Role of P/Q-Ca2+ Channels in Metabotropic Glutamate Receptor 2/3-Dependent Presynaptic Long-Term Depression at Nucleus Accumbens Synapses

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The Journal of Neuroscience, June 1, 2002, 22(11):4346-4356

Role of P/Q-Ca²⁺ Channels in Metabotropic Glutamate Receptor 2/3-Dependent Presynaptic Long-Term Depression at Nucleus Accumbens Synapses
David Robbe¹, Gérard Alonso², Séverine Chaumont³, Joël Bockaert¹, and Olivier J. Manzoni¹
Centre National de la Recherche Scientifique ¹ Unité Propre de Recherche 9023, ² Unité Mixte de Recherche 5101, and ³ Unité Propre de Recherche 1142, 34094 Montpellier Cedex 05, France

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The nucleus accumbens (NAc) is an important cerebral area involved in reward and spatial memory (Pennartz et al., 1994), butlittle is known about synaptic plasticity in this region. Here,electron microscopy revealed that, in the NAc, metabotropic glutamatereceptors 2/3 (mGlu2/3) immunostaining was essentially associatedwith axonal terminals and glial processes, whereas postsynapticdendrites and neuronal cell bodies were unstained. Electrophysiologicaltechniques in the NAc slice preparation demonstrated that activationof mGlu2/3 with synaptically released glutamate or specific exogenousagonist, such as LY354740 (200 nM, 10 min), induced long-termdepression of excitatory synaptic transmission (mGlu2/3-LTD).Tetanic-LTD and pharmacological mGlu2/3-LTD occluded each other,suggesting common mechanisms. The mGlu2/3-LTD did not requiresynaptic activity but depended on the cAMP-protein kinase A cascade.Selective inhibition of P/Q-type Ca²⁺ channels with $omega$ -agatoxin-IVA occluded the expression of mGlu2/3-LTD,and, conversely, the inhibitory effects of $omega$ -agatoxin-IVA wereabolished during mGlu2/3-LTD. Thus, mGlu2/3 play an importantrole in the control of use-dependent synaptic plasticity at prelimbiccortex-NAc synapses: their activation causes a form of LTD mediatedby the long-lasting reduction of P/Q-type Ca²⁺channels contribution to transmitterrelease.

Key words: nucleus accumbens; long-term depression; metabotropic glutamate receptors; mGlu2/3; presynaptic inhibition; mice; prelimbic cortex; calcium channels

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The nucleus accumbens (NAc) is a structure of particular interest because of its role in connecting the limbic system to thebasal ganglia and to extrapyramidal motor system, its involvementin spatial memory and adaptative processes, and its implicationin the mechanisms at the origin of the rewarding properties ofmany drugs of abuse (Schacter et al., 1989; Pennartz et al., 1994).Glutamate is the excitatory neurotransmitter at the synapses betweenprelimbic cortex afferents and medium spiny neurons of the NAc(Horne et al., 1990). Pennartz and collaborators showed that high-frequencystimulation of prelimbic afferents could cause long-term depression(LTD), long-term potentiation (LTP), or no change in the gainof excitatory synaptic transmission (Pennartz et al., 1993). Whatdetermines the fate of these synapses during phasic activity ofprelimbic afferents? LTP (but not LTD) induction partially dependedon NMDA receptors, and both LTD and LTP were independent of dopaminereceptors (Pennartz et al., 1993; Kombian and Malenka, 1994).Morphological and physiological studies have described variousmetabotropic glutamate receptor (mGlu) subtypes at the glutamatergicafferents to the NAc (Ohishi et al., 1993a,b; Shigemoto et al.,1993; Manzoni et al., 1997). Converging reports indicate that,during tetanic stimulation of glutamatergic synapses, activationof mGlu induces LTD (for review, see Anwyl, 1999). Among the variousmGlu subtypes (for review, see Conn and Pin, 1997), mGlu2/3 playkey roles in the control of LTD in hippocampal mossy fibers (Kobayashiet al., 1996; Yokoi et al., 1996; Tzounopoulos et al., 1998),the dentate gyrus (Huang et al., 1997, 1999), the amygdala (Linet al., 2000), the prefrontal cortex (Otani et al., 1999), andthe dorsal striatum (Kahn et al., 2001).

This study shows that mGlu2/3 play an important role in the control of use-dependent synaptic plasticity at prelimbic cortex-NAcsynapses: their activation causes a form of LTD mediated by areduction of P/Q-type Ca²⁺ channels contribution to transmitterrelease.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Immunohistochemistry-electron microscopy. After being deeply anesthetized with sodium pentobarbital (50 mg/kg), mice wereperfused through the ascending aorta with PBS, pH 7.4, followedby 300 ml of fixative composed of 4% paraformaldehyde and 0.5%glutaraldehyde in 0.1 M phosphate buffer, pH 7.4. The brain wasthen dissected and fixed by immersion in the fixative withoutglutaraldehyde for 12 hr at 4°C. It was then cut sagittally witha vibratome into 40- to 50-µm-thick sections. After careful rinsingin PBS, sections were successively incubated as follows: (1) for48 hr at 4°C with the antibody anti-mGlu2/3 (diluted 1:500; Chemicon,Temecula, CA), (2) for 12 hr at 4°C with a peroxidase-labeledFab fragment of goat IgG anti-rabbit IgG (Biosys, Compiègne,France), diluted 1:1000, and (3) with 0.1% 3,3' diaminobenzidinediluted in 0.05 M Tris buffer, pH 7.3, in the presence of 0.2%H₂O₂. The primary and secondary antibodies were diluted in PBScontaining 1% BSA, 1% normal goat serum, and 0.1% saponin. Immunostainedsections were either mounted in Permount and observed under alight microscope or further treated for electron microscopy. Forthis, they were carefully rinsed in 0.1 M cacodylate buffer, pH7.3, and postfixed in 1% OsO₄ in the same buffer. They were thendehydrated in graded concentrations of ethanol and embedded inaraldite. Punches of 1.5 mm in diameter were cut through the accumbensnucleus and mounted on araldite blocks. After being cut into ultrathinsections, they were observed in an electron microscope (modelH 7110; Hitachi, Tokyo, Japan) without counterstaining or withslight uranyl acetatestaining.

