[35S]Guanosine-5'-O-(3-thio)triphosphate Binding as a Measure of Efficacy at Human Recombinant Dopamine D4.4 Receptors: Actions of Antiparkinsonian and Antipsychotic Agents

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Vol. 282, Issue 1, 181-191, 1997

[³⁵S]Guanosine-5 $'$ -O-(3-thio)triphosphate Binding as a Measure of Efficacy at Human Recombinant Dopamine D_4.4 Receptors: Actions of Antiparkinsonian and Antipsychotic Agents

A. Newman-Tancredi, V. Audinot, C. Chaput and L.Verrièle and M. J. Millan

Department of Psychopharmacology, Institut de Recherches Servier, 78290 Croissy-sur-Seine, France

	Abstract

Top Abstract Introduction Methods Results Discussion References

Recombinant human dopamine D_4.4 receptor-mediated G protein activation was characterized in membranes of transfected mammalian(Chinese hamster ovary) cells by the use of [³⁵S]guanosine-5 $'$ -O-(3-thio)triphosphate ([³⁵S]GTP $gamma$ S) binding. An initial series of experiments defined theconditions (3 µM GDP, 100 mM NaCl, 3 mM MgCl₂) under which optimalstimulation (2.2-fold increase in specific [³⁵S]GTP $gamma$ S binding) was achieved with the endogenous agonist dopamine.The number of dopamine-activated G proteins in Chinese hamsterovary-D_4.4 membranes was determined through [³⁵S]GTP $gamma$ S isotopic dilution saturation binding, yielding a B_maxvalue of 2.29 pmol/mg. This compared with a D_4.4 receptor B_maxvalue of 1.40 pmol/mg determined by [³H]spiperone saturation binding, indicating that 1 or 2 G proteinswere activated per D_4.4 receptor and that there were few or no"spare receptors" in this cell line. Under these conditions, theefficacy for stimulation of [³⁵S]GTP $gamma$ S binding at D_4.4 receptors of 12 dopaminergic agonistswas determined. Several antiparkinsonian drugs, including ropinirole,quinerolane and lisuride, exhibited agonist activity at D_4.4 receptors(E_max = 74.3%, 72.4% and 32.2%, respectively, compared with dopamine= 100%). The EC₅₀ values for agonist stimulation of [³⁵S]GTP $gamma$ S binding correlated well with the inhibition constantsderived from competition binding with [³H]spiperone (r = +.99). However, other antiparkinsonian drugs(bromocriptine, L-DOPA and terguride) showed low affinity and/orwere devoid of agonist activity at D_4.4 receptors. The potencyat D_4.4 receptors of the novel, selective D_4.4 receptor antagonistL 745,870 was determined, indicating that it has high affinity(K_i = 1.99 nM) without detectable agonist activity. Furthermore,L 745,870 completely inhibited dopamine-stimulated [³⁵S]GTP $gamma$ S binding with a K_b value of 1.07 nM. The actionof an additional 20 chemically diverse dopaminergic ligands, includingclozapine, ziprasidone, sertindole, olanzapine and several other"atypical" antipsychotics, in advanced development was investigated.Each of these ligands shifted the dopamine stimulation curve tothe right in a parallel manner consistent with competitive antagonismat this site and yielding K_b values (32.6, 22.4, 17.2and 26.5 nM, respectively) that agreed closely with their K_ivalues (38.0, 14.9, 18.5 and 26.1 nM). In contrast, racloprideand seroquel exhibited low affinity at D_4.4 receptors (K_i> 1000 nM). Other compounds that showed antagonist activity atD_4.4 receptors included the 5-hydroxytryptamine_2A receptor antagonistfananserin (RP 62203), the sigma ligand BMY 14,802 and the D₃receptor antagonist GR 103,691. In conclusion, dopamine D_4.4 receptoractivity is unlikely to be an important factor in the clinicaleffectiveness of antiparkinsonian drugs, although low agonistefficacy at D_4.4 receptors might be associated with a lesser incidenceof side effects. Furthermore, antagonist activity at D_4.4 receptorsis a common property of many typical and atypical antipsychoticagents.

	Introduction

Top Abstract Introduction Methods Results Discussion References

Molecular biology techniques have enabled the cloning and pharmacological characterization of multiple dopamine receptor subtypesbelonging to two families. D₁ and D₅ receptors exhibit high structuralhomology and similar pharmacological profiles (Sunahara et al.,1991). Likewise, D₂, D₃ and D₄ receptors exhibit similaritiesin both their pharmacological profiles and their coupling to Gproteins and signal transduction pathways (Levesque et al., 1992;O'Hara et al., 1996; Tang et al., 1994; Werner et al., 1996).The D₄ receptor is of particular interest for several reasons.First, in situ hybridization, autoradiographic and immunohistochemicalstudies indicate the existence of D₄-like receptor sites in limbicstructures, such as cerebral cortex and hippocampus, associatedwith regulation of mood and cognition (Lahti et al., 1995; Matsumotoet al., 1996; Meador-Woodruff et al., 1996; Mrzljak et al., 1996).In contrast, only low levels of D₄ receptors are detected in regionsassociated with control of locomotor activity, such as the striatum(Meador-Woodruff et al., 1996; Seeman et al., 1993b). Furthermore,the atypical antipsychotic clozapine, which is known to act asan antagonist at dopamine D₂ and 5-HT_2A receptors (Canton et al.,1994; Meltzer, 1996), an inverse agonist at 5-HT_2C receptors (Labrecqueet al., 1995) and a partial agonist at 5-HT_1A receptors (Newman-Tancrediet al., 1996a), also has significant affinity at dopamine D₄ receptors(Van Tol et al., 1991). This suggests that these sites may mediatesome of the therapeutic actions of atypical antipsychotics. Infact, D₄-like receptor up-regulation in postmortem schizophrenicbrain has been observed using indirect binding techniques (Murrayet al., 1995a; Seeman et al., 1993a). Second, D₄ receptors haverecently been discovered to display a "promiscuous" pharmacologicalprofile, binding epinephrine and norepinephrine with high affinity,similar to that of dopamine (Lanau et al., 1997; Newman-Tancrediet al., 1997a). Hence, D₄ receptors may play a role in integratingdopaminergic and adrenergic transmission. Furthermore, D₄ receptoractivation by norepinephrine is blocked by clozapine (Lanau etal., 1997; Newman-Tancredi et al., 1997a), suggesting that someof its clinical effects may be mediated by the antagonism of noradrenergicactivity at D₄ receptors. Indeed, it has been suggested that noradrenergicoveractivity may contribute to acute exacerbation of psychosis(Hornykiewicz, 1982; Van Kammen et al., 1990). Third, D₄ receptorsmay be implicated in the secondary action of antiparkinsoniandrugs because clozapine, which has high affinity at D₄ receptors,is effective in the treatment of L-DOPA-induced psychoses (Factoret al., 1995; Meltzer et al., 1995). In fact, although dopaminergicagonists such as bromocriptine are known to be effective in alleviatingthe symptoms of PD (Weddell and Weiser, 1995), the dopaminergicreceptor subtypes involved remain to be further defined (De Keyseret al., 1995; Jenner, 1995).

