Presynaptic Effects of NMDA in Cerebellar Purkinje Cells and Interneurons

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The Journal of Neuroscience, January 15, 1999, 19(2):511-519

Presynaptic Effects of NMDA in Cerebellar Purkinje Cells and Interneurons
M. Glitsch and A. Marty
Arbeitsgruppe Zelluläre Neurobiologie, Max-Planck-Institut für biophysikalische Chemie, 37077, Göttingen, Germany

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

NMDA receptors (NMDARs) are generally believed to mediate exclusively postsynaptic effects at brain synapses. Here we searchedfor presynaptic effects of NMDA at inhibitory synapses in ratcerebellar slices. In Purkinje cells, application of NMDA enhancedthe frequency of miniature IPSCs (mIPSCs) but not that of miniatureEPSCs (mEPSCs). This increase in frequency was dependent on theexternal Mg²⁺ concentration. In basket and stellate cells, NMDA induced aneven larger mIPSC frequency increase than in Purkinje cells, whereasmEPSCs were again not affected. Moreover, NMDA induced an inwardcurrent in both types of interneuron, which translated into asmall depolarization (~10 mV for 30 µM NMDA) under current-clampconditions. In paired recordings of connected basket cell-Purkinjecell synapses, depolarizations of 10-30 mV applied to the basketcell soma enhanced the frequency of postsynaptic mIPSCs, suggestingthat somatic depolarization was partially transmitted to the terminalsin the presence of tetrodotoxin. However, this effect was smalland unlikely to account fully for the effects of NMDA on mIPSCs.Consistent with a small number of dendritic NMDARs, evoked EPSCsin interneurons had a remarkably small NMDA component. EvokedIPSCs at interneuron-interneuron synapses were inhibited by NMDA,and the rate of failures was increased, indicating again a presynapticsite of action. We conclude that activation of NMDARs in interneuronsexerts complex presynaptic effects, and that the correspondingreceptors are most likely located in the axonal domain of thecell.

Key words: cerebellum; GABA; NMDA; presynaptic receptors; axon; stellate cell; basket cell

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Postsynaptic NMDA receptors (NMDARs) play a fundamental role in synaptic transmission in the brain, where they mediate analmost ubiquitous component of excitatory synaptic currents (Collingridgeet al., 1988; Hestrin et al., 1990) and where they participatein diverse processes such as neuronal plasticity (Collingridgeand Singer, 1990) and neurotoxicity (Meldrum and Garthwaite, 1990).By contrast, presynaptic actions of NMDARs are far less welldocumented.

Several recent reports provide immunohistochemical evidence for NMDARs on presynaptic terminals (e.g., in the visual cortex:Aoki et al., 1994; DeBiasi et al., 1996; in the spinal cord: Liuet al., 1994; in the cerebellum: Petralia et al., 1994; in theamygdala: Farb et al., 1995). This raises the intriguing possibilitythat, in addition to its well characterized postsynaptic actions,NMDARs might also regulate neurotransmitter release. Indeed thereis evidence that NMDAR activation can increase the release ofnoradrenaline (Pittaluga et al., 1990; Wang et al., 1992) andof dopamine (Krebs et al., 1991; Wang, 1991) in synaptosomes.At neuromuscular synapses from Xenopus in culture, glutamate,kainate, or NMDA has been shown to enhance transmitter releaseby activation of axonal receptors. This effect was resistant toaddition of tetrodotoxin (TTX; Fu et al., 1995). In the spinalcord of the lamprey, inward currents reflecting the activationof both AMPA-selective receptors and of NMDARs were obtained inaxonal recordings; these currents may correspond to the activationof receptors of axo-axonal synapses (Cochilla and Alford, 1997).In mammalian brain slices, there have been a few reports of presynapticeffects of ionotropic glutamate receptor agonists on synapticcurrents (for review, see McGehee and Role, 1996; see furtherreferences in Discussion). In the entorhinal cortex, applicationof the selective NMDAR antagonist D-APV leads to a decrease inthe frequency of miniature EPSCs (mEPSCs) (Berretta and Jones,1996), indicating a facilitatory presynaptic role for NMDARs.Despite these scattered reports, however, the physiological significanceof presynaptic NMDARs has remained largelyunexplored.

