Cannabinoid Agonist Signal Transduction in Rat Brain: Comparison of Cannabinoid Agonists in Receptor Binding, G-Protein Activation, and Adenylyl Cyclase Inhibition

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Vol. 295, Issue 1, 328-336, October 2000

Cannabinoid Agonist Signal Transduction in Rat Brain: Comparison of Cannabinoid Agonists in Receptor Binding, G-Protein Activation, and Adenylyl Cyclase Inhibition¹

Christopher S. Breivogel and Steven R. Childers

Department of Physiology and Pharmacology, Center for the Neurobiological Investigation of Drug Abuse, and Center for Investigative Neuroscience, Wake Forest University School of Medicine, Winston-Salem, North Carolina

	Abstract

Top Abstract Introduction Experimental Procedures Results Discussion References

To investigate differences in agonist affinity, potency, and efficacy across rat brain regions, five representative cannabinoidcompounds were investigated in membranes from three differentrat brain regions for their ability to maximally stimulate [³⁵S]guanosine-5'-O-(3-thio)triphosphate (GTP $gamma$ S) binding and bindto cannabinoid receptors (measured by inhibition of [³H]antagonist binding) under identical assay conditions. In allthree brain regions, the rank order of potency for the stimulationof [³⁵S]GTP $gamma$ S binding and the inhibition of [³H]SR141716A binding for these compounds were identical, with CP55940 $approx$ levonantradol > WIN55212-2 $>=$ $Delta$ ⁹-tetrahydrocannabinol ( $Delta$ ⁹-THC) > methanandamide. The rank order of efficacy was not relatedto potency, and relative maximal agonist effects varied acrossregions. Receptor binding fit to a three-site model for most agonists,stimulation of [³⁵S]GTP $gamma$ S binding fit to a two-site model for all agonists, andhigh-affinity receptor binding did not appear to produce any stimulationof [³⁵S]GTP $gamma$ S binding. WIN55212-2, methanandamide, and $Delta$ ⁹-THC also were assayed for the inhibition of adenylyl cyclasein cerebellar membranes. The rank orders of potency and efficacywere similar to those for [³⁵S]GTP $gamma$ S binding, but the efficacies and potencies of methanandamideand $Delta$ ⁹-THC compared with WIN55212-2 were higher for adenylyl cyclaseinhibition, implying receptor/G-proteinreserve.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

Cannabinoids include a family of compounds derived from Cannabis sativa, the most biologically active of which is $Delta$ ⁹-tetrahydrocannabinol ( $Delta$ ⁹-THC) (Gaoni and Mechoulam, 1964). In addition, a number of compoundshave been developed as specific receptor ligands, including agonistsand antagonists (Compton et al., 1993; Rinaldi-Carmona et al.,1994). CB₁ receptors, and splice variant CB_1A (Shire et al., 1995),represent the principle cannabinoid receptor type so far foundin rat brain (Matsuda et al., 1990), and mediate the central nervoussystem actions of cannabinoid compounds (Compton et al., 1993).Their actions are transduced via the activation of G-proteins(Howlett et al., 1986) that results in the inhibition (Howlett,1984) or stimulation of adenylyl cyclase (Glass and Felder, 1997;Maneuf and Brotchie, 1997), inhibition of Ca²⁺ conductance (Mackie and Hille, 1992; Mackie et al., 1995), stimulationof K⁺ conductance (Mackie et al., 1995), and stimulation of the mitogen-activatedprotein kinase pathway (Bouaboula et al., 1995). Cannabinoid receptorscouple to at least six different G-subunits in brain membranes(Prather et al., 2000).

Receptor activation of G-proteins can be measured by agonist-stimulated binding of the hydrolysis-resistant GTP analog [³⁵S]guanosine-5'-O-(3-thio)triphosphate (GTP $gamma$ S) to G-protein $alpha$ -subunitsin membranes (Hilf et al., 1989; Selley et al., 1996) or brainsections (Sim et al., 1995). This technique is sensitive to differencesin agonist efficacy and potency for G-protein activation (Lorenzenet al., 1996; Selley et al., 1997, 1998). Previous results withagonist-stimulated [³⁵S]GTP $gamma$ S binding have demonstrated that $Delta$ ⁹-THC is a weak partial agonist (Sim et al., 1996), and anandamideis an intermediate efficacy partial agonist (Burkey et al., 1997)compared with WIN55212-2 or CP55940 in rodent brain membranes.Other studies have reported partial agonist activity of $Delta$ ⁹-THC and anandamide for inhibition of adenylyl cyclase (Howlettet al., 1986; Childers et al., 1994) and CP55940 for inhibitionof Ca²⁺ currents (Shen et al., 1996). Previous work from our laboratorynot only confirmed these differences in agonist efficacy (Breivogelet al., 1998) but also demonstrated that cannabinoid receptoractivity varies across different regions of rat brain becausereceptors in each region exhibit different catalytic amplificationfactors, defined as the number G-proteins activated per agonist-occupiedreceptor (Breivogel et al., 1997).

Cannabinoid compounds inhibit adenylyl cyclase activity in cell lines (Howlett, 1984; Slipetz et al., 1995) and in brain membranes(Bidaut-Russell et al., 1990; Pacheco et al., 1991; Childers etal., 1994). In general terms, the pharmacology of cannabinoid-inhibitedadenylyl cyclase matches that of cannabinoid receptor binding(Pacheco et al., 1991)_, including competitive antagonism by SR141716A(Rinaldi-Carmona et al., 1994). However, inhibition of adenylylcyclase in membranes from different regions of rat brain was onlydetectable in cerebellum and striatum (Pacheco et al., 1991; Childerset al., 1994).

