Metabotropic Glutamate Receptors in the Rat Nucleus Accumbens Contribute to Amphetamine-Induced Locomotion

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Vol. 284, Issue 1, 317-322, 1998

Metabotropic Glutamate Receptors in the Rat Nucleus Accumbens Contribute to Amphetamine-Induced Locomotion¹

Jeong-Hoon Kim and Paul Vezina

Department of Psychiatry, The University of Chicago, Chicago, Illinois

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

This study examined the role played by metabotropic glutamate receptors in the nucleus accumbens in dopamine agonist-inducedlocomotion. Rats received microinjections into this nucleus ofthe selective metabotropic glutamate receptor antagonist, (RS)- $alpha$ -methyl-4-carboxyphenylglycine,alone or with amphetamine and their locomotor activity was subsequentlymeasured for 2 hr. None of the doses of (RS)- $alpha$ -methyl-4-carboxyphenylglycinetested (0.025, 0.25, 2.5, or 25 nmol/0.5 µl/side) when administeredalone produced effects on locomotion that differed significantlyfrom those observed after saline. However, when co-injected withamphetamine (6.8 nmol [2.5 µg]/side) into the nucleus accumbens,a moderately high dose of (RS)- $alpha$ -methyl-4-carboxyphenylglycine(25 nmol/side) completely blocked, whereas a lower dose (0.25nmol/side) potentiated the locomotor effects of amphetamine. (RS)- $alpha$ -Methyl-4-carboxyphenylglycine(25 nmol/side) also blocked the locomotor-activating effects ofapomorphine (32.9 nmol [10 µg]/side), when co-injected with thisdirect dopamine receptor agonist into the nucleus accumbens. Theseresults suggest that metabotropic glutamate receptors in the nucleusaccumbens contribute to amphetamine-induced locomotion and thatthis contribution may be mediated, at least in part, by metabotropicglutamate receptors expressed by intrinsic nucleus accumbens cellslocated postsynaptic to dopamine neuron terminals.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

In the rat, low doses of amphetamine produce increases in locomotor activity when administered acutely by systemic injection.Considerable evidence now indicates that this effect is mediatedby actions of this drug on mesolimbic dopaminergic neurotransmission.Thus, the locomotor activation produced by amphetamine is associatedwith an increase in extracellular levels of DA in the NAcc, whichreceives dense axonal projections from mesolimbic DA neurons (Clarkeet al., 1988; Kuczenski and Segal, 1989; Meredith et al., 1993).AMPH injections into the NAcc increase locomotion, whereas injectionsof DA receptor antagonists into the NAcc and lesions of DA nerveterminals in this region block amphetamine-induced locomotion(Roberts et al., 1975; Kelly and Iversen, 1976; Joyce and Koob,1981; Vezina et al., 1991).

Glutamatergic projections to the NAcc originating from prefrontal cortex, hippocampus and amygdala (Christie et al., 1987;Meredith et al., 1993) also regulate locomotor activity by interactingwith dopaminergic neurotransmission. Anatomical studies of theNAcc provide the basis for a possible interaction between DA andglutamate at the level of nerve terminals in this site (Sesackand Pickel, 1990, 1992). Consistent with the results of thesestudies, it has been shown that agonists of iGluRs, includingAMPA and NMDA, increase extracellular levels of DA and locomotoractivity when infused into the NAcc and these effects are inhibitedby drugs that interfere with dopaminergic neurotransmission (Donzantiand Uretsky, 1983; Boldry and Uretsky, 1988; Imperato et al.,1990; Youngren et al., 1993). Furthermore, the application ofglutamate receptor antagonists to the NAcc attenuates the locomotoreffects of psychomotor-stimulant drugs. For example, it has beenshown that the infusion of AMPA/kainate glutamate receptor antagonistsinto the NAcc reduces the increases in locomotor activity andin the levels of extracellular DA in this site produced by eitherAMPH or cocaine (Pulvirenti et al., 1989; Willins et al., 1992;Kaddis et al., 1993; Pap and Bradberry, 1995). NMDA receptor antagonistshave also been reported to decrease such psychomotor stimulant-inducedeffects (Pulvirenti et al., 1991; Kelley and Throne, 1992; Burnset al., 1994; Moghaddam and Bolinao, 1994). These results suggestthat increases in glutamatergic neurotransmission as well as indopaminergic neurotransmission contribute to AMPH-induced locomotion.

