Comparison of Pharmacological Activities of Buprenorphine and Norbuprenorphine: Norbuprenorphine Is a Potent Opioid Agonist

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Vol. 297, Issue 2, 688-695, May 2001

Comparison of Pharmacological Activities of Buprenorphine and Norbuprenorphine: Norbuprenorphine Is a Potent Opioid Agonist

Peng Huang, George B. Kehner, Alan Cowan and Lee-Yuan Liu-Chen

Department of Pharmacology, Temple University Medical School, Philadelphia, Pennsylvania

	Abstract

Top Abstract Introduction Experimental Procedures Results Discussion References

Buprenorphine (BUP) is an oripavine analgesic that is beneficial in the maintenance treatment of opiate-dependent individuals.Although BUP has been studied extensively, relatively little isknown about norbuprenorphine (norBUP), a major dealkylated metaboliteof BUP. We now describe the binding of norBUP to opioid and nociceptin/orphaninFQ (ORL1) receptors, and its effects on [³⁵S]guanosine-5'-O-( $gamma$ -thio)triphosphate ([³⁵S]GTP $gamma$ S) binding mediated by opioid or ORL1 receptors and in themouse acetic acid writhing test. Chinese hamster ovary cells stablytransfected with each receptor were used for receptor bindingand [³⁵S]GTP $gamma$ S binding. NorBUP exhibited high affinities for µ-, $delta$ -,and $kappa$ -opioid receptors with K_i values in the nanomolar or subnanomolarrange, comparable to those of BUP. NorBUP and BUP had low affinitiesfor the ORL1 receptor with K_i values in the micromolar range.In the [³⁵S]GTP $gamma$ S binding assay, norBUP displayed characteristics distinctfrom BUP. At the $delta$ -receptor, norBUP was a potent full agonist,yet BUP had no agonist activity and antagonized actions of norBUPand DPDPE. At µ- and $kappa$ -receptors, both norBUP and BUP were potentpartial agonists, with norBUP having moderate efficacy and BUPhaving low efficacy. At the ORL1 receptor, norBUP was a full agonistwith low potency, while BUP was a potent partial agonist. In thewrithing test, BUP and norBUP both suppressed writhing in an efficaciousand dose-dependent manner, giving A₅₀ values of 0.067 and 0.21mg/kg, s.c., respectively. These results highlight the similaritiesand differences between BUP and norBUP, each of which may influencethe unique pharmacological profile of BUP.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

Buprenorphine (BUP) (Fig. 1), an oripavine derived from thebaine, has antinociceptive activities in animal pain models andis used clinically for treatment of moderate-to-severe pain (Cowanand Lewis, 1995). BUP is 25 to 40 times more potent than morphineas an analgesic after parenteral injection (Cowan et al., 1977;Lewis, 1995). Since it is associated with less physical dependenceand reinforcing effects than many other opioids (Negus and Woods,1995), BUP is being developed as a potential pharmacotherapy foropioid abuse anddependence.

[³H]BUP administered in vivo preferentially labels µ-opioid receptor sites (Sadee et al., 1982). Although BUP was reportedto have pharmacological effects on $delta$ - and $kappa$ -opioid receptors (Belchevaet al., 1993, 1996; Pick et al., 1997), its analgesic effectshave been ascribed mostly to actions on the µ-receptor (Dum andHerz, 1981; Kamei et al., 1997). At the biochemical level, BUPis a partial agonist at the µ-opioid receptor (Traynor and Nahorski,1995; Selley et al., 1998; Toll et al., 1998; Lee et al., 1999),or an antagonist (Romero et al., 1999). At the $kappa$ -opioid receptor,BUP acts as a low-efficacy partial agonist (Zhu et al., 1997)or as an antagonist (Romero et al., 1999) or shows no agonistactivity (Toll et al., 1998). At the $delta$ -opioid receptor, BUP showsno agonistic effects (Toll et al., 1998; Lee et al., 1999; Romeroet al., 1999). BUP exhibited pure antagonism at rat brain ORL1receptors, but acted as a partial agonist or a full agonist atthe recombinant human ORL1 receptor (Wnendt et al., 1999; Hashimotoet al., 2000; Hawkinson et al., 2000).