Electrophysiology. Whole-cell patch-clamp and extracellular field recordings were made from medium spiny neurons in parasagittalslices of mouse nucleus accumbens. This method has been describedpreviously (Manzoni et al., 1997; Robbe et al., 2001). In brief,mice (male C57BL/6, 4-6 weeks) were anesthetized with isofluraneand decapitated. The brain was sliced (300-400 µm) in the parasagittalplane using a vibratome and maintained in physiological salineat 4°C. Slices containing the NAc were stored at least 1 hr atroom temperature before being placed in the recording chamberand superfused (2 ml/min) with artificial CSF (in mM: 126 NaCl,2.5 KCl, 1.2 MgCl₂, 2.4 CaCl_2, 18 NaHCO₃, 1.2 NaH₂PO₄, and 11glucose) and was equilibrated with 95% O₂-5% CO₂. All experimentswere done at room temperature. The superfusion medium containedpicrotoxin (100 µM) to block GABA_A receptors. All drugs were addedat the final concentration to the superfusionmedium.

For field EPSPs (fEPSPs), the recording pipette was filled with a 3 M NaCl solution, and both the fEPSP slope (calculatedwith a least-square method) and fEPSP amplitude were measured(graphs depict amplitudes). For patch-clamp experiments, cellswere visualized using an upright microscope with infrared illumination,and recordings were made with whole-cell electrodes containingthe following (in mM): 128 Cs-gluconate, 20 NaCl, 1 MgCl₂, 1 EGTA,0.3 CaCl₂, 2 Mg-ATP, 0.3 GTP, and 0.2 cAMP, buffered with 10 HEPES,pH 7.3. Electrode resistance was 4 M $Omega$ , acceptable access resistancewas <20 M $Omega$ , and the holding potential was $-$ 70 mV. An Axopatch-1D(Axon Instruments, Foster City, CA) was used to record the data,which were filtered at 1-2 kHz, digitized at 5 kHz on a DigiData1200 interface (Axon Instruments), and collected on a personalcomputer using ACQUIS-1 software (Bio-Logic, Claix, France). Toevoke synaptic currents, stimuli (100-150 µsec duration) weredelivered at 0.033 Hz through bipolar tungsten electrodes placedat the prefrontal cortex-accumbens border (Manzoni et al., 1997,1998). Recordings were made in the rostromedial dorsal accumbensclose to the anterior commissure. According to the atlas of mousebrain in stereotaxic coordinates (Paxinos and Franklin, 2001),slices were located between lateral 1.44 and 0.6 mm to the midline.Electrodes of stimulation were placed rostrally and close to therecordingelectrode.

Miniature and spontaneous EPSCs (mEPSCs and sEPSCs) were recorded in the presence or absence of tetrodotoxin (TTX) (300 nM),respectively, using Axoscope 1.1.1. mEPSC amplitude and inter-intervaltime were measured using Axograph 3.6. For this analysis, a templateof mEPSCs having the width and time course of a typical synapticevent [a double exponential: f(t) = exp( $-$ t/Rise) $-$ exp( $-$ t/Decay),where Rise is 0.5 msec and Decay is 3 msec] was slid along thedata trace one point at a time. At each position, this templateis optimally scaled and offset to fit the data, and a detectioncriterion is calculated. The detection criterion is the template-scalingfactor divided by the goodness-of-fit at each position. An eventis detected when this criterion exceeds a threshold and reachesa sharp maximum. The limit of detection was 2 pA (Manzoni andWilliams, 1999; Robbe et al., 2001).

The fitting of concentration-response curves were calculated according to y = {y_max $-$ y_min/1 + (x/EC₅₀)n} + y_min (where y_maxindicates response in the absence of agonist, y_min indicates responseremaining in presence of maximal agonist concentration, x indicatesconcentration, EC₅₀ indicates concentration of agonist producing50% of the maximal response, and n indicates slope) with Kaleidagraphsoftware (Abelbeck Software, Reading, PA). All values are givenas mean ± SEM. Statistical analyses were done with the Mann-WhitneyU test, the Fisher's exact test for distribution in Figure 3A,the Kolmogorov-Smirnov tests using Statview for cumulative distributionanalysis of mEPCSs and sEPSCs (Abacus Concepts, Calabasas, CA),and the paired Student's t test for mean frequency and amplitudeof mEPSCs and sEPSCs. p < 0.05 was taken as indicating statisticalsignificance (*p < 0.05 and **p < 0.01).

Drugs used were as follows: (+)-5-methyl-10,11-dihydro-5H-dibenzo [a,d] cyclohepten-5,10-imine maleate (MK801), L-AP-5, picrotoxin,forskolin, and nimodipine (Sigma, St. Louis, MO); 2-amino-2-(2-carboxycyclopropan-1-yl)-3-(dibenzopyran-4-yl)propanoic acid (LY341495), (2S,1'S,2'S)-2-(carboxycyclopropyl)glycine(LCCG1) and (2S)- $alpha$ -ethylglutamate (eGlu) (Tocris Cookson, Ballwin,MO); H 89, KT 5720, and $omega$ -agatoxin-IVA (Alexis, San Diego, CA);tetrodotoxin and $omega$ -conotoxin-GVIA (Alomone, Jerusalem, Israel);and (+)-2-aminobicyclo-[3.1.0]hexane-2,6-dicarboxylic acid (LY354740)[gift of Drs. A. Schoepp and Monn (Eli-Lilly, Indianapolis, IN)].Other chemicals were from the highest commercial gradeavailable.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Localization of mGlu2/3 in the NAc

Examination of immunostained sections under the light microscope indicated that, throughout all of the forebrain regions examined,the organization of the mGlu2/3-immunostained structures conformedto previous descriptions in the rat (Petralia et al., 1996; Mineffand Valtschanoff, 1999) and mice (Ohishi et al., 1998; Tamaruet al., 2001). Within the nucleus accumbens, as in the surroundingregions including the striatum, mGlu2/3 labeling was essentiallyassociated with elongated processes and with numerous dot structuresdispersed between unlabeled neuronal cell bodies (Fig. 1A). Theexamination of immunostained sections at the electron microscopiclevel indicated that, throughout the nucleus accumbens of C57BL/6mice, mGlu2/3 immunostaining was essentially associated with axonalterminals and glial processes, postsynaptic dendrites and neuronalcell bodies being unstained (Fig. 1B,D). Throughout the nucleus,the mGlu2/3-immunostained glial processes closely surround bothlabeled and unlabeled synaptic axon terminals (Fig. 1C,D). mGlu2/3-immunostainedaxon terminals represented ~20% of total axon terminals (identifiedby their content in synaptic-like vesicles). When identified,these mGlu2/3-immunostained terminals form typical asymmetricsynaptic contacts with unlabeled dendrites (Fig. 1B). These resultsare in agreement with a previous detailed study by Tamaru andcolleagues, who have described subcellular localization and thepresence of mGlu3 immunostaining in striatal presynaptic terminalsof BALB/c mice (Tamaru et al., 2001).

