatched columns)-containing buffer. The cross-hatchedcolumn represents the effect of 1 µM naloxone on the ICI 174864(3 µM)-mediated response in K⁺-containing buffer. Basal [³⁵S]GTP $gamma$ S binding was 76.2 ± 3.2 fmol/mg in Na⁺-containing buffer and 102.4 ± 9.8 fmol/mg in K⁺-containing buffer. Assays were performed as described in Materialsand Methods, using the appropriate buffer, for 60 min at 30°C.Points represent mean ± S.E.M. from three separate determinationsperformed in duplicate. *P < .01 compared with effect caused by3000 nM ICI 174864 alone.

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Fig. 10. Diprenorphine stimulation of [³⁵S]GTP $gamma$ S (100 pM) binding to NG108-15 membranes relative to that afforded by DSLET (3 µM) inNa⁺ (100 mM; $bullet$ )- or K⁺ (100 mM; $black-square$ )-containing buffer. Basal [³⁵S]GTP $gamma$ S binding was 53.2 ± 6.8 fmol/mg in Na⁺-containing buffer and 78.5 ± 12.0 fmol/mg in K⁺-containing buffer. [³⁵S]GTP $gamma$ S binding in the presence of DSLET (3 µM) was 102.8 ± 1.1fmol/mg in Na⁺-containing buffer and 112.6 ± 13.6 fmol/mg in K⁺-containing buffer. Assays were performed as described in Materialsand Methods, using the appropriate buffer, for 60 min at 30°C.Points represent mean ± S.E.M. from three separate determinationsperformed in duplicate.

To further characterize the delta opioid receptor in NG108-15 membranes, displacement of [³H]diprenorphine (0.50 nM) binding by BNTX and NTB was studied(fig. 11). Surprisingly, both antagonists afforded shallow displacementcurves, with Hill coefficients of 0.45 ± 0.02 and 0.51 ± 0.05for BNTX and NTB, respectively. Such shallow slopes suggest thepresence of receptor heterogeneity, and computer modeling of thedata using the program LIGAND (Munson and Rodbard, 1980

) revealedthat a two-site model gave a significantly better fit of the datathan a one-site model (P < .01). As expected from the relativeability of the two antagonists to shift the [³⁵S]GTP $gamma$ S binding curve for DPDPE, the affinity of NTB was higherat both sites than that of BNTX (table 1). In contrast, displacementof [³H]diprenorphine by the delta agonist DPDPE was monophasic witha Hill coefficient of 0.95 ± 0.06 and an affinity (K_i) of 1.64± 0.07 nM (fig. 11).

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Fig. 11. Displacement of the specific binding of [³H]diprenorphine (0.5 nM) to membranes from NG108-15 cells by NTB ( $black-square$ ), BNTX ( $bullet$ ) andDPDPE ( $black-triangle$ ). Experiments were performed in Tris·HCl buffer (50 mM,pH 7.4) for 60 min at 25°C as described in Materials and Methods.Points represent mean ± S.E.M. for four experiments performedin duplicate.

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TABLE 1
Binding affinities of BNTX and NTB at the delta opioid receptor in NG108-15 cell membranes
Data were obtained from the displacement of specific binding of [³H]diprenorphine (0.5 nM) to membranes from NG108-15 cells by BNTXand NTB (see fig. 11) and fitted using the LIGAND program (Munsonand Rodbard, 1980

). The two-site model gave a significantly betterfit of the data than a single-site model (P < .01).

	Discussion

Abstract Introduction Materials & Methods Results Discussion References

The NG108-15 cell membranes used in this study were shown to express the same number of delta opioid receptors measured byeither the delta agonist [³H]DPDPE or the delta antagonist [³H]diprenorphine. Because this cell line expresses only opioidreceptors of the delta type, this demonstrates that in Tris bufferthe receptors are all (within the limits of measurement) in aconformational state recognized with high affinity by both agonistsand antagonists. According to the ternary complex model of receptor/Gprotein interaction (Birnbaumer et al., 1990), this would indicatethat the receptors are in a form tightly coupled to G protein.