Norbuprenorphine (norBUP) (Fig. 1), the N-dealkylated product of BUP, is a major metabolite of BUP in humans and rats (Coneet al., 1985; Garrett and Chandran, 1990). Ohtani et al. (1989)showed that norBUP was measurable in plasma between 2 to 3 h aftera sublingual dose of BUP in a human volunteer. Kuhlman et al.(1998) demonstrated that the mean steady-state plasma concentrationof norBUP exceeded that of buprenorphine after daily administrationof sublingual buprenorphine to humans, whereas Tzeng et al. (2000)reported that plasma levels of BUP and norBUP declined in a multipleexponential manner inrats.

Although the pharmacology of BUP has been studied extensively, relatively little is known about norBUP. Ohtani et al. (1995)reported that norBUP was considerably less hydrophobic than BUP,and the intrinsic analgesic activity of i.c.v. norBUP was aboutone-fourth that of BUP in the rat tail-flick test. Additionally,these researchers have reported that norBUP does not readily crossthe blood-brain barrier into the rat brain. Intravenous administrationof norBUP at 1 to 3 mg/kg decreased respiratory rate, whereasBUP had no effect up to 3 mg/kg (Ohtani et al., 1997). The respiratorydepression induced by norBUP appeared to be mediated by µ-opioidreceptors in the lung rather than in the brain (Ohtani et al.,1997).

In the present study, we compared the pharmacological profiles of BUP and norBUP on opioid and nociceptin/orphanin FQ (ORL1)receptors. We determined their binding properties to these receptors,and their potencies and efficacies in stimulating these receptorsto enhance [³⁵S]GTP $gamma$ S binding in Chinese hamster ovary (CHO) cells stably transfectedwith the µ-, $delta$ -, or $kappa$ -opioid receptor or ORL1 receptor. In addition,we compared the antinociceptive effects of norBUP and BUP in anin vivo assay $---$ the mouse acetic acid writhingtest.

	Experimental Procedures

Top Abstract Introduction Experimental Procedures Results Discussion References

Materials. Norbuprenorphine was purchased from Ultrafine (Manchester, England). ( $-$ )-Buprenorphine HCl and U50,488H were supplied by theNational Institute on Drug Abuse. (+)-Buprenorphine HCl was synthesizedby Drs. N. A. Grayson and K. C. Rice of the National Instituteof Digestive and Kidney Disease, National Institutes of Health.[15,16-³H]Diprenorphine (56 Ci/mmol), [leucyl-3,4,5-³H]nociceptin/orphanin FQ (N/OFQ) (87.7 Ci/mmol), [³⁵S]guanosine-5'-O-(3-thio)triphosphate ([³⁵S]GTP $gamma$ S) (1250 Ci/mmol), and [³H]cAMP (30-40 Ci/mmol) were obtained from NEN Life Science Products,Inc. (Boston, MA). DAMGO and nociceptin/OFQ were purchased fromPhoenix Pharmaceuticals, Inc. (Belmont, CA) The following compoundswere obtained as indicated: naloxone HCl (Sigma, St. Louis, MO),GTP $gamma$ S (Boehringer-Mannheim, Indianapolis, IN), geneticin (G418)(Cellgro, Mediatech, Inc., Herndon, VA), and DPDPE (ICI, Downingtown,PA). Bovine serum albumin (BSA; 1 mg/ml) was added to all BUPsolutions, and 0.05 mg/ml bacitracin and 1 mg/ml BSA were includedin all buffers for nociceptin/OFQ.

CHO Cell Lines. CHO cells stably transfected with the rat µ-opioid receptor (Chen et al., 1993) was established as we described previously(Chen et al., 1995). CHO cells stably expressing the mouse $delta$ -opioidreceptor (Evans et al., 1992) were kindly supplied by Dr. Ping-YiLaw, Department of Pharmacology, University of Minnesota Schoolof Medicine, Minneapolis, MN. CHO cells with stable expressionof the human $kappa$ -opioid receptor (Zhu et al., 1995) was establishedpreviously (Zhu et al., 1997). CHO cells stably transfected withthe human ORL1 receptor were a gift from Dr. Lawrence Toll, SRIInternational, Menlo Park, CA (Adapa and Toll, 1997).

