Abstract
Salvinorin A [(2S,4aR,6aR,7R,9S,10aS,10bR)-9-(acetyloxy)-2-(3-furanyl)-dodecahydro-6a,10b-dimethyl-4,10-dioxo-2h-naphtho[2,1-c]pyran-7-carboxylic acid methyl ester] is a hallucinogenic κ-opioid receptor agonist that lacks the usual basic nitrogen atom present in other known opioid ligands. Our first published studies indicated that Salvinorin A weakly inhibited μ-receptor binding, and subsequent experiments revealed that Salvinorin A partially inhibited μ-receptor binding. Therefore, we hypothesized that Salvinorin A allosterically modulates μ-receptor binding. To test this hypothesis, we used Chinese hamster ovary cells expressing the cloned human opioid receptor. Salvinorin A partially inhibited [3H]Tyr-d-Ala-Gly-N-Me-Phe-Gly-ol (DAMGO) (0.5, 2.0, and 8.0 nM) binding with EMAX values of 78.6, 72.1, and 45.7%, respectively, and EC50 values of 955, 1124, and 4527 nM, respectively. Salvinorin A also partially inhibited [3H]diprenorphine (0.02, 0.1, and 0.5 nM) binding with EMAX values of 86.2, 64, and 33.6%, respectively, and EC50 values of 1231, 866, and 3078 nM, respectively. Saturation binding studies with [3H]DAMGO showed that Salvinorin A (10 and 30 μM) decreased the μ-receptor Bmax and increased the Kd in a dose-dependent nonlinear manner. Saturation binding studies with [3H]diprenorphine showed that Salvinorin A (10 and 40 μM) decreased the μ-receptor Bmax and increased the Kd in a dose-dependent nonlinear manner. Similar findings were observed in rat brain with [3H]DAMGO. Kinetic experiments demonstrated that Salvinorin A altered the dissociation kinetics of both [3H]DAMGO and [3H]diprenorphine binding to μ receptors. Furthermore, Salvinorin A acted as an uncompetitive inhibitor of DAMGO-stimulated guanosine 5′-O-(3-[35S]thio)-triphosphate binding. Viewed collectively, these data support the hypothesis that Salvinorin A allosterically modulates the μ-opioid receptor.
Salvia divinorum is a plant from the sage family that has been used in the traditional spiritual practices by the Mazatec Indians of Oaxaca, Mexico to produce “mystical” or hallucinogenic experiences. The active ingredient isolated from the leaves of S. divinorum is Salvinorin A, a neoclerodane diterpene. Current evidence suggests that Salvinorin A-induced hallucinogenic effects are mediated by activation of κ-opioid receptors (for review, see Sheffler and Roth, 2003).
Salvinorin A, a κ-opioid receptor agonist (Roth et al., 2002), is a unique opioid receptor ligand. It bears little structural similarity to other structural classes of nonpeptidic opioid receptor ligands, including κ agonists, such as U50,488H and U69,593 (Harding et al., 2005). The common structural motif among all of these compounds is the presence of a basic amino group. Until recently, it had been assumed that the presence of a positively charged nitrogen atom in opioid compounds represented an absolute requirement for their interaction with opioid receptors (Rees and Hunter, 1990). The general assumption was that this cationic amino charge on the opioid ligand would interact with the side chain carboxyl group of an aspartate residue located in transmembrane III of the opioid receptor (Surratt et al., 1994; Eguchi, 2004). Given the lack of a basic nitrogen in Salvinorin A, this interaction is not an absolute requirement.
The pharmacology of Salvinorin A differs from that of other κ agonists (Wang et al., 2005). Although Salvinorin A and U50,488H stimulated [35S]GTPγS binding with similar potency in Chinese Hamster ovary cells (CHO) expressing the cloned human κ receptor, salvinorin A was ∼40-fold less potent than U50,488H in promoting receptor internalization. As observed with other κ agonists (Devine et al., 1993), Salvinorin A produces decreases in extracellular dopamine in both mouse caudate (Zhang et al., 2005) and rat nucleus accumbens (Carlezon et al., 2006).