The NAcc expresses high amounts of mGluRs (Albin et al., 1992; Shigemoto et al., 1992; Testa et al., 1994; Romano et al.,1995). The mGluRs represent a large family of G protein-coupledreceptors that activate multiple second messenger systems leadingto various signal transduction processes (Nakanishi, 1994). Therecent development of mGluR-selective ligands (Eaton et al., 1993;Birse et al., 1993; Hayashi et al., 1994) has introduced importantroles for mGluRs in the modulation of voltage- and ligand-gatedion channels, the induction of long-term changes in synaptic strengthand in spatial and olfactory memory formation (Schoepp and Conn,1993; Pin and Bockaert, 1995; Pin and Duvoisin, 1995; Miller etal., 1995). It has also been shown that the local applicationof the selective mGluR agonist, (1S,3R)-ACPD, to the NAcc canmodulate extracellular levels of DA in this site (Ohno and Watanabe,1995; Taber and Fibiger, 1995) and increase locomotor activityin a DA-dependent manner (Kim and Vezina, 1997). These resultsprovide evidence for functional interactions between mGluRs andDA terminals in the NAcc. However, whereas the contribution ofNAcc iGluRs to AMPH-induced locomotion is well established, therehave been no studies of the potential role of NAcc mGluRs in themediation of such an effect. The present experiment, therefore,used the selective mGluR antagonist, MCPG, to investigate thecontribution of this receptor to the locomotor effects producedby acute injections of AMPH into the NAcc.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Subjects and surgery. Male Sprague-Dawley rats weighing 250 to 275 g on arrival from Harlan Sprague-Dawley (Madison, WI) were used. They were housedindividually in a 12-hr light/dark reverse cycle room, with foodand water available at all times. Four to seven days after arrival,rats were anesthetized with ketamine (1 mg/kg i.p.) followed byxylazine (0.3 mg/kg i.p.) and placed in a stereotaxic instrumentwith the incisor bar at 5.0 mm above the interaural line (Pellegrinoet al., 1979). They were then implanted with chronic bilateralguide cannulae (22 gauge, Plastics One, Roanoke, VA) aimed atthe NAcc (A/P, +3.4; L, ±1.5; D/V, $-$ 7.5 from bregma and skull).Cannulae were angled at 10° to the vertical and positioned 1 mmabove the final injection site. All cannulae were secured withdental acrylic cement anchored to stainless steel screws fixedto the skull. After surgery, 28 gauge obturators were insertedto a depth 1 mm below the guide cannula tips and rats were returnedto their home cages for a 10-day recovery period. All proceduresinvolving animals were conducted according to an approved InstitutionalAnimal Care and Use Committee protocol.

Drugs. D-Amphetamine sulfate (National Institute on Drug Abuse, Rockville, MD) was dissolved in sterile 0.9% saline. (RS)-MCPG (TocrisCookson, St. Louis, MO) was dissolved in equimolar NaOH (0.1 N;Fisher Scientific, Fair Lawn, NJ) and small aliquots were storedat $-$ 80°C. Immediately before use, frozen aliquots of the drugswere diluted in sterile 0.9% saline. They were prepared eitherseparately or as a cocktail. R( $-$ )-Apomorphine hydrochloride (ResearchBiochemicals Internationals, Natick, MA) was dissolved eitherin oxygen-free boiled water or in 50 mM (RS)-MCPG solution.