Cell Membrane Preparation. Membranes were prepared according to a modified procedure of (Zhu et al., 1997). Cells were washed twice and harvested inVersene solution (EDTA 0.54 mM, NaCl 140 mM, KCl 2.7 mM, Na₂HPO₄8.1 mM, KH₂PO₄ 1.46 mM, and glucose 1 mM) and centrifuged at 500gfor 3 min. The cell pellet was suspended in buffer A [5 mM Tris(pH 7.4), 5 mM EDTA, 5 mM EGTA, and 0.1 mM phenylmethylsulfonylfluoride], passed through a 26-gauge <FR><NU>3</NU><DE>8</DE></FR> needlefive times and then centrifuged at 46,000g for 30 min. The pelletwas resuspended in buffer A and centrifuged again. The membranepellet was resuspended in buffer B [50 mM Tris-HCl (pH 7.0) and0.32 mM sucrose], aliquoted at about 600 µg/ml, frozen in dryice/ethanol, and stored at $-$ 80°C. All procedures were performedat 4°C.

Receptor Binding. Ligand binding experiments were carried out with [³H]diprenorphine for opioid receptors and [³H]nociceptin/OFQ for the ORL1receptor.

Saturation binding of [³³H]diprenorphine to µ-, $delta$ -, and $kappa$ -opioid receptors was performed with at least six concentrations of[³³H]diprenorphine (ranging from 25 pM to 1-2 nM), and K_d and B_maxvalues were determined. Competition inhibition by BUP, norBUP,or (+)-BUP of [³H]diprenorphine (0.4 nM) binding to opioid receptors was performedin the absence or presence of various concentrations of each drug.Binding was carried out in 50 mM Tris-HCl buffer containing 1mM EGTA (pH 7.4) at room temperature for 1 h in duplicate in afinal volume of 1 ml with ~10 to 20 µg of membrane protein. Naloxone(10 µM) was used to define nonspecific binding. Bound and free[³H]diprenorphine were separated by filtration under reduced pressurewith GF/B filters presoaked with 0.1 mg/ml BSA and 0.2% polyethyleneimine.Radioactivity on filters was determined by liquid scintillationcounting. Each experiment was performed in duplicate and repeatedat least three times. Binding data were analyzed with the EBDAprogram (McPherson, 1983

). K_i values of each drug were determined(Cheng and Prusoff, 1973

Saturation binding of [³H]nociceptin/OFQ to the ORL1 receptor was performed with at least six concentrations of [³H]nociceptin/OFQ (ranging from 25 pM to 2 nM), and K_d and B_maxvalues were determined. Competition inhibition by BUP, norBUP,or (+)-BUP of [³H]nociceptin/OFQ (0.3 nM) binding to the ORL1 receptor was performed,and K_i values of each drug were determined. Nociceptin/OFQ (150nM) was used to define nonspecificbinding.

[³⁵S]GTP $gamma$ S Binding. Determination of [³⁵S]GTP $gamma$ S binding to G proteins was carried out using a modified procedure of Zhu et al. (1997). Immediatelybefore the [³⁵S]GTP $gamma$ S binding assay, membranes were thawed at 37°C, chilledon ice, and diluted with buffer C [50 mM HEPES (pH 7.4), 100 mMNaCl, 5 mM MgCl₂, and 1 mM EDTA]. Membranes (10 µg) were incubatedin buffer C containing [³⁵S]GTP $gamma$ S (200 pM, 300,000-500,000 dpm) and 15 µM GDP with or withouta ligand (10¹² to 10⁴ M) in a total volume of 0.5 ml for 60 min at 30°C. Nonspecificbinding was defined by incubation in the presence of 10 µM GTP $gamma$ S.Bound and free [³⁵S]GTP $gamma$ S were separated by filtration with GF/B filters under reducedpressure. Radioactivity on filters was determined by liquid scintillationcounting. EC₅₀ values and maximal responses (E_max) of drugs weredetermined by curve fitting to the equation for a sigmoidal curveE = [E_max/]1 + ([D]/EC₅₀)ⁿ + basal level, where E is effect produced by a certain concentrationof the drug, [D], E_max is the maximal response elicited by thedrug, and n is a fittingparameter.

