[3H]RY 80: A High-Affinity, Selective Ligand for gamma -Aminobutyric AcidA Receptors Containing Alpha-5 Subunits,

Assistant Professor of Medicine (Clinician-Educator)

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Vol. 283, Issue 2, 488-493, 1997

[³H]RY 80: A High-Affinity, Selective Ligand for $gamma$ -Aminobutyric Acid_A Receptors Containing Alpha-5 Subunits¹^,²

Phil Skolnick, Rona J. Hu, Christine M. Cook, Stephen D. Hurt, Joseph D. Trometer, Ruiyan Liu, Qi Huang and James M. Cook

Laboratory of Neuroscience, National Institute of Diabetes and Digestive and Kidney Diseases, National Institutes of Health, Bethesda, Maryland (R.J.H., C.M.C., P.S.), New England Nuclear, Boston, Massachusetts (S.D.H., J.D.T.), and Department of Chemistry, University of Wisconsin-Milwaukee, Milwaukee, Wisconsin (R.L., Q.H., J.M.C.)

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

The radiochemical synthesis and pharmacological properties are described of [³H]RY 80 (ethyl-8-acetylene-5,6-dihydro-5-methyl-6-oxo-4H-imidazo[1,5a][1,4]benzodiazepine-3-carboxylate,[ethyl-³H]). This compound is one of a series of 8-substituted imidazobenzodiazepinesthat exhibits both high affinity and selectivity for $gamma$ -aminobutyricacid (GABA)_A receptors containing alpha-5 subunits. Saturable,high-affinity (K_d ~0.7 nM) binding of [³H]RY 80 was observed in hippocampal membranes. The maximum number(B_max) of [³H]RY 80 binding sites was ~18% of that obtained with [³H]flunitrazepam, a radioligand that labels all "diazepam-sensitive"GABA_A receptors. This value is consistent with previous estimates(10-20%) of the proportion of rat hippocampal GABA_A receptorscontaining alpha-5 subunits determined by immunoprecipitationwith selective antibodies and competition experiments using analpha-5-selective ligand. In recombinant GABA_A receptors composedof alpha-5 beta-3 gamma-2 subunits, the K_d of [³H]RY 80 (~0.5 nM) was consistent with the value obtained in hippocampus,whereas the B_max value was not significantly different from thatobtained with [³H]flunitrazepam. The potencies of several benzodiazepine siteligands to inhibit [³H]RY 80 binding to hippocampal membranes were in agreement withthe values obtained in recombinant (alpha-5 beta-3 gamma-2) GABA_Areceptors. [³H]RY 80 was used both in a "GABA shift" assay to correctly predictthe in vivo actions of a novel, alpha-5-selective ligand and tocharacterize a population of GABA_A receptors containing alpha-5subunits in neonatal rat cortex. These findings demonstrate that[³H]RY 80 can be used as a radioligand to examine the propertiesof GABA_A receptors containing alpha-5 subunits.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

GABA_A receptors possess multiple, allosterically linked modulatory sites that are loci for drug action (reviewed in Skolnickand Paul, 1988; Johnston, 1996). However, from a therapeutic anddrug development perspective, benzodiazepine binding sites areperhaps the most important. Thus, benzodiazepine binding sitesmediate the principal therapeutic actions of 1,4-benzodiazepines(e.g., diazepam and flurazepam) as well as a large group of structurallyunrelated molecules including imidazopyridines (e.g., zolpidem),cyclopyrrolones (e.g., zopiclone) and $beta$ -carbolines (e.g., abecarnil).