Our initial binding studies showed that Salvinorin A weakly inhibited μ- and δ-opioid receptor binding (Roth et al., 2002), a finding replicated by others (Wang et al., 2005). In a subsequent report (Harding et al., 2005), using the radioligand [125I]IOXY, we generated more detailed Salvinorin A inhibition curves and observed that Salvinorin A and certain other Salvinorin A analogs partially inhibited [125I]IOXY binding to the cloned human μ receptor expressed in CHO cells (hMOR-CHO cells). In the present study, we characterized the interaction of Salvinorin A with μ-opioid receptors. We report evidence that Salvinorin A allosterically modulates μ-receptor binding.
Materials and Methods
Cell Culture and Membrane Preparation. The recombinant CHO cells (hMOR-CHO) were produced by stable transfection with the human opioid receptor cDNA and provided by Dr. Larry Toll (SRI International, Menlo Park, CA). The cells were grown on plastic flasks in Dulbecco's modified Eagle's medium/F-12 (50%/50%) medium (hMOR-CHO) containing 10% fetal bovine serum, 100 U/ml penicillin, 100 μg/ml streptomycin, and 0.20–0.25 mg/ml G-418 under 95% air/5% CO2 at 37°C. Cell monolayers were harvested and homogenized using a Polytron grinding apparatus in 50 mM Tris-HCl, pH 7.4, containing 4 μg/ml leupeptin, 2 μg/ml chymostatin, 10 μg/ml bestatin, and 100 μg/ml bacitracin, The homogenate was centrifuged at 15,000 rpm for 10 min at 4°C, and the supernatant was discarded. The membrane pellets were resuspended in binding buffer and used for [35S]GTPγS binding assays. For drug pretreatment experiments, the medium was changed, and then cells were incubated with various test drugs for 20 h. Cells were washed three times with phosphate-buffered saline (pH 7.4), and cell membranes were prepared as described above. This treatment produces tolerance to opioid drugs (Xu et al., 2003).
[35S]GTPγS Binding Assays. [35S]GTPγS binding was determined as described previously (Xu et al., 2001). In brief, test tubes received the following additions: 50 μl of buffer A (50 mM Tris-HCl, pH 7.4, containing 100 mM NaCl, 10 mM MgCl2, and 1 mM EDTA), 50 μl of GDP in buffer A (final concentration = 50 μM), 50 μl of drug in buffer A/0.1% bovine serum albumin, 50 μl of [35S]GTPγS in buffer A (final concentration = 50 pM), and 300 μl of cell membranes (50 μg of protein) in buffer B. The final concentrations of reagents in the [35S]GTPγS binding assays were: 50 mM Tris-HCl, pH 7.4, containing 100 mM NaCl, 10 mM MgCl2, 1 mM EDTA, 1 mM dithiothreitol, and 0.1% bovine serum albumin. Incubations proceeded for 2 h at 25°C. Nonspecific binding was determined using GTPγS (40 μM). Bound and free [35S]GTPγS were separated by vacuum filtration through Whatman GF/B filters. The filters were punched into 24-well plates, to which 0.6 ml of liquid scintillation cocktail (Cytoscint; MP Biomedicals, Irvine, CA) was added. Samples were counted after an overnight extraction in a Trilux liquid scintillation counter at 60% efficiency.
Opioid Binding Assays. We used [3H][d-Ala2-MePhe4,Glyol5]enkephalin ([3H]DAMGO) (SA = 46 Ci/mmol), [3H]diprenorphine (SA = 54.9 Ci/mmol), and [125I]IOXY (SA = 2200 Ci/mmol) to label μ-binding sites. All assays took place in 50 mM Tris-HCl, pH 7.4, with a protease inhibitor cocktail [bacitracin (100 μg/ml), bestatin (10 μg/ml), leupeptin (4 μg/ml), and chymostatin (2 μg/ml)] in a final assay volume of 0.5 ml. Nonspecific binding was determined using 20 μM levallorphan. Triplicate samples were filtered with Brandel cell harvesters (Biomedical Research and Development Inc., Gaithersburg, MD) over Whatman GF/B filters after a 2- to 3-h incubation at 25°C. For the [125I]IOXY experiments, the filters were punched into 12 × 75-mm glass test tubes and counted in a Micromedic gamma counter at 80% efficiency. For the 3H-ligand binding assays, the filters were punched into 24-well plates, to which was added 0.6 ml liquid scintillation cocktail (Cytoscint). Samples were counted, after an overnight extraction, in a Trilux liquid scintillation counter at 44% efficiency. Opioid binding assays using membranes prepared from hMOR-CHO cells had ∼30-μg protein per assay tube.