Determination of Adenylate Cyclase Activity. The cAMP assay is based on the method described by Cote et al. (1982). CHO cells expressing the ORL1 receptor were added toassay tubes containing isobutylmethylxanthine, forskolin, andN/OFQ in serum-free Dulbecco's modified Eagle's medium (finalvolume 250 µl, final 2.5 mM isobutylmethylxanthine, and 25 µMforskolin). For the basal level, forskolin and agonist were omitted.Assay mixtures were incubated at 37°C for 10 min, and the reactionwas terminated by placing the tubes in boiling water for 5 min.The amounts of cAMP in the sample tubes were determined with thecAMP binding protein method. Briefly, [³H]cAMP (~30,000 dpm in 0.02 M citrate phosphate buffer, pH 5.0)was added to all sample tubes and standard tubes (from 1.25-40pmol of cAMP) on ice. cAMP binding protein partially purifiedfrom bovine adrenal glands was added to each tube at an amountthat gave 10,000 to 20,000 dpm [³H]cAMP binding in the absence of cold cAMP, except the blanks.The mixture (final 170 µl) was incubated on ice or at 4°C forat least 2 h. Bound and free [³H]cAMP were separated by absorption of free [³H]cAMP by charcoal (100 µl of 10% Norit A, 4% BSA, and 1% AntifoamA) and centrifugation. Radioactivity of bound [³H]cAMP in an aliquot of the supernatant was determined by liquidscintillation counting. The amounts of cAMP were calculated basedon the standardcurve.

Acetic Acid Writhing Test. Male Swiss albino mice (24-27 g; n = 7-12) were injected s.c. with either saline or test agent. After 20 min, acetic acid(0.6%) was injected i.p. (0.25 ml/25 g). A further 5 min later,the number of writhes was counted for 10 min. The number of writhesin each test period was then normalized to the mean number shownby the control group, and antinociceptive-50 (A₅₀) values wereobtained by nonlinear regressionanalysis.

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

Determination of Receptor Expression Levels of CHO-µ, CHO- $delta$ , and CHO- $kappa$ , and CHO-ORL1 Cells. The rat µ-opioid receptor, mouse $delta$ -opioid receptor, human $kappa$ -opioid receptor, and human ORL1 receptor were stably transfectedinto CHO cells. Saturation binding of [³H]diprenorphine to µ-, $delta$ -, and $kappa$ -opioid receptors and [³H]nociceptin/OFQ to the ORL1 receptor was performed on membranes,and K_d and B_max values were determined. [³H]Diprenorphine exhibited high affinities for µ-, $delta$ -, and $kappa$ -opioidreceptors, with K_i values of 0.14 ± 0.03 nM, 0.33 ± 0.04 nM, and0.15 ± 0.03 nM, respectively (mean ± S.E.M., n = 3-5) and theB_max values of 2.1 ± 0.5, 1.1 ± 0.3, and 1.3 ± 0.2 pmol/mg ofprotein, respectively (mean ± S.E.M., n = 3-5). [³H]nociceptin/OFQ bound to the ORL1 receptor with high affinitywith a K_i value of 0.14 ± 0.02 nM and a B_max value of 5.0 ± 0.7pmol/mg of protein (mean ± S.E.M., n = 3).

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Fig. 1. Chemical structures of BUP and norBUP.

Binding Affinities of norBUP and BUP to Opioid Receptors and ORL1 Receptor. Competitive inhibition of [³H]diprenorphine to opioid receptors or [³H]nociceptin/OFQ to ORL1 receptor by BUP, norBUP, and (+)-BUPwas conducted to determine binding affinities of these ligandsto µ-, $delta$ -, and $kappa$ -opioid receptors or the ORL1 receptor (Fig. 2,Table 1). NorBUP exhibited high affinities for µ-, $delta$ -, and $kappa$ -opioidreceptors, with K_i values in inhibiting [³H]diprenorphine binding in the subnanomolar and nanomolar rangewith a ratio of 1:45:13 for µ: $delta$ : $kappa$ . In contrast, norBUP had a lowaffinity for the ORL1 receptor, with a K_i value in inhibiting[³H]N/OFQ binding in the micromolar range. Similarly, BUP had highaffinities for µ-, $delta$ -, and $kappa$ -opioid receptors, with K_i valuesin the subnanomolar range and had a low affinity for the ORL1receptor, with a K_i value in the micromolar range. (+)-BUP didnot bind to µ-, $delta$ -, or $kappa$ -opioid receptors or the ORL1 receptor.

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Fig. 2. Competitive inhibition by BUP, norBUP, and (+)-BUP of [³H]diprenorphine binding to µ-, $delta$ -, and $kappa$ -opioid receptors and [³H]nociceptin/OFQ binding to the ORL1 receptor. Membranes were prepared from CHO cells stably transfected with the µ-, $delta$ -, or $kappa$ -opioid receptor or the ORL1 receptor. Binding of opioid receptors and the ORL1 receptor was carried out with ~0.4 nM [³H]diprenorphine and ~0.3 nM [³H]nociceptin/OFQ, respectively, in the presence and absence of various concentrations of BUP, norBUP, and (+)-BUP as described under Experimental Procedures. Specific [³H]diprenorphine and [³H]nociceptin/OFQ binding was ~7,600 dpm/tube and ~12,000 dpm/tube, respectively, and the corresponding nonspecific binding was 400 to 600 dpm/tube and 1,000 dpm/tube, respectively. Data were normalized to percentage of specific binding. Each value represents the mean ± S.E.M of at least three independent experiments performed in duplicate. Apparent K_i values are shown in Table 1.