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Figure 1. Immunolocalization of mGlu2/3 in the nucleus accumbens. A, At the light microscope level, immunostaining is associated with elongated processes (arrows) and dot structures dispersed between unlabeled neuronal cell bodies (N). B-D, At the electron microscope level, immunostaining is essentially associated with axon terminals containing numerous synaptic-like vesicles (ax) and glial processes (gl), whereas dendritic profiles (D) always appear unstained. Note that labeled axon terminals frequently form typical synaptic contacts with unlabeled dendrites (arrowheads in B and C), whereas labeled glial processes frequently enwrap either labeled (C) or unlabeled (D) synaptic axon terminals. Asterisks in B-D indicate the unlabeled axon terminals. Scale bars: A, 25 µm; B-D, 1 µm.

LTD can be induced by specific group 2 mGlu agonist

We decided to evaluate the effects of the direct stimulation of presynaptic mGlu2/3. Conventional extracellular field recordingwere first chosen because of the non-invasive nature of the technique.fEPSPs were measured in mice NAc core (Manzoni et al., 1997, 1998;Robbe et al., 2001). It was found that application of the highlyselective mGlu2/3 agonist LY354740 (Schoepp et al., 1997) (200nM) for 10 min caused a rapid and strong inhibition of fEPSP,which was maximal at the end of the application of the drug (62.7± 3.0% of inhibition; n = 34) (Fig. 2A). After washout of thedrug, the amplitude of the fEPSP was only partially recoveredto a stable response that was depressed at 60 min by 25.7 ± 2.5%relative to baseline value (LTD; n = 34) (Fig. 2A). LTD was alsotriggered by another mGlu2/3 agonist, LCCG1; application of thisdrug at 10 µM for 5 min induced an initial inhibition of the fEPSPof 67.05 ± 5.56% (n = 8), which was followed by an LTD of 34.79± 7.94% (n = 8) at 60 min (data not shown).

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Figure 2. Characterization of pharmacological mGlu2/3-induced LTD. A, Summarized data showing that application of LY354740 (200 nM) resulted in an initial depression, which was followed during washout by an LTD. Inset shows traces (average of 10 consecutive fEPSPs) taken at the points indicated in a typical experiment. Calibration: 0.3 mV, 10 msec. B, Typical whole-cell experiment showing LTD induced by LY354740. Inset shows traces (average of 10 consecutive eEPSCs) taken at points indicated on the graph. Calibration: 100 pA, 25 msec. C, Inhibition of eEPSC 30 min after LY354740 is accompanied by an increase in the paired-pulse ratio. D, In presence of the group 2 mGlu antagonist LY341495 (200 nM), the initial depression induced by LY354740 was reduced and the LTD was prevented. E, Application of LY341495 (200 nM) 60 min after LTD induced by LY354740 did not reverse the LTD. F, Dose-response curves for the LY354740-induced initial inhibition of the fEPSP and for LTD.

To verify that LTD is a synaptic phenomenon and does not result from a decrease of cell excitability, we use patch-clamp recordingin the whole-cell configuration. Figure 2B depicts a typical experiment,and it is clear that LTD could be obtained even when the cellswere held at $-$ 70 mV, without modification of the input resistance;on average, 30 min after LY354740, excitatory EPSCs (EPSCs) measured72 ± 11% of baseline (n = 6; data not shown). The paired-pulseratio was increased 30 min after LY354740 by 45 ± 12% (n = 6)(Fig. 2C). That increase was significantly correlated with themagnitude of LTD induced by LY354740 (r = 0.80; Spearmann's rankcorrelation; p < 0.0005) (Fig. 2C). Together, these experimentsdemonstrated that, at the NAc glutamatergic synapses, direct activationof mGlu2/3 induces LTD. Moreover, the accompanying increase ofpaired-pulse ratio suggested a presynaptic locus ofexpression.

Pharmacological characterization of the mGlu2/3-LTD

To demonstrate that the effects of group 2 mGlu agonists were attributable to genuine interactions with mGlu2/3 receptors,the following experiments were performed. First, slices were treatedwith the highly specific mGlu2/3 antagonist LY341495 (Ornsteinet al., 1998) (200 nM, 15 min before, during, and 10 min aftersuperfusion of LY354740). In this condition, LY354740 induceda smaller initial depression of the fEPSP than in control medium(34.11 ± 10.11%, n = 5 vs 62.7 ± 3%, n = 34; p < 0.05) (Fig. 2D),consistent with the antagonist actions of LY341495 at mGlu2/3.The acute mGlu2/3 inhibition was completely reversed 10 min afterwashout of the agonist, and LTD was never observed. A similarresult was obtained with eGlu, another selective mGlu2/3 antagonist(Pin et al., 1999): in slices treated with eGlu (200 µM), theinitial LY354740 depression of fEPSP was reduced compared withcontrol (32.31 ± 10.13%, n = 5 vs 62.7 ± 3%, n = 34; p < 0.05)and completely reversed after 5 min of washout of LY354740 (datanot shown). Accordingly, in slices treated with eGlu (200 µM),the initial LCCG1 depression of fEPSP was reduced compared withcontrol (29.2 ± 13.6%, n = 5 vs 67.05 ± 5.56%, n = 8; p < 0.05)and completely reversed after 5 min of washout of LCCG1 (datanot shown). Together, these results clearly show the efficacyof group 2 antagonists (LY341495 and eGlu) at inhibiting the actionsof group 2 mGlu agonists. Finally, slices were treated with 10µM LY341495 to ensure the total blockade of mGlu2/3. In this condition,fEPSP measured 103.73 ± 5.82% of baseline at the end of LY354740application (n = 4; data not shown) and 111.22 ± 0.88% 60 minafter LY354740 application (n = 3; data notshown).

Figure 2E illustrates that superfusion of the mGlu2/3 antagonist LY341495 (200 nM) for 10 min (1 hr after agonist perfusion)did not reverse mGlu2/3-induced LTD. In a similar experiment,superfusion of eGlu (200 µM) for 10 min, 30 min after LCCG1 washout,did not reverse LCCG1-induced LTD (data not shown). These resultsshow that mGlu2/3-induced LTD is not attributable to the incompletewashout of LY354740 or LCCG1. The EC₅₀ values for the initialdepression of the fEPSP attributable to LY354740 and LTD were33.09 ± 0.6 nM and 79.89 ± 8.75 µM, respectively (Fig. 2F). TheLCCG1-induced effects were also dose dependent, and the EC₅₀ forthe initial depression and the LTD were 1.4 ± 0.8 and 2.0 ± 0.4µM, respectively (data notshown).