Inhibition curves were generated by displacing a single concentration of radioligand by 10 concentrations of drug. For binding surface experiments (Rothman, 1986; Rothman et al., 1991), two different concentrations of radioligand were each displaced by ten concentrations of nonradioactive ligand agents in the absence or presence of various blockers.
Cyclic AMP Assays. Functional coupling of the cloned μ-opioid receptor to adenylate cyclase was determined by measuring changes in the levels of cellular cAMP. The assay procedures followed the protocol provided by CatchPoint cyclic-AMP fluorescent assay kit (a horseradish peroxidase-based competitive immunoassay kit). For acute studies, hMOR-CHO cells were grown to 80 to 90% confluence in 96-well black-walled, clear bottom plates that had been treated with poly-l-lysine. After aspirating the medium, cells were washed with 300-μl/well Krebs-Ringer bicarbonate buffer with glucose (KRBG, pH 7.4). KRBG containing 0.75 mM 3-isobutyl-1-methylxanthine and 1 mg/ml bovine serum albumin and appropriate agonists were added to each well (90 μl). After a 30-min incubation at 37°C, 100 μM forskolin in KRBG containing 0.75 mM 3-isobutyl-1-methylxanthine and 1 mg/ml bovine serum albumin was added to each well in a volume of 10 μl. Cyclic AMP production was terminated 40 min later by the addition of 50 μl of a cell-lysing solution (Molecular Devices, Sunnyvale, CA). For chronic studies, cells were grown to 80% confluence in 96-well black-walled, clear bottom plates (number 3603, Corning Inc., Corning, NY) that had been treated with poly-l-lysine. After treatment with medium or 10 μM drug for 20 h, cells were rinsed three times with 300-μl/well KRBG (pH 7.4) and assayed as described above. This assay was sensitive between 0.1 and 10 pmol of cAMP in a 40-μl sample volume. A FlexStation II (Molecular Devices) was used to read and quantitate fluorescence intensity of the plate. Data from three experiments were analyzed using the program Prism (version 3.0; GraphPad Software, Inc., San Diego, CA). Results are presented as the mean ± S.E.M.
Stimulation of p42/p44 MAPK Phosphorylation. The assay procedures followed the protocol provided by PhosphoPlus p44/42 MAPK (Thr202/Tyr204) antibody kit (Cell Signaling, Beverly, MA). In brief, cells were grown to 80 to 90% confluence in six-well plates. The assay started by the addition of any agonists and stopped after 5 min by rinsing the cells with ice-cold 1× phosphate-buffered saline. Cells were lysed by adding SDS sample buffer (100 μl) and immediately scraped to a microcentrifuge tube on ice, sonicated for 10 to 15 s, and boiled for 5 min. Samples (20 μl) were loaded onto SDS-polyacrylamide gel electrophoresis gel as described previously (Xu et al., 2005). Western blots were digitized and quantified using densitometric analysis (NIH Image software). Results from at least three experiments were analyzed using the program Prism.
Data Analysis and Statistics. For [35S]GTPγS binding experiments, the percentage stimulation of [35S]GTPγS binding was calculated according to the following formula: (S – B)/B × 100, where B is the basal level of [35S]GTPγS binding and S is the stimulated level of [35S]GTPγS binding (Xu et al., 2004). EC50 values (the concentration that produces 50% maximal stimulation of [35S]GTPγS binding) and EMAX (percentage of maximal stimulation in the [35S]GTPγS binding) were determined using the program MLAB-PC (Civilized Software, Bethesda, MD).
The amount of cAMP in the samples was measured using a cAMP standard curve. Forskolin (100 μM)-stimulated cAMP formation in the absence of agonist was defined as 100%. The EC50 (the concentration of agonist that produces 50% inhibition of forskolin-stimulated cAMP formation) and EMAX (percentage of maximal inhibition of forskolin-stimulated cAMP) were calculated using the program Prism.