GABA_A receptors are a heterogeneous family of ligand-gated ion channels that may be assembled from at least 15 structurallyrelated subunits (alpha, beta, gamma, delta and rho) (reviewedin Stephenson, 1995). Immunochemical studies have demonstratedthat GABA_A receptors most often exist as ternary complexes composedof alpha, beta, and gamma subunits (; DeBlas, 1996; Fritschy andMohler, 1993) arranged as pentamers (Nayeem et al., 1994). AlthoughGABA_A receptor subunit stoichiometry remains controversial (Backuset al., 1993; Chang et al., 1996; Tretter et al., 1997), boththe affinities and efficacies of drugs acting at this family ofligand-gated ion channels (including benzodiazepine site ligands)appear to be defined by subunit composition. For example, studiesin recombinant GABA_A receptors have shown that the alpha subunitis a primary determinant of ligand affinity at benzodiazepinebinding sites (Hadingham et al., 1993; Lüddens et al., 1990;Pritchett and Seeburg, 1990), with the gamma subunit playing asmaller, albeit significant role for some ligands (Benke et al.,1996; Lüddens et al., 1994). Ligand efficacy at benzodiazepinebinding sites appears to be determined primarily by the gammasubunit (Ducic et al., 1993; von Blankenfeld et al., 1990; Waffordet al., 1993). These studies in recombinant receptors have providedvaluable insights that explain many aspects of the pharmacologicalheterogeneity of wild-type GABA_A receptors, which has been recognizedfor almost 20 years (Klepner et al., 1979; Lippa et al., 1982;Young et al., 1981).

With few exceptions (e.g., GABA_A receptors in the cerebellum containing alpha-6 subunits, the so-called "diazepam-insensitiveGABA_A receptors"; Gunnersen et al., 1996; Lüddens et al., 1990;Wong et al., 1995), it is inherently more difficult to study thepharmacological properties of benzodiazepine site ligands at specificsubpopulations of wild-type compared with recombinant GABA_A receptors.This is due, in part, to a remarkable receptor heterogeneity presentat the cellular level (Fritschy and Mohler, 1995; McKernan andWhiting, 1996; Wisden et al., 1992) and the paucity of high-affinity,selective ligands capable of discriminating among these receptorsubpopulations. Based on the ~10-fold selectivity of Ro 15-4513for recombinant GABA_A receptors containing alpha-5 subunits (comparedwith receptors containing alpha-1, alpha-2 or alpha-3 subunits);Hadingham et al., 1993; Lüddens et al., 1994), a series of novel8-substituted imidazobenzodiazepines (Liu et al., 1995, 1996)were prepared in an attempt to increase this selectivity. Severalof these compounds exhibited both high-affinity (K_i ~0.4-5 nM)and selectivity (up to 75-fold) for recombinant GABA_A receptorscontaining alpha-5 subunits. Moreover, these imidazobenzodiazepinesinhibited [³H]flunitrazepam binding to rat hippocampal membranes (that arerelatively enriched in GABA_A receptors containing alpha-5 subunits;McKernan et al., 1991a) with the characteristics of high-affinity,subtype-selective ligands (Liu et al., 1996). The present studydescribes the radiochemical synthesis and pharmacological propertiesof one member of this series, [³H]RY 80 (ethyl-8-acetylene-5,6-dihydro-5-methyl-6-oxo-4H-imidazo[1,5a][1,4]benzodiazepine-3-carboxylate, [ethyl-³H]). The results obtained in both wild-type and recombinant GABA_Areceptors indicate that [³H]RY 80 is a useful radioligand for studying specific receptorpopulations containing alpha-5 subunits.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Cell culture and transfection. HEK 293 cells (American Type Culture Collection, Rockville, MD) were maintained at 37° in 5% CO₂ as previously described (Gunnersenet al., 1996). Cells were transfected with cDNAs for the rat alpha-5,beta-3 and gamma-2 (8, 8 and 5 µg of DNA/10-cm² dish containing ~4 × 10⁶ cells) subunits by calcium phosphate precipitation (Gorman etal., 1990). The cells were harvested ~48 hr later, and a washedmembrane suspension was prepared as previously described (Gunnersenet al., 1996). These membrane suspensions were stored at ~70°until assayed. The beta-3 and gamma-2s cDNAs were subcloned intopCDNA1 and pcDNA3 vectors, respectively (Gunnersen et al., 1996;Harris et al., 1995). The alpha-5 cDNA (the gift of Dr. H. Lüddens,University of Mainz) was subcloned from a BlueScript to a CMVvector by standard techniques.