Synaptic activation of mGlu2/3 induces LTD and occludes pharmacological mGlu2/3-LTD

We next tested whether synaptically released glutamate, similar to exogenous mGlu2/3 agonist, can induce mGlu2/3 presynapticLTD. First, we reproduced the observation of Pennartz and collaborators:in rat NAc slices, high-frequency stimulation of prelimbic cortex-NAcsynapses resulted in LTP, LTD, or no change in synaptic efficacy(Pennartz et al., 1993). As summarized Figure 3A, tetanic stimulation(three times for 1 sec at 100 Hz, 20 sec intervals) of prelimbicglutamatergic afferents in mice NAc slices (black bars) causedLTD in a majority of the experiments (in 60% of the slices; 15of 25) (a typical experiment is shown Fig. 3B). In the remainingslices, tetanic stimulation caused either no change (28% of slices;7 of 25; No Plasticity) or rarely LTP (12% of slices; 3 of 25).There was no correlation between the magnitude of basal fEPSPsand the direction of plasticity (r = 0.210). When all of the sliceswere averaged, tetanus induced an overall LTD of 14.05 ± 3.61%(n = 25) (Fig. 3C, black circles). Based on the aforementionedresults, we reasoned that stimulation of presynaptic mGlu2/3 duringintense synaptic activity should induce LTD. Indeed, perfusionof the slices with the mGlu2/3 antagonist LY341495 (200 nM, 15min) clearly reduced the number of slices expressing LTD in responseto tetanic stimulation (12.5% of the slices; one of eight; p <0.05 vs control Fisher's exact test) (Fig. 3A) but had no effecton basal synaptic transmission (data not shown). Comparing allof the slices revealed that synaptic activation of mGlu2/3 drivesthe prelimbic cortex-NAc synapses to express LTD (Fig. 3C) [30min after tetanus, fEPSP measured 85.95 ± 3.67% of baseline incontrol (n = 25) and 106.01 ± 8.44% of baseline in LY341495-treatedslices (n = 8); p < 0.05]. Finally, we confirmed the results ofPennartz et al. and found that tetanic-LTD was independent ofNMDA receptors (NMDARs) (60 and 50% of tetanized slices exhibitedLTD in control and after 50 µM L-APV treatment, respectively;p > 0.05; Fisher's exact test; data not shown).

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Figure 3. Induction of synaptic mGlu2/3-LTD and mutual occlusion with pharmacological LTD. A, High-frequency tetanus (3 times for 1 sec at 100 Hz, 20 sec interval) can induce LTD, LTP, or no plasticity in the NAc. Summarized histogram showing the percentage of slices exhibiting LTD (defined as a inhibition of at least 10% of baseline fEPSP, 30 min after tetanus), LTP (defined as an enhancement of at least 10% of baseline fEPSP, 30 min after tetanus), or no plasticity in control conditions or after perfusion with the highly selective mGlu2/3 antagonist LY341495 (200 nM, 15 min). Blocking mGlu2/3 receptors during the tetanus clearly reduced the number of slices expressing LTD and increased the number of slices exhibiting either LTP or no change in synaptic efficacy. B, Typical experiment showing tetanus-induced LTD in control medium. The inset shows traces (average of 10 consecutive fEPSPs) taken at the points indicated. Calibration: 0.4 mV, 5 msec. C, Summary of all of the experiments comparing the effects of high-frequency stimulation of prelimbic afferents in control conditions and after blockade of mGlu2/3. D, Typical experiment showing that, after inducing the mGlu2/3-LTD with LY354740 (200 nM), the tetanus induces no more LTD (here it induces LTP). E, Summary of all of the experiments showing the occlusion of tetanus-induced LTD after induction of mGlu2/3-LTD with LY354740. F, Typical experiment showing that, after saturation of tetanus-induced LTD, LY354740 (200 nM) did not induce LTD. G, Summary of all of the experiments showing the occlusion of mGlu2/3-LTD induced with LY354740 (200 nM) after induction of tetanus-induced LTD. Tet, Tetanus (three times at 1 sec at 100 Hz). *p < 0.05; **p < 0.01.

Occlusion experiments were performed to test whether mGlu2/3 agonist-induced LTD and tetanus-induced LTD shared similar mechanisms.LTD was first induced by perfusion with LY354740, and, 70 minafter agonist application, tetanus (three times for 1 sec at 100Hz, 20 sec intervals) were given. Tetanus-induced LTD was neverobserved in slices in which mGlu2/3-LTD was already triggered(zero of seven; p < 0.05 vs control; Fisher's exact test), demonstratingthe complete occlusion between these two forms of LTD (Fig. 3D,typical experiment, E, average data) [fEPSP at 30 min after measured85.95 ± 3.67% (n = 25) in control vs 110.73 ± 7.84% (n = 7) afterinducing LTD with LY354740; p < 0.05). Occlusion from mGlu2/3-LTDwas also observed in slices in which tetanus-induced LTD was inducedfirst. Figure 3F shows a typical experiment in which, after inductionof tetanic-LTD (note that tetanic-LTD is already saturated afterthe first tetanus), LY354740 causes acute inhibition but not LTD.Figure 3G presents average data. LY354740 initial effect is reducedcompared with control (46.32 ± 3.29 vs 62.71 ± 3.03%; p < 0.05)and completely reversed 20 min after washout. Together, theseexperiments showed the existence of common mechanisms betweenmGlu2/3-LTD and tetanus-inducedLTD.