In receptor binding experiments, for drugs that produced inhibition curves without apparent plateaus, the data were fit to the two-parameter logistic equation for the best-fit estimates of the IC50 and n values (Nightingale et al., 2005). For curves with apparent plateaus, the data were transformed to “percentage inhibition” and fit to a two-parameter dose-response curve model: Y = EMAX × ([D]/([D] + EC50), for the best fit estimates of the EMAX and EC50 using either KaleidaGraph version 3.6.4 or MLAB-PC (Nightingale et al., 2005). Radioligand binding surfaces generated with [3H]DAMGO or [3H]diprenorphine were fit to one-site binding models using MLAB-PC as described elsewhere (Rothman et al., 1991). Statistical significance among binding parameters was determined using the F-test (Rothman et al., 1991). Dissociation experiments were conducted with minor modification of published procedures, in which the data were fit to a two-component dissociation model (Rothman et al., 1991). Statistical significance among kinetic model parameters was determined using the Student's t test.
Sources. [35S]GTPγS (SA = 1250 Ci/mmol) was obtained from DuPont NEN (Boston, MA). Various opioid peptides were provided by Multiple Peptide System via the Research Technology Branch (National Institute on Drug Abuse, Baltimore, MD). [125I]IOXY was prepared as described previously (de Costa et al., 1992; Ni et al., 1993). The sources of other agents are published elsewhere (Xu et al., 2004). Salvinorin A and herkinorin were synthesized as described previously (Harding et al., 2005). For experiments using Salvinorin A or herkinorin, drug dilution curves were made up from freshly prepared 10 mM stock solutions in dimethyl sulfoxide. As is our standard operating procedure, all drug dilution curves used buffer with 1 mg/ml bovine serum albumin.
Results
Ligand Binding Experiments. Our initial experiments demonstrated that Salvinorin A, whose structure is shown in Fig. 1, partially inhibited [125I]IOXY (0.9 nM) binding to membranes prepared from hMOR-CHO cells (Fig. 1), with an EC50 value of 1728 nM and an EMAX value of 48%. Similar results were observed in rat brain membranes using [3H]DAMGO to label μ receptors (Fig. 2). In this case, Salvinorin A partially inhibited μ-receptor binding with an EC50 value of 2322 nM and an EMAX value of 60%.
To further characterize Salvinorin A-mediated partial inhibition of μ-receptor binding, we generated Salvinorin A inhibition curves using three concentrations of [3H]DAMGO (0.5, 2.0, and 8.0 nM) designed to produce varying levels of μ-receptor occupation (the Kd is ∼2 nM), using membranes prepared from hMOR-CHO cells. As reported in Fig. 3, Salvinorin A partially inhibited μ-receptor binding at all three [3H]DAMGO concentrations. The EC50 and EMAX values are reported in Table 1. These results show that the Salvinorin A inhibition curve observed with 8.0 nM [3H]DAMGO resulted in a significantly lower EMAX value and a higher EC50 value compared with the two lower [3H]DAMGO concentrations.
Likewise, we generated Salvinorin A inhibition curves using three concentrations of [3H]diprenorphine (0.02, 0.1, and 0.5 nM) designed to produce varying levels of μ-receptor occupation (the Kd is ∼0.7 nM), using membranes prepared from hMOR-CHO cells. As reported in Fig. 4A, Salvinorin A partially inhibited μ-receptor binding at all three [3H]diprenorphine concentrations. The EC50 and EMAX values are reported in Table 1. These results show that the Salvinorin A inhibition curve observed with 0.5 nM [3H]diprenorphine resulted in a significantly lower EMAX value and a higher EC50 value compared with the two lower [3H]diprenorphine concentrations. It is apparent from these inhibition curves that Salvinorin A is correctly identified as being “inactive” or having less than 50% inhibition of μ-receptor binding at a concentration of 10 μM when higher [3H]ligand concentrations are used (Roth et al., 2002). In contrast to the results observed for Salvinorin A, both (–)-U50,488, a κ agonist, and naloxone, a μ-receptor antagonist, fully inhibited [3H]diprenorphine binding, producing classic inhibition curves consistent with simple competitive inhibition (Fig. 4B; Table 1).