Intracranial microinjection. Bilateral intracranial microinjections into the NAcc were made in the freely moving rat. Injection cannulae (28 gauge) connectedto 1-µl syringes (Hamilton, Reno, NV) via PE-20 tubing were insertedto a depth 1 mm below the guide cannula tips. Injections weremade in a volume of 0.5 µl/side during 30 sec. Sixty seconds later,the injection cannulae were withdrawn, the obturators replacedand the rat placed immediately in an activity box.

Locomotor activity. A bank of 12 activity boxes was used to measure locomotor activity. Each box (22 × 43 × 33 cm) was constructed of opaque plastic(rear and two side walls), a Plexiglas front-hinged door and atubular stainless steel ceiling and floor. Two photocells, positioned3.5 cm above the floor and spaced evenly along the longitudinalaxis of each box, estimated horizontal locomotion. Two additionalphotocells, positioned on the side walls 16.5 cm above the floorand 5 cm from the front and back walls, estimated rearing. Separateinterruptions of photocell beams were detected and recorded viaan electrical interface by a computer situated in an adjacentroom. The activity boxes were kept in a room lighted dimly withred light.

Design and procedure. In all experiments, rats were injected and tested only during their dark cycle (between 10:00 A.M. and 6:00 P.M.). Brief exposureto light was unavoidable during transport from the housing tothe testing room and at the time of injection. Rats were randomlyassigned to five different groups. On each of two occasions, ratsin each group were administered a bilateral microinjection intothe NAcc of one of five doses of (RS)-MCPG (0, 0.025, 0.25, 2.5and 25 nmol/side). On one occasion, these microinjections weremade alone with saline. On the other, they were made in a cocktailwith AMPH (6.8 nmol [2.5 µg]/side). The two microinjections wereseparated by 3 days, and their order (MCPG alone or in cocktailwith AMPH) was counterbalanced in all groups. Individual ratswere administered only one dose of the mGluR antagonist. Immediatelyafter the microinjections, rats were placed in activity boxes,and their locomotor activity was measured for 2 hr. Additionalgroups of rats were tested to assess the possible contributionof mGluRs to postsynaptic components of DA neurotransmission.Three different groups of rats received either saline (0.5 µl/side),apomorphine (32.9 nmol [10 µg]/side) or a cocktail of apomorphine(32.9 nmol/side) plus (RS)-MCPG (25 nmol/side). Rats were placedin the activity boxes immediately after injection and their locomotionwas measured for 2 hr. The behavior of some rats was simultaneouslyfilmed with a closed-circuit video system to permit the subsequentobservation and recording of stereotyped, seizure-like (e.g.,motor convulsions, foreleg clonus, wet dog shakes and hyper salivation;see Burns et al., 1994) and other behaviors not detected by photobeaminterruptions.

Histology. After completion of the experiments, the rats were anesthetized and perfused via intracardiac infusion of saline and 10% formalin.Brains were removed and postfixed further in 10% formalin for3 to 5 days. Coronal sections (40 µm) were subsequently stainedwith cresyl violet for verification of cannulae tip placements.

Data analyses. The data were analyzed either with one-way ANOVA or with between-within ANOVA with dose of (RS)-MCPG as the between factorand injection [(RS)-MCPG alone or co-injected with AMPH] as thewithin factor. Post hoc Scheffé comparisons were made accordingto Kirk (1968).