In Purkinje cells of rat cerebellar slices, bath application of NMDA lead to an increase in the frequency of spontaneous inhibitorysynaptic currents (Farrant and Cull-Candy, 1991; Llano et al.,1991). However, just how NMDA accomplished this was not investigated.If, as commonly assumed, such effects were caused by the increasein the firing of presynaptic neurons after activation of "postsynaptic"(somatodendritic) receptors, then they should be abolished byapplication of TTX. In a recent study of presynaptic metabotropicglutamate receptors at inhibitory synapses onto Purkinje cells,we noticed that the unspecific glutamatergic agonist L-AP3 increasedthe frequency of spontaneous IPSCs, that this effect was blockedby the specific NMDAR antagonist APV, and that it was resistantto the application of TTX (Glitsch et al., 1996). These resultsimplied that NMDA could exert a presynaptic action at this synapse.Here we investigate this possibilityfurther.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Tissue preparation. Sagittal cerebellar slices were prepared from rats aged 12-14 d, after the procedure described by Llanoet al. (1991). Briefly, rats were decapitated after cervical dislocation,and the cerebellar vermis was dissected out and glued to the stageof a vibroslicer after a cooling period of 2-4 min in ice-coldbicarbonate-buffered saline (BBS; see composition below). Slicesof 180-200 µm thickness were consequently cut and incubated inoxygenated BBS at 31-33°C for at least 45 min before their usein electrophysiologicalrecordings.

Electrophysiological recordings. Tight-seal whole-cell recordings were obtained from Purkinje cells and interneurons as explainedin Llano et al. (1991) and Llano and Gerschenfeld (1993). Duringexperiments, slices were visualized through a 63× water immersionobjective. Basket and stellate cells were differentiated on thebasis of their position within the molecular layer: interneuronsin the lower third were considered basket cells, and those inthe upper two thirds were considered stellate cells (Palay andChan-Palay, 1974).

The cell surface was not cleaned before recording. Experiments were performed with an EPC-9 patch-clamp amplifier (Heka Electronics,Lambrecht, Germany) and an additional EPC-7 patch-clamp amplifier(List Medical, Darmstadt, Germany) in the case of paired recordings.Patch-clamp pipettes had resistances of 2-2.5 M $Omega$ (Cs⁺-containing internal solution for recordings from Purkinje cells;see composition below) or of 4-5 M $Omega$ (K⁺-containing internal solution for recordings from interneurons;see composition below). Pipettes were coated with dental wax toreduce the input capacitance during recording. Cancellation ofcapacitive current and series resistance compensation (~70%) wereperformed for Purkinje cell recordings as described in Llano etal. (1991). Experiments were abandoned when series resistanceincreased >12 (Purkinje cells) or 20 M $Omega$ (interneurons) or whenthe holding current exceeded $-$ 500 (Purkinje cells) or $-$ 70 pA (interneurons),measured at a holding potential of $-$ 60 mV. For current-clamp experiments,a holding current was applied such that the resting potentialwas $-$ 60mV.

Paired recordings. For paired recordings, a whole-cell recording was first established on a Purkinje cell. Cell-attached recordingswere then obtained for one or several basket cells located within50 µm (distance measured between somata centers) of the Purkinjecell. Spontaneous action potentials (Llano and Gerschenfeld, 1993)were monitored from the basket cell, and if a functional connectionwas observed, presynaptic and postsynaptic signals were recordedfor 1-2 min. The experiment proceeded by addition of TTX to thebath, which resulted in a loss of presynaptic action potentials.In TTX-containing BBS, the whole-cell configuration was also establishedin the basket cell. From a holding potential of $-$ 60 mV, repetitivecycles of 1-sec-long depolarizing steps were applied to the basketcell immediately afterward, and the corresponding miniature IPSCs(mIPSCs) were registered in the Purkinje cell. After breakinginto the basket cell, recordings never exceeded 10 min. This procedureallowed to minimize the rundown of the synaptic connection thatoccurs at this synapse after the onset of presynaptic whole-cellrecording (Vincent and Marty, 1996).

Evoked IPSCs and EPSCs. Evoked IPSCs and EPSCs were obtained in interneurones using a saline-filled pipette as stimulationelectrode. Voltage pulses (20-90 V; duration, 0.4 msec; rate,0.33-0.5 Hz) were applied between the pipette interior and a platinumelectrode coiled around the pipette. To obtain evoked IPSCs, thestimulation pipette was positioned in the molecular layer, ~100µm away from the recorded cell, and the bath was perfused withNBQX. To obtain evoked EPSCs, the stimulation pipette was positionedin the granule cell layer, ~50 µm away from the Purkinje celllayer, and the bath was perfused withbicuculline.