Using the method of binding surface analysis, we determined the effect of fixed concentrations of Salvinorin A on the Kd and Bmax of [3H]DAMGO binding to membranes prepared from both MOR-CHO cells and rat brain. As reported in Table 2, Salvinorin A had complex actions on the Kd and Bmax values in hMOR-CHO cells. Salvinorin A increased the Kd value in a dose-dependent manner, producing a maximal increase to ∼8.9 nM. After increasing the Bmax value at a concentration of 6400 nM, Salvinorin A proceeded to decrease the Bmax value at higher concentrations. These data, normalized as percentage changes, are reported in Fig. 5, A and B. The data clearly show that Salvinorin A increased the Kd in dose-dependent nonlinear manner with an EC50 value of 1730 nM and an EMAX value of 248%. In contrast, a competitive inhibitor increased the Kd in a strictly linear manner. In rat brain, 1000 nM Salvinorin A increased the Kd without changing the Bmax. A higher concentration of Salvinorin A (5000 nM) substantially reduced the Bmax by 48% while increasing the Kd to a smaller extent than 1000 nM Salvinorin A.
We also determined the effect of Salvinorin A on the Kd and Bmax of [3H]diprenorphine binding to hMOR-CHO cells. As reported in Table 3, both 10,000 and 40,000 nM Salvinorin A decreased the Bmax value by ∼34% and increased the Kd by ∼2-fold. Consistent with the plateau reported in Fig. 4, increasing the Salvinorin A concentration 4-fold from 10,000 to 40,000 nM had no additional effect on [3H]diprenorphine binding. On the other hand, naloxone (10 nM) acted as a competitive inhibitor of [3H]diprenorphine binding to hMOR-CHO cells (Table 3).
Kinetic Experiments. To determine whether Salvinorin A altered the rate of [3H]DAMGO dissociation from the μ-opioid receptor, membranes prepared from hMOR-CHO cells were incubated with 1 nM [3H]DAMGO for 120 min at 25°C. At this point, defined as time 0, baseline samples were filtered, and then drugs were added into paired samples to generate the following conditions: control (no addition), DAMGO (10 μM), Salvinorin A (30 μM), and DAMGO (10 μM) + SA (30 μM). Samples were then filtered at the indicated time points. As reported in Fig. 6, the addition of Salvinorin A to DAMGO seemed to slightly speed up the dissociation [3H]DAMGO binding, whereas the addition of Salvinorin A appeared to slow the dissociation [3H]DAMGO binding. Quantitative analysis of these data revealed that a two-component dissociation model fit the data much better than a one-component model (P < 1E-10) (Table 4) and that the addition of Salvinorin A to the DAMGO condition significantly increased the dissociation rate constant (K2) of the faster-dissociating component. Salvinorin A significantly decreased (1.5-fold) the dissociation rate constant (K1) of the slower-dissociating component, accounting for the apparent slower dissociation rate observed in this condition.
Hoping to conduct a dissociation experiment under conditions of a one-component dissociation model, we repeated this experiment using the antagonist [3H]diprenorphine. These experiments were conducted at 37°C, because [3H]diprenorphine dissociation was too slow at 25°C. As reported in Fig. 7 and Table 5, the addition of 10 μM diprenorphine resulted in a fairly rapid dissociation that was best described by a two-component dissociation model. Salvinorin A alone (30 μM) resulted in a much slower dissociation of [3H]diprenorphine, an observation mainly accounted for by a decreased value of K1 from 0.021 to 0.0025 min–1 (Table 5). Interestingly, the addition of an approximate IC50 concentration, (–)-U50,488 (1 μM), produced a dissociation curve not significantly different from Salvinorin A. It is noteworthy that the diprenorphine + Salvinorin A condition resulted in statistically significant changes in the kinetic parameters compared with the diprenorphine condition: decreased A1, decreased K1, and increased A2.
Functional Experiments. Using the [35S]GTPγS binding assay, we assessed the effect of Salvinorin A on measures of μ-receptor function. As reported in Fig. 8A and Table 6, Salvinorin A weakly stimulated [35S]GTPγS binding with an EC50 of approximately 65,000 nM and an extrapolated EMAX value (202%) approximately 40% lower than that of DAMGO. Interestingly, 10 nM naloxone reduced Salvinorin A-stimulated [35S]GTPγS binding in a noncompetitive manner, significantly reducing the EMAX value without changing the ED50 value.