The present study compares the efficacies and potencies of several commonly used cannabinoid compounds for the stimulationof [³⁵S]GTP $gamma$ S binding and displacement of [³H]SR141716A binding in rat brain membranes from three brain regionsunder identical assay conditions. Inhibition of adenylyl cyclaseby several of these agonists also is determined in rat cerebellarmembranes to compare the efficacies and potencies of agonistsfor G-protein activation with those for a downstream effectorsystem. Although the efficacies of these compounds have previouslybeen determined in rat cerebellar membranes, the relationshipof agonist receptor occupancy to G-protein activation was notdetermined, and it is not known whether these efficacy differencesare maintained in membranes from different regions of rat brain.To test the hypothesis that efficacy is related to receptor density,two regions were chosen that contain either similar (hippocampus)or different (hypothalamus) levels of cannabinoid receptors andcannabinoid-activated G-proteins compared with cerebellum. Furthermore,direct comparison of receptor binding and G-protein activationunder identical conditions allows determination of the receptorstates that are involved in agonist activity. Finally, determinationof efficacy for adenylyl cyclase inhibition by these agonistswill test the hypothesis that cannabinoid receptors in cerebellumexhibit greater receptor reserve at this effector than at G-proteins.

	Experimental Procedures

Top Abstract Introduction Experimental Procedures Results Discussion References

Materials. Male Sprague-Dawley rats were purchased from Zivic Miller Laboratories, Inc. (Zelienople, PA). [³⁵S]GTP $gamma$ S (1250 Ci/mmol), [ $alpha$ -³²P]ATP (800 Ci/mmol), and [³H]cAMP (25 Ci/mmol) were purchased from New England Nuclear Corp.(Boston, MA). [³H]SR141716A (53-55 Ci/mmol) was obtained from Amersham Life Sciences(Arlington Heights, IL). CP55940 and levonantradol were obtainedfrom Pfizer, Inc. (Groton, CT). $Delta$ ⁹-THC was provided by National Institute on Drug Abuse/ResearchTriangle Institute (Research Triangle Park, NC). WIN55212-2, anandamide,and R-(+)-methanandamide were purchased from Research BiochemicalsInternational (Natick, MA). SR141716A was a generous gift fromDr. Francis Barth at Sanofi Recherché (Montpellier, France).GDP and GTP $gamma$ S were purchased from Boehringer Mannheim (New York,NY). All other reagent grade chemicals and enzymes were obtainedfrom Sigma Chemical Co. (St. Louis, MO) or Fisher Scientific (Pittsburgh,PA).

Agonist-Stimulated [³⁵S]GTP $gamma$ S Binding and [³H]SR141716A Competition Assays. Cerebellum, hippocampus, and hypothalamus were dissected from fresh rat brains on ice and pooled. Each region was homogenizedwith a Tissumizer (Tekmar, Cincinnati, OH) in cold membrane buffer(50 mM Tris-HCl, pH 7.4, 3 mM MgCl₂, 0.2 mM EGTA, 100 mM NaCl,pH 7.7) and centrifuged at 48,000g for 10 min at 4°C. Pelletswere resuspended in membrane buffer, and then centrifuged againat 48,000g for 10 min at 4°C. Pellets from the second centrifugationwere homogenized in membrane buffer and stored at $-$ 80°C untiluse. Frozen membranes were thawed and diluted in membrane buffer,homogenized, and preincubated for 10 min at 30°C in 0.004 U/mladenosine deaminase (240 U/mg of protein; Sigma Chemical Co.)to remove endogenous adenosine, and then assayed for protein contentbefore addition to assay tubes. Assays were conducted at 30°Cfor 2 h in membrane buffer, including 8 to 10 µg (cerebellum andhippocampus) or 10 to 20 µg (hypothalamus) of membrane proteinwith 0.1% (w/v) BSA, 50 µM GDP, 0.5 nM SR141716A (³H-labeled for competition assays), and 0.05 nM GTP $gamma$ S (³⁵S-labeled in stimulation assays) in a final volume of 1 ml. Bothassays were performed simultaneously by incubating membranes withvarious concentrations of each ligand. Each rack also includeddetermination of [³⁵S]GTP $gamma$ S binding with 3 µM levonantradol to be able to normalizethe amount of stimulation by each agonist to that obtained witha maximally effective concentration of levonantradol. Nonspecificbinding was determined in the absence of agonists and the presenceof 30 µM unlabeled GTP $gamma$ S ([³⁵S]GTP $gamma$ S assays) or 10 µM unlabeled SR141716A ([³H]SR141716A assays). Reactions were terminated by rapid filtrationunder vacuum through Whatman GF/B glass fiber filters, followedby three washes with cold Tris buffer, pH 7.4. For [³H]SR141716A binding, filters were presoaked for approximately2 h in Tris buffer containing 0.5% (w/v) BSA, and cold Tris rinsebuffer contained 0.05% (w/v) BSA. Bound radioactivity was determinedby liquid scintillation spectrophotometry at 95% efficiency for³⁵S or 45% efficiency for ³H after overnight extraction of the filters in 4 ml of ScintiSafeEcono 1 scintillation fluid (Fisher Scientific). Typical [³⁵S]GTP $gamma$ S binding results included 500 to 700 dpm for nonspecificbinding, 200 to 450 dpm [³⁵S]GTP $gamma$ S bound/mg of protein basal binding (depending on the region),and 850 to 1100 dpm/mg bound in the presence of maximally effectiveconcentrations oflevonantradol.