In view of the above considerations, the efficacy and potency of a range of agonists and antagonists at dopamine D₄ receptorswere investigated. Previous studies have revealed the existenceof D₄ receptor alleles, differing in the number of a 16-aminoacid repeat sequence found in the putative third intracellularloop of the receptor (Van Tol et al., 1992). However, all of thesealleles are negatively coupled to adenylyl cyclase activity (Asghariet al., 1995; McHale et al., 1994) and have similar binding andG protein interaction profiles (Asghari et al., 1994), althoughthey may differ in their sensitivity to monovalent cations (VanTol et al., 1992). Previous studies have determined the affinitiesof some dopaminergic ligands at D₄ receptors by radioligand competitionbinding (Lawson et al., 1994; Roth et al., 1995). This techniquehas yielded estimates of agonist efficacies at D_4.4 receptorsby comparing their affinities at different receptor states (Lahtiet al., 1996). Other studies have investigated the agonist/antagonistactivity at D₄ receptors of a limited number of compounds (e.g.,dopamine and quinpirole as agonists and/or clozapine and haloperidolas antagonists) by adenylyl cyclase determinations (Asghari etal., 1995; Bouvier et al., 1995; Tang et al., 1994). Hence, todate, no study of a broad range of agonist efficacies and antagonistpotencies in a functional test has been conducted. The presentstudy addressed this issue by evaluation of [³⁵S]GTP $gamma$ S binding (Chabert et al., 1994) to membranes of mammalian(CHO) cells transfected with the D_4.4 receptor (four repeat sequence),the most common allele in humans (Chang et al., 1996; Lichteret al., 1993). Agonist stimulation of [³⁵S]GTP $gamma$ S binding, a nonhydrolyzable analog of GTP, provides a measureof receptor-mediated G protein activation (Hilf et al., 1989;Lazareno et al., 1993). An initial characterization defined theexperimental conditions under which optimum agonist stimulationof [³⁵S]GTP $gamma$ S binding was observed. Previous studies in other receptorsystems (Gierschik et al., 1991; Hilf et al., 1989; Lazareno etal., 1993; Lorenzen et al., 1993) have highlighted the importanceof monovalent and divalent cations (particularly Na⁺ and Mg⁺⁺) and of GDP as being critical for modulation of agonist activationof [³⁵S]GTP $gamma$ S binding. Furthermore, given the importance of receptordensity and/or receptor reserve on functional responses, the numberof receptor-coupled G proteins activated by the endogenous agonistdopamine was determined in relation to the density of receptorspresent in the cell line. Indeed, the stoichimetric relationshipbetween receptors and G proteins can significantly affect thedefinition of agonist efficacies (Adham et al., 1993; Kenakin,1996; Newman-Tancredi et al., 1997c). The potency and efficacyfor stimulation of [³⁵S]GTP $gamma$ S binding of 12 dopaminergic agonists, including severalantiparkinsonian drugs currently in development, were determined.Finally, in view of the potential use of D₄ receptors as a targetfor antipsychotic activity, the potency of a large series of antipsychoticsfor blocking dopamine-induced [³⁵S]GTP $gamma$ S binding was determined and compared with the action ofreference dopaminergic antagonists. In addition to the neuroleptichaloperidol and the "atypical" antipsychotic clozapine, we examinedthe action of ziprasidone, olanzapine, sertindole, seroquel andother putatively atypical antipsychotics in late-stage development(Goldstein, 1995). Furthermore, the action of the novel selectiveD₄ receptor antagonist L 745,870 (Kulagowski et al., 1996), wasinvestigated.

	Methods

Top Abstract Introduction Methods Results Discussion References

[³H]Spiperone binding to CHO-D_4.4 cell membranes. Saturation binding at D_4.4 receptors was carried out with 8 concentrations of [³H]spiperone (100 Ci/mmol; Amersham, Les Ulis, France) from 0.02to 2.5 nM. For competition binding experiments, the concentrationof [³H]spiperone was 0.5 nM. Membranes (10-20 µg of protein) from transfectedCHO cells stably expressing the human dopamine D_4.4 receptor (ReceptorBiology, Baltimore, MD) were incubated with [³H]spiperone at 25°C for 60 min in a buffer containing 50 mM Tris,pH 7.4, 120 mM NaCl, 5 mM KCl, 1 mM EDTA and 5 mM MgCl₂. Nonspecificbinding was defined with haloperidol (10 µM). Affinity (inhibitionconstants, K_i) at hD_4.4 receptors was determined in [³H]spiperone competition binding experiments. Isotherms were analyzedby nonlinear regression using the program Prism (GraphPAD Software,San Diego, CA) to yield IC₅₀ values. Inhibition constants (K_i)were derived from IC₅₀ values according to the Cheng-Prusoff equation:K_i = IC₅₀/(1 + L/K_d), where L is the concentration of radioligandand K_d is the dissociation constant of [³H]spiperone at D_4.4 receptors (0.37 nM).

Isotopic dilution [³⁵S]GTP $gamma$ S saturation binding to CHO-D_4.4 cell membranes. Receptor-linked G protein activation at D_4.4 receptors was determined by measuring the stimulation of [³⁵S]GTP $gamma$ S (1332 Ci/mmol; New England Nuclear, Les Ulis, France)binding. Except where stated otherwise, CHO-D_4.4 membranes (50µg of protein) were incubated (20 min, 22°C) with agonists and/orantagonists in a buffer containing 20 mM HEPES, pH 7.4, 3 µM GDP,3 mM MgCl₂, 100 mM NaCl and 0.1 nM [³⁵S]GTP $gamma$ S. Nonspecific binding was defined with GTP $gamma$ S (10 µM). Inisotopic dilution experiments, the basal and dopamine (10 µM)-stimulatedbinding of radiolabeled [³⁵S]GTP $gamma$ S was inhibited with unlabeled GTP $gamma$ S. Two concentrationranges of GTP $gamma$ S were tested: 0 to 10 µM and 0 to 45 nM. For theformer, IC₅₀ values were derived by nonlinear regression. Forthe latter, saturation binding curves were derived to estimatethe number of G proteins activated by dopamine. The total amountof ligand bound to G protein (BOUND_TOT) was calculated by equation1: BOUND_TOT = [³⁵S]GTP $gamma$ S_BOUND× GTP $gamma$ S_TOT/[³⁵S]GTP $gamma$ S_CONC, where [³⁵S]GTP $gamma$ S_BOUND is observed dopamine-dependent binding in the tubes(fmol/mg), [³⁵S]GTP $gamma$ S_CONC is [³⁵S]GTP $gamma$ S concentration in the tubes (0.1 mM) and GTP $gamma$ S_TOT is [³⁵S]GTP $gamma$ S_CONC plus GTP $gamma$ S concentration.