mGlu2/3-LTD is independent of presynaptic activity and intracellular Ca²⁺ levels

Compared with tetanus-induced LTD, agonist-induced mGlu2/3-LTD offered an easy and reliable assay to study the LTD of prelimbiccortex-NAc and particularly its transduction pathways. Is thesimple activation of presynaptic mGlu2/3 sufficient to LTD induction?At excitatory synapses of the hippocampus (Huang et al., 1997,1999; Tzounopoulos et al., 1998) or the amygdala (Lin et al.,2000), an additional component that depended on presynaptic terminalactivity was required to produce LTD. Thus, test stimulation wasstopped during perfusion and washout of LY354740 (for a totalof 40 min). Figure 4A clearly demonstrates that concurrent presynapticactivity was not necessary for the induction of mGlu2/3-LTD [LTDat 60 min measured 22.90 ± 5.91% (n = 6) of baseline vs 25.69± 2.24% (n = 34) in control; p > 0.05] (Kahn et al., 2001). Totest the importance of intracellular Ca²⁺ levels (and especially presynaptic Ca²⁺), intracellular Ca²⁺ was lowered with BAPTA AM (50 µM). Similar to other studies usingmembrane-permeant Ca²⁺ chelators (Tzounopoulos et al., 1998; Casado et al., 2000; Linet al., 2000), BAPTA AM markedly reduced the fEPSP (45.5 ± 7.2%of baseline in BAPTA AM; n = 4; data not shown), suggesting thatthis concentration effectively buffered intracellular Ca²⁺. In marked contrast with studies in which bath perfusion withCa²⁺ chelator reduced mGlu2/3-LTD (Tzounopoulos et al., 1998; Linet al., 2000), in the NAc, the initial depression or the LTD inducedby LY354740 are unaltered [LTD at 60 min measured 36.51 ± 11.43%(n = 4) vs 25.69 ± 2.24% (n = 34) in control; p > 0.05; data notshown). Together, these results suggested that activity-dependentchanges in intracellular Ca²⁺ are unlikely to participate in mGlu2/3-LTD.

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Figure 4. Transduction pathways of mGlu2/3-LTD. A, mGlu2/3-LTD was not blocked in the absence of presynaptic activity. Summary of all of the experiments in which evoked synaptic stimulation was stopped during bath perfusion of LY354740 (200 nM) and 30 min after the washout. B, Summarized data showing that treatment with the adenylate cyclase activator forskolin (10 µM) inhibited the initial depression attributable to LY354740 and completely abolished mGlu-LTD. C, Summary of the effects the PKA inhibitor KT 5720 (1 µM) on basal synaptic transmission. D, Summary of all of the experiments in which the slices were preincubated at least 2 hr with the PKA inhibitor KT 5720 at 1 µM. In this condition, the initial depression of fEPSP by LY354740 was slightly decreased, and LTD at 60 min was totally prevented. E, Summary of the effects the PKA inhibitor H 89 (10 µM) on basal synaptic transmission. F, Summary of the experiments in which slices have been treated 20 min before, during, and 10 min after LY354740 application with the PKA inhibitor H 89 (10 µM). In this condition, the LTD induced by LY354740 was completely prevented at 60 min. *p < 0.05; **p < 0.01.

Role of the cAMP/protein kinase A-signaling cascade in the mGlu2/3-LTD

Because group 2 mGlu are coupled to adenylate cyclase via G-protein of the G_i/o family (Conn and Pin, 1997) and because mGlu2/3-LTDhas been shown to be dependent on both group 2 mGlu activationand the cAMP-protein kinase A (PKA) cascade (Tzounopoulos et al.,1998; Huang et al., 1999; Lin et al., 2000) (but see Otani etal., 1999; Kahn et al., 2001), the involvement of the cAMP-PKAcascade in the mGlu2/3-LTD at the NAc synapses was tested. Theadenylate cyclase activator forskolin (10 µM) caused a large increaseof the NAc fEPSP (150.05 ± 10.24% of basal fEPSP; n = 9; datanot shown), demonstrating the sensitivity of these synapses tothe elevation of cAMP levels (Manzoni et al., 1998; Robbe et al.,2001). Figure 4B shows that, in slices treated with forskolin(20 min before agonist perfusion and thereafter, 10 µM), the initialdepression of fEPSP induced by LY354740 was reduced compared withcontrol [36.95 ± 7% inhibition (n = 3) vs 62.7 ± 3% (n = 34);p < 0.05], and the LTD at 60 min was completely abolished [2.15± 1.02% of baseline (n = 3) vs 25.69 ± 2.45% (n = 34) in control;p < 0.05]. Similar results were obtained with the LCCG1-inducedLTD that was prevented in slices treated with forskolin [3.2 ±0.8% of baseline (n = 4) vs 25.69 ± 2.45% (n = 34); p < 0.05;data not shown].

Is protein kinase A involved in the mGlu2/3-LTD? The PKA inhibitor KT 5720 (1 µM) alone depressed basal synaptic transmission(25.5 ± 5.5% inhibition; 60 min; n = 3), as shown in Figure 4C(Tzounopoulos et al., 1998). Accordingly, pretreatment of theslices for at least 2 hr with KT 5720 (1 µM) completely abolishedLY354740-induced LTD at 60 min [0.8 ± 13% of baseline (n = 6)vs 25.69 ± 2.49% (n = 34); p < 0.05] (Fig. 4D). Another PKA inhibitorstructurally unrelated to KT 5720, H 89 (10 µM, applied 20 minbefore, during, and 10 min after LY354740) also caused the inhibitionof fEPSP (12.8 ± 4.82% of inhibition at 20 min; n = 15) (Fig.4E) (Lin et al., 2000), mimicking and clearly occluding mGlu2/3-LTD(9.4 ± 6.6%, n = 4 vs 25.69 ± 2.49%, n = 34; p < 0.05) (Fig. 4F).It was also found that the LCCG1-induced LTD was blocked by treatmentwith H 89 (0.2 ± 8.6%; n = 3; p < 0.05; data not shown). Fromthis set of experiments, it was concluded that activation of mGlu2/3-LTDat the NAc synapses involved the cAMP-PKA cascade. More specifically,the data suggested that mGlu2/3 activation induced LTD via thereduction of PKAactivity.

At the mossy fiber synapses, both LTD and LTP are cAMP-PKA mediated (Weisskopf et al., 1993; Huang et al., 1994; Tzounopouloset al., 1998). In contrast, we found that, in experimental conditionsfavoring the occurrence of LTP (i.e., in the presence of mGlu2/3antagonist), the PKA-inhibitor KT 5720 had no effect on the tetanus-inducedLTP (LTP was observed in three of eight slices in control andfive of eight with KT 5720; p = 0.31; Fisher's exact test; datanot shown), suggesting that modulation of the cAMP-PKA cascadeis important to presynaptic LTD but not toLTP.