Agonist Inhibition of Adenylyl Cyclase. Assays were performed according to the method of Salomon (1979) with some modifications. Fresh cerebella were dissected onice and homogenized in membrane buffer with a ground glass homogenizer.Membrane suspensions were centrifuged at 48,000g for 10 min at4°C, and then pellets were resuspended and homogenized in membranebuffer. Membranes were assayed for protein content before additionto assay tubes. Membranes (~15 µg) were incubated for 10 min at30°C in membrane buffer in the presence of various concentrationsof each agonist with 50 µM cAMP, 50 µM GTP, and 50 µM ATP plus1.5 µCi [ $alpha$ -³²P]ATP with 10 mM theophylline, 5 mM phosphocreatine, 20 U/ml creatinephosphokinase (250 U/mg of protein; Sigma Chemical Co.), and 0.1%(w/v) BSA in a final volume of 0.1 ml. Reactions were terminatedby boiling for 3 min and addition of stopping solution (2% sodiumlauryl sulfate, 45 mM ATP, and 1.3 mM cAMP in Tris buffer, pH7.5). [³H]cAMP standard (50 µl; ~15,000 cpm) and 1 ml of deionized waterwere added to each tube before addition of samples to Dowex columnsand processing according to a previously published method (Salomon,1979). Recovery of ³²P and ³H were determined by liquid scintillation spectrophotometry at99% efficiency for ³²P and 45% efficiency for ³H in 3.5 ml of 0.1 M imidazole buffer, pH 7.3, and 18 ml of scintillationfluid. The solvents used to dissolve the cannabinoid compounds(dimethyl sulfoxide for WIN55212-2 and 95% ethanol for all others)had no effect on cAMP formation at the highest concentration ofeach vehicle present in the assay (0.1%).

Data Analysis. Net agonist-stimulated [³⁵S]GTP $gamma$ S binding values were calculated by subtracting basal binding values (obtained in the absenceof agonist) from agonist-stimulated values (obtained in the presenceof agonist) and were normalized to the values obtained for a maximallyeffective concentration of levonantradol (3 µM) measured in thesame assay rack. The amount of [³²P]cAMP formed was determined by normalizing ³²P cpm to the fraction of total ³H cpm recovered from the columns. Data analyses, including agonistconcentration-effect curves and displacement curves, were conductedby iterative nonlinear regression by using JMP for Macintosh (SAS,Cary, NC) or Prism for Windows (GraphPad Software, San Diego,CA) to obtain EC₅₀, E_max, IC₅₀, I_max, and n_H (Hill slope) values.Determination of which model best fit the data was made by anF test with Prism to compare two models simultaneously. [³⁵S]GTP $gamma$ S binding and [³H]SR141716A displacement data were found to fit better to two-or three-component models than to a one-component model with variableHill slope. Percentage of total [³H]SR141716A binding data was fit to two- or three-component modelswith specific binding constrained to between 0 and 100%. K_i, andK_s values were estimated from IC₅₀ and EC₅₀ values, respectively,by the Cheng-Prusoff equation and antagonist K_B values were determinedby the equation K_B = [Ant]/(CR $-$ 1), where [Ant] is the concentrationof antagonist and CR is the ratio of the agonist EC₅₀ values inthe presence and absence of antagonist (Pratt and Taylor, 1990).Differences among agonists and regions were determined by ANOVAfollowed by the Tukey-Kramer test for multiple comparisons atP < .05. Unless otherwise indicated, all data presented are mean± S.E. of at least three experiments performed induplicate.

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

Stimulation of [³⁵S]GTP $gamma$ S Binding and Inhibition of [³H]SR141716A Binding by Cannabinoid Agonists. Concentration-effect curves were generated for both the stimulation of [³⁵S]GTP $gamma$ S binding and competition for [³H]SR141716A binding by the cannabinoid agonists WIN55212-2, levonantradol,CP55940, $Delta$ ⁹-THC, and methanandamide in rat cerebellar (Fig. 1), hippocampal,and hypothalamic membranes. Both assays were performed under thesame conditions, with 0.5 nM SR141716A in [³⁵S]GTP $gamma$ S binding assays and 0.05 nM GTP $gamma$ S in [³H]SR141716A binding assays. Both assays included 50 µM GDP and100 mM NaCl, both of which favor agonist stimulation of [³⁵S]GTP $gamma$ S binding and promote the low-affinity state of cannabinoidreceptors for agonist binding. Agonist-stimulated [³⁵S]GTP $gamma$ S binding in cerebellar membranes was blocked by the CB₁-selectiveantagonist SR141716A (data not shown), and the K_B value of SR141716Ain shifting WIN55212-2 concentration-effect curves to the rightwas 0.24 ± 0.08 nM, similar to the previously reported K_D valuefor [³H]SR141716A obtained by Scatchard analysis in cerebellar membranes(0.19 ± 0.01 nM; Breivogel et al., 1997), and consistent withcompetitive antagonism of CB₁ receptors.

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Fig. 1. Concentration-effect curves for cannabinoid stimulation of [³⁵S]GTP $gamma$ S binding (A) and displacement of [³H]SR141716A binding (B) in rat cerebellar membranes. Assays were performed under identical conditions as described under Experimental Procedures. Net agonist-stimulated [³⁵S]GTP $gamma$ S binding is shown as percentage of that obtained with 3 µM levonantradol. Curve fits are to a one-site model with variable Hill slope. Data are mean ± S.E. from four assays performed in duplicate.