Tissue preparation. Adult male and juvenile (6-8 days postpartum; both sexes) Sprague-Dawley rats (Taconic Farms, Germantown, NY) were killedby decapitation. The brains were rapidly removed and placed inbeakers containing ice-cold 50 mM Tris-citrate buffer, pH 7.8.After dissection, the tissues were disrupted in 50 volumes ofice-cold Tris-citrate buffer using a Polytron (20 sec; setting6-7) (Brinkmann Instruments, Westbury, NY). The homogenates werecentrifuged at 20,000 × g (4°C) for 20 min. The supernatants werediscarded and the pellets resuspended in an equal volume of bufferand recentrifuged. This "washing" procedure was repeated a totalof five times. Tissue suspensions were frozen on solid CO₂ andstored at $-$ 70°C until assayed.

Radioligand binding. Studies in recombinant receptors were performed in a final volume of 1 ml consisting of: tissue suspension (~0.2 mg of protein),0.2 M NaCl, [³H]RY 80 or flunitrazepam and 50 mM Tris-citrate buffer, pH 7.8,to volume. For studies in wild-type receptors (from adult hippocampusand juvenile cerebral cortex), the volume of membrane suspensionwas varied to yield between 0.02 and 0.1 mg of protein/assay.In competition experiments, 50 µl of buffer was replaced by drugsand/or GABA (30 µM); the concentration of [³H]RY 80 routinely used in competition experiments was ~0.5 to0.6 nM. Nonspecific binding was defined with Ro 15-1788 (10 µM).In pilot experiments to optimize incubation conditions, specificbinding of [³H]RY 80 was obtained at a range of temperatures (4°, 25° and 37°),with the optimum ratio of specific and nonspecific binding achievedat 4°. Under these assay conditions, [³H]RY 80 (0.8 nM) binding to hippocampal membranes reached equilibriumby 30 min and was maintained for $>=$ 2 hr. Samples were routinelyharvested at 2 hr. Assays (4°C) were terminated after 2 hr byrapid filtration (Brandel M-48R, Gaithersburg, MD) through GF/Bfilters followed by two 5-ml washes with ice-cold 50 mM Tris-citratebuffer. Radioactivity retained by the filters was measured inan LS 6500 liquid scintillation counter (Beckman Instruments,Palo Alto, CA). Data were analyzed with GraphPAD InPlot 4 (GraphPADSoftware, San Diego, CA). Protein concentrations were determinedusing the BCA protein assay reagent (Pierce, Rockford, IL).

In vivo studies. Adult, male NIH/Swiss mice (~30 g) were injected (0.1 ml i.p.) with graded doses of QHII-066 (7-acetyleno-1,3-dihydro-1-methyl-5-phenyl-2H-1,4-benzodiazepin-2-one)or vehicle (10% diluted Emulphor/90% saline). Mice were placedin individual plastic cages and administered either RY-24 [t-butyl-8-acetylene-5,6-dihydro-5-methyl-6-oxo-4H-imidazo[1,5a][1,4]benzodiazepine-3-carboxylate;20 mg/kg i.p.) or DMCM (7.5 mg/kg i.p.) 10 min. later. Animalswere observed (10 min) for the presence of tonic and clonic convulsions(Liu et al., 1996).

Synthesis of [³H]RY 80. 8-Acetylene-5,6-dihydro-5-methyl-6-oxo-4H-imidazo[1,5a][1,4]benzodiazepine-3-carboxylic acid (15 mg; 0.05 mmol) was addedto a 10-ml round-bottom flask and dissolved in N, N $'$ -dimethylformamide(DMF) (1 ml). After the addition of 0.2 M lithium hydroxide (0.25ml), the reaction was stirred at room temperature for 1 hr andthen heated (70°C) for 30 min. The reaction mixture was cooledto room temperature, and the solvents were removed under reducedpressure. The residue was taken up in DMF (1 ml) and transferredto a 5-ml tritiation flask. [³H]Ethyl iodide (0.1 mmol) was added to this mixture, and the reactionwas stirred at 70°C for 16 hr (fig. 1). The labiles were removedwith ethanol, and the residue was taken up in 10 ml of ethanol.Thin-layer chromatography (ethyl acetate/hexanes 10:1) of thecrude reaction mixture revealed two major components with R_F valuesof ~0.4 (RY 80) and ~0.1 (presumed to be the quaternary salt ofRY 80). The crude reaction mixture was purified by high performanceliquid chromatography on a Zorbax RX-C8 analytical column witha mobile phase of 1% triethylammonium acetate (pH 4.0)/acetonitrile(75:25) at a flow rate of 1 ml/min. The material correspondingto product (detected by UV absorbance at 274 nm) had a retentiontime of ~25 min. The solvents were removed with multiple ethanolazeotropes, and the residue was taken up in 50 ml of ethanol.The specific activity of [ethyl-³H]RY 80 was 55.4 Ci/mmol, as determined by FAB mass spectroscopy.The radiochemical purity of [³H]RY 80 was 99%, as determined by high performance liquid chromatography.