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

(RS)-MCPG modulates the locomotor-activating effects of NAcc AMPH. Consistent with previous reports (Taylor and Robbins, 1984; Vezina and Stewart, 1990; Burns et al., 1994) microinjection ofAMPH into the NAcc significantly increased both horizontal andvertical locomotor activity when compared with saline controlinjections (fig. 1). These effects of AMPH were either unaffectedor progressively and significantly enhanced by increasing concentrationsof the four lower doses of (RS)-MCPG tested (0, 0.025, 0.25 and2.5 nmol/side). Co-injection with a moderately high dose of (RS)-MCPG(25 nmol/side) completely blocked the locomotor-activating effectsof NAcc AMPH. None of the doses of (RS)-MCPG tested when administeredalone into the NAcc produced effects on locomotion that differedsignificantly from those observed after injections of saline.Time-course analyses showed that the locomotor-activating effectsof NAcc AMPH persisted for approximately 1 hr of testing, consistentwith previous reports (Vezina and Stewart, 1990). The abilityof (RS)-MCPG to block these effects was apparent throughout thistime course. The ANOVA conducted on the data obtained in the first30 min of testing revealed significant effects of groups [betweendifferent doses of (RS)-MCPG; F(4,50) = 5.26, P < .002 and F(4,50)= 4.28, P < .005 for horizontal and vertical activity, respectively],injections [saline versus AMPH at all levels of (RS)-MCPG; F(1,50)= 100.99, P < .0001 and F(1,50) = 72.58, P < .0001] and a groups× injections interaction [F(4,50) = 4.57, P < .004 and F(4,50)= 4.45, P < .004]. Post hoc Scheffé comparisons revealed thatAMPH produced significantly greater locomotor activity than salineat the four lower doses (P < .001) but not at the highest doseof (RS)-MCPG tested. In addition, 0.25 nmol (RS)-MCPG significantlyenhanced (P < .05, horizontal and approached, P < .075, statisticalsignificance for vertical) and 25 nmol (RS)-MCPG significantlydecreased (P < .05, horizontal and vertical) the locomotor activityproduced by AMPH relative to that observed in animals having receivedAMPH with 0 nmol (RS)-MCPG. The ANOVA conducted on the data obtainedin the second 30 min of testing also revealed significant effectsof injections [F(1,50) = 36.73, P < .0001 and F(1,50) = 28.84,P < .0001 for horizontal and vertical locomotion, respectively].Again, post hoc Scheffé comparisons revealed that AMPH producedsignificantly greater locomotor activity than saline (P < .05-0.01)but not when it was co-injected with either the 2.5 (vertical)or the 25 nmol (horizontal and vertical) doses of (RS)-MCPG.

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Fig. 1. Effects of (RS)-MCPG on the locomotor-activating effects of NAcc AMPH. Data are shown as group mean (+S.E.M.) horizontal andvertical locomotor activity counts for each 30-min period of the2-hr test after microinjection of the indicated dose of (RS)-MCPG(0, 0.025, 0.25, 2.5 and 25 nmol/side) with saline or AMPH (6.8nmol/side). Numbers of rats in each group are indicated at thebase of the different columns. Individual animals were testedwith only one concentration of (RS)-MCPG, once co-injected withsaline and once co-injected with AMPH. Symbols indicate significantdifferences as revealed by post hoc Scheffé comparisons afterbetween-within ANOVA. ***P < .001, **P < .01 and *P < .05, AMPHcompared with saline at the indicated dose of (RS)-MCPG. $dagger$ P <.05, AMPH at the indicated dose of (RS)-MCPG compared with AMPHat (RS)-MCPG (0 nmol/side).

To determine whether the microinjection of (RS)-MCPG into the NAcc also produced effects on other behaviors not detected bythe photobeam interruptions, some rats were filmed after injectionto permit the subsequent observation and recording of variousbehaviors (e.g., grooming, sniffing, licking/gnawing). No evidenceof stereotyped or seizure-like behaviors was detected in ratsadministered either (RS)-MCPG alone or in combination with AMPH.

(RS)-MCPG blocks the locomotor-activating effects produced by NAcc infusions of the direct DA receptor agonist apomorphine. When microinjected into the NAcc, apomorphine (32.9 nmol [10 µg]/side) produced a significant increase in horizontal locomotoractivity during the second hour of testing. This finding, togetherwith the lack of effect of these infusions on vertical activity,is consistent with those reported previously by others (Jacksonet al., 1975; Cools, 1986). As shown in figure 2, co-injecting(RS)-MCPG (25 nmol/side) with apomorphine into the NAcc completelyblocked this effect. The ANOVA conducted on these data revealeda significant effect of groups [F(2,16) = 5.54, P < .02] duringthe second hour of testing. Apomorphine, at the dose tested, producedsignificantly greater locomotion than that produced by salineor apomorphine + (RS)-MCPG (P < .05 as revealed by post hoc Scheffécomparisons).