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TABLE 1
Apparent K_i values (nM) of BUP and norBUP for the opioid receptors and the ORL1 receptor
Apparent K_i values were calculated from the equation K_i = IC₅₀/(1 ⁺ [L]/K_d); IC₅₀ values were derived from the competition curves shown in Fig. 2. Each value represents the mean ± S.E.M. n = number of independent experiments performed in duplicate.

Potencies and Efficacies of norBUP and BUP in the [³⁵S]GTP $gamma$ S Binding Assay. [³⁵S]GTP $gamma$ S binding to membranes of CHO cells stably transfected with the µ-, $delta$ -, and $kappa$ -opioid receptor or the ORL1 receptorin response to norBUP, BUP, and (+)-BUP was examined, with a prototypicalfull agonist as the control for each receptor (Fig. 3). EC₅₀ valuesand maximal responses are shown in Table 2. NorBUP was a partialagonist at µ- and $kappa$ -receptors and a full agonist at the $delta$ -receptor,with EC₅₀ values in the nanomolar range, whereas it was a fullagonist at ORL1 receptor with low potency, with EC₅₀ values inthe micromolar range. BUP was a partial agonist at the µ- andORL1 receptors, with EC₅₀ values in the nanomolar range. In addition,BUP demonstrated weak agonism at the $kappa$ -receptor giving a maximalresponse of 10% and was inactive at the $delta$ -receptor. (+)-BUP didnot activate µ-, $delta$ -, or $kappa$ -opioid receptors or the ORL1 receptor.

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Fig. 3. Stimulation of [³⁵S]GTP $gamma$ S binding to membranes of CHO cells stably transfected with the µ-, $delta$ -, $kappa$ -opioid or the ORL1 receptor by BUP, norBUP, and a full agonist for each receptor. [³⁵S]GTP $gamma$ S binding was performed as described under Experimental Procedures. Nonspecific binding, estimated using 10 µM cold GTP $gamma$ S, was ~500 dpm and was subtracted from each datum. Basal [³⁵S]GTP $gamma$ S binding in the absence of added drugs was 3000 to 5000 dpm. Data were normalized to percentage of the basal [³⁵S]GTP $gamma$ S binding. Each value represents the mean ± S.E.M. of at least three independent experiments performed in duplicate. EC₅₀ values and maximal responses are shown in Table 2.

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TABLE 2
EC₅₀ values and maximal effects of BUP and norBUP in stimulating [³⁵S]GTP $gamma$ S binding to membranes of CHO cells stably transfected with the µ-, $delta$ -, or $kappa$ -opioid or the ORL1 receptor
DAMGO, DPDPE, U50,488H, and N/OFQ were used as full agonists for the µ-, $delta$ -, $kappa$ -opioid and the ORL1 receptors, respectively. Data were derived from the curves in Fig. 3.

Effects of BUP and norBUP on ORL1 Receptor-Mediated Inhibition of Forskolin-Stimulated Adenylate Cyclase. Our finding that BUP is a partial agonist at the ORL1 receptor in stimulating [³⁵S]GTP $gamma$ S binding differs from those of Wnendt et al. (1999) andHashimoto et al. (2000). These researchers demonstrated that BUPwas a potent full agonist at the ORL1 receptor in inhibiting forskolin-stimulatedadenylate cyclase activity. The difference may be due to the differentfunctional assays used. We thus determined potencies and efficaciesof BUP and norBUP at the ORL1 receptor in inhibiting forskolin-stimulatedadenylate cyclase activity. As shown in Fig. 4, BUP and norBUPinhibited forskolin-stimulated adenylate cyclase to similar extentsas N/OFQ, indicating that both compounds are full agonists inthis assay. The EC₅₀ values were determined to be 26.2 nM and1360 nM, respectively, indicating that BUP is approximately 52times more potent than norBUP.