Levonantradol significantly increased [³⁵S]GTP $gamma$ S binding in all three brain regions; net agonist-stimulated binding (pmol/mg)was approximately the same in the three regions, but percentageof stimulation by levonantradol over basal ranged from 140 to620% (Table 1). These differences in percentage of stimulationby agonist were due to differences in basal [³⁵S]GTP $gamma$ S binding levels across regions. CB₁ receptor binding, measuredwith 0.5 nM [³H]SR141716A, ranged from 1.5 to 3.9 pmol/mg (Table 1). Becausethe K_D of SR141716A in brain membranes is 0.24 nM and does notvary between regions (Breivogel et al., 1997

), B_max values of[³H]SR141716A binding can be estimated (Table 1) between 2.3 and5.9 pmol/mg. These values are similar to those previously reportedin these tissues (Breivogel et al., 1997

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TABLE 1
Binding parameters for cannabinoid-stimulated [³⁵S]GTP $gamma$ S binding and [³H]SR141716A binding in brain membranes
Membranes from the indicated regions were analyzed for maximal stimulation of [³⁵S]GTP $gamma$ S binding by 3 µM levonantradol and for [³H]SR141716A binding. Data for [³⁵S]GTP $gamma$ S binding are presented as net levonantradol-stimulated binding (pmol/mg), and percentage of stimulation of [³⁵S]GTP $gamma$ S binding over basal by levonantradol. Data for [³H]SR141716A binding are presented as specific binding determined with 0.5 nM [³H]SR141716A, and the estimated B_max of [³H]SR141716A binding assuming a K_D of 0.24 nM for SR141716A. Data are mean values ± S.E. from four separate experiments.

Concentration-effect curves of all five agonists in stimulating [³⁵S]GTP $gamma$ S binding (A) and displacing [³H]SR141716A binding (B) in cerebellar membranes are shown in Fig.1. The efficacies (E_max) of the agonists for stimulating [³⁵S]GTP $gamma$ S binding to cerebellar membranes were similar to thosepreviously determined (Breivogel et al., 1998

). E_max values normalizedto maximal stimulation produced by levonantradol are presentedin the text and Table 2. In cerebellar membranes, WIN55212-2(106%) was only slightly more efficacious than levonantradol,but this difference was not significant. However, levonantradoland WIN55212-2 were both more efficacious than the other agonists(P < .05), and CP55940 (74%) was more efficacious than methanandamide(65%), which was more efficacious than $Delta$ ⁹-THC (20%) (Fig. 1). In hippocampal and hypothalamic membranes(Table 2), WIN55212-2 was significantly the most efficaciousagonist, stimulating 128 and 130% of the [³⁵S]GTP $gamma$ S binding stimulated by levonantradol, respectively. CP55940was significantly less efficacious than levonantradol in hippocampus(87 ± 3%), but not in hypothalamus (82 ± 5%). Methanandamide wassignificantly different from levonantradol in hippocampus (86%),but not in hypothalamus (104%). In each region, $Delta$ ⁹-THC was the least efficacious agonist and was different fromthe other agonists, yielding 27 and 12% of the stimulation bylevonantradol in hippocampus and hypothalamus, respectively. Thus,although normalized E_max values of each cannabinoid agonist acrossregions were similar, there were some significant differences.Agonist K_s values in stimulating [³⁵S]GTP $gamma$ S binding also were determined, and compared with K_i valuesfor cannabinoid receptor binding determined under the same assayconditions. Agonist potencies for both assays followed the orderCP55940 $approx$ levonantradol > WIN55212-2 > $Delta$ ⁹-THC $>=$ methanandamide. Figure 2 shows a comparison of the bindingcurves for one representative agonist, levonantradol, in all threebrain regions. These curves show that although the potency oflevonantradol for stimulating [³⁵S]GTP $gamma$ S binding appeared to vary across regions (most potent inhippocampus and least potent in cerebellum), the potency of levonantradolfor displacing [³H]SR141716A binding did not vary significantly across regions.This trend appeared for all agonists except $Delta$ ⁹-THC. The results of curve fitting parameters for fits to one-sitemodels are shown in Table 3, and confirm this trend.

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TABLE 2
Relative agonist efficacies for the stimulation of [³⁵S]GTP $gamma$ S binding and inhibition of adenylyl cyclase ([³²P]cAMP) determined using a one-site model
Agonist concentration-effect curves were generated for stimulation of [³⁵S]GTP $gamma$ S binding and inhibition of adenylyl cyclase ([³²P]cAMP) in brain membranes. E_max values for [³⁵S]GTP $gamma$ S binding and I_max values for adenylyl cyclase inhibition were normalized to the values obtained by maximally effective concentrations of levonantradol (3 µM) or WIN55212-2 (1 µM), respectively, before curve fitting. Normalized values for adenylyl cyclase inhibition are shown in parentheses. Data are mean values ± S.E. from four separate experiments.

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Fig. 2. Comparison of levonantradol-stimulated [³⁵S]GTP $gamma$ S binding (A) and inhibition of [³H]SR141716A binding (B) in rat cerebellar, hippocampal, and hypothalamic membranes. Net agonist-stimulated [³⁵S]GTP $gamma$ S binding is shown as percentage of maximum stimulation obtained in each region. Curve fits are to a one-site model with variable Hill slope. Data are mean ± S.E. from four assays performed in duplicate.