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Fig. 2. The mGluR antagonist, (RS)-MCPG, blocks the locomotor-activating effects of NAcc apomorphine (APO). Data are shown as groupmean (+S.E.M.) horizontal locomotor activity counts obtained inthe second hour. Note that when microinjected into the NAcc, apomorphine(32.9 nmol/side) compared with saline produced a significant increasein locomotor activity during the second hour of testing in a mannerconsistent with previous reports (Jackson et al., 1975

; Cools,1986

). The same dose of (RS)-MCPG (25 nmol/side) found to be effectivefor blockade of AMPH-induced locomotor activity was used. Thenumber of rats in each group is indicated at the base of eachcolumn. Symbols indicate significant differences as revealed bypost hoc Scheffé comparisons after one-way ANOVA. *P < .05, apomorphinecompared with saline and apomorphine + (RS)-MCPG.

Histology. Figure 3 shows the location of the injection cannula tips in the NAcc for all animals tested and included in the statisticalanalyses. Only data from rats with injection cannula tips locatedbilaterally in the NAcc were considered. Eight rats were excludedfor failing to meet this criterion. Also shown are representativephotomicrographs illustrating the guide and injection cannulatracks (aimed at the rostral pole, A, and more caudally into thecore, B, subregions of the NAcc) of two of the animals tested.Little evidence for neurotoxicity beyond the mechanical damageproduced by penetration of the cannulae was detected. Most injectionswere made bilaterally into the rostral pole (fig. 3A) and core(fig. 3B) subregions of the NAcc. Some animals received injectionseither bilaterally into the shell subregion of this nucleus orinto the core on one side and the shell on the other. No evidencewas obtained from the small number of such animals tested to indicatethat infusions of (RS)-MCPG either alone or in combination withAMPH into the shell subregion produced differential effects onhorizontal and vertical locomotion relative to infusions intoother subregions of the NAcc.

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Fig. 3. Location of the microinjection cannula tips in the NAcc of rats included in the data analyses (C). The line drawings are fromPaxinos and Watson (1986)

. Numbers to the right indicate millimetersrostral to bregma. The different symbols refer to the differentmicroinjections administered: open circles, (RS)-MCPG (0 nmol/side)microinjected either alone (with saline) or in combination withAMPH; filled circles, the remaining doses of (RS)-MCPG microinjectedeither alone (with saline) or in combination with AMPH; open triangles,apomorphine; filled triangles, apomorphine + (RS)-MCPG. Also shownare representative photomicrographs illustrating the guide andinjection cannula tracks of one rat that received microinjectionsinto the rostral pole subregion (A) and another that receivedmicroinjections more caudally into the core subregion (B) of theNAcc. Note the lack of neurotoxicity beyond the mechanical damageproduced by penetration of the injection cannulae.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