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Fig. 1. Radiochemical preparation of [³H]RY 80.

Materials. [³H]Flunitrazepam (specific activity, 85.8 Ci/mmol) was purchased from Dupont-New England Nuclear (Boston, MA). 3-Carbomethoxy- $beta$ -carboline,QHII-066 (the 7-acetyleno-congener of diazepam; Huang et al.,1996), RY-24 (the t-butyl ester congener of RY 80; Liu et al.,1996) and 8-acetylene-5,6-dihydro-5-methyl-6-oxo-4H-imidazo[1,5a][1,4]benzodiazepine-3-carboxylatewere synthesized at the University of Wisconsin-Milwaukee. Ro15-1788 was donated by Hoffmann-LaRoche (Nutley, NJ). Zolpidemwas the gift of Synthelabo (Laboratoire Experimental RechercheSynthelabo; Paris, France). DMCM was purchased from Research Biochemicals(Natick, MA). All other reagents and chemicals were obtained fromstandard commercial sources.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

[³H]RY 80 binding to recombinant alpha-5 beta-3 gamma-2 receptors and hippocampal membranes. Saturable, high-affinity (K_d, 0.53 ± 0.09 nM) binding of [³H]RY 80 was observed in membranes prepared from HEK 293 cells transfectedwith cDNAs encoding alpha-5 beta-3 gamma-2 subunits (fig. 2A).The maximum number of binding sites (B_max) obtained with [³H]RY 80 (173 ± 9 fmol/mg of protein) was not significantly differentfrom the values obtained using [³H]flunitrazepam (190 ± 12 fmol/mg of protein; K_d, 1.3 ± 0.18 nM)(fig. 2A). The apparent affinity of [³H]RY 80 in hippocampal membranes (K_d, 0.68±.04 nM vs. 1.5 ± 0.12nM for [³H]flunitrazepam) was comparable to that obtained in recombinantreceptors, whereas the B_max value was ~17.6% of that obtainedwith [³H]flunitrazepam (302 ± 21 fmol/mg of protein vs. 1712 ± 156 fmol/mgof protein, respectively) (fig. 2B). In identically prepared cerebellarmembranes, saturable binding of [³H]RY 80 was not observed using radioligand concentrations of $<=$ 20nM (data not shown). To confirm that the receptor population labeledby [³H]RY 80 corresponds to GABA_A receptors containing alpha-5 subunits,the effects of several ligands with well defined characteristicsat these receptors were examined. Zolpidem, which binds with low(µM) affinity to recombinant receptors containing alpha-5 beta-3gamma-2 receptors (Graham et al., 1996; Lüddens et al., 1994;Pritchett and Seeburg, 1990) did not produce a concentration-dependentinhibition of [³H]RY 80 binding to either recombinant alpha-5 beta-3 gamma-2 receptors(fig. 3A) or hippocampal membranes (fig. 3B). In contrast, thepotency of an alpha-5-selective ligand, RY-24 (the t-butyl estercongener of RY 80) (Liu et al., 1995), to inhibit [³H]RY 80 binding was similar in recombinant receptors and hippocampalmembranes (IC₅₀, 0.95 ± 0.22 and 0.82 ± 0.13 nM, respectively)(fig. 3). The potency of QHII-066 (the 7-acetyleno congener ofdiazepam), which exhibits a moderate selectivity for recombinantalpha-5-containing receptors (Huang et al., 1996), was similarin recombinant alpha-5 beta-3 gamma-2 receptors and hippocampalmembranes (IC₅₀, 41 ± 5 vs. 56 ± 10 nM, respectively). GABA increasedthe potency of QHII-066 to inhibit [³H]RY 80 binding by ~2.5-3-fold in both preparations (IC₅₀, 17± 3 vs. 18 ± 7 nM, respectively) (fig. 3).