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TABLE 3
Agonist potencies for inhibition of [³H]SR141716A binding, stimulation of [³⁵S]GTP $gamma$ S binding, and inhibition of adenylyl cyclase ([³²P]cAMP) determined using a one-site model
Agonist concentration-effect curves were generated under identical assay conditions for competition for [³H]SR141716A binding and stimulation of [³⁵S]GTP $gamma$ S binding. Three representative compounds also were assayed in cerebellar membranes for inhibition of adenylyl cyclase ([³²P]cAMP). Curves were fit by iterative nonlinear regression to one-site models with variable Hill slopes to obtain IC₅₀ and EC₅₀ values. K_i and K_s values for binding were calculated as described under Experimental Procedures. Data shown are mean ± S.E. from four assays performed in duplicate.

Comparison of the potencies of these agonists for displacing [³H]SR147161A binding and stimulating [³⁵S]GTP $gamma$ S binding for each region also can be seen in Table 3.The rank order of potency of these agonists for receptor binding(CP55940 = levonantradol > WIN55212-2 > $Delta$ ⁹-THC > methanandamide) was approximately the same as for stimulationof [³⁵S]GTP $gamma$ S binding. However, EC₅₀ values for $Delta$ ⁹-THC did not follow this order for [³⁵S]GTP $gamma$ S binding, possibly due to error resulting from the lowefficacy of $Delta$ ⁹-THC in this assay. However, correlation of the K_i and K_s valuesfor each agonist (r = 0.90 in cerebellum, r = 0.92 in hippocampus,and r = 0.98 in hypothalamus) were significant by ANOVA (P < .05).Moreover, each agonist was usually ( $Delta$ ⁹-THC again being the exception) more potent in receptor bindingthan in stimulating [³⁵S]GTP $gamma$ S binding (Table 3). This leads to a problem in interpretationbecause it implies that greater than full receptor occupancy isrequired to achieve maximal effect, an issue that will be addressedby multicomponent binding analyses (seebelow).

Agonist Inhibition of Adenylyl Cyclase. Three agonists that exhibited a wide range of efficacies for stimulating the binding of [³⁵S]GTP $gamma$ S (WIN55212-2, methanandamide, and $Delta$ ⁹-THC) were used to assess the concentration-effect relationshipfor inhibition of adenylyl cyclase in rat cerebellar membranes.All three agonists produced significant (ANOVA, P < .005 for eachagonist) concentration-dependent inhibition of adenylyl cyclase(Fig. 3). The effects of each agonist on adenylyl cyclase werecompletely blocked by 100 nM SR141716A, which had no effect onadenylyl cyclase by itself (data not shown). IC₅₀ values for thethree cannabinoid agonists in inhibiting adenylyl cyclase rangedfrom 32 to 155 nM, and they were significantly more potent thanthe corresponding EC₅₀ values of each agonist in stimulating [³⁵S]GTP $gamma$ S binding, but were similar to their K_i values in displacing[³H]SR141716A binding (Table 3). The cannabinoid agonists alsoexhibited different efficacies (I_max values) for inhibiting adenylylcyclase (Table 2), with WIN55212-2 and methanandamide producingsimilar levels of inhibition, and $Delta$ ⁹-THC producing approximately 50% of the maximal inhibition producedby WIN55212-2 (P < .05, Tukey-Kramer test). The I_max values ofmethanandamide and $Delta$ ⁹-THC for adenylyl cyclase inhibition normalized to WIN55212-2(85 ± 5 and 53 ± 4%, respectively) were significantly higher (P< .05, Mann-Whitney rank sum test) than those for [³⁵S]GTP $gamma$ S binding normalized to WIN55212-2 (61 ± 4 and 19 ± 1%,respectively).

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Fig. 3. Cannabinoid inhibition of adenylyl cyclase in rat cerebellar membranes. Assays were performed by incubating membranes with various concentrations of each agonist as described under Experimental Procedures. Data are percentage of inhibition of basal adenylyl cyclase activity presented as mean ± S.E. from four assays performed in duplicate.

Multicomponent Analysis of Agonist-Stimulated [³⁵S]GTP $gamma$ S Binding and Agonist-Inhibited [³H]SR141716A Binding Curves. Inspection of the agonist concentration-effect curves for the stimulation of [³⁵S]GTP $gamma$ S binding and inhibition of [³H]SR141716A binding revealed relatively shallow curves. In fact,all data fit better to a one-site model with variable slope (andall Hill slope values were less than one) than to a one-site modelwith Hill slope constrained to one. Moreover, comparison of thebinding and stimulation curves in each region showed that eachagonist appeared to occupy cannabinoid receptors at lower concentrationsthan those that stimulated [³⁵S]GTP $gamma$ S binding (Fig. 4). In each region, approximately 10 to30% of [³H]SR141716A binding was inhibited before any stimulation of [³⁵S]GTP $gamma$ S binding occurred. For example, in hippocampus, 1 nM levonantradoldisplaced 25% of [³H]SR141716A binding, but it did not stimulate [³⁵S]GTP $gamma$ S binding (Fig. 4). In contrast, complete receptor occupancyby each agonist, indicated by 100% inhibition of [³H]SR141716A binding, occurred at nearly the same concentrationof agonist as maximal stimulation of [³⁵S]GTP $gamma$ S binding (e.g., 3 µM levonantradol; Fig. 4).

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Fig. 4. Multicomponent analysis of cannabinoid stimulation of [³⁵S]GTP $gamma$ S binding (A) and displacement of [³H]SR141716A binding (B) in hippocampal membranes. Data are mean ± S.E. from seven assays performed in duplicate. Net agonist-stimulated [³⁵S]GTP $gamma$ S binding is shown as percentage of that obtained with 3 µM levonantradol. Curve fits are to two- and three-site models as appropriate.