High-dose (RS)-MCPG blocks the locomotor-activating effects of NAcc AMPH. The present findings are consistent with those of previous studies showing that glutamate receptor antagonists microinjectedinto the NAcc attenuate the locomotor effects of psychomotor-stimulantdrugs (Pulvirenti et al., 1989; Willins et al., 1992; Kaddis etal., 1993; Burns et al., 1994). For example, the selective NMDAreceptor antagonist 2-amino-5-phosphonopentanoic acid has beenshown to dose-dependently reduce the effectiveness of NAcc AMPHto produce locomotion (Kelley and Throne, 1992). The intra-accumbensadministration of the AMPA/kainate antagonist, DNQX, has alsobeen shown to antagonize the locomotor-stimulant response to cocaineadministered either systemically or directly into the NAcc (Kaddiset al., 1993). The present study extended these findings to mGluRs.In a manner similar to iGluR antagonists, a moderately high dose(25 nmol/side) of (RS)-MCPG completely blocked the locomotor effectsof NAcc AMPH. The dose dependence of this effect and the effectivedose of (RS)-MCPG (25 nmol/side) found to produce it is reasonablysimilar to the effects obtained with iGluR antagonists and theeffective doses of these antagonists reported. For instance, 4nmol/side of DNQX and 21 nmol/side of GAMS, both AMPA/kainatereceptor antagonists, have been used to inhibit the locomotorstimulation produced by AMPH (0.5 mg/kg s.c.) (Willins et al.,1992), whereas 98 nmol/side of GDEE, a quisqualate receptor antagonist,was used to significantly reduce AMPH (0.75 mg/kg s.c.) locomotoreffects (Pulvirenti et al., 1989). For the NMDA receptor, 2.5to 5 nmol of 2-amino-5-phosphonopentanoic acid was shown to effectivelyreduce the locomotor effects of AMPH (13.6 nmol [5 µg]) microinjectedinto the NAcc (Kelley and Throne, 1992). More importantly, wheninjected alone into the NAcc, the dose of (RS)-MCPG (25 nmol/side)used to effectively block the locomotor effects of NAcc AMPH (aswell as all other doses tested) in this study produced no significanteffects on various types of behaviors including locomotor activityand stereotypy. As revealed from the time-course analyses, thisblockade by (RS)-MCPG of NAcc AMPH-induced locomotion persistedfor the duration of the latter drug's effect (approximately 1hr). A similar persistence in the ability to block NAcc AMPH-inducedlocomotion was reported previously for the NMDA receptor antagonist,2-amino-5-phosphonopentanoic acid (Kelley and Throne, 1992).

(RS)-MCPG blocks the locomotor-activating effect of NAcc apomorphine. Consistent with previous reports (Cools, 1986), infusion into the NAcc of the direct DA receptor agonist, apomorphine, produceda significant increase in horizontal locomotion during the secondhour of a 2-hr test. Again, (RS)-MCPG when co-injected with apomorphineinto the NAcc blocked this effect, which suggests that (RS)-MCPGcan act postsynaptically at mGluRs expressed by intrinsic NAccneurons. High concentrations of mGluRs are known to be expressedon both pre- and postsynaptic sites in the NAcc (Albin et al.,1992; Ohishi et al., 1993; Testa et al., 1994; Romano et al.,1995). The mGluRs are known to activate multiple second messengersystems via G proteins, including phosphotidylinosite hydrolysisand inhibition or activation of cAMP (Nakanishi, 1994). Thus,it is possible that mGluRs located on the dendritic processesof intrinsic NAcc cells may regulate incoming dopaminergic signalsby acting on second messenger systems with which mGluRs are coupled.Recent ultrastructural studies of the NAcc have indicated thatsome of the terminals of the descending excitatory amino acidprojections from cortex and those of ascending DA mesencephalicprojections not only come in close apposition to each other butform synaptic contacts with the same intrinsic NAcc neurons aswell (Sesack and Pickel, 1990, 1992). This anatomical arrangementprovides the basis for a possible interaction between glutamateand DA at the same synaptic sites in the NAcc. However, it doesnot preclude the possibility that receptor antagonists such as(RS)-MCPG can modulate the release of DA by AMPH by acting atmGluRs located presynaptically on dopaminergic nerve terminalsin the NAcc. Indeed, it was recently shown that the local applicationof (1S,3R)-ACPD (1 mM) to the NAcc via reverse dialysis can regulatethe extracellular levels of DA in this site (Ohno and Watanabe,1995; Taber and Fibiger, 1995). Although such results may reflectthe contribution of mGluRs located on nondopaminergic (e.g., serotonergic)afferents to the NAcc or, as recently suggested for iGluRs (Taberet al., 1996), of mGluRs expressed by intrinsic NAcc cells sendingreciprocal projections to DA perikarya in the ventral tegmentalarea, they are also consistent with a contribution by mGluRs locatedon DA neuron terminals. This latter possibility, together withthe ability of AMPH to release DA in an action potential-independentmanner, suggests that mGluRs may be linked to postreceptor pathwayswithin DA neuron terminals that are capable of influencing thestimulation of DA release by AMPH. Thus, although the presentresults support a contribution by mGluRs located postsynapticallyto DA neuron terminals to dopaminergic neurotransmission in theNAcc, they cannot exclude an equally important contribution bymGluRs located presynaptically on DA neuron terminals in thissite.