To demonstrate delta opioid agonist stimulation of [³⁵S]GTP $gamma$ S binding in membranes from NG108-15 and CHO cells, the presenceof GDP, or its hydrolysis resistant analog GDP $beta$ S, was necessary.This dependence on GDP has also been observed in studies on thestimulation of [³⁵S]GTP $gamma$ S binding by mu opioid agonists in SH-SY5Y cell membranes(Traynor and Nahorski, 1995) and in C6 cells expressing the clonedµ receptor (Emmerson et al., 1996), adenosine A₁ agonists in bovinebrain (Lorenzen et al., 1993), muscarinic agonists in porcinecardiac membranes and CHO cells (Hilf et al., 1989; Lazareno etal., 1993) and chemotactic peptide fMet-Leu-Phe in membranes fromHL-60 cells (Gierschik et al., 1991). GDP is thought to bind toempty guanine nucleotide binding sites on G proteins and hencereduce the basal level of [³⁵S]GTP $gamma$ S binding (Wieland et al., 1992), such that agonist-inducedexchange of GDP for [³⁵S]GTP $gamma$ S can be observed. However, GDP and GDP $beta$ S affected bothbasal and agonist-stimulated [³⁵S]GTP $gamma$ S binding in the NG108-15 cell membranes in a complex manner.Thus, GDP and GTP $beta$ S reduced binding of [³⁵S]GTP $gamma$ S at concentrations below 3 µM, but above this concentrationan increase in [³⁵S]GTP $gamma$ S binding was observed, and this reverted to an inhibitionat higher concentrations.

The delta opioid-mediated stimulation of [³⁵S]GTP $gamma$ S binding was not observed if GDP or GDP $beta$ S was replaced by GMP, ADP or UDP.These latter nucleotides did not inhibit basal [³⁵S]GTP $gamma$ S binding but did stimulate the binding of [³⁵S]GTP $gamma$ S in the absence of opioid agonist. Indeed, for ADP, UDPand GMP, the level of stimulation was far in excess of that seenwith GDP or GDP $beta$ S. A number of explanations are possible for thisfinding. The nucleotides may be stimulating the binding of [³⁵S]GTP $gamma$ S via a G protein-coupled "nucleotide" receptor, althoughno nucleotide receptor with such a profile is known. However,a preliminary metabolism study suggests the presence of the secondunlabeled nucleotide protects [³⁵S]GTP $gamma$ S from breakdown, probably by various nucleotidases andphosphatases present in the membrane preparation (Wieland et al.,1992), thereby increasing the level of [³⁵S]GTP $gamma$ S available to bind to G protein. This is supported by thefinding that a reduced level of agonist stimulated [³⁵S]GTP $gamma$ S binding was seen at 37°C, whereas stimulation was increasedat 20°C. The decrease in binding at higher concentrations of GDPor GDP $beta$ S (>30 µM) presumably results from a competition betweenthe guanine dinucleotides and [³⁵S]GTP $gamma$ S for the nucleotide binding site on the G protein(s). Asa consequence, this effect is not seen with ADP, UDP or GMP dueto the specificity of the nucleotide binding site on the G protein(Rodbell et al., 1971, 1980).

These complex effects of GDP on [³⁵S]GTP $gamma$ S binding in NG108-15 cell membranes are not a property of the delta opioid receptorsystem because a similar relationship is not seen in membranesfrom CHO cells expressing the mouse delta receptor. Thus, theeffect is cell, not receptor, specific and is independent of theability of the agonist bound form of the delta receptor to stimulate[³⁵S]GTP $gamma$ S binding. The difference in GDP requirements for expressionof delta agonism at the same receptor expressed in different cellshighlights considerations that must be examined when looking atreceptor-mediated responses outside endogenous systems (Kenakin,1996).

The ionic environment is also a very important parameter in modulating [³⁵S]GTP $gamma$ S binding. To observe agonist stimulation of [³⁵S]GTP $gamma$ S binding in NG108-15 cell membranes, Mg⁺⁺ ions were required. It is difficult to conclude the mechanismby which Mg⁺⁺ is causing its effects because this cation has many actions onG protein events (Birnbaumer et al., 1990). However, the increasein both basal and agonist-stimulated [³⁵S]GTP $gamma$ S binding may be accounted for by the increased rate ofdissociation of GDP (Higashijima et al., 1987) and an increasedrate of association of [³⁵S]GTP $gamma$ S (Bokoch et al., 1984; Sternweis et al., 1981) with a decreasedrate of dissociation (Higashijima et al., 1987). In addition,delta opioid binding is likely to be enhanced by Mg⁺⁺ (Rodriguez et al., 1992; Standifer et al., 1993), resulting ina differential increase in agonist-stimulated over basal [³⁵S]GTP $gamma$ S binding. Above 10 mM, Mg⁺⁺ had a strong inhibitory effect on both basal and agonist-stimulated[³⁵S]GTP $gamma$ S binding.