Role of Ca²⁺ channels in mGlu2/3-LTD

What is the locus of expression of mGlu2/3-LTD? Previous studies have suggested preferential interactions between mGlu2/3and high-voltage-activated (HVA) Ca²⁺ channels (Chavis et al., 1994; Glaum and Miller, 1995; Choi andLovinger, 1996; Stefani et al., 1996). Moreover, the influenceof the cAMP-PKA cascade on HVA Ca²⁺ currents has been clearly identified (Surmeier et al., 1995;Fukuda et al., 1996; Huang et al., 1996; Kaneko et al., 1998).Of particular interest, enhanced PKA activity was shown to potentiateN-, Q-, and P-type HVA Ca²⁺ currents (Fukuda et al., 1996; Huang et al., 1998). We reasonedthat the mGlu2/3-induced reduction of PKA activity could leadto inhibition of presynaptic HVA and reduction of synaptic efficacy.To test this hypothesis, two types of experiments were performed.We estimated the effects of selectively blocking L-, N-, or P/Q-typeHVA Ca²⁺ channels (Manzoni et al., 1997; Robbe et al., 2001) (with 1 µMnimodipine, 1 µM $omega$ -conotoxin-GVIA, or 200 nM $omega$ -agatoxin-IVA, respectively)on control synaptic transmission and on the expression of mGlu2/3-LTD.Figure 5A shows in a representative experiment that $omega$ -conotoxin-GVIA-sensitiveCa²⁺ channels (N-type) are responsible for most of the evoked transmissionin mice NAc (average fEPSP inhibition measured after 15 min of $omega$ -conotoxin-GVIA was 62.90 ± 3.62%; n = 13) (Fig. 5H) (Robbe etal., 2001). In the presence of $omega$ -conotoxin-GVIA, neither mGlu2/3initial depression nor LTD was modified (19.49 ± 5.46%, n = 8vs 25.69 ± 2.49%, n = 34 in control; p > 0.05) (Fig. 5A-D). Strikingly,bath perfusion with $omega$ -agatoxin-IVA to selectively block P/Q-typechannels reduced by 29.46 ± 7.35% (n = 5) (for a typical experiment,see Fig. 5B,H) synaptic transmission (Robbe et al., 2001) andcompletely abolished the expression of mGlu2/3-LTD (1.25 ± 4.02%,n = 8 vs 25.69 ± 2.49%, n = 34 in control; p < 0.05) (Fig. 5B-D)but not the initial depression (66.22 ± 5.11%, n = 8 vs 62.7 ±3%, n = 34 in control; p > 0.05) (for a representative experiment,see Fig. 6B). In contrast, perfusing nimodipine to selectivelyblock L-type channels (Robbe et al., 2001) had no effect on mGlu2/3-LTD(19.62 ± 6.3%, n = 4 vs 25.69 ± 2.49%, n = 34 in control; p >0.05) or initial depression (59.49 ± 5.71%, n = 4 vs 62.7 ± 3%,n = 34 in control; p > 0.05) (Fig. 5C,D).

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Figure 5. mGlu2/3-LTD is attributable to the reduction of P/Q-type Ca²⁺ channels to evoked synaptic transmission. A-D, The mGlu2/3-LTD requires P/Q-type Ca²⁺ channels. A, Typical experiment in which the slice was perfused with $omega$ -conotoxin-GVIA (1 µM). The fraction of synaptic transmission insensitive to $omega$ -conotoxin-GVIA displayed a normal form of mGlu2/3-LTD. B, Typical experiment in which the slice was perfused with $omega$ -agatoxin-IVA (200 nM). The fraction of synaptic transmission insensitive to $omega$ -agatoxin-IVA did not display mGlu2/3-LTD. C, Typical experiment in which the slice was perfused with nimodipine (1 µM). This treatment had no effect on the mGlu2/3-LTD. D, Summary of all of the experiments performed as above. The histogram of the mGlu2/3-LTD at 60 min reveals that blocking P/Q-type HVA Ca²⁺ channels suppressed mGlu2/3-LTD. E-H, P/Q-type Ca²⁺ channels do not contribute to synaptic transmission when mGlu2/3-LTD is induced. E-G, Typical experiments in which, after induction of mGlu2/3-LTD with LY354740 (200 nM), the slices were perfused with $omega$ -conotoxin-GVIA (1 µM), $omega$ -agatoxin-IVA (200 nM), and nimodipine (1 µM), respectively. H, Summary of all of the experiments performed as above. The histogram represents mean fEPSP inhibition (i.e., fEPSP contribution) induced by $omega$ -conotoxin-GVIA, $omega$ -agatoxin-IVA, and nimodipine and taken after 15-20 min of drug application. It reveals that P/Q-type Ca²⁺ channels do not contribute to synaptic transmission once mGlu2/3-LTD is induced. Conversely, N-type contribution is augmented. *p < 0.05; **p < 0.01.

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Figure 6. mGlu2/3-LTD is reduced on Ca²⁺-independent spontaneous EPSCs. A, B, Spontaneous EPSCs recorded in the absence of TTX express both acute and long-term effects of mGlu2/3 activation. A, Typical experiment. Representative consecutive 1 sec current sweeps from a cell (holding potential of $-$ 70 mV) in which sEPSCs were recorded in the absence, during, or 45 min after LY354740 (200 nM). Calibration: 30 pA, 200 msec. The distribution of sEPSC inter-event intervals was altered after bath-perfusion of LY354740. B, Mean frequency of sEPSCs was equally reduced during and 45 min after LY354740 perfusion. **p < 0.01. n.s., Not significant. C, D, Action potential-independent miniature EPSCs recorded in the presence of TTX (300 nM) express acute but reduced long-term effects of mGlu2/3 activation. C, Typical experiment. Representative consecutive 1 sec current sweeps from a cell (holding potential of $-$ 70 mV) in which mEPSCs were recorded in the absence, during, or 45 min after LY354740 (200 nM). Calibration: 30 pA, 200 msec. The distribution of mEPSC inter-event intervals was altered during application of the mGlu2/3 agonist but was back to normal after 45 min. The distribution of mEPSC amplitude was unchanged after bath perfusion of LY354740. D, Mean frequency of sEPSCs was significantly more reduced during than 45 min after LY354740 perfusion. *p < 0.05; **p < 0.01.

If mGlu2/3-LTD is expressed via the inhibition of P/Q-type HVA Ca²⁺ channels, then one expects a modification of the relative participationof these Ca²⁺ channels to evoked transmission during the plateau phase of mGlu2/3-LTD.