In the analysis of evoked IPSCs (see Fig. 8), failure rates were determined by counting events with an onset occurring duringa time window that was determined empirically from the controldata (typically, 1-4 msec after each stimulationartifact).

Analysis. Miniature synaptic currents were analyzed off-line using an event-detection routine. Detection thresholds were adjustedbetween 8 and 15 pA for both Purkinje cells and interneurons,depending on the noise of the recording. In experiments performedon Purkinje cells, the ionotropic glutamate antagonist NBQX (seebelow) was added to the saline to block mEPSCs. NBQX was not includedin miniature current recordings on interneurons, so that in theseexperiments mEPSCs were recorded together with mIPSCs. However,the decay kinetics of mEPSCs are much faster than that of mIPSCs(Llano and Gerschenfeld, 1993), allowing unambiguous distinctionof the two classes of events duringanalysis.

Paired recording experiments started with an initial period during which the presynaptic interneuron was recorded with thecell-attached configuration. To analyze the results of this firstpart, presynaptic action currents were identified using a spikedetector. Postsynaptic traces were aligned with respect to thespikes and were averaged to calculate the mean amplitude of evokedIPSCs.

Statistical deviations from mean values given in the text, and error bars in figures, indicate ± SEM across experiments, nbeing the number ofexperiments.

Bath perfusion. The recording chamber was perfused at a rate of 1-1.5 ml/min with BBS. Experiments were performed at roomtemperature (22-25°C).

To examine the effect of a drug or a modified external solution on miniature synaptic currents, membrane currents were recordedover a control period of 3 min in BBS, then the bath was exchangedto the test solution. After a period of 3-4 min to allow completebath exchange, data acquisition was resumed. Recordings were typicallyof 3 min duration under each experimental condition. Only onecell per slice was used to circumvent possible long-term effectsof the drugsused.

Solutions and drugs. The standard external solution (BBS) contained (in mM): 125 NaCl, 2.5 KCl, 2 CaCl₂, 1 MgCl₂, 1.25 NaH₂PO₄,26 NaHCO₃, and 10 glucose, pH 7.4 when equilibrated with a mixtureof 95% O₂ and 5% CO₂. In experiments in which the effect of extracellularMg²⁺ on NMDA-induced synaptic currents was investigated, either theexternal solution contained no MgCl₂ or the concentration wasraised to 8 mM MgCl₂ without changing any othercomponent.

The intracellular solution for Purkinje cells consisted of (in mM): 150 CsCl, 10 HEPES, 1 EGTA 0.1 CaCl₂, 4.6 Na-ATP, 0.4Na-GTP, and 4.6 MgCl₂. The internal solution for interneuronswas the same, except that 150 mM CsCl was substituted by 150 mMKCl. The pH was set to 7.3 with CsOH or KOH,respectively.

NMDA, ( $-$ )-bicuculline methochloride (bicuculline), 6-nitro-7-sulfamoylbenzo[f]quinoxaline-2,3-dione (NBQX), and D( $-$ )-2-amino-5-phosphonopentanoicacid (D-APV) were obtained from Tocris Cookson (Bristol, UK).CGP 62349 was kindly provided by Ciba Geigy. All other drugs andchemicals were purchased from Sigma (St. Louis, MO). Drug stockswere prepared as follows: 100 mM NMDA, 10 mM D-APV, and 1 mM NBQXin equimolar NaOH; 10 mM CGP 62349 in DMSO; and 1 mM bicucullinein H₂O. TTX was purchased as 1 mg aliquots containing 5 mg citratebuffer; 0.2 mM stocks were prepared in H₂O. Stocks were aliquoted,frozen, and dissolved daily in BBS to reach the desiredconcentration.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

NMDAR activation leads to an increase in the frequency of mIPSCs in Purkinje cells

mIPSCs were recorded in Purkinje cells dialyzed with a high intracellular Cl concentration solution at a holding potential of $-$ 60 mV. Amplitudesranged from ~10 pA to several hundreds of pA (Fig. 1A, top leftpanel). In these experiments, Na⁺-dependent action potentials and glutamatergic synaptic currentswere blocked, respectively, with 0.2 µM TTX and 10 µM NBQX. Underthese conditions, bath-application of 15 µM NMDA led to a massiveincrease in the frequency of mIPSCs (top right panel). In agreementwith previous work (Llano et al., 1991), there was no effect ofNMDA on the holding current of the Purkinje cell.