Consistent with the partial agonist profile described above, Salvinorin A significantly reduced the EMAX value of DAMGO-stimulated [35S]GTPγS binding (Fig. 8B; Table 6) by 31 and 42% at 10 and 50 μM, respectively. Salvinorin A also increased the DAMGO ED50 values. At a concentration of 10 μM, Salvinorin A increased the ED50 for DAMGO from 39 to 192 nM, resulting in a calculated Ke (antagonist Ki value) of 2549 nM. If simple competitive antagonism of Salvinorin A at the μ receptor were responsible for this 4.9-fold increase in the DAMGO ED50, one would predict that a 5-fold increase in the Salvinorin A concentration to 50 μM should further increase the DAMGO ED50 to 804 nM, such that the same Ke value would result. However, 50 μM Salvinorin A increased the DAMGO ED50 only an additional 1.13-fold to 218 nM. In contrast, 10 nM naloxone, a competitive antagonist, increased the DAMGO ED50 more than predicted based on its Ke determined with a 2.5 nM dose.
We determined the effect of Salvinorin A (50 μM) and DAMGO (10 μM) on basal and forskolin-stimulated cAMP levels. As reported in Fig. 9A, DAMGO and Salvinorin A did not alter basal cAMP levels. As expected, DAMGO almost completely inhibited forskolin-stimulated cAMP accumulation. Salvinorin A inhibited forskolin-stimulated cAMP accumulation by 44%. We compared the effect of naloxone (a competitive inhibitor) and Salvinorin A on DAMGO-mediated inhibition of forskolin-stimulated cAMP accumulation in the hMOR-CHO cells. As reported in Table 7, 50 μM Salvinorin A significantly increased the ED50 value. The calculated apparent Ke was 27 μM. Salvinorin A also decreased the EMAX value by ∼9%. In contrast, naloxone increased the ED50 without decreasing the EMAX. Thus, in the cAMP assay, Salvinorin A demonstrated partial agonist activity.
The cellular adaptations produced by chronic opioids are generally accepted as signs of opioid dependence. We next determined the effect of Salvinorin A (50 μM) on the cellular adaptations produced by chronic treatment of cells with DAMGO (10 μM) and the novel μ-opioid agonist herkinorin (10 μM) (Harding et al., 2005). Cells were treated for 20 h with DAMGO or herkinorin in the absence and presence of Salvinorin A. We measured two endpoints: forskolin-stimulated cAMP, which detects cAMP superactivation, and naloxone-stimulated cAMP in the presence of forskolin, which detects the presence of constitutively active receptors. As reported in Fig. 9B, chronic DAMGO treatment produced cAMP superactivation without a naloxone overshoot. Chronic herkinorin treatment reduced forskolin-stimulated cAMP, but the addition of naloxone revealed the occurrence of cAMP superactivation and the presence of constitutively active receptors. Salvinorin A did not change the cellular response to either treatment. However, chronic Salvinorin A treatment produced signs of cAMP superactivation.
In contrast to the activity of Salvinorin A in functional assays that measured changes in the level of cellular cAMP, Salvinorin A was inactive in the MAPK assay, which is activated by the Gβγ subunit. As reported in Fig. 10, DAMGO stimulated the phosphorylation of MAPK. Salvinorin A alone had no effect and did not alter the effect of DAMGO in this assay.
Discussion
As described in a recent review (Christopoulos and Kenakin, 2002), allosteric modulators of G protein-coupled receptors may be of interest as potential targets for medication development. There are few reports of allosteric modulators of opioid receptors that we are aware of. In 1987, Vaysse et al. (1987) reported that cannabidiol noncompetitively inhibited radioligand binding to μ- and δ-opioid receptors, a finding consistent with allosteric modulation. Subsequent work by another laboratory provided additional evidence for this hypothesis by showing that cannabidiol accelerated the dissociation of [3H]DAMGO and [3H]naltrindole from rat brain μ and δ receptors, respectively (Kathmann et al., 2006). We reported in 1991 that pretreating rat brain membranes with (+)-cis-methylfentanyl increased the dissociation rate of μ receptors labeled with [3H]ohmfentanyl (Xu et al., 1991).
In our recent article (Roth et al., 2002), we briefly noted that Salvinorin A, a potent κ-opioid receptor agonist, partially inhibited [125I]IOXY binding to μ-opioid receptors (see Table 1 in Harding et al., 2005). In the present study, we tested the hypothesis that Salvinorin A allosterically modulates μ-opioid receptors. Several lines of evidence support this hypothesis.