Measurement of agonist efficacy and antagonist potency at D_4.4 receptors. Agonist efficacy is expressed relative to that of DA (100%), which was tested at a maximally effective concentration (10 µM)in each experiment. For antagonist tests, membranes were preincubatedwith dopamine and a single concentration of antagonist for 30min before the addition of [³⁵S]GTP $gamma$ S. For concentration-response curves of the inhibition ofdopamine-stimulated [³⁵S]GTP $gamma$ S binding, K_b values were calculated by equation 2: K_b =IC₅₀/{([agonist]/EC₅₀) + 1}, where [agonist] is agonist concentration.

For the dopamine concentration-response curves determined in the presence of a fixed concentration of antagonist, antagonistpotency values (K_b) were calculated by equation 3: K_b = [antagonist]/[(EC₅₀ $'$ /EC₅₀) $-$ 1], where [antagonist] is antagonist concentration, EC₅₀ $'$ wasdetermined in the presence of antagonist and EC₅₀ was determinedin the absence of antagonist (dopamine alone).

Experiments were terminated by rapid filtration through Whatman GF/B filters (pretreated with 0.1% polyethyleneimine in thecase of [³H]spiperone binding) using a Brandel cell harvester. Radioactivityretained on the filters was determined by liquid scintillationcounting. Protein concentration was determined colorimetricallyusing a bicinchonic acid assay kit (Sigma, S. Quentin Fallavier,France). All results are expressed as mean ± S.E.M. of three ormore independent determinations.

Compounds. Fananserin (RP 62203) was obtained from Rhone-Poulenc Rorer (Vitry-sur-Seine, France). Lisuride and terguride were from Schering(Berlin, Germany). Ocaperidone was from Janssen (Beerse, Belgium).ORG 5222 (trans-5-chloro-2-methyl-2,3,3a,12b-tetrahydro-1H-dibenz[2,3:6,7]oxepino-[4,5-c]pyrrole)was from Organon (Oss, Netherlands). Olanzapine and quinerolanewere from Eli Lilly (Indianapolis, IN). Raclopride was from Astra(Sodertalje, Sweden). Seroquel was from Zeneca (Macclesfield,UK). Sertindole was from Lundbeck (Copenhagen, Denmark). Tiaspironeand BMY 14802 (1-[4-(4-fluorophenyl)-4-hydroxybutyl]-4-(5-fluoropyrimidin-2-yl)-piperazine)was from Bristol-Myers (Wallingford, CT). (+)-7-OH-DPAT [7-hydroxy-2-(di-n-propylamino)tetralin]was from CNRS (Paris, France). dp-ADTN (5,6-dihydroxy-2-di-n-propylamino-1,2,3,4-tetrahydronaphthalene)was kindly donated by Dr. Ann Mills-Duggan (Glaxo-Wellcome, Stevenage,UK). Ropinirole, piribedil, FG 5893 (2-[4-[4,4-bis(4-fluorophenyl)butyl]-1-piperazinyl]pyridine-3-carboxylicacid), GR 103,691 (4 $'$ -acetyl-N-{4-[(2-methoxyphenyl)-piperazin-1-yl]butyl-biphenyl-4-carboxamide), risperidone, ziprasidone and L745,870 (3-(4-[4-chlorophenyl]piperazin-1-yl)methyl-1H-pyrrolo-[2,3b]pyridine)were synthesized by J.-L. Peglion and G. Lavielle (Servier). Clozapine,bromocriptine, ( $-$ )-quinpirole and spiperone were purchased fromRBI (Natick, MA). Haloperidol, ( $-$ )-apomorphine and L-DOPA werepurchased from Sigma.

	Results

Top Abstract Introduction Methods Results Discussion References

[³H]Spiperone competition binding at D_4.4 receptors. D_4.4 receptor density in CHO-D_4.4 membranes was determined by [³H]spiperone saturation binding. The isotherms were monophasic,with a dissociation constant (K_d) of 0.37 ± 0.05 nM (n = 4) anda B_max value of 1.40 ± 0.12 pmol/mg protein (4) (fig. 1). In [³H]spiperone competition binding experiments, agonist isothermswere shallow, with pseudo-Hill coefficients of <0.8 (table 1).In contrast, the antagonist competition isotherms were steeperand exhibited pseudo-Hill coefficients close to unity.

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Fig. 1. Saturation binding of [³H]spiperone to CHO-D_4.4 cell membranes. Saturation binding was carried out by incubating [³H]spiperone (0.02-2.5 nM) with CHO-D_4.4 membranes. Analysis wasby nonlinear regression using the program Prism. A, Representativesaturation binding isotherm. Points shown are mean of triplicatedeterminations from an experiment repeated on at least three occasions.B, Scatchard transformation of specific binding data from A.

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TABLE 1
Action of dopaminergic agonists at cloned human dopamine D_4.4 receptors
Affinities (K_i) at human dopamine D_4.4 receptors stably expressed in CHO cells were determined from competition bindingexperiments with [³H]spiperone. Agonist potencies (EC₅₀) and efficacies were determinedby [³⁵S]GTP $gamma$ S binding. Efficacy is expressed relative to that of dopamine(100%) that stimulated specific [³⁵S]GTP $gamma$ S binding 2.2-fold from basal values of 3950 ± 440 dpm toa maximum of 8810 ± 480 dpm. Nonspecific [³⁵S]GTP $gamma$ S binding (defined with 10 µM GTP $gamma$ S) amounted to 1030 ±130 dpm. Results are expressed as mean ± S.E.M. of at least threeindependent experiments.