Similarly, iGluRs in the NAcc have also been shown to regulate dopaminergic neurotransmission. Perfusion of the NAcc withselective agonists of iGluRs increases extracellular levels ofDA in this site (Imperato et al., 1990

; Youngren et al., 1993

),whereas infusion of iGluR antagonists attenuates dopaminergicneurotransmission induced by either direct or indirect DA agonists(Pulvirenti et al., 1989

, 1991

; Kelley and Throne, 1992

; Willinset al., 1992

; Kaddis et al., 1993

). Taken together, the presentresults confirm and extend to mGluRs the notion that glutamateregulates dopaminergic neurotransmission by acting at sites pre-and postsynaptic to DA neuron terminals in the NAcc.

Different subtypes of mGluRs exist in the NAcc. Based on their sequence homology, transduction mechanisms and pharmacology, the mGluR family, consisting of at least eightdifferent subtypes of receptors, has been divided into three groups(Pin and Bockaert, 1995; Pin and Duvoisin, 1995; Miller et al.,1995). Whereas receptors belonging to group I (mGluR1 and mGluR5)are coupled to G-proteins which lead to activation of phospholipaseC, those in group II (mGluR2 and mGluR3) and group III (mGluR4,mGluR6, mGluR7 and mGluR8) are negatively coupled to G-proteinsand inhibit adenylyl cyclase. Among these, mGluR5 and mGluR3 mRNAsare expressed most abundantly in the NAcc (Testa et al., 1994).It is known that (RS)-MCPG acts as an antagonist at both mGluR5(group I) and mGluR3 (group II) (Pin and Bockaert, 1995). Thus,it is possible that either or both of these receptors may be involvedin mediating the effect of (RS)-MCPG in blocking the locomotor-activatingeffects of DA agonists in the NAcc. The mechanisms mediating theseeffects, however, remain to be determined.

Low-dose (RS)-MCPG potentiates the locomotor-activating effects of NAcc AMPH. In the lower range of doses of (RS)-MCPG tested (0, 0.025, 0.25 nmol/side), increasing the dose of this mGluR antagonist progressivelyenhanced the locomotor-activating effects of NAcc AMPH. Althoughthe magnitude of this effect was small, it did achieve statisticalsignificance at the 0.25 dose of (RS)-MCPG for horizontal activity(P < .05, AMPH + 0.25 (RS)-MCPG vs. AMPH + 0 (RS)-MCPG) and approachedstatistical significance at this dose (P < .075) for verticalactivity, which suggests that this mGluR antagonist may have biphasiceffects on NAcc AMPH-induced locomotion. Such a possibility isnot without precedent. For example, it was recently reported thatwhereas a low concentration of the mGluR agonist (1S,3R)-ACPDdecreased levels of extracellular DA in the NAcc, a higher concentrationproduced the opposite effect (Taber and Fibiger, 1995). The presentfindings (enhancement of NAcc AMPH-induced locomotion by a lowdose of (RS)-MCPG and its blockade by a higher dose) are entirelyconsistent with these results. The mechanisms underlying theseeffects are unknown. It is conceivable, however, as suggestedby some (Schoepp and Conn, 1993; Taber and Fibiger, 1995; Kimand Vezina, 1997), that opposing actions by different concentrationsof mGluR agonists and antagonists may reflect the different affinitiesfor such ligands displayed by mGluR subtypes (Pin and Bockaert,1995; Pin and Duvoisin, 1995) and their differential activationby the different doses. Given the different transduction mechanismsassociated with mGluR3 and mGluR5 described above, it is likelythat their selective recruitment would lead to opposing actions(Schoepp and Conn, 1993; Taber and Fibiger, 1995; Kim and Vezina,1997).