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Fig. 2. Saturation studies of: [³H]RY 80 binding to (A) recombinant alpha-5 beta-3 gamma-2 receptors and (B) hippocampal membranesHEK 293 cells were transiently transfected with cDNAs encodingrat alpha-5 beta-3 gamma-2 subunits. The cells were harvested~48 hr after transfection and membranes prepared as described.Hippocampal membranes were prepared as described. A, Representativesaturation isotherm of [³H]RY 80 ( $bullet$ ) and [³H]flunitrazepam ( $black-square$ ). The K_d and B_max values in these experimentswere 0.43 nM and 182 fmol/mg of protein and 1.3 nM and 183 fmol/mgof protein for [³H]RY 80 and [³H]flunitrazepam, respectively. In pilot experiments, the bindingof [³H]RY 80 to cerebellar membranes was not saturable using radioligandconcentrations of $<=$ 20 nM (data not shown). B, In this representativeexperiment, the K_d and B_max values were 0.71 nM and 314 fmol/mgof protein and 1.2 nM and 1707 fmol/mg of protein for [³H]RY 80 and [³H]flunitrazepam, respectively. Insets, Rosenthal (Scatchard) analysisof the respective saturation isotherms in (A) recombinant tissueand (B) hippocampal membranes. The radioligand concentrationsranged from ~0.12 to 3.7 nM and ~0.5 to 12.6 nM for [³H]RY 80 and [³H]flunitrazepam, respectively. These experiments were repeatedthree or more times (see Results) with [³H]RY 80 and [³H]flunitrazepam.

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Fig. 3. Inhibition of [³H]RY 80 binding to (A) recombinant alpha-5 beta-3 gamma-2 receptors and (B) hippocampal membranes: [³H]RY 80 binding to recombinant and hippocampal membranes was assayedas described. These are representative experiments repeated atleast three times. $triangle$ , RY-24; $bullet$ , QHII-066 + GABA; $open circle$ , QHII-066;*, zolpidem. The x axes depicts the log of concentrations used.[³H]RY 80 was used at a concentration of ~0.5 nM in these experiments.The IC₅₀ values (in nM) in recombinant and hippocampal membraneswere 0.83 and 1.03 for RY-24, 34 and 53 for QHII-066 and 14.3and 20.9 for QHII-066 + GABA, respectively. The IC₅₀ values forzolpidem could not be estimated. Consistent with the describedinverse agonist properties of RY 80 demonstrated both in vitroand in vivo (Liu et al., 1995

, 1996

), GABA (30 µM) inhibited [³H]RY 80 binding by 48.7 ± 4.1% and 41 ± 1.8% in recombinant receptorsand hippocampal membranes, respectively. The IC₅₀ values calculatedfor QHII-066 in the presence of GABA reflect this inhibitory effectof GABA. The Hill slopes in recombinant and hippocampal membraneswere 0.84 ± 0.1 and 0.72 ± 0.04 for RY-24, 0.99 ± 0.03 and 0.84± 0.1 for QHII-066 and 1.05 ± 0.05 and 0.79 ± 0.12 for QHII-066+ GABA, respectively. These experiments were repeated at leastthree times (see Results).

Anticonvulsant actions of QHII-066. The anticonvulsant actions of QHII-066 were examined because GABA increased the potency of this compound in vitro (i.e., apositive "GABA-shift") (fig. 3). Consistent with previous findings(Liu et al., 1996), parenteral administration of DMCM (7.5 mg/kg)and RY-24 (20 mg/kg) produced tonic and clonic convulsions in100% and 80% of mice, respectively. Higher doses of RY-24 didnot result in a greater percentage of animals exhibiting convulsions(Liu et al., 1996; and data not shown). QHII-066 reduced bothRY-24- and DMCM-induced convulsions in a dose-dependent mannerwith ED₅₀ values of ~0.6 and ~2.9 mg/kg, respectively (fig. 4)