Definition of [³⁵S]GTP $gamma$ S binding conditions. Dopamine (10 µM) stimulated [³⁵S]GTP $gamma$ S binding to CHO-D_4.4 membranes in a linear manner over the first 20 min (3) of time courseexperiments, and a standard incubation time of 20 min was thereforeused. In contrast, no stimulation of [³⁵S]GTP $gamma$ S binding was observed in membranes of untransfected CHOcells (results not shown). Basal (nonagonist-stimulated) bindingof [³⁵S]GTP $gamma$ S to CHO-D_4.4 membranes was dependent on the concentrationof GDP present in the buffer (fig. 2B) and was reduced from ~90,000dpm in the absence of GDP to ~4000 dpm at a GDP concentrationof 3 µM. In contrast, agonist-dependent [³⁵S]GTP $gamma$ S binding (i.e., the difference between agonist-stimulatedand basal binding) amounted to ~5000 dpm (see legend to table1) and was not decreased by GDP concentrations of $<=$ 3 µM. Thedecrease in basal binding augmented the ratio of agonist-stimulatedto basal [³⁵S]GTP $gamma$ S binding to 2.2-fold at GDP concentrations of 3 µM (fig.2B, inset). Like GDP, NaCl reduced basal [³⁵S]GTP $gamma$ S binding, from 13,000 dpm in the absence of NaCl to 4000dpm at a concentration of 100 mM (fig. 2C). However, high concentrationsof NaCl ( $>=$ 200 mM) also decreased agonist-dependent [³⁵S]GTP $gamma$ S binding. Although the latter was observed in both thepresence and absence of GDP and NaCl, it exhibited an absolutedependence on the presence of magnesium in the incubation medium(fig. 2D). Agonist stimulation of [³⁵S]GTP $gamma$ S binding was observed over a wide range of MgCl₂ concentrations,from 0.1 to 30 mM. The effect of MgCl₂ on both basal and agonist-dependent[³⁵S]GTP $gamma$ S binding was biphasic, increasing to a first maximum at~0.1 mM and then to a second, higher, maximum at 3 to 10 mM. Aset of standard experimental conditions was defined (3 µM GDP,3 mM MgCl₂, 100 mM NaCl, 20-min incubation) that yielded the highestagonist stimulation of [³⁵S]GTP $gamma$ S binding and was used in all subsequent experiments.

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Fig. 2. Effect of (A) time, (B) GDP, (C) NaCl and (D) MgCl₂ on [³⁵S]GTP $gamma$ S binding to membranes of CHO cells stably expressing clonedhuman D_4.4 receptors. Except where shown, experiments were carriedout in a buffer containing HEPES (20 mM, pH 7.4), GDP (3 µM),MgCl₂ (3 mM) and [³⁵S]GTP $gamma$ S (0.1 nM) for 20 min at 22°C. Nonspecific binding was definedwith GTP $gamma$ S (10 µM). Points shown are mean of triplicate determinationsfrom representative experiments repeated on at least three independentoccasions. DA, dopamine. $square$ , Basal [³⁵S]GTP $gamma$ S binding (no dopamine). $black-square$ , Agonist-stimulated [³⁵S]GTP $gamma$ S binding (with 10 µM dopamine). A, Specific basal and dopamine-stimulated[³⁵S]GTP $gamma$ S binding determined over time points ranging from 1 to60 min. B, Specific basal and dopamine-stimulated [³⁵S]GTP $gamma$ S binding determined in the presence of GDP concentrationsbetween 0 and 100 µM. Inset, effect of GDP concentration on agoniststimulation ratio. The stimulation ratio was calculated as specificdopamine-stimulated [³⁵S]GTP $gamma$ S binding divided by specific basal [³⁵S]GTP $gamma$ S binding. C, Specific basal and dopamine-stimulated [³⁵S]GTP $gamma$ S binding determined in the presence of concentrations ofNaCl between 0 and 200 mM. D, Specific basal and dopamine-stimulated[³⁵S]GTP $gamma$ S binding determined in the presence of concentrations ofMgCl₂ between 0 and 100 mM. Inset, effect of MgCl₂ concentrationon agonist stimulation ratio.

Isotopic dilution [³⁵S]GTP $gamma$ S saturation binding. Inhibition of basal [³⁵S]GTP $gamma$ S binding to CHO-D_4.4 membranes with GTP $gamma$ S (0.1 nM to 10 µM) exhibited a low affinity component(IC₅₀ = 110 ± 18 nM). In contrast, inhibition of dopamine (10µM)-stimulated [³⁵S]GTP $gamma$ S binding produced biphasic isotherms with IC_50(high) =4.4 ± 1.9 nM (4) and IC_50(low) = 257 ± 67 nM (4) (fig. 3A). [³⁵S]GTP $gamma$ S saturation binding isotherms were derived for the high-affinitybinding component by isotopic dilution with GTP $gamma$ S (0-45 nM; fig.3B). These yielded an apparent K_d for [³⁵S]GTP $gamma$ S binding to the high-affinity (agonist-dependent) bindingsite of 15.0 ± 4.2 nM and a B_max of 2.29 ± 0.44 pmol/mg (4) (fig.3B). The K_d value did not differ significantly from the IC_50(high)value above (P > .05, two-tailed t test).

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Fig. 3. Effect of GTP $gamma$ S on [³⁵S]GTP $gamma$ S binding to membranes of CHO stably expressing cloned human D_4.4 receptors. Experiments were carriedout in a buffer containing HEPES (20 mM, pH 7.4), GDP (3 µM),MgCl₂ (3 mM) and [³⁵S]GTP $gamma$ S (0.1 nM) for 20 min at 22°C. Representative curves areshown in which each point is the mean of duplicate determinations.Similar results were obtained in at least three independent experiments.A, Basal and dopamine (10 µM)-stimulated [³⁵S]GTP $gamma$ S binding determined in the presence of concentrations ofGTP $gamma$ S between 0 and 10 µM. B, Basal and dopamine (10 µM)-stimulated[³⁵S]GTP $gamma$ S binding determined in the presence of concentrations ofGTP $gamma$ S between 0 and 45 nM. These data were transformed as describedin the text to generate a saturation binding isotherm for agonist-dependent[³⁵S]GTP $gamma$ S binding. Inset, Scatchard plot of the saturation bindingisotherm.