To more accurately determine the potency and affinity of each ligand, a representative region (hippocampus) was assayed byusing 34 concentrations of each agonist for displacement of [³H]SR141716A binding and stimulation of [³⁵S]GTP $gamma$ S binding. Table 4 provides the analysis of displacementand stimulation curves for WIN55212-2, levonantradol, CP55940,and methanandamide. Data for $Delta$ ⁹-THC are not presented because the combination of low aqueoussolubility and low affinity for this agonist made multicomponentanalysis of the data unreliable. In all cases, for both [³H]SR141716A and [³⁵S]GTP $gamma$ S binding, all agonists displayed Hill slope (n_H) valuessignificantly less than one, with most Hill slope values approximately0.5 (Table 4), suggesting the presence of multiple binding sites.Multicomponent analyses of agonist displacement and stimulationcurves confirmed this suggestion. For [³⁵S]GTP $gamma$ S binding, agonist stimulation curves were best fit to atwo-site model for all agonists, with high-affinity sites makingup approximately 14 to 60% of the total number of sites. For receptorbinding, the agonist displacement curves were best fit to a three-sitemodel for all agonists except methanandamide, which fit best toa two-site model, consistent with its higher Hill slope (0.86)compared with those of other agonists (Table 4). For the threeagonists producing a three-site fit, individual K_i values wereat least 10-fold different from the other two K_i values for thatagonist, with high-affinity sites ranging from 0.16 to 1 nM, intermediate-affinitysites ranging from 3 to 50 nM, and low-affinity sites rangingfrom 44 to 3200 nM. Although the potencies of levonantradol andCP55940 at each calculated site were very similar, each exhibitedgreater potency than WIN55212-2 at the corresponding site (Table4).

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TABLE 4
Multicomponent analysis of agonist displacement of [³H]SR141716A and stimulation of [³⁵S]GTP $gamma$ S binding in hippocampal membranes
Agonist concentration-effect curves were generated under identical assay conditions for displacement of [³H]SR141716A binding and stimulation of [³⁵S]GTP $gamma$ S binding. Data were normalized to percentage of total specific (or agonist-stimulated) binding. Pooled data from seven separate experiments were fit to multicomponent equations by nonlinear regression, as described under Experimental Procedures. The "%" column refers to the percentage of total binding sites that are of high, intermediate, or low affinity as fit by nonlinear regression. IC₅₀ and EC₅₀ values are presented as mean log values ± S.E. of each fit, with corresponding K_i and K_s values in nM listed in parentheses. K_i/K_s ratios are shown for receptor binding and [³⁵S]GTP $gamma$ S-stimulating sites that are hypothesized to correspond to one another.

The data in Table 4 allow a direct comparison between agonist potencies for displacement of [³H]SR141716A binding compared with stimulation of [³⁵S]GTP $gamma$ S binding. However, because the [³⁵S]GTP $gamma$ S data were best fit with two-site models and [³H]SR141716A data were fit to three-site models, it is not obvioushow to determine which of the three receptor-binding sites bestcorrelate with the two G-protein activation sites. The resolutionof this problem is illustrated in Fig. 5, which shows the occupancyof receptors for levonantradol (Fig. 5A) and methanandamide (Fig.5B). For levonantradol, whose [³H]SR141716A displacement curve was best fit to three sites, itis clear that occupancy of receptors occurred at lower concentrationsof levonantradol than did stimulation of [³⁵S]GTP $gamma$ S binding. For example, 1 nM levonantradol produced 25%occupancy of receptor binding, but produced approximately 5% ofmaximal [³⁵S]GTP $gamma$ S stimulation. Therefore, for levonantradol, there is nohigh-affinity G-protein activation site that corresponds to thehighest affinity receptor-binding site. For this reason, in Table4, the "high"-affinity [³⁵S]GTP $gamma$ S site is compared directly with the intermediate receptor-bindingsite, and the low-affinity sites for both assays are comparedwith each other. The same situation existed for WIN55212-2 andCP55940: the low concentrations of agonist corresponding to thehighest affinity receptor-binding site produced little or no stimulationof [³⁵S]GTP $gamma$ S binding (data not shown). In contrast, the situation wasdifferent for methanandamide (Fig. 5B), where receptor bindingand [³⁵S]GTP $gamma$ S curves were essentially identical, and there was closeto a 1:1 relationship between receptor occupancy by this agonistand stimulation of [³⁵S]GTP $gamma$ S binding. This agrees with the basic finding of multicomponentanalysis of methanandamide curves that showed that a two-sitemodel best fit the data for both assays (Table 4).

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Fig. 5. Comparison of levonantradol (A) and methanandamide (B) stimulation of [³⁵S]GTP $gamma$ S binding and cannabinoid receptor occupancy. Data are mean ± S.E. from seven assays performed in duplicate. Net agonist-stimulated [³⁵S]GTP $gamma$ S binding is shown as percentage of maximum obtained with each agonist. Curve fits are to two- and three-site models as appropriate.

Now that the different affinity states for agonist displacement of [³H]SR141716A binding and stimulation of [³⁵S]GTP $gamma$ S binding can be matched, K_i/K_s ratios can be calculatedbetween receptor-binding and G-protein activation potencies (Table4). With the exception of the low-affinity sites for WIN55212-2,which exhibited a K_i/K_s ratio of 16, the K_i/K_s ratios were allfairly similar for all agonists, and all close to one, indicatinglittle if any receptor reserve for these agonists for the stimulationof [³⁵S]GTP $gamma$ S binding via cannabinoidreceptors.