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Fig. 4. Anticonvulsant actions of QHII-066. Mice were injected (0.1 ml i.p.) with varying doses of QHII-066 or vehicle (5-20 mice/dose).At 10 min later, the mice were injected with RY-24 (20 mg/kg i.p.)or DMCM (7.5 mg/kg i.p.) and observed (10 min) for the presenceof convulsions. RY-24 and DMCM produced a maximum of 80% (16 of20) and 100% (10 of 10) convulsions, respectively. The inabilityof RY-24 to produce convulsions in 100% of the mice is consistentwith previous data (Liu et al., 1996

). The ED₅₀ values of QHII-066were 0.6 and 2.9 mg/kg vs. RY-24 and DMCM, respectively.

[³H]RY 80 binding to neonatal rat cortex. High-affinity (K_d, 0.81 ± 0.25 nM), saturable (B_max, 464 ± 104 fmol/mg of protein) binding of [³H]RY 80 was obtained in cortical membranes prepared from 6- to8-day-old rat pups (fig. 5). This binding was zolpidem insensitiveand inhibited by RY-24 in a concentration-dependent fashion (IC₅₀,2.2 ± 0.4 nM) (fig. 5, inset). The B_max value obtained with [³H]RY 80 was ~31% of the value obtained with [³H]flunitrazepam (1461 ± 317 fmol/mg of protein; K_d, 1.2 ± 0.1nM).

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Fig. 5. [³H]RY 80 binding to neonatal rat cortex demonstrates a comparison with [³H]flunitrazepam. Cortical membranes were prepared from 6- to 8-day-oldrat pups as described in the text. In this representative experiment,(A) the K_d and B_max values for RY 80 ( $bullet$ ) and flunitrazepam ( $black-square$ )were 0.62 and 1.5 nM and 322 and 1160 fmol/mg of protein, respectively.B, Rosenthal (Scatchard) plot of the saturation isotherm representedin A. C, [³H]RY 80 binding (0.75 nM) was insensitive to zolpidem ( $open circle$ ) butpotently inhibited (IC₅₀ ~ 2.9 nM) by RY-24 ( $diamond$ ). The abscissaeare in log units. These experiments were repeated three times.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

The high-affinity and selectivity of several novel imidazobenzodiazepines for recombinant GABA_A receptors containing alpha-5subunits (Liu et al., 1995) suggest that a radiolabeled form ofone (or more) of these compounds could be used to examine thepharmacological properties of the corresponding wild-type receptors.Although GABA_A receptors containing alpha-5 subunits are minorconstituents of the total GABA_A receptor pool, both in situ hybridization(Khrestchatisky et al., 1989; Wisden et al., 1992) and immunochemicalstudies (Endo and Olsen, 1993; McKernan et al., 1991a, 1991b;Mertens et al., 1993; Thompson et al., 1992) indicate the rodenthippocampus is relatively enriched in this subunit compared withother brain regions. The feasibility of selectively labeling thisreceptor subpopulation in hippocampus was supported by competitionstudies with RY-24, the t-butyl ester congener of RY 80. Thus,RY-24 inhibition of [³H]flunitrazepam binding to hippocampal membranes is best fit toa two-site competition curve, with the high-affinity component(IC₅₀ ~ 0.6 nM) representing 16 ± 4% of the sites labeled by [³H]flunitrazepam (Liu et al., 1996). This high-affinity of RY-24is consistent with both the value obtained in recombinant receptorscomposed of alpha-5 beta-3 gamma-2 subunits (Liu et al., 1995)and the proportion of these high-affinity sites corresponds tothe values obtained by immunoprecipitation with alpha-5 subunit-specificantibodies in rat hippocampus (McKernan et al., 1991a; Mertenset al., 1993). Although other imidazobenzodiazepines in this seriesexhibit a greater selectivity for recombinant GABA_A receptorsbearing alpha-5 subunits than RY 80 ( $<=$ ~75-fold compared with 60-foldfor RY 80; Liu et al., 1995, 1996), this compound was the simplestto prepare in its radiolabeled form (fig. 1).