Agonist and antagonist action at D_4.4 receptors. The EC₅₀ values for stimulation of [³⁵S]GTP $gamma$ S binding by agonists, including the antiparkinsonian drugs quinerolane, ( $-$ )-apomorphine,(+)7-OH-DPAT and lisuride, correlated (r = .99, P < .01) withtheir binding affinity (K_i; table 1; see fig. 5B). In contrast,other clinically used antiparkinsonian drugs (e.g., bromocriptine,piribedil) had low affinity and/or efficacy at D_4.4 receptors.None of the compounds, other than dopamine, acted as full agonistsfor stimulation of [³⁵S]GTP $gamma$ S binding.

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Fig. 5. Agonism and antagonism at cloned human D_4.4 receptors defined by [³⁵S]GTP $gamma$ S binding. Experiments were carried out in a buffer containingHEPES (20 mM, pH 7.4), GDP (3 µM), MgCl₂ (3 mM) and [³⁵S]GTP $gamma$ S (0.1 nM) for 20 min at 22°C. Nonspecific binding was definedwith GTP $gamma$ S (10 µM). Points shown are mean of triplicate determinationsfrom representative experiments repeated on at least three independentoccasions. [³⁵S]GTP $gamma$ S binding is expressed as a percentage of the maximal stimulationgiven by dopamine. A, Agonist concentration-response curves. B,Correlation of minus log EC₅₀ values (pEC₅₀) for agonist stimulationof [³⁵S]GTP $gamma$ S binding with minus log K_i values (pK_i;table 1) for inhibition of [³H]spiperone binding. The correlation coefficient was .99 (P <.001). C, Shift of dopamine concentration-response [³⁵S]GTP $gamma$ S binding curve in the presence of fixed concentrationsof antagonists (table 2). D, Correlation of minus log K_bvalues (pK_b) for antagonist potency with minus log K_ivalues (pK_i, table 2) for inhibition of [³H]spiperone binding. The correlation coefficient was .99 (P <.001). The point corresponding to FG 5893 was not included inthe calculation of the correlation.

The antagonist activity of a range of dopaminergic ligands was tested, including the novel, selective D₄ receptor ligand L745,870 (K_i = 1.99 nM). Like spiperone, haloperidol and clozapine,L 745,870 concentration-dependently and completely blocked thestimulation of [³⁵S]GTP $gamma$ S binding induced by 1 µM dopamine (K_b = 1.07 nM; fig. 4and table 2). L 745,870 (100 nM) also shifted the dopamine concentration-responsecurve to the right, with an 89-fold increase in EC₅₀ (8910 ± 1250nM), yielding a K_b value of 1.19 nM (table 3 and fig. 5C). Othercompounds that showed antagonist activity were the dopamine D₃receptor ligand GR 103,691, the serotonin 5-HT_2A receptor antagonistfananserin (RP 62,203), the sigma ligand BMY 14,802 and the antiparkinsoniandrug terguride.

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Fig. 4. Competition binding and antagonism at cloned human D_4.4 receptors by dopaminergic antagonists. A, Representative [³H]spiperone competition binding isotherms. B, Antagonism of dopamine(1 µM)-stimulated [³⁵S]GTP $gamma$ S binding. Points shown are mean of triplicate determinationsfrom representative experiments repeated on at least three occasions.

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TABLE 2
Antagonism of dopamine-stimulated [³⁵S]GTP $gamma$ S binding to CHO-D_4.4 membranes
Antagonist potencies (K_b) were calculated from IC₅₀ values for the inhibition of dopamine (1 µM)-stimulated [³⁵S]GTP $gamma$ S binding. Results are expressed as mean ± S.E.M. of atleast three independent experiments.

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TABLE 3
Action of dopaminergic antagonists at cloned human D_4.4 receptors
Affinities (K_i) at human dopamine D_4.4 receptors stably expressed in CHO cells were determined from competition bindingexperiments with [³H]spiperone. Antagonist potencies (K_b) were determinedby the shift in the dopamine stimulation curve of [³⁵S]GTP $gamma$ S binding to a higher concentration (EC₅₀ $'$ ) in the presenceof a fixed concentration of antagonist. Dopamine alone yieldedan EC₅₀ of 100.6 ± 13.7 nM (table 1). Results are expressed asmean ± S.E.M. of at least three independent experiments.

The effect on [³⁵S]GTP $gamma$ S binding of a range of antipsychotics was tested, including clozapine, olanzapine, risperidone and ziprasidone,none of which altered [³⁵S]GTP $gamma$ S binding from basal levels when tested alone. However,fixed concentrations of antagonist shifted the dopamine concentration-responsecurve to the right in a parallel manner, consistent with competitiveantagonism at D_4.4 receptors (table 3). For all the compoundstested, the K_b values calculated from these shifts agreed closelywith their respective K_i values (r = .99, P < .01; fig. 5D), exceptFG 5893, which showed a 6-fold lower K_b value than K_i value (P< .05, table 3) and was not included in the calculation of correlationcoefficient.

	Discussion

Top Abstract Introduction Methods Results Discussion References

Effects of GDP, NaCl and MgCl₂ on [³⁵S]GTP $gamma$ S binding to CHO-D_4.4 membranes. [³⁵S]GTP $gamma$ S binding affords a measure of receptor-mediated G protein activation (the first step of the signal transduction pathway)and is applicable regardless of the second-messenger system(s)involved. In CHO-D_4.4 cell membranes, [³⁵S]GTP $gamma$ S binding was modulated by buffer concentrations of GDP.The latter reduced the level of basal (non-agonist-stimulated)binding, without affecting agonist-dependent binding. Hence, asGDP concentration increased, the ratio of agonist-stimulated tobasal [³⁵S]GTP $gamma$ S binding increased to 2.2-fold at a GDP concentration of3 µM (fig. 2B, inset). This compares with stimulation ratios of1.4-, 2.2-, 2.5- and 3-fold for 5-HT_1D, 5-HT_1D, muscarinicand 5-HT_1A receptors, respectively (Hilf et al., 1989; Newman-Tancrediet al., 1996b; Thomas et al., 1995). Like GDP, NaCl reduced basalbinding of [³⁵S]GTP $gamma$ S but reduced dopamine-stimulated binding only at concentrationsof >100 mM. Similar data have been reported for agonist stimulationof [³⁵S]GTP $gamma$ S binding at alpha-2 adrenoceptors (Tian et al., 1994).