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Figure 1. NMDAR activation increases the mIPSC frequency in Purkinje cells. A, Top two traces show mIPSCs recorded from a representative Purkinje cell under control conditions (left) and in the presence of 15 µM NMDA (right). Bottom traces, After washing NMDA, the bath was perfused with a solution containing 50 µM D-APV. Further addition of 15 µM NMDA did not alter the pattern of mIPSCs. B, Pooled results from seven experiments. In the absence of 50 µM D-APV, 15 µM NMDA leads to a 141 ± 45% increase in the frequency of mIPSCs. In the presence of 50 µM D-APV, the increase in the frequency is almost completely blocked (15 ± 4%). All experiments were performed in the presence of 0.2 µM TTX and 10 µM NBQX.

The specific NMDAR antagonist D-APV blocked the NMDA-induced frequency increase (Fig. 1A, bottom panel). Figure 1B shows pooleddata from seven NMDA-treated Purkinje cells in the absence andpresence of D-APV. NMDA induced a large and consistent frequencyincrease, and this effect was reduced almost 10-fold in the presenceof 50 µM D-APV. These results indicate that activation of NMDARsresults in an increase in the frequency of mIPSCs in Purkinjecells.

Application of D-APV slightly decreased the frequency of mIPSCs (to 82 ± 5% of the control, n = 9; Fig. 2). In six of ninecells, this decrease was statistically significant (Kolmogorov-Smirnovtest; p < 0.05), whereas there was no significant change in theremaining three cells. The mean amplitude of mIPSCs was not modifiedby D-APV (mean ratio to the control, 95 ± 6%; n = 9). These resultsindicate that a tonic activation of NMDARs, caused by backgroundglutamate, may permanently enhance the rate of miniatures.

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Figure 2. D-APV reduces the frequency of mIPSCs in Purkinje cells. A, Raw traces, showing mIPSCs under control conditions (left, 0.2 µM TTX + 10 µM NBQX) and after addition of 50 µM D-APV (right). B, After addition of D-APV, the cumulated amplitude histogram is not modified (left), whereas the cumulated interval histograms indicate a change to a lower event frequency (right). Same cell as in A. Total number of events (5 min recording periods in each condition): 831 in control saline, and 615 in the presence of D-APV. Mean amplitudes: 166 pA in control, and 170 pA in D-APV.

NMDA primarily enhances the frequency of small mIPSCs

Close inspection of the traces in Figure 1A and in similar experiments suggested that the NMDA-induced frequency increaseconcerned primarily small amplitude mIPSCs, whereas large amplitudemIPSCs were less affected. To quantify this effect, we comparedthe cumulated amplitude distributions of mIPSCs in control conditions(in the presence of TTX and NBQX) and after addition of NMDA.Figure 3 illustrates pooled amplitude histograms from all sevencells in control conditions (Fig. 3A), in NMDA (Fig. 3B), andfor the difference events (NMDA-induced events; Fig. 3C). Cleardifferences can be seen in the corresponding cumulative histograms(Fig. 3D). In individual experiments, cumulative distributionsof mIPSC amplitudes in the presence and absence of NMDA were statisticallysignificant in six of seven cells (Kolmogorov-Smirnov test; p< 0.01). On average, NMDA decreased the mean current amplitudeto 86 ± 4% of control values (n = 7).

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Figure 3. NMDAR activation preferentially increases the frequency of small events. A, Average amplitude distribution of mIPSCs of seven cells under control conditions (0.2 µM TTX and 10 µM NBQX). Histograms were taken from 3-min-long recordings and were normalized to the total number of events. Bin width is 10 pA. B, Normalized average amplitude distribution of mIPSCs of the same cells in the presence of 15 µM NMDA. C, Normalized average amplitude distribution of NMDA-induced events, obtained by subtracting the distributions in NMDA from the control ones. D, Comparison of integrals of the plots in A-C (cumulative amplitude histograms). NMDA-induced events are on average smaller than control events.