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Fig. 4. Inhibition of cAMP accumulation by nociceptin/OFQ, BUP, and norBUP in CHO cells stably transfected with the ORL1 receptor. CHO cells stably expressing ORL1 receptors were incubated in serum-reduced medium with 10 µM forskolin and 1 mM isobutylmethylxanthine with and without different concentrations of drugs. cAMP contents were determined as described under Experimental Procedures and normalized to percentage of the forskolin-stimulated cAMP level. Each value represents the mean ± S.E.M. of at least three independent experiments performed in duplicate.

Antagonistic Effect of Buprenorphine at the $delta$ -Opioid Receptor. Since BUP had high affinity for the $delta$ -receptor, yet no agonist activity, we examined whether BUP had antagonistic effectson norBUP-stimulated [³⁵S]GTP $gamma$ S binding to membranes of CHO- $delta$ cells. BUP shifted the dose-responsecurves of norBUP to the right in a parallel fashion (Fig. 5A).The potency of BUP in antagonizing the action of norBUP at the $delta$ -receptor was determined. Schild analysis was performed, andthe slope was determined to be 1.09, indicating that BUP is acompetitive antagonist at the $delta$ - receptor (Fig. 5B). The pA₂ valueof BUP was determined to be 9.31 ± 0.14 (0.49 nM) (n = 3).

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Fig. 5. A, antagonistic effects of BUP on norBUP-stimulated [³⁵S]GTP $gamma$ S binding to membranes of CHO cells stably transfected with $delta$ -opioid receptor. B, Schild plot of BUP in antagonizing norBUP-induced increase in [³⁵S]GTP $gamma$ S binding. [³⁵S]GTP $gamma$ S binding was performed as described under Experimental Procedures, with various concentrations of norBUP in the absence or presence of a fixed concentration (10⁹, 3 × 10⁹, 10⁸, or 3 × 10⁸ M) of BUP. Nonspecific binding, estimated using 10 µM cold GTP $gamma$ S, was ~500 dpm and was subtracted from each datum. Basal [³⁵S]GTP $gamma$ S binding in the absence of added drugs was 3000 to 5000 dpm. Data were normalized to percentage of the basal [³⁵S]GTP $gamma$ S binding. Each value represents the mean ± S.E.M. of at least three independent experiments performed in duplicate.

Antinociceptive Activity of norBUP and BUP. NorBUP was a relatively potent analgesic, suppressing writhing with an efficacy similar to that of BUP (Fig. 6). The antinociceptiveactivity of norBUP was dose-dependent, giving an A₅₀ value of0.21 mg/kg, approximately 3 times greater than that of BUP.

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Fig. 6. Antinociceptive effects of BUP, norBUP, and (+)-BUP in the mouse acetic acid writhing test. The mice (n = 7-12) were pretreated s.c. with either saline or test compound. After 20 min, the mice received 0.6% acetic acid i.p., and a further 5 min later, the number of writhes was counted for 10 min. Each point represents the mean (±S.E.M.) percentage inhibition of writhing relative to the saline-control group.

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

In the present study, we have shown that norBUP has a distinctly different pharmacological profile from BUP although bothhave high affinities for µ-, $delta$ -, and $kappa$ - opioid receptors and lowaffinities for the ORL1 receptor. NorBUP is a full agonist atthe $delta$ -receptor, whereas BUP is an antagonist. Both are partialagonists at µ- and $kappa$ -receptors, with norBUP having higher efficacythan BUP. NorBUP and BUP are less efficacious at the $kappa$ -receptorrelative to the µ-receptor. To the best of our knowledge, thisrepresents the first characterization of pharmacological activitiesof norBUP at cloned µ-, $delta$ -, and $kappa$ - opioid receptors and the ORL1receptor.