The binding of [³H]RY 80 to recombinant alpha-5 beta-3 gamma-2 receptors was saturable (fig. 2A), with a K_d value (0.53 ± 0.09nM) comparable to the K_i value (~0.5 nM) obtained in recombinanthuman receptors composed of alpha-5 beta-3 gamma-2 subunits (Liuet al., 1995). Moreover, the B_max value obtained with [³H]RY 80 was not significantly different from the value obtainedwith [³H]flunitrazepam, indicating that both radioligands label the samereceptor populations (fig. 2B). Although saturable, high-affinitybinding (K_d, 0.69 ± 0.07 nM) of [³H]RY 80 was also detected in hippocampal membranes, the B_max valuewas only ~18% of the value obtained with [³H]flunitrazepam, a radioligand thought to label all "diazepam-sensitive"GABA_A receptor isoforms. The fraction of hippocampal GABA_A receptorslabeled by [³H]RY 80 is consistent with the values obtained by both immunoprecipitationwith alpha-5-selective antibodies (~15-16%) (Mertens et al., 1993;McKernan et al., 1991a) and competition studies using the alpha-5-selectiveligand RY-24 (16%) (Liu et al., 1996). In contrast, saturablebinding of [³H]RY 80 (at concentrations of $<=$ 20 nM) was not observed in cerebellarmembranes (fig. 2, legend), an observation consistent with boththe low expression of alpha-5 subunits in this brain region (McKernanet al., 1991b; Wisden et al., 1992) and the selectivity of RY80 for recombinant GABA_A receptors bearing this subunit (Liu etal., 1995).

Zolpidem binds with very low (µM) affinity to both recombinant GABA_A receptors containing alpha-5 subunits (Pritchett andSeeburg, 1990; Hadingham et al., 1993 Lüddens et al., 1994; fig.3A) and hippocampal GABA_A receptors that have been immunoprecipitatedwith alpha-5-selective antibodies (Mertens et al., 1993; McKernanet al., 1991a). Thus, the inability of zolpidem to significantlyreduce [³H]RY 80 binding in hippocampal membranes (fig. 3B) is consistentwith the hypothesis that this radioligand selectively labels GABA_Areceptors bearing alpha-5 subunits. This hypothesis is also consistentwith the agreement in potency of RY-24 (an alpha-5-selective ligand)to inhibit [³H]RY 80 binding to hippocampal membranes (fig. 3B) and recombinantGABA_A receptors with alpha-5 subunits (fig. 3A and Liu et al.,1995) and to inhibit a component of [³H]flunitrazepam binding to hippocampal membranes representing~16% of the total receptor pool (Liu et al., 1996).

The ability of GABA to modulate the affinity of benzodiazepine site ligands (the "GABA shift") remains a robust neurochemicalmeasure of efficacy. GABA shift assays traditionally use brainmembranes (Skolnick et al., 1982) containing heterogeneous receptorpopulations. The resulting values thus represent an average efficacybecause this measure is dependent on subunit composition (Grahamet al., 1996; von Blankenfeld et al., 1990). To determine whetherligand efficacy could be correctly predicted in a subpopulationof hippocampal GABA_A receptors using [³H]RY 80, we examined the effect of GABA on QHII-066, the 7-acetylenocongener of diazepam. This compound was recently reported to bindwith moderate ( $>=$ 7-fold) selectivity to recombinant alpha-5 beta-3gamma-2 receptors compared with isoforms containing other alphasubunits (Huang et al., 1996). GABA produced a ~2.7-fold increasein the potency of QHII-066 in both hippocampal membranes and recombinantalpha-5 beta-3 gamma-2 receptors (fig. 3). If the positive GABAshift obtained with QHII-066 in hippocampal membranes is predictiveof in vivo efficacy, then this compound should exhibit some ofthe pharmacological properties common to other benzodiazepinesite agonists. To test this hypothesis, we examined the anticonvulsantproperties of QHII-066. This measure was selected because severalof the alpha-5-selective imidazobenzodiazepines, such as RY-24,are inverse agonists at alpha-5 beta-3 gamma-2 receptors expressedin Xenopus oocytes (Liu et al., 1995) and are convulsant in mice(Liu et al., 1996). As predicted from its efficacy in hippocampalmembranes, QHII-066 blocked RY-24 induced convulsions in a dose-dependentfashion and was ~5-fold less potent against DMCM-induced convulsions(fig. 4). These observations indicate that [³H]RY 80 may be useful in evaluating ligand efficacies at wild-typeGABA_A receptors bearing alpha-5 subunits. Although more speculative,the higher potency of QHII-066 in blocking RY-24 compared withDMCM-induced convulsions suggests its anticonvulsant propertiesmay be related to an action at GABA_A receptors containing alpha-5subunits.