1) Salvinorin A partially inhibits μ-receptor binding using both the cloned human μ receptor expressed in CHO cells, as well as the native μ receptor present in rat brain membranes. We observed a partial inhibition pattern with three radioligands: [3H]DAMGO, [3H]diprenorphine, and [125I]IOXY. As reported in Figs. 3 and 4, the presence of a plateau is most readily observed using radioligand concentrations sufficient to occupy a substantial fraction of μ receptors, such as 0.9 nM [125I]IOXY (Fig. 1), 8 nM [3H]DAMGO (Fig. 3), or 0.5 nM [3H]diprenorphine (Fig. 4). The partial inhibition pattern we observed, where the inhibition curve shifts to the right with a lower EMAX value as the radioligand concentration is increased, is consistent with the theoretical predictions made by Ehlert (1988) for negative allosteric modulators. This partial inhibition pattern is unique to Salvinorin A, because (–)-U50,488, a potent κ agonist, and naloxone, a competitive μ antagonist, produce “normal” inhibition curves without any evidence of a plateau.
2) Salvinorin A affects the Kd and Bmax of the μ receptor in a manner inconsistent with competitive binding. Using [3H]DAMGO and hMOR-CHO cells, Salvinorin A first increased the μ-receptor Bmax followed by highly significant decreases in the Bmax at higher concentrations. It is noteworthy that Salvinorin A increased the Kd of the μ receptor in a dose-dependent manner (Fig. 5A), rather than a linear manner, as would observed with a competitive inhibitor (Ehlert, 1988). Thus, the ability of Salvinorin A to increase the Kd reaches a ceiling at approximately 200% of control. Salvinorin A-mediated uncompetitive inhibition of μ-receptor binding was also observed in rat brain (Table 2) and in hMOR-CHO cells using [3H]diprenorphine (Table 3).
3) Salvinorin A alters the kinetics of radioligand dissociation. It is well known that allosteric modulators can alter the rate of radioligand dissociation (Kostenis and Mohr, 1996). As reported in Table 4, [3H]DAMGO dissociation from μ receptors expressed in hMOR-CHO cells was biexponential, with readily measurable slower (K1 = 0.006 min–1) and faster (K2 = 0.10 min–1) components. The addition of Salvinorin A to DAMGO increased the faster dissociation rate by 160% to 0.16 min–1 and decreased the A2 value by 24 to 26%. Interestingly, the addition of Salvinorin A alone decreased K1 by 33% to 0.004 min–1. When the μ receptors were labeled with an antagonist ([3H]diprenorphine), the addition of Salvinorin A alone substantially slowed [3H]diprenorphine dissociation (Fig. 7), mainly by decreasing K1 by more than 10-fold. Viewed in context with the other findings, such as the partial inhibition pattern, these data are consistent with an allosteric effect. However, the addition of a nonallosteric compound, (–)-U50,488, at an approximate IC50 concentration resulted in a similarly slowed dissociation of [3H]diprenorphine, making it more difficult to interpret the slowed [3H]diprenorphine dissociation produced by Salvinorin A. However, the concurrent addition of Salvinorin A and diprenorphine decreased the A1 value by 31%, decreased the K1 value by 43%, and increased the K2 value by 162%, providing direct evidence for an allosteric effect of Salvinorin A.
4) Salvinorin A acts as an uncompetitive inhibitor of DAMGO-stimulated [35S]GTPγS binding (Fig. 8B). As reported in Table 6, Salvinorin A produced a dose-dependent decrease in the EMAX and failed to increase the ED50 value significantly when the Salvinorin A concentration was increased from 10 to 50 μM, as was observed for a competitive inhibitor, naloxone. We believe that these four lines of data support the hypothesis that Salvinorin A allosterically modulates μ-receptor binding and function.