To test this prediction and evaluate the relative contribution of N-, P/Q-, and L-type HVA Ca²⁺ channels during mGlu2/3-LTD, LTD was first induced by bath applicationof LY354740 (10 min, 200 nM), and, at the time at which LTD hadreached its plateau, selective Ca²⁺ channels blockers were perfused. Figure 5E-H shows that the $omega$ -conotoxin-GVIAinhibition was significantly larger during mGlu2/3-LTD than incontrol conditions (83.65 ± 7.65%, n = 4 after LTD vs 62.90 ±3.62%, n = 13 in control; p < 0.05). Remarkably, $omega$ -agatoxin-IVA,which normally reduced by 29.46 ± 7.35% (n = 5) synaptic transmission,had no effect when mGlu2/3-LTD was already induced (2.25 ± 3.8%;n = 4; p < 0.05) (Fig. 5F-H). In contrast, the inhibitory effectsof nimodipine were identical during mGlu2/3-LTD and in controlconditions (respectively, 20.09 ± 5.84%, n = 3 and 15.28 ± 4.91%,n = 8; p > 0.05), excluding the participation of L-type HVA Ca²⁺ channels in the expression of LTD (Fig. 5G,H). These experimentsreinforced the idea that inhibition of presynaptic P/Q-type Ca²⁺ channels is the principal mechanisms of expression of mGlu2/3-LTD.

mGlu2/3-LTD is reduced on mEPSCs compared with sEPSCs

If mGlu2/3-LTD is mediated by the inhibition of presynaptic P/Q-type Ca²⁺ channels, one predicts that action potential-dependent, spontaneouslyoccurring EPSCs (sEPSCs) express both mGlu2/3-induced acute inhibitionand LTD, whereas action potential-independent EPSCs (mEPSCs, previouslyshown to be Ca²⁺-independent; Robbe et al., 2001) only express acute mGlu2/3-LTDacute inhibition. Figure 6, A and B, shows that LY354740 (200nM, 10 min) significantly altered the inter-event interval distributions(p < 0.05; n = 9; Kolmogorov-Smirnov test; data not shown) andreduced the mean frequency of sEPSCs during and 45 min after itsapplication: the mean frequency in control was 2.23 ± 0.44 Hzcompared with 1.01 ± 0.24 Hz during LY354740 and 1.12 ± 0.27 Hz45 min after LY354740 (n = 9; p < 0.01). Note that there was nostatistical difference between the mean frequency during applicationof LY354740 and after 45 min washout (p > 0.05; n = 9) (Fig. 6B)or between cumulative distributions (p > 0.05; n = 9; data notshown). Amplitudes of sEPSCs were not affected during these experiments:the mean amplitude in control was 17.59 ± 8.84 pA compared with18.26 ± 1.08 pA 10 min after LY354740 and 16.76 ± 0.96 pA 45 minafter washout (n = 9; p > 0.05; paired t test) or their cumulativeamplitude distributions (p > 0.05, n = 9, Kolmogorov-Smirnov test,notshown).

In marked contrast, whereas action potential-independent mEPSCs in presence of the voltage-dependent Na⁺ channel blocker TTX (300 nM) were still highly sensitive to theacute effect of LY354740, the expression of mGlu2/3-LTD was clearlyreduced. At the end of the 10 min LY354740 application, both theinter-event interval distributions (p < 0.05; n = 8) and the meanfrequency of the mEPSCs were modified (mean frequency was 2.17± 0.57 Hz in control compared with 0.91 ± 0.28 Hz during LY354740;n = 8; p < 0.01) (Fig. 6C,D). In contrast, Figure 6, C and D,shows that the acute effects of LY354740 are partially reversed45 min after LY354740 application: the mean frequency 45 min afterLY354740 was 1.63 ± 0.52 Hz compared with 0.91 ± 0.28 Hz duringLY354740 application (n = 8; p < 0.05; the cumulative distributionwas also different, p < 0.05; data not shown). Amplitudes of sEPSCswere not affected during these experiments: the mean amplitudein control was 17.29 ± 0.84 pA, 18.26 ± 1.08 pA during LY354740,and 16.76 ± 0.96 pA 45 min after LY354740 (n = 8; p > 0.05 betweenthe three conditions). Accordingly, the cumulative amplitude distributionswere also identical (p > 0.05 between the three conditions; n= 8; data not shown). These results show that TTX can reduce thelong-term effect ofLY354740.

In addition to confirming the electron microscopy observations showing the presynaptic localization of mGlu2/3 and the whole-cellexperiments on paired-pulse ratio, these experiments indicatethat different effectors mediate the acute and long-term effectsof mGlu2/3.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study describes the mechanisms of mGlu2/3-LTD at the prelimbic cortex-NAc synapses: mGlu2/3 autoreceptors cause a long-lastinginhibition of presynaptic P/Q-type Ca²⁺ channels, which is responsible forLTD.

Synapses have developed a number of strategies to modulate their gain in response to high-frequency or simply repetitive stimulation.Short-term forms of synaptic plasticity include paired-pulse andfrequency-dependent facilitation or depression (Thomson, 2000a,b;Sudhof, 2001). Noteworthy, the central role of both Ca²⁺ channels and mGlus in these regulations has been well identified(Scanziani et al., 1997; Wu and Saggau, 1997; Anwyl, 1999; Meiret al., 1999; Zucker, 1999; Cartmell and Schoepp, 2000; Parnaset al., 2000). It was not known, however, whether these local,short-living means of controlling synaptic gain were implicatedin longer-lasting forms of synapticplasticity.

Until now, there was no data concerning the final target of presynaptic mGlu2/3-LTD in the NAc or in other brain areas. Althoughreduction of Ca²⁺ channels is a classical intermediary of acute receptor-mediatedpresynaptic inhibition (Miller, 1990; Wu and Saggau, 1997), sucha mechanism has never been linked to LTD. Our finding that inhibitionof presynaptic P/Q-type Ca²⁺ channels is the principal mechanisms of expression of mGlu2/3-LTDat the prelimbic cortex-NAc synapses is in accord with the wellknown modulatory role of the cAMP/PKA cascade on HVA Ca²⁺ currents (Surmeier et al., 1995; Fukuda et al., 1996; Huang etal., 1996; Kaneko et al., 1998). It will be interesting to determinewhether a reduction of presynaptic Ca²⁺ channel contribution is a general feature of all mGlu2/3-LTD-expressingsynapses. Determining factors will certainly include the subtypesof adenylyl cyclase and Ca²⁺ channels linked to the transmitter release machinery at individualsynapses.

This study is reminiscent of a first work of our team on mGlu regulation of glutamatergic transmission in the NAc of rat (Manzoniet al., 1997). Because we focused on acute mGlu-mediated inhibitions,the LCCG1-induced long-term effects were unfortunately overlooked.Using the highly selective mGlu2/3 agonist LY354740, we have sincereproduced these results and found that, similar to the mice NAcslices, mGlu2/3-LTD can be induced in rat NAc slices: 1 hr aftera 10 min perfusion with 200 nM LY354740, the fEPSP measured 64.92± 8.53% of baseline (n = 4) (L. Kahn and O. J. Manzoni, unpublisheddata).