NorBUP was a more efficacious but slightly less potent partial agonist than BUP at the µ-receptor, with an 81% maximal [³⁵S]GTP $gamma$ S binding response and an EC₅₀ of 1.5 nM. Our finding thatBUP stimulated [³⁵S]GTP $gamma$ S binding to CHO-µ membranes with an E_max of 38% and anEC₅₀ of 0.08 nM is consistent with several previous reports. Inthese reports, BUP was a potent partial agonist at the µ-opioidreceptor and enhanced [³⁵S]GTP $gamma$ S binding to varying extents: E_max of about 50% in C6 gliomacells expressing the rat µ-receptor (Lee et al., 1999), 73% inhuman neuroblastoma SH-SY5Y cells (Traynor and Nahorski, 1995),43% in CHO cells stably transfected with the mouse µ-receptor,and 10% in the rat thalamus (Selley et al., 1998). In addition,with inhibition of forskolin-stimulated adenylate cyclase as theendpoint, BUP displayed agonism at the mouse µ-receptor expressedin HEK293 cells (Blake et al., 1997) and the human µ-receptorexpressed in CHO cells (Yu et al., 1997). In contrast, BUP failedto stimulate [³⁵S]GTP $gamma$ S binding in guinea pig caudate membranes and showed antagonismunder certain conditions (Romero et al., 1999). The differencesin the efficacy of BUP in these preparations may be related toseveral factors, including different species of µ-opioid receptorsused, the number of µ-opioid receptors, the repertoire and levelof G proteins to which the receptor can be coupled, and the receptor/Gproteinratio.

NorBUP acted as a full agonist at the $delta$ -opioid receptor with an EC₅₀ value of 30.4 nM. In contrast, BUP had no agonistic activityand was a potent competitive antagonist against effects of norBUPon [³⁵S]GTP $gamma$ S binding at the $delta$ -opioid receptor. The pA₂ value (0.49nM) of BUP at $delta$ -receptors is similar to its K_i value (0.42 nM).Our observation that BUP has no agonist activity at the $delta$ -opioidreceptor is in accord with previous reports (Toll et al., 1998;Lee et al., 1999; Romero et al., 1999). Thus, depending on theconcentrations of BUP and its metabolite norBUP, BUP administrationcan have varying activities in vivo at the $delta$ -receptor, rangingfrom being predominantly antagonistic to largely agonistic. Sincechronic buprenorphine increased $delta$ ₂-binding sites in some brainregions without changing $delta$ ₁-sites (Belcheva et al., 1993, 1996),buprenorphine may have different actions on the two subtypes of $delta$ -receptor invivo.

We have shown that norBUP is a potent partial agonist at the $kappa$ -opioid receptor with an E_max of 60% and an EC₅₀ of 7.2 nM instimulating [³⁵S]GTP $gamma$ S binding, having higher efficacy than BUP. That BUP actedas a partial agonist with low efficacy at the $kappa$ -opioid receptoris similar to our previous report (Zhu et al., 1997). In contrast,BUP failed to stimulate [³⁵S]GTP $gamma$ S binding (Toll et al., 1998; Romero et al., 1999) and inhibited $kappa$ -agonist-promoted [³⁵S]GTP $gamma$ S binding with high potency (Romero et al., 1999). In addition,BUP is a potent antagonist at the $kappa$ -receptor in several in vivotests (Leander, 1987, 1988; Negus and Dykstra, 1988). The differencein efficacy of buprenorphine in different preparations may beattributed to variations in the receptor level, the populationand level of G proteins, and receptor/G protein ratio as mentionedabove.

NorBUP was found to be a full agonist at the ORL1 receptor with low potency, having an EC₅₀ >1 µM in both [³⁵S]GTP $gamma$ S binding and inhibition of forskolin-stimulated adenylatecyclase. In contrast, BUP was a partial agonist at the ORL1 receptor,with an EC₅₀ of 35 nM and an E_max of 60% in stimulating [³⁵S]GTP $gamma$ S binding (see Table 2) and BUP acted as a full agonistwith an EC₅₀ of 26 nM when evaluated by inhibition of forskolin-stimulatedadenylate cyclase. The difference in the efficacy of BUP in thetwo endpoints may be due to the possibility that full inhibitionof adenylyl cyclases requires only partial activation of G proteins.Our results with BUP on the ORL1 receptor are consistent withthose of Wnendt et al. (1999), Bloms-Funke et al. (2000), Hashimotoet al. (2000), and Hawkinson et al. (2000). Using [³⁵S]GTP $gamma$ S binding as the functional measure, Bloms-Funke et al.(2000) and Hawkinson et al. (2000) showed that BUP exhibited partialagonism at the human ORL1 receptor. In contrast, with inhibitionof forskolin-stimulated adenylate cyclase as the endpoint, BUPwas reported to be a full agonist at the ORL1 receptor (Wnendtet al., 1999; Hashimoto et al., 2000).