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

For these studies, five agonists representing a wide range of efficacies and potencies for G-protein activation in rat cerebellarmembranes were chosen to determine whether these differences forG-protein activation persisted in other brain regions, and whetherthey also were manifested at the level of a downstream effectorsystem, adenylyl cyclase. Hippocampus and hypothalamus were comparedwith cerebellum because hippocampus exhibited similar levels ofcannabinoid receptors and cannabinoid-activated G-proteins, whereashypothalamus exhibited lower levels of cannabinoid receptors andhigher levels of cannabinoid-activated G-proteins (Breivogel etal., 1997). Methanandamide, a stable analog, was used insteadof the endogenous cannabinoid anandamide because previous resultsdemonstrated that these agonists acted essentially identicallyfor both [³⁵S]GTP $gamma$ S binding (Breivogel et al., 1998) and receptor binding(Abadji et al., 1994) (provided that the membranes had been pretreatedwith an esteraseinhibitor).

It is clear that the responses measured in these studies were mediated by CB₁ receptors as assessed by using the CB₁-selectiveantagonist SR141716A. Agonist-receptor binding was measured byinhibition of [³H]SR141716A binding, stimulation of [³⁵S]GTP $gamma$ S binding was inhibited by SR141716A with a potency consistentwith mediation by CB₁, and agonist inhibition of adenylyl cyclasewas blocked potently by SR141716A. Furthermore, the relative affinitiesfor each agonist agreed with previously published relative affinitiesat CB₁ cannabinoid receptors (Rinaldi-Carmona et al., 1996).

Results of this study indicated that relative agonist potency is determined by agonist receptor affinity because agonist potenciesfor functional responses (activation of G-proteins and the inhibitionof cAMP accumulation) correlated with agonist receptor-bindingaffinities. Although there were no apparent differences in agonistaffinities across regions, most agonists (except $Delta$ ⁹-THC where efficacy was low) were most potent for [³⁵S]GTP $gamma$ S binding in hippocampus and least potent in cerebellum.This may be explained by regional differences in receptor reserve,with reserve being highest in hippocampus and lowest in cerebellum.However, agonist receptor affinities did not vary across regions,and the K_i/K_s ratios in hippocampus were all close to one, indicatinglittle, if any, cannabinoid receptor reserve for [³⁵S]GTP $gamma$ S binding. This agrees with the observation that near completereceptor occupancy is required to obtain maximal stimulation of[³⁵S]GTP $gamma$ S binding (Fig. 4).

Results (Tables 1 and 2) showed significant differences in relative agonist efficacy (E_max) and potency across regions,but the reasons for these differences are not clear. The numbersof cannabinoid-activated G-proteins and cannabinoid receptorsand the ratios between them (catalytic amplification factors)in these brain regions were previously reported by our laboratory.These factors were very similar for cerebellum and hippocampus,but hypothalamus exhibited higher amplification factors (Breivogelet al., 1997). Neither differences in receptor density nor amplificationfactor correlated with differences in relative agonist E_max orpotency across these regions because relative agonist E_max valuesand potencies were most similar in hippocampus and hypothalamus.However, it is possible that the types of G-proteins activatedby cannabinoid receptors in these regions vary. This is supportedby the observation that cannabinoid-inhibited adenylyl cyclaseis measurable in cerebellar but not in hippocampal or hypothalamicmembranes, indicating that perhaps there is a higher ratio ofadenylyl cyclase-inhibiting G-proteins (G_i or certain Gcomplexes) to other types of G-proteins coupling to cannabinoidreceptors in cerebellum (Pacheco et al., 1991; Childers et al.,1994). However, data obtained in another study by using a photoaffinityGTP analog, azidoanilido [³²P]GTP, found no evidence for a regional difference in activationof G-protein $alpha$ -subunits that would account for this variation(Prather et al., 2000). Alternatively, it may be that these agonistsacting at CB_1A or at undiscovered cannabinoid receptor subtypesdisplay different efficacies, and that the multiple receptor subtypesare present in different ratios across these threeregions.

In cerebellar membranes, it is clear that the potencies of each agonist, and the efficacies of the partial agonists relativeto WIN55212-2, are higher for inhibition of adenylyl cyclase thanfor stimulation of [³⁵S]GTP $gamma$ S binding. This is consistent with the existence of receptor/G-proteinreserve for adenylyl cyclase inhibition, or greater receptor reservefor adenylyl cyclase inhibition than for G-protein activation.Receptor/effector reserve for the adenylyl cyclase would be predictedto produce greater apparent potency for the agonists because lowerlevels of receptor occupancy would be required to obtain the maximaleffect. Because full agonists would activate excess G-proteinsover what is necessary for maximal inhibition of adenylyl cyclase,partial agonists would have greater efficacy relative to a fullagonist (e.g., WIN55212-2) for adenylyl cyclase inhibition thanfor G-proteinactivation.

This study clearly shows that cannabinoid agonists exhibit a wide range of efficacies for G-protein activation, translatinginto efficacy differences for at least one downstream effectorsystem, adenylyl cyclase. Some of these differences were reportedpreviously by other measurements. For example, both anandamideand CP55940 were partial agonists for inhibiting Ca²⁺ currents (Mackie et al., 1993; Shen et al., 1996). Chronic treatmentswith agonists of different efficacies have shown that more tolerancedevelops to agonists of greater efficacy (Elliott et al., 1997).Cultured N18TG2 cells exhibited greater desensitization of cannabinoid-inhibitedcAMP after chronic desacetyllevonantradol than $Delta$ ⁹-THC treatment (Dill and Howlett, 1988), and mice treated chronicallywith CP55940 showed greater behavioral tolerance than those treatedwith $Delta$ ⁹-THC (Fan et al., 1994). Although it is difficult to demonstrateacute efficacy differences behaviorally (Fan et al., 1994), thesechronic data suggest in vivo efficacy differences. Thus, it appearsthat these differences in efficacy at different effector systemsare produced at the level of G-protein activation. Differencesin efficacy may have profound implications for both drug abuseand for the use of cannabinoids as medicinal agents, particularlywith long-termuse.