Na⁺ ions were not essential to produce an agonist-mediated increase in [³⁵S]GTP $gamma$ S binding. The effect of Na⁺ ions on [³⁵S]GTP $gamma$ S binding was to decrease both basal and agonist-stimulated[³⁵S]GTP $gamma$ S binding. However, in the presence of DPDPE (1 µM), theeffect of Na⁺ was shifted, leading to an increased stimulation window at Na⁺ concentrations of 10 to 100 mM. This inhibitory effect of Na⁺ on G protein activity has been interpreted as reflecting a modulationof the affinity of "empty" opioid delta receptors for G protein,that is, reducing the activity of constitutively active receptors(Costa et al., 1990, 1992; Lefkowitz et al., 1993). As expected,because delta opioid receptors are known to couple to G proteinsof the G_i/G_o family (Laugwitz et al., 1993; Offermanns et al.,1991; Prather et al., 1994; Roerig et al., 1992), treatment ofNG108-15 cells with pertussis toxin (100 ng/ml; 24 hr) completelyabolished delta opioid receptor-mediated stimulation of [³⁵S]GTP $gamma$ S binding. Furthermore, pertussis toxin pretreatment reducedcontrol [³⁵S]GTP $gamma$ S binding. Because pertussis toxin only uncouples G proteinsfrom receptors and does not alter other properties of G proteins,such as their ability to bind GTP and interact functionally withadenylyl cyclase (Katada et al., 1986), this provides evidencefor the presence of constitutively active receptors in membranepreparations of NG108-15 cells.

Only a single delta opioid receptor has been cloned from NG108-15 cells (Evans et al. 1992; Kieffer et al., 1992). However,the agonist effect of DPDPE was antagonized by the nonselectiveopioid antagonist naloxone and by the putative delta-1 antagonistBNTX and putative delta-2 antagonist NTB. The higher sensitivityof DPDPE to blockade by NTB, rather than BNTX, suggests the homogeneousdelta receptor in NG108-15 cells is of the delta-2 subtype, aconclusion also reached by studying the cloned delta receptorfrom NG108-15 cells expressed in CHO cells (Law et al., 1994).The K_e values reported in the CHO cells for the two antagonists(Law et al., 1994) suggests they have lower affinities for thetransfected receptor in CHO cells than for the endogenous receptorin NG108-15 cells. Moreover, the displacement of binding of [³H]diprenorphine by BNTX and NTB in delta receptor containing CHOmembranes is approximately linear, whereas the displacement of[³H]diprenorphine binding by these compounds in the NG108-15 membraneswas biphasic. This biphasic recognition by both BNTX and NTB maydepend on the environment, such as the type of associated G proteins,which allows differentiation of the receptor into two apparentbinding affinities for these antagonists. However, the agonistDPDPE recognizes only a single site. Because agonists are highlysusceptible to the presence of Na⁺ ions and guanine nucleotides (Childers and Snyder, 1980; Kellyet al., 1982) and therefore to the state of coupling of the receptor,this suggests that the biphasic activity of BNTX and NTB resultsfrom a combination of the chemical nature of the compounds themselvesand the membrane environment.

Several opioid agonist alkaloids and peptides were examined for their ability to stimulate [³⁵S]GTP $gamma$ S binding by using maximally effective concentrations asreported for their activity against adenylyl cyclase in thesecells (Childers et al., 1993; Law et al., 1983; Roerig et al.,1996). The most efficacious were the peptides, although DSLETwas more efficacious than either DPDPE or [D-Ala²,Glu⁴]deltorphin II. Etorphine was equally efficacious with DPDPE and[D-Ala²,Glu⁴]deltorphin II, but other alkaloid derivatives were partial agonists.The relative ability to stimulate [³⁵S]GTP $gamma$ S binding among these compounds was similar to their abilityto inhibit adenylyl cyclase. Of the antagonists examined, diprenorphinehad some activity, as previously seen at the delta receptor inNG108-15 cells (Law et al., 1983), as did naltrindole, which isreported to have agonist effects at supraspinal delta receptorsin the mouse (Stapelfeld et al., 1992). BNTX, NTB and TIPP hadno efficacy in this system. In contrast, the antagonist ICI 174864,a delta opioid ligand with negative intrinsic activity (Costaand Herz, 1989), reduced the basal binding of [³⁵S]GTP $gamma$ S in membranes of NG108-15 cells, confirming the presenceof constitutively active receptors of the delta type.

The effect of ICI 174864 in lowering basal [³⁵S]GTP $gamma$ S was not as pronounced as that of pertussis toxin. This is in contrastwith the findings of Mullaney et al. (1996), using the clonedmouse delta receptor expressed in Rat 1 fibroblasts, in whichpertussis toxin and ICI 174864 inhibited basal [³⁵S]GTP $gamma$ S binding to the same extent and suggested ICI 174864 wasan inverse agonist with high intrinsic activity. The observeddifference could be explained by the fact that in the NG108-15cells ICI 174864 may not be a full inverse agonist or that otherreceptors present in NG108-15 cells and also linked to G_o/G_i proteinsare active in the agonist-unoccupied state. Such receptors includemuscarinic M₄ receptors (Graeser and Neubig, 1993; Lazareno etal., 1990; Michel et al., 1989), alpha-2B adrenergic (Graeserand Neubig, 1993; McClue and Milligan, 1990) and cannabinoid (Caulfieldand Brown, 1992; Mackie et al., 1993).