Comparison between the EC₅₀ values of norBUP and BUP in stimulating [³⁵S]GTP $gamma$ S binding (see Table 2) and their K_i values in inhibiting[³H]diprenorphine binding to µ-, $delta$ -, and $kappa$ -opioid receptors (seeTable 1) reveals that EC₅₀ values for norBUP or BUP are similaror greater than their corresponding K_i values. In contrast, forthe ORL1 receptor, the K_i values of norBUP or BUP are more than4 times greater than their corresponding EC₅₀ values. These resultsindicate that there are spare receptors for norBUP and BUP intheir stimulation of the ORL1 receptor, but not opioid receptors,to activate Gproteins.

(+)-BUP does not bind to or activate µ-, $delta$ -, and $kappa$ -opioid receptors or the ORL1 receptor, indicating that binding of BUP tothese receptors isstereospecific.

Results from the acetic acid writhing test showed that norBUP, injected s.c. in mice, has comparable antinociceptive efficacyto BUP, with BUP being about 3 times more potent than norBUP.As noted previously (Cowan et al., 1977), the dose-response relationshipfor BUP is sigmoidal in this procedure. In contrast, BUP producesbell-shaped curves in several other rodent antinociceptive assays(e.g., Rance et al., 1980; Dum and Herz, 1981; Bryant et al.,1983; Wheeler-Aceto and Cowan, 1991; Woods et al., 1992). Thus,BUP is associated with antinociception at low doses, yet higherdoses are often less effective. N/OFQ displays pronociceptiveor hyperalgesic activity in different animal pain models afterintracerebroventricular administration (Meunier et al., 1995;Reinscheid et al., 1995; Hara et al., 1997), which has been attributedto an inhibition of stress-induced analgesia (Mogil et al., 1996a,b).As hypothesized by Wnendt and colleagues (Wnendt et al., 1999;Bloms-Funke et al., 2000), the ORL1 agonistic activity of BUPmay contribute to its bell-shaped dose-response curve in, forexample, the mouse tail-flick test. BUP is a potent partial agonistat the µ-receptor, and norBUP is a potent partial agonist at theµ- and $kappa$ -receptors and a potent full agonist at the $delta$ -receptor,with EC₅₀ values in the subnanomolar or nanomolar range, whichcontribute to the antinociceptive effect of low doses of BUP administeredin vivo. At the ORL1 receptor, BUP is a potent partial agonistin stimulating [³⁵S]GTP $gamma$ S binding and a full agonist in inhibiting forskolin-stimulatedadenylate cyclase, with EC₅₀ values of about 30 nM. The actionof BUP at the ORL1 receptor at higher concentrations may counterthe antinociception produced by BUP and norBUP on opioid receptors,resulting in less antinociception at higher doses and thus thebell-shaped dose-response curves. This hypothesis is currentlybeing tested. Although norBUP is a full agonist at the ORL1 receptor,its low potency (EC₅₀ of 1.4 µM) makes it less likely to contributesignificantly to the action on ORL1 receptors invivo.

In conclusion, BUP and norBUP displayed distinct pharmacological properties at µ-, $delta$ -, and $kappa$ -opioid receptors and the ORL1receptor. Since norBUP is a major metabolite of BUP in vivo andits mean steady-state plasma concentration is comparable to oreven exceeds that of BUP following sublingual BUP (Kuhlman etal., 1998), it is likely to contribute to the overall pharmacologicaleffects of BUP invivo.

	Footnotes

Accepted for publication January 17, 2001.

Received for publication October 5, 2000.

This work was supported in part by grants from the National Institute on Drug Abuse (DA04745, DA11263, DA13429, and T32DA07237).

Send reprint requests to: Dr. Lee-Yuan Liu-Chen, Department of Pharmacology, Temple University School of Medicine, 3420 N. Broad St., Philadelphia, PA 19140. E-mail: lliuche{at}astro.temple.edu

	Abbreviations

BUP, buprenorphine; norBUP, norbuprenorphine; ORL1, nociceptin/orphanin FQ receptor; [³⁵S]GTP $gamma$ S, [³⁵S]guanosine-5'-O-(3-thio)triphosphate; DAMGO, Tyr-D-Ala-Gly-N-(Me)Phe-Gly-ol; DPDPE, Tyr-D-Pen-Gly-Phe-D-Pen-OH (disulfide bridge between D-Pen² and D-Pen⁵); CHO cell, Chinese hamster ovary cell; ( $-$ )-U50,488H, (trans)-3,4-dichloro-N-methyl-N-[2-(1-pyrrolidiny)-cyclohexyl]benzeneacetamide methanesulfonate; N/OFQ, nociceptin/orphanin FQ; BSA, bovine serum albumin.

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