The effects of Salvinorin A in the functional assays deserve additional study. For example, Salvinorin A stimulates [35S]GTPγS binding with low potency and an extrapolated EMAX value of approximately 42% that of DAMGO. The simplest explanation of these data is that Salvinorin A is a weak partial μ agonist. This finding is supported by the ability of Salvinorin A to decrease forskolin-stimulated cAMP accumulation and to induce cAMP superactivation (Fig. 9). However, naloxone noncompetitively inhibits Salvinorin A-stimulated [35S]GTPγS binding, suggesting that Salvinorin A acts at a site on the μ receptor distinct from that of typical μ ligands. This viewpoint is supported by point four in the previous paragraph and the fact that Salvinorin A, unlike DAMGO, had no activity in the MAPK assay (Fig. 10). Viewed collectively, the functional data indicate that Salvinorin A may have some partial agonist activity at μ receptors in addition to the allosteric effects described above. Assuming that Salvinorin A has partial agonist activity at μ receptors, it might be possible to detect μ-mediated antinociception following administration of Salvinorin A. However, Salvinorin A-induced antinociception was not observed in κ receptor knockout mice (Ansonoff et al., 2006), suggesting that the potency of Salvinorin A as a partial μ agonist is probably too low to produce detectable antinociception.
The ultimate significance of this work remains to be seen. However, the immediate significance of our findings is the clear demonstration that the μ-opioid receptor possesses an allosteric modulator site. A major challenge of subsequent work will be to identify more potent ligands for the allosteric site. Toward this end, we note that certain analogs of Salvinorin A also partially inhibit μ-opioid receptors (Tidgewell et al., 2006) as well as δ-opioid receptors (R. B. Rothman and T. E. Prisinzano, unpublished data). Thus, we anticipate that the Salvinorin A structural template will yield a number of allosteric modulators of opioid receptors. A more complete structure-activity profile of the allosteric site will be used to design more potent allosteric ligands. Once these are available, it will be possible to determine the in vivo effects and potential therapeutic application of allosteric modulators of μ-opioid receptors. It is possible, as observed with other classes of medications that work via allosteric mechanisms (benzodiazepines), that allosteric modulators of opioid receptors will have therapeutic value. Because a positive allosteric modulator will enhance the action of endogenous ligands acting via μ receptors, such a drug could produce analgesia with fewer adverse effects than that produced by direct μ-receptor agonists. Furthermore, it is unfortunate that we do not yet know the molecular basis of the allosteric actions of Salvinorin A at the μ-opioid receptor. Site-directed mutagenesis studies, such as those that delineated the interaction of Salvinorin A at the κ-opioid receptor (Yan et al., 2005), will be necessary to definitively prove that the Salvinorin A-induced allosteric effects reported here are mediated via a binding site on the μ receptor distinct from the binding site of other μ ligands.
Footnotes
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This work was supported by the Intramural Research Program of the National Institutes of Health and National Institute on Drug Abuse Grant R01 DA018151-01A2 (to T.E.P.).
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Article, publication date, and citation information can be found at http://jpet.aspetjournals.org.
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doi:10.1124/jpet.106.113167.
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ABBREVIATIONS: CHO, Chinese hamster ovary cells; hMOR-CHO, CHO cells expressing the cloned human μ-opioid receptor; DAMGO, Tyr-d-Ala-Gly-N-Me-Phe-Gly-ol; herkinorin, (2S,4aR,6aR,7R,9S,10aS,10bR)-9-(benzoyloxy)-2-(3-furanyl)dodecahydro-6a,10b-dimethyl-4, 10-dioxo-2H-naphtho-[2,1-c]pyran-7-carboxylic acid methyl ester; [35S]GTPγS, guanosine 5′-O-(3-[35S]thio)triphosphate; U50,488H, (±)-trans-3,4-dichloro-N-methyl-N-[2-(1-pyrrolidinyl)-cyclohexyl]-benzeneacetamide; U69,593, 5α,7α,8β-(–)-N-methyl-N-[7-(1-pyrrolidinyl)-1-oxaspiro(4,5)dec-8-yl]-phenyl-benzeneacetamide; Salvinorin A, (2S,4aR,6aR,7R,9S,10aS,10bR)-9-(acetyloxy)-2-(3-furanyl)-dodecahydro-6a,10b-dimethyl-4,10-dioxo-2H-naphtho[2,1-c]pyran-7-carboxylic acid methyl ester; SA, specific activity; MAPK, mitogen-activated kinase protein; KRBG, Krebs-Ringer bicarbonate buffer with glucose; [125I]IOXY, 6β-iodo-3,14-dihydroxy-17-cyclopropylmethyl-4,5α-epoxymorphinon.
- Received August 29, 2006.
- Accepted October 20, 2006.
- The American Society for Pharmacology and Experimental Therapeutics