Finally, determining the location of the mGluR subtype in the NAcc and the manner in which it contributes to the potentiationof the locomotor-activating effects of AMPH is currently difficult.AMPH-induced locomotion could be potentiated by enhancing itsability to elevate extracellular levels of DA in the NAcc. Thiscould be achieved directly by mGluR-mediated actions at DA neuronterminals or indirectly by mGluR actions at nondopaminergic afferentsto the NAcc (e.g., to decrease serotonin inhibition of DA release)or at intrinsic NAcc cells (to increase DA neuron firing via theirdescending projections to ventral tegmental area; see Taber etal., 1996

). Alternatively, AMPH-induced locomotion could alsobe potentiated by changes in the regulation of incoming dopaminergicsignals by mGluRs located on intrinsic NAcc motor output neurons.The present findings with apomorphine indicate that these neuronsexpress at least one mGluR subtype and that its blockade preventsthe locomotion produced by this agonist. It is possible that theseneurons also express another mGluR subtype that is recruited bylower doses of (RS)-MCPG. Confirmation of this possibility wouldbe aided by the direct observation of different mGluR subtypeson these neurons or the demonstration that apomorphine-inducedlocomotion is enhanced by these doses of (RS)-MCPG in the absenceof changes in the availability of extracellular DA resulting frompotential presynaptic apomorphine-(RS)-MCPG interactions.

Conclusion. The present results demonstrate that the mGluR antagonist, (RS)-MCPG, can block the locomotor-activating effects of both directand indirect DA agonists when these are infused into the NAcc.Although these results can be interpreted to suggest that mGluRslocated on intrinsic NAcc cells postsynaptic to DA neuron terminalsmediate this effect, a contribution by presynaptically expressedmGluRs remains a possibility. The additional finding that lowand high doses of (RS)-MCPG produced opposing effects indicates,in a manner consistent with previous reports, that this mGluRantagonist exerts biphasic effects on NAcc AMPH-induced locomotoractivity. The contribution of the locally expressed mGluR3 andmGluR5 subtypes to these effects as well as their pre- and postsynapticlocus and site of action in the NAcc remain to be elucidated.

Along with the results of previous reports, the present results confirm and extend to mGluRs the notion that glutamate interactswith DA neurotransmission in the NAcc to influence behavior.

	Footnotes

Accepted for publication September 8, 1997.

Received for publication June 25, 1997.

¹ Supported by grants to P.V. from The Brain Research Foundation.

Send reprint requests to: Paul Vezina, Department of Psychiatry, The University of Chicago, 5841 South Maryland Avenue, MC 3077, Chicago, IL 60637.

	Abbreviations

DA, dopamine; NAcc, nucleus accumbens; AMPH, amphetamine; iGluRs, ionotropic glutamate receptors; AMPA, $alpha$ -amino-3-hydroxy-5-methyl isoxazole-4-propionic acid; NMDA, N-methyl-D-aspartate; mGluRs, metabotropic glutamate receptors; (1S,3R)-ACPD, 1-aminocyclopentane-trans-1,3-dicarboxylic acid; (RS)-MCPG, (RS)- $alpha$ -methyl-4-carboxyphenylglycine; ANOVA, analysis of variance; DNQX, 6,7-dinitroquinoxaline-2,3-dione; GAMS, $gamma$ -d-glutamylaminomethylsulfonate; GDEE, L-glutamic acid diethyl ester.

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