NMDA selectively enhances GABA release

The finding that NMDA selectively enhanced the frequency of small miniature synaptic currents was rather unexpected. In viewof the recent demonstration of glycinergic currents in cerebellarGolgi cells (Dieudonné, 1995), the possibility was consideredthat NMDA was recruiting a previously unrecognized non-GABAergic,nonglutamatergic input to Purkinje cells. Therefore, the effectsof NMDA were reinvestigated in the presence of bicuculline. Totest simultaneously for possible effects of NMDA on mEPSCs, NBQXwas omitted from these experiments. mEPSCs recorded in the presenceof bicuculline had a mean amplitude of 29 ± 3 pA (n = 7). Additionof NMDA under these conditions did not lead to any modificationin mEPSC amplitude, nor to any increase in activity (control,8 ± 2 mEPSCs/min; in NMDA, 6 ± 3 mEPSCs/min; n = 7). After washingout bicuculline, NMDA evoked an increase in mIPSC frequency, confirmingthat NMDA was effective (n = 3). These results confirm that NMDA-inducedevents are GABAergic, and they show that the frequency increaseis specific of inhibitorysynapses.

Mg²⁺ dependence of NMDA effect

It is well established that NMDA channels are blocked in a voltage-dependent manner by Mg²⁺ (Mayer et al., 1984; Nowak et al., 1984). All experiments describedso far were performed in the presence of 1 mM Mg²⁺. To investigate the Mg²⁺ dependence of the NMDA effect, we established dose-response curvesfor NMDA in external solutions containing different concentrationsof Mg²⁺. As the extracellular Mg²⁺ concentration increased, the stimulatory effect of NMDA on synapticactivity was reduced (Fig. 4).

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Figure 4. Mg²⁺ dependence of NMDA effect. Plot of NMDA-induced increase in mIPSC frequency in Purkinje cells in different external Mg²⁺ concentrations. Open circles, 0 mM Mg²⁺; gray circles, 1 mM Mg²⁺ (normal BBS); black squares, 8 mM Mg²⁺. For 0 Mg²⁺, only two NMDA concentrations were tested. Experiments were performed in the presence of 0.2-0.5 µM TTX and 10 µM NBQX (n = 3-7).

NMDA enhances the mIPSC frequency in interneurons

Purkinje cells receive inhibitory inputs from interneurons of the molecular layer, basket, and stellate cells (Llinas andWalton, 1990). It is therefore likely that the increase in mIPSCsobserved in Purkinje cells was the result of NMDA acting on receptorslocated on these interneurons. Interneurons not only contact Purkinjecells but also make inhibitory contacts with each other (Palayand Chan-Palay, 1974). Because the effects of NMDA on Purkinjecell IPSCs were apparently presynaptic, it seemed plausible thatinterneuron-interneuron synaptic contacts would be influencedas well. NMDA (30 µM) increased the frequency of mIPSCs in bothstellate and basket cells (Fig. 5A,B). The frequency ratio overcontrol values was 24.1 ± 10.6 in basket cells (n = 6) and 21.7± 3.4 in stellate cells (n = 5) (pooled data, 23.0 ± 5.8; n =11), and thus about fourfold bigger than in Purkinje cells (5.6± 1.3). This suggests that interneuron-interneuron synapses aremore sensitive to NMDAR activation than Purkinje cell-interneuronsynapses. Figure 5C shows the amplitude distribution of mIPSCsfor the same stellate cell as shown in A under control conditions(0.2 µM TTX) and in the additional presence of 30 µM NMDA. Onaverage, both basket and stellate cells showed a slight, statisticallyinsignificant mean amplitude increase in the presence of 30 µMNMDA when compared with control (ratio of mean amplitude in 30µM NMDA and control, 1.15 ± 0.24; n = 11; six basket cells andfive stellate cells). Thus, the decrease in miniature size observedin Purkinje cells was not reproduced in interneurons.

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Figure 5. NMDA enhances synaptic activity in stellate and basket cells. A, Synaptic currents recorded from a representative stellate cell under control conditions (0.2 µM TTX, left trace) and in additional presence of 30 µM NMDA (right trace). B, Same as A, except that the recorded cell was a basket cell. Dotted lines in right traces in A and B indicate control holding current to show the NMDA-induced inward current in interneurons (26 and 24 pA, respectively). C, Amplitude distribution of mIPSCs of same stellate cell as in A under control conditions (0.2 µM TTX, left) and in additional presence of 30 µM NMDA (right). Three minute recordings were used for each histogram. Ratio of mean amplitudes in NMDA-control, 1:3.

To determine whether NMDA had a potentiating effect on mEPSCs in interneurons, we looked at the number of mEPSCs in 15 µMbicuculline and compared it with the frequency of excitatory currentsin 15 µM bicuculline +30 µM NMDA. The control number of mEPSCsduring a 3 min recording in bicuculline was 12 ± 3, and therewas no difference to the number of mEPSCs recorded in the additionalpresence of NMDA (13 ± 2), suggesting that NMDA did not have anystimulatory effect on glutamate release (n = 10; six of whichwere stellatecells).