The inverse agonist effect of ICI 174864 was much more pronounced in buffer in which the Na⁺ ions had been replaced with K⁺ ions, an effect previously reported for the inverse agonist activityof ICI 174864 when determined by measures of GTPase activity (Costaand Herz, 1989). Seven-transmembrane domain G protein-linked receptorsexist in equilibrium between an inactive (R) and active conformation(R*). In the presence of agonist (A), the R* form is greatly favoredand interacts with G protein to form the active ternary complex(AR*G) (Birnbaumer et al., 1990). Constitutive activity occurswhen receptors exist in the R* state and are able to spontaneouslycouple to G proteins in the absence of agonist. Ligands with negativeintrinsic activity shift the equilibrium in favor of R and therebylead to a reduction in constitutive activity, manifest in thepresent experiments as a reduction in basal [³⁵S]GTP $gamma$ S binding. Thus, despite the fact that Na⁺ ions and ICI 174864 are acting through different mechanisms,the presence of Na⁺ will mask the inverse agonist effect of ICI 174864 because bothbring about the same result, namely, a reduction in R* with aconcomitant rise in R. When Na⁺ ions in the medium are replaced with K⁺ ions, the basal binding of [³⁵S]GTP $gamma$ S is considerably higher, so the inverse agonist effectof ICI 174864 is apparently greater.

The increase in the basal level of binding of [³⁵S]GTP $gamma$ S afforded by removal of Na⁺ ions should also have an effect on agonist responses. In thepresence of 100 mM Na⁺, diprenorphine only produced $approx$ 30% of the maximal stimulationof [³⁵S]GTP $gamma$ S binding produced by the full agonist DSLET. However, whenNa⁺ ions were replaced by K⁺ ions in the reaction buffer, diprenorphine produced 70% of theDSLET response. Thus, because there is a finite number of G proteinsthat can be labeled by [³⁵S]GTP $gamma$ S, the relative efficacies of compounds can be varied byalteration of the basal level of coupling through changes in theconcentration of Na⁺ ions.

In conclusion, delta opioid agonists have been shown to stimulate [³⁵S]GTP $gamma$ S binding to pertussis toxin-sensitive G proteins in membranesfrom NG108-15 cells in a naloxone-reversible manner. Optimal conditionsfor this assay have been established to provide a rapid, sensitiveand reproducible method to measure the potency and intrinsic activityof G protein activation at an endogenously expressed delta opioidreceptor. The relative efficacy of a series of compounds is governedby the level of G protein, which places a ceiling on the maximumeffect that can be obtained. Therefore, through judicious manipulationof assay conditions, it should be possible to match the relativedelta opioid efficacies in this cell system with those seen indifferent tissues and thus design screening conditions suitablefor the detection of different pharmacological and side effectprofiles.

	Footnotes

Accepted for publication August 19, 1997.

Received for publication February 21, 1997.

¹ This work was supported by an EPSRC Research Studentship (P.G.S.) and United States Public Health Service Grant DA-00254-25.

Send reprint requests to: Dr. J. R. Traynor, Department of Pharmacology, University of Michigan Medical School, 1301 MSRBIII, Ann Arbor, MI 48109-0632. E-mail: jtraynor{at}umich.edu

	Abbreviations

[D-Ala², Glu⁴]deltorphin II, [Tyr-D-Ala-Phe-Glu-Val-Val-Gly-NH₂]; DPDPE, [D-Pen²,D-Pen⁵]enkephalin; DSLET, [D-Ser²,Leu⁵]enkephalin-Thr⁶; BNTX, 7-benzylidenenaltrexone; NTB, naltriben; TIPP, Tyr-Tic-Phe-Phe (Tic = tetrahydroisoquinoline-3-carboxylic acid); GTP $gamma$ S, guanosine-5 $'$ -O-(3-thio)triphosphate; DAMGO, [D-Ala², MePhe⁴, Glyol⁵]enkephalin; CHO, Chinese hamster ovary; DMEM, Dulbecco's modified Eagle's medium.

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Delta Opioid Modulation of the Binding of Guanosine-5-O-(3-[35S]thio)triphosphate to NG108-15 Cell Membranes: Characterization of Agonist and Inverse Agonist Effects1

Delta Opioid Modulation of the Binding of Guanosine-5 $'$ -O-(3-[³⁵S]thio)triphosphate to NG108-15 Cell Membranes: Characterization of Agonist and Inverse Agonist Effects¹