[³⁵S]GTP $gamma$ S binding to CHO-D_4.4 membranes has an absolute requirement for magnesium, similar to that observed for A₁ adenosinereceptors (Lorenzen et al., 1993

). In the present study, the modulatoryeffects of magnesium were complex, exhibiting a biphasic actionon agonist-dependent [³⁵S]GTP $gamma$ S binding (fig. 2D). The [³⁵S]GTP $gamma$ S binding peak at a MgCl₂ concentration of 3 to 10 mM probablyreflects conditions that favor the formation of a ternary complexof agonist/receptor/G protein. In contrast, agonist stimulationof [³⁵S]GTP $gamma$ S binding at a MgCl₂ concentration of 0.1 mM is low, becausethese conditions may be less favorable for the formation of theternary complex. However, MgCl₂ also had a biphasic effect onbasal [³⁵S]GTP $gamma$ S binding, suggesting that Mg⁺⁺ ions may have modulatory effects on G proteins themselves. Thesemay reflect altered levels of G protein attachment to cell membranes.For example, transducin solubility increases at Mg⁺⁺ concentrations of <0.1 mM (Bornancin et al., 1989

), suggestingthat the association of G proteins to membrane-bound receptorswould be favored by higher Mg⁺⁺ concentrations. Although the exact mechanistic basis for thebiphasic action of magnesium is unclear, the present observationsagree with similar biphasic effects reported for muscarinic acetylcholinereceptors (Hilf et al., 1989

) and fMet-Leu-Phe (fMet) chemotacticreceptors (Gierschik et al., 1991). For subsequent experiments,a magnesium concentration of 3 mM was selected, providing thehighest ratio of dopamine-stimulated over basal [³⁵S]GTP $gamma$ S binding (fig. 2D).

The buffer composition chosen was similar to that of Chabert et al. (1994)

for [³⁵S]GTP $gamma$ S binding to D_4.4 -transfected Sf9 insect cells and forthe other receptors mentioned above. This suggests that bufferconditions that yield optimal agonist stimulation of [³⁵S]GTP $gamma$ S binding may be similar for many receptor and cell types.Furthermore, the present data show that there is no necessityfor agonist to be present for G protein activation to occur. Rather,G protein activation can be induced, in the absence of agonist,by selecting conditions that favor coupling of G protein to receptor(millimolar magnesium, low sodium and low GDP). These factorsdo not, however, appear to influence the ability of dopamine tofurther stimulate [³⁵S]GTP $gamma$ S binding, suggesting that an active receptor conformationis induced by agonists that is not achieved by merely manipulatingbuffer conditions. Thus, basal and agonist-stimulated [³⁵S]GTP $gamma$ S binding may reflect different activation states of theD_4.4 receptor. In addition, the presence of a basal level of receptor-mediatedG protein activation enables, in principle, the identificationof compounds that inhibit G protein activation (inverse agonists).Xanthine amine congener, for example, lowers basal G protein activationat A₁ adenosine receptors (Freissmuth et al., 1991

), whereas methiothepinand ketanserin inhibit [³⁵S]GTP $gamma$ S binding to membranes of CHO cells stably expressing 5-HT_1Dand 5-HT_1D receptors (Thomas et al., 1995

). In the presentsystem, however, the level of basal [³⁵S]GTP $gamma$ S binding was minimized to facilitate the definition ofagonist effects. Hence, reduction of basal binding by inverseagonists, may be relatively small. Furthermore, the ability todetect inverse agonist activity may depend on the presence ofa high receptor to G protein ratio. Indeed, in a CHO cell linemanipulated to express a high level of 5-HT_1A receptors (withouta change in G protein number), the inverse agonist spiperone exhibitedincreased negative efficacy (Newman-Tancredi et al., 1997b

, 1997c

Determination of G protein number in CHO-D_4.4 membranes by [³⁵S]GTP $gamma$ S isotopic dilution. Unlabeled GTP $gamma$ S inhibited basal [³⁵S]GTP $gamma$ S binding to CHO-D_4.4 monophasically and with low affinity [IC_50(low) = 110 nM]. Incontrast, GTP $gamma$ S inhibited agonist-stimulated [³⁵S]GTP $gamma$ S binding biphasically, with an additional high-affinitysite [IC_50(high) = 4.4 nM] as well as a low-affinity binding component.Two points should be made regarding these data. First, the IC₅₀values are a function of the GDP concentration in the assays,because GTP $gamma$ S in effect competes with GDP for binding to G proteins.Second, whereas the low-affinity binding component reflects inhibitionof the endogenous GDP/GTP exchange rate of all CHO-D_4.4 G proteins,the high-affinity binding component reflects only inhibition ofagonist-stimulated GDP/GTP exchange at D_4.4 receptor-linked Gproteins (fig. 3A; Tian et al., 1994). The K_d value for this high-affinitycomponent (15 ± 4.2 nM) was not significantly different from theIC_50(high) above, but serotonin-activated recombinant human 5-HT_1Areceptors, also expressed in CHO cells, display a K_d value for[³⁵S]-GTP $gamma$ S of only 1.29 ± 0.13 nM (Newman-Tancredi et al., 1977cP < .01, two-tailed t test, compared with the K_d value for D_4.4receptors). This suggests that D_4.4 and 5-HT_1A receptors may differentlyactivate G proteins in the same host cell line. In fact, CHO-K1cells express G_i₂ and G_i₃, both of which can coupleto 5-HT_1A receptors (Raymond et al., 1993), whereas D_4.4 receptorcoupling to G_i₂ may be a cell-dependent property becauseit is observed in mouse fibroblast CCL1.3 cells but not MN9D mesencephaliccells (Tang et al., 1994). Additional studies are therefore requiredto determine which G protein subtype or subtypes are activatedby D₄ receptors in CHO cells.

Information regarding the receptor/G protein stoichiometry in CHO-D_4.4 cells can be obtained from the B_max values for dopamine-stimulated[³⁵S]GTP $gamma$ S binding in CHO-D_4.4 cells (2.29 pmol/mg) and the B_maxvalue for D_4.4 receptor expression (1.40 pmol/mg). These dataindicate that 1 or 2 dopamine-activated G proteins are labeledin CHO-D_4.4 membranes per D_4.4 receptor. This is similar to thatseen for atrial natriuretic factor receptors (1 G protein/receptor;Khurana and Pandey, 1995

) and for mu opioid receptors (2 G proteins/receptor;Traynor and Nahorski, 1995

). However, much higher degrees of amplificationhave been observed for fMet chemotactic receptors (20 G proteins/receptor;Gierschik et al., 1991) and for human cardiac muscarinic acetylcholinereceptors (50-80 G proteins/receptor; Böhm et al., 1994). Furtherinvestigation is required to elucidate the origin of these widelyvarying ratios, but they may be a function of the rapidity ofcycling between different receptor subtypes and their respectiveG proteins. Indeed, in a comparative study in rat striatal membranes,mu and sigma opioid receptors activated 20 G proteins/receptor,whereas cannabinoid receptors only activated 3 G proteins/receptor(Sim et al., 1996

Agonist stimulation of [³⁵S]GTP $gamma$ S binding to CHO-D_4.4 membranes. The action at D_4.4 receptors of 12 dopaminergic agonists was characterized. Their EC₅₀ values for activation of [³⁵S]GTP $gamma$ S binding correlated closely with the K_i values obtainedfor inhibition of [³H]spiperone binding, and their order of potency agrees with thatpreviously reported for D₄ receptors (Chabert et al., 1994; Tanget al., 1994; Van Tol et al., 1991). In the case of agonist competitionbinding isotherms, the presence of more than one receptor affinitystate was suggested by the low (<.8) pseudo-Hill coefficients(table 1), probably reflecting ligand binding to G protein-coupledand -uncoupled forms of the receptor.