In situ hybridization studies have shown mRNA encoding the alpha-5 subunit is relatively abundant in the neonatal rat brain(Laurie et al., 1992). This expression diminishes substantiallyduring development, and in the adult brain, mRNA encoding thealpha-5 subunit is relatively abundant only in the hippocampus(Wisden et al., 1992). In contrast, either undetectable (McKernanet al., 1991b) or very low levels (Sieghart et al., 1993) of thecorresponding protein have been detected with subunit-specificantibodies. Based on a comparison of the B_max values obtainedwith [³H]RY 80 and flunitrazepam in cortical membranes from 6- to 8-day-oldrat pups, GABA_A receptors bearing alpha-5 subunits represent ~31%of the receptor pool (Results and fig. 5). Although it could beargued that [³H]RY 80 is labeling other GABA_A receptor isoforms in the neonatalcortex, its K_d value (0.81 ± 0.25 nM) is similar to that obtainedin both adult hippocampus and recombinant receptors (fig. 2).Moreover, [³H]RY 80 binding to juvenile cortex is zolpidem-insensitive andpotently inhibited by the alpha-5-selective ligand RY-24 (fig.5, inset). The apparent discrepancy between the low levels ofalpha-5 immunoreactive protein relative to both an abundance ofmRNA encoding this subunit and the B_max value estimated with [³H]RY 80 may be attributable to the extensive glycosylation ofalpha-5 subunits (Sieghart et al., 1993) that may interfere withthe antigen-antibody reaction in neonatal brain.

In summary, [³H]RY 80 appears to label specific populations of GABA_A receptors containing an alpha-5 subunit and may be usedin much the same manner as [³H]zolpidem to study receptor populations bearing alpha-1 subunits(DeVaud and Morrow, 1994). As such, [³H]RY 80 may be used to evaluate the potency and efficacy of compoundsat wild-type GABA_A receptors containing alpha-5 subunits, as aradioligand for autoradiographic studies and as a probe for examiningthese receptors after physiological and pharmacological manipulations.

	Footnotes

Accepted for publication July 29, 1997.

Received for publication March 19, 1997.

¹ Portions of this work were presented at the 35th Annual Meeting of the American College of Neuropsychpharmacology, December9-13, 1996, San Juan, PR.

² This work was supported in part by a predoctoral fellowship from the American Society for Pharmacology and Experimental Therapeutics(C.M.C.) and NIMH Grant MH-46851 (J.M.C.). R.J.S. is a PRAT Fellow,NIGMS.

Send reprint requests to: Dr. P. Skolnick, Chief, Laboratory of Neuroscience, NIDDK/NIH, Building 8/111, Bethesda, MD 20892-0008. E-mail: dpopa{at}helix.nih.gov

	Abbreviations

GABA, $gamma$ -aminobutyric acid; DMCM, methyl-6,7-dimethoxy-4-ethyl- $beta$ -carboline-3-carboxylate; HEK, human embryonic kidney.

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				T.-J. Zhao, M. Li, T. H. Chiu, and H. C. Rosenberg Decreased Benzodiazepine Binding with Little Effect on gamma -Aminobutyric Acid Binding in Rat Brain After Treatment with Antisense Oligodeoxynucleotide to the gamma -Aminobutyric AcidA Receptor Gamma-2 Subunit J. Pharmacol. Exp. Ther., November 1, 1998; 287(2): 752 - 759. [Abstract] [Full Text]

[3H]RY 80: A High-Affinity, Selective Ligand for -Aminobutyric AcidA Receptors Containing Alpha-5 Subunits1,2

[³H]RY 80: A High-Affinity, Selective Ligand for $gamma$ -Aminobutyric Acid_A Receptors Containing Alpha-5 Subunits¹^,²