Synaptic activity has been shown to be negatively regulated by mGlu2/3 at many central synapses of the CNS (Kobayashi et al.,1996; Yokoi et al., 1996; Tzounopoulos et al., 1998; Anwyl, 1999;Huang et al., 1999; Lin et al., 2000). The majority of these studiesshowed the involvement of the cAMP/PKA cascade in mGlu2/3-LTD(hippocampal mossy fibers, dentate gyrus, and amygdala). Accordingly,we found that both activation of adenylate cyclases with forskolin(Seamon and Daly, 1986) and inhibition of the PKA pathway (withH 89 or KT 5720) abolished the expression of LTD. Interestingly,mGlu2/3 can be negatively (Manzoni et al., 1992; Prézeau et al.,1992) or positively coupled to the adenylate cyclases (Conn andPin, 1997), and analysis of genetically modified mice have shownthat mice with defective cAMP-dependent protein kinases displaysevere deficit in hippocampal postsynaptic LTP and LTD (Brandonet al., 1995; Qi et al., 1996). Considering our observations thatelevation of cAMP levels enhances NAc-fEPSP (present report, Manzoniet al., 1998; Robbe et al., 2001) and that PKA inhibitors alonereduce NAc synaptic transmission (present report; Tzounopouloset al., 1998; Lin et al., 2000), it was concluded that inhibitionof PKA activity is a necessary early step of mGlu2/3-LTD. In allcases, our data show the crucial role of the cAMP-PKA cascadein mGlu2/3-LTD at the prelimbic cortex-NAcsynapses.

In conditions favoring the induction of LTP (i.e., in the presence of mGlu2/3 antagonist), it was found that LTP was completelyblocked by NMDAR antagonist, confirming previous reports of apostsynaptic NMDAR-dependent LTP (three of eight slices in thepresence of LY341495 alone vs zero of six in LY341495 and MK801)(Pennartz et al., 1993; Kombian and Malenka, 1994). Together withthe lack of effect of KT 5720 on the tetanus-induced LTP, ourstudy indicates that modulation of the cAMP-PKA cascade is importantto presynaptic LTD but not to LTP. Thus, unlike the mossy fibersynapses that exhibit both presynaptic cAMP-PKA-mediated LTD andLTP (Weisskopf et al., 1993; Huang et al., 1994; Tzounopouloset al., 1998), it is conceivable that prelimbic cortex-NAc synapsesare not capable of expressing activity-dependent forms of LTPin response to increased PKA activity. However, considering thatwe consistently observed synaptic enhancement in response to forskolinapplication (present study; Manzoni et al., 1998; Robbe et al.,2001), another interpretation is that the experimental conditions(tetanus, external Ca²⁺ levels, temperature, etc... . ) were inadequate to activate thecAMP/PKA-dependent enhancingcascade.

Extending the pioneer study of Pennartz et al. (1993) who showed that tetanizing prelimbic cortex-NAc synapses induced a mixtureof LTP, LTD, or no change in synaptic efficacy, we found thatsimple antagonism of mGlu2/3 turns "indecisive synapse" into LTP-expressingones. What can explain the apparent discrepancy with Kombian andMalenka (1994) who reported an overall increase of fEPSPs duringtetanic stimulation of prelimbic cortex afferents, whereas weobserved an overall LTD of excitatory synapses (Fig. 1)? The choiceof species (rat vs mice), the age of the animals, and more importantlythe stimulation protocols might be of importance: we repeatedthe 1 sec 100 Hz tetanus three times, whereas Kombian and Malenkaonly applied it once. It is possible that a single tetanus, whichis unable release sufficient glutamate to activate presynapticmGlu2/3 receptors and induce presynaptic LTD, still allows theinduction of postsynaptic NMDAR-dependentLTP.

Recently, evidences have been provided that glial cells contribute to the regulation of synaptic transmission by controllingglutamate concentration in the extracellular space (Rothsteinet al., 1996; Oliet et al., 1997; Bergles and Jahr, 1998). Similarto what we observed in the NAc, the occurrence of mGlu2/3 on thelimiting membrane of glial processes enwrapping axon terminalshas been described in a number of brain regions (Petralia et al.,1996; Mineff and Valtschanoff, 1999). In the NAc, the functionsof glial mGlu2/3 receptors remain to be determined, and it ispossible that these receptors contribute to synaptic transmissionand plasticity: mGlu2/3 may regulate glial glutamate transportersand affect extracellular glutamate levels. In all cases, the involvementof P/Q-channels in mGlu2/3-LTD indicates a predominant role ofneuronal mGlu2/3 in LTD of the prelimbic cortex-NAcsynapses.

How are mGlu2/3 and in particular mGlu2/3-LTD involved in the functions of the nucleus accumbens? The therapeutic potentialsof mGlu2/3 drugs might provide indications in this regard. Itis indeed intriguing that agonists of these receptors reduce withdrawalsyndromes from nicotine (Helton et al., 1997) and opiates (Fundytusand Coderre, 1997; Fundytus et al., 1997) have anxiolytic properties(Helton et al., 1998) and can modulate drug-evoked behaviors (Cartmellet al., 1999, 2000a,b). Interestingly, chronic morphine treatmentaugmented mGlu-induced inhibition of neurotransmission in nucleusaccumbens and the ventral tegmental area (Manzoni and Williams,1999; Martin et al., 1999). Together with the importance of mGlu2/3in controlling synaptic plasticity at the prelimbic cortex-NAcsynapses, these observation reinforce the idea that mGlu2/3 canparticipate in drug-related behaviors andaddiction.

  FOOTNOTES

Received Nov. 9, 2001; revised March 7, 2002; accepted March 11, 2002.

The work in the laboratory of O.J.M. was supported by grants from Mission Interministérielle de Lutte contre la Drogue etla Toxicomanie and Ministère de la Recherche (Les Actions ConcertéesIncitatives Jeunes Chercheurs). We thank Dr. P. M. Lledo and Dr.P. Castillo for critical reading of this manuscript, M. Passamafor the artworks, and Dr. Monn and Dr. Shoepp at Eli Lilly (Indianapolis,IN) for their generous gift of LY-354740.

Correspondence should be addressed to Dr. O. Manzoni, Centre National de la Recherche Scientifique Unité Propre de Recherche9023, 34094 Montpellier Cedex 5, France. E-mail: manzoni{at}ccipe.montp.inserm.fr.

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