In measurements of [³⁵S]GTP $gamma$ S binding, all the agonists exhibited efficacies (relative to dopamine) of markedly <100%, withthe highest (~74%) observed with ropinirole and quinerolane. Incontrast to the present data, Lahti et al. (1996)

reported thatthe efficacy of ( $-$ )-apomorphine at D_4.4 receptors, estimated bythe ratio of ligand affinities for G protein-coupled and -uncoupledreceptor states, was about double (80%) that seen here ( $approx$ 40%;table 1). Similarly, Chabert et al. (1994)

found that ( $-$ )-apomorphineexhibited an efficacy of 85%, whereas two further partial agoniststested here (dp-ADTN and ( $-$ )-quinpirole) were full agonists atD_4.4 receptors expressed in insect Sf9 cells. At least two possibilitiesmay account for these differences. First, although buffer conditionswere similar, the incubation temperature in the present studywas lower (22°C) than that used by Chabert et al. (1994)

(30°C).A temperature rise may augment the apparent efficacy of partialagonists through thermodynamic facilitation of GDP release fromG proteins (Lorenzen et al., 1996

). However, in control experimentsincubated at 30°C, the efficacy of ( $-$ )-apomorphine was increasedby only 5% to 10%,¹ which is insufficient to account for the 45% difference in efficacies.Second, the D_4.4 receptor B_max value in the CHO cells used here(1.40 pmol/mg) was 4-fold lower than that in the Sf9 cells usedby Mills et al. (1993)

(5-6 pmol/mg). This suggests that apparentagonist efficacies in Sf9 cells may be higher due to the presenceof "spare" receptors. Indeed, a high ratio of receptor to G proteinin Sf9 cells would be expected to increase agonist efficacy, ashas been shown for weak partial agonists such as pindolol at 5-HT_1Breceptors and eltoprazine at 5-HT_1A receptors (Adham et al., 1993

;Newman-Tancredi et al., 1997c

The agonists tested in the present study include several compounds that are in development for the treatment of PD, such asquinerolane, bromocriptine and ropinirole. Dopaminergic agonistsare known to alleviate the symptoms of PD (De Keyser et al., 1995

;Wolters et al., 1995

), but their exact mechanism of action isunclear, and may involve multiple dopamine receptor subtypes (Jenner,1995

). Quinerolane, ( $-$ )-apomorphine and lisuride displayed highaffinity for D_4.4 receptors, but bromocriptine and piribedil displayedlow or negligible affinity at this site. Furthermore, althoughquinerolane was an efficacious agonist (E_max = 72.4%), lisuridehad only weak partial agonist activity (E_max = 32.2%), and tergurideis an antagonist at D_4.4 receptors (see tables 1 and 2). Itis concluded that no correlation exists between the antiparkinsonianeffects of these drugs and their activity at D_4.4 receptors. However,given that dopaminergic agonists can have propsychotic actions(Factor et al., 1995

) and the possible importance of D_4.4 receptorsin mediating mood dysfunctions, an antiparkinsonian drug withantagonist activity at D_4.4 , such as the ergot terguride (trans-dihydrolisuride),may present a therapeutic advantage. Indeed, terguride attenuatesparkinsonian symptoms in 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine-lesionedmonkeys and suppresses hyperactivity induced by apomorphine treatment(Akai et al., 1993

), whereas in clinical trials, terguride waseffective against PD with only a low incidence of psychotic sideeffects (Filipova et al., 1988

). Thus, it may be hypothesizedthat antiparkinsonian drugs with low efficacy at D_4.4 receptorsmay induce less-pronounced psychotic side effects. This is consistentwith the observed effectiveness of clozapine, which has significantaffinity and antagonist activity at D₄ receptors, in counteringL-DOPA-induced psychosis in PD patients (Factor et al., 1995

;Meltzer et al., 1995

Antagonism of dopamine-stimulated [³⁵S]GTP $gamma$ S binding to CHO-D_4.4 membranes. In agreement with previous reports, clozapine showed marked affinity (K_i = 38 nM) at D_4.4 receptors (table 3). This indicatesthat in our hands, clozapine is ~2-fold selective for D_4.4 comparedwith D₂ receptors (K_i = 76 nM) (Millan et al., 1995), althoughusing different radioligands and experimental conditions, otherauthors have reported selectivities of $<=$ 17-fold (Durcan et al.,1995; Lawson et al., 1994; Van Tol et al., 1991). In contrast,the novel D₄ receptor antagonist L 745,870 has negligible affinityat D₂ receptors (K_i = 890 nM)² but high affinity at D_4.4 receptors. Its K_i value (1.99 nM) isin the same range as that (0.4 nM) reported by Kulagowski et al.(1996). Although it has no effect alone, L 745,870 completelyantagonized dopamine-stimulated [³⁵S]GTP $gamma$ S binding (fig. 4B), with a K_b value of 1.07 nM, and shiftedthe dopamine concentration-response curve to the right with aK_b value of 1.19 nM (table 2), confirming its high potency atD_4.4 receptors.