[³⁵S]GTP $gamma$ S binding assays produced multicomponent concentration-effect curves for all agonists. Some of this heterogeneity maybe due to the simultaneous presence of G-protein-coupled and -uncoupledcannabinoid receptors because both guanine nucleotides and sodiumdecrease high-affinity agonist binding to cannabinoid receptorsby decreasing receptor/G-protein coupling (Devane et al., 1988;Pacheco et al., 1994). Alternatively, the two apparent potenciesobserved for the stimulation of [³⁵S]GTP $gamma$ S binding may have been due to coupling to different subtypesof G-protein $alpha$ -subunits, as previously suggested (Prather et al.,2000).

The identity of the three apparent receptor-binding sites is not clear. The highest affinity sites probably represent precoupledcannabinoid receptors because these values were similar to thosepreviously determined under high-affinity agonist binding conditions(Rinaldi-Carmona et al., 1996). Previous data indicating thatcoupling to different G-subtypes occurred with differentpotencies (Prather et al., 2000) suggest that the multiple agonistreceptor-binding affinities observed for the agonists were dueto this differential coupling. Coupling to different G-proteinshas previously been proposed as the source of three receptor-bindingaffinities observed for muscarinic receptors in cardiac membranes(Green et al., 1997). Another possible explanation for the threeapparent receptor-binding sites is that high-affinity receptorbinding occurs when receptors are coupled to G-proteins that arenot binding either GDP or GTP( $gamma$ S), and the remaining states arisefrom receptor coupling to different subtypes of G-proteins thathave guanine nucleotidebound.

These data do not directly identify the receptor affinity state(s) responsible for G-protein activation, but they do provideevidence via a strong correlation. In this study, it appearedthat highest affinity agonist-binding sites contributed to basal,and not to agonist-stimulated [³⁵S]GTP $gamma$ S binding. For example, a previous study suggested thatthe GDP affinity on receptor precoupled G-proteins is approximately30-fold lower than on uncoupled G-proteins, and is decreased only8-fold further by a cannabinoid full agonist (Breivogel et al.,1998). Thus, receptor/G-protein coupling may promote some [³⁵S]GTP $gamma$ S binding even in the absence of agonist. A mathematicalmodeling study by Shea and Linderman (1997) supports the suggestionthat precoupling of receptors and G-proteins may lead to complexbinding and activation curves as were observed experimentallyin the present study. Intermediate- and low-affinity receptor-bindingsites appeared to correspond to the high- and low-affinity [³⁵S]GTP $gamma$ S-stimulating sites. This interpretation is somewhat complicatedby findings with WIN55212-2 (Table 4), where the percentage ofintermediate receptor sites (59%) more closely corresponded tothe percentage of low-affinity [³⁵S]GTP $gamma$ S sites (68%). Nevertheless, for the other agonists, thepercentage of low-affinity receptor sites corresponds well withthe percentage of low-affinity [³⁵S]GTP $gamma$ S sites. The lack of correspondence between the percentagesof intermediate receptor sites and high-affinity [³⁵S]GTP $gamma$ S sites can be explained by the existence of high-affinityreceptor-binding sites that reduce the percentage of intermediatereceptor sites. Previous findings that the ratio between cannabinoidreceptor number and cannabinoid-activated G-proteins is not constantacross brain regions (Breivogel et al., 1997) would predict thatthe ratio between these individual sites also might not beconstant.

In contrast to the three-site model that fit receptor-binding data for WIN55212-2, levonantradol, and CP55940, methanandamideappeared to recognize only two-receptor-binding sites, indicatingthat this ligand binds to two of the sites recognized by the otherligands with equal or very similar affinity. Perhaps the inabilityof methanandamide to recognize a high-affinity receptor-bindingsite (higher than those stimulating [³⁵S]GTP $gamma$ S binding) is related to its lower efficacy for stimulating[³⁵S]GTP $gamma$ S binding. Regardless of the interpretation, these datashow that cannabinoid receptors exhibit multiple affinities forat least some agonists, and that agonist occupancy of cannabinoidreceptors often occurs at lower concentrations than are able tostimulate [³⁵S]GTP $gamma$ S binding to G-proteins.

	Footnotes

Accepted for publication June 21, 2000.

Received for publication March 20, 2000.

¹ This work was supported by DA-06784 (to S.R.C.) and DA-07246 (to C.S.B.) from National Institute on DrugAbuse.

Send reprint requests to: Steven R. Childers, Department of Physiology and Pharmacology, Wake Forest University School of Medicine, Medical Center Blvd., Winston-Salem, NC 27157.

	Abbreviations

$Delta$ ⁹-THC, tetrahydrocannabinol; GTP $gamma$ S, guanosine-5'-O-(3-thio)triphosphate.

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Cannabinoid Agonist Signal Transduction in Rat Brain: Comparison of Cannabinoid Agonists in Receptor Binding, G-Protein Activation, and Adenylyl Cyclase Inhibition¹