The present study tested the antagonist activity and/or affinity of 19 other dopaminergic ligands at D_4.4 receptors, includingseveral antipsychotics in late-stage development. Olanzapine,which was designed to exhibit a similar receptorial profile tothat of clozapine (which is also a dibenzazepine derivative),displayed a similar affinity at D_4.4 receptors (K_i = 26.1 nM).However, other dibenzazepine derivatives, ORG 5222 and seroquel,displayed widely differing affinities at this site (K_i = 0.78and 2290 nM, respectively). In fact, seroquel has generally lowaffinity at a range of receptors, including dopamine D₁, D₂ andD₃ (pK_i = 5.4, 6.2 and 6.5, respectively; Schotte et al., 1996

).All the butyrophenone compounds tested (spiperone, haloperidol,ocaperidone, risperidone and ziprasidone) showed marked affinityat D_4.4 receptors, as did the arylpiperazines tiaspirone and FG5893. Interestingly, BMY 14,802 (another arylpiperazine), originallydescribed as a selective sigma-site ligand (Taylor and Dekleva,1987

), had significant affinity at D_4.4 receptors (K_i = 24.5 nM),whereas other sigma ligands, DUP 734 and rimcazole, did not (K_i> 1000 nM). Similarly, fananserin (RP 62203), originally presentedas a selective 5-HT_2A antagonist (Doble et al., 1992

), has highaffinity at D_4.4 receptors (K_i = 4.99 nM). This result agreeswith Heuillet et al. (1996)

, who reported a K_i value of 2.9 nMat CHO-D_4.2 receptors. Ligands selective for D₁ (SCH 23,390) andD₂/D₃ receptors (raclopride) showed low affinity, but the D₃ receptorantagonist GR 103,691 exhibited moderate affinity at D_4.4 receptors(K_i = 83.6 nM), which is in agreement with previous reports (63nM) (Murray et al., 1995b

Previous studies have shown the antagonist activity of clozapine and haloperidol at D₄ receptors (Asghari et al., 1995

; Chabertet al., 1994

). The present study confirms these findings and characterized19 other compounds, showing that K_b values corresponded closelyto respective K_i values (r = .99, fig. 4D). In contrast, Asghariet al. (1995)

found, surprisingly, that clozapine and haloperidolwere equipotent for antagonism of dopamine-inhibited adenylylcyclase activity, and Chabert et al. (1994)

reported pA₂ valuesfor clozapine and haloperidol 1 order of magnitude lower thanthe K_b values here. These discrepancies may be due to the differentcell lines used, the different receptor expression levels or thedifferent functional test adopted ([³⁵S]GTP $gamma$ S binding or adenylyl cyclase). Nevertheless, the presentdata demonstrate the ability of all the antipsychotics testedto shift the dopamine stimulation curve to the right in a parallelmanner, which is consistent with competitive antagonism at D₄receptors. The K_b values of spiperone, L 745,870, haloperidoland clozapine calculated for inhibition of dopamine-stimulated[³⁵S]GTP $gamma$ S binding agreed closely with those calculated for the shiftin the dopamine concentration-response curves (tables 2 and 3).None of the drugs tested, including L 745,870, terguride and clozapine,exhibited any intrinsic agonist activity. This indicates thatthey act as "neutral" or "silent" antagonists in this system,although experiments in a cell line with a high receptor expressionlevel might reveal weak agonist activity (Newman-Tancredi et al.,1997c

). Taken together, the present data found no distinctionin (lack of) intrinsic activity at D_4.4 receptors between typicalantipsychotics such as haloperidol and atypical antipsychoticssuch as clozapine, risperidone and olanzapine.

The physiological significance of D₄ receptors is unclear, but the controversial up-regulation of D₄-like receptors in postmortemschizophrenic brain tissue (Murray et al., 1995

;//Reynolds, 1996

;Seeman et al., 1993a

) suggests that an interaction at these sitesmay be involved in the etiology of the disease. However, the benzamideantipsychotic raclopride, which is effective in countering productiveschizophrenic symptoms, has low affinity at D_4.4 receptors (table3), whereas the potent and selective D₄ receptor antagonist L745,870 is ineffective in treating acutely psychotic patients(Kramer et al., 1996

). Nevertheless, raclopride induces a highincidence of extrapyramidal symptoms and poorly treats negativeschizophrenic symptoms, whereas L 745,870 did not induce extrapyramidalsymptoms, and its therapeutic interest in treating negative andcognitive symptoms is as yet unknown. These observations, togetherwith the known distribution of D₄-like receptors in frontal cortexand hippocampus and on GABAergic neurons (Matsumoto et al., 1996

;Meador-Woodruff et al., 1996

; Mrzljak et al., 1996

), suggest thatthe functional significance of D₄ receptors may be related todeficit symptoms, cognitive dysfunction or anxiodepressive states.Indeed, the D₄ receptor antagonist (and antiparkinsonian drug)terguride significantly attenuated negative, but not positive,schizophrenic symptoms in clinical trials (Olbrich and Schanz,1988

, 1991

Conclusions. [³⁵S]GTP $gamma$ S binding methodology has been applied to recombinant human dopamine D_4.4 receptors expressed in a mammalian (CHO)cell line. In this system, high experimental concentrations ofGDP (3 µM), NaCl (100 mM) and MgCl₂ (3 mM) are necessary to obtainoptimum ratios of agonist-induced over basal [³⁵S]GTP $gamma$ S binding. CHO-D_4.4 cells display a high ratio of dopamine-activatedG proteins to receptors, indicating the absence of spare receptorsand enabling partial agonist activity to be defined. A range ofantiparkinsonian drugs exhibited widely varying affinities andefficacies at D_4.4 receptors, suggesting that activity at thissite is not an important factor in their clinical effectiveness,although D_4.4 receptor agonism may be associated with side effectson mood. In contrast, a range of neuroleptic and atypical antipsychoticsantagonized the dopamine-induced stimulation of [³⁵S]GTP $gamma$ S binding, suggesting that D₄ receptor antagonism may bea potentially clinically important feature of many antipsychoticdrugs.

	Acknowledgments

We thank Paul Chazot, Chris Breivogel, Frederic Bornancin and Ann Mills-Duggan for helpful discussions.

	Footnotes

Accepted for publication March 17, 1997.

Received for publication September 23, 1996.

¹ A. Newman-Tancredi and C. Chaput, unpublished observations.

² A. Newman-Tancredi and C. Chaput, unpublished observations.

Send reprint requests to: Dr. Adrian Newman-Tancredi, Department of Psychopharmacology, Institut de Recherches Servier, 125, Chemin de Ronde, 78290 Croissy-sur-Seine (Paris), France. E-mail: 101511,274{at}compuserve.com

	Abbreviations

5-HT, 5-hydroxytryptamine; CHO, Chinese hamster ovary; CHO-D_4.4 , Chinese hamster ovary cells expressing dopamine D_4.4 receptors, GTP $gamma$ S, guanosine-5 $'$ -O-(3-thio)triphosphate; PD, Parkinson's disease; HEPES, 4-(2-hydroxyethyl)-1-piperazineethanesulfonic acid.

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