NMDA induces inward current and somatic depolarization in interneurons

In the above experiments examining the effects of NMDA on mIPSCs in interneurons, NMDA was found to reversibly induce an inwardcurrent (Fig. 5). To rule out the possibility that this currentcould be a consequence of an activation of GABA_A receptors, becauseof the higher rate of mIPSCs in NMDA, we performed NMDA applications(30 µM) in the presence of 15 µM bicuculline. Under these conditionsthere was still a clear inward current response (14 ± 3 pA; n= 10 cells, six of which were stellate cells), suggesting thatthe inward current was directly due to activation of NMDARs inthe recordedcells.

Membrane potential changes associated with the NMDA-induced current were measured under current clamp in the presence of 0.2µM TTX. Experiments were performed both in the presence and absenceof bicuculline; no significant difference was found between thetwo conditions. Overall, application of 30 µM NMDA induced a depolarizationof 11 ± 1 mV (n = 16; pooled data of stellate and basket cellswith or without bicuculline). There was no sign of regenerativevoltage signals superimposed on thesedepolarizations.

Can electrotonic spread of somatic depolarization account for the enhancement in mIPSC frequency by NMDA?

The results obtained so far do not allow to specify whether the NMDARs responsible for the increase in the frequency of mIPSCsare located in the axon or in the somatodendritic compartmentof the presynaptic interneurons. The fact that the frequency ofmIPSCs was enhanced suggested at first sight an axonal location.However, we also considered the alternative hypothesis that theenhancement of mIPSC frequency would be secondary to activationof somatodendritic NMDARs in the presynaptic cells. Because thedistance between soma and terminals is short in interneurons,this depolarization could be transmitted to the terminals despitethe presence of TTX, as previously shown for Cs⁺-dialyzed cells (Vincent and Marty, 1996; Llano et al., 1997).Therefore, we next performed paired recordings between presynapticbasket cells and postsynaptic Purkinje cells to test if a somaticdepolarization of the basket cell could lead to an increase inthe mIPSC frequency in the Purkinjecell.

The experiments were performed on a series of seven connected basket cell-Purkinje cell pairs. In a first part of each experiment,the spontaneous firing of the presynaptic basket cell was monitoredin the cell-attached configuration while the evoked IPSCs wereregistered with whole-cell recording (Fig. 6A1,A2). The averageevoked IPSC was 43 pA in the example shown. This average valuetimes the number of presynaptic action potentials was used todetermine the "weight" of the connection (in this case, 2.4%)by comparing it to the cumulative amplitude of all IPSCs recordedin the Purkinje cell over the same time period. Then TTX was addedto the bath, leading to a loss of presynaptic action potentials.In TTX, a whole-cell recording was established in the basket cell,and 1 sec-long depolarizing steps were applied up to $-$ 30 mV tothe presynaptic soma. Although no clear response could be distinguishedin individual sweeps (Fig. 6B), on average the frequency of mIPSCswas correlated to the presynaptic steps (Fig. 6C; in the pairedrecording shown the frequency at $-$ 30 mV is 1.44 times higher thanat $-$ 60 mV, and this ratio is statistically different from 1 withp < 0.001). The same trend, albeit weaker, was found in each ofthe other cases. Figure 6D shows summary results for the sevenexperiments. At $-$ 30 mV, the frequency ratio was on average 1.18± 0.06 (n = 7; p < 0.05; test performed across experiments), butat $-$ 50 mV (roughly corresponding to the 11 mV depolarization measuredwith 30 µM NMDA), the ratio was only 1.08 ± 0.05. As will be furtherdiscussed below, such small changes are unlikely to underlie theeffects of NMDA on mIPSCs.

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Figure 6. In TTX, somatic depolarization of an interneuron increases the mIPSC frequency in a postsynaptic Purkinje cell. All data obtained from paired recordings with presynaptic basket cells (BC) and postsynaptic Purkinje cells (PC). A-C are from the same pair. A1, Average of spikes recorded in the basket cell in cell-attached mode. A2, Superimposed IPSCs recorded in the Purkinje cell. B, Results obtained after superfusion with 0.2 µM TTX, shortly after breaking into the basket cell. Top trace shows the presynaptic depolarization protocol (repetitive cycles from $-$ 60 to $-$ 30 mV in 10 mV steps, holding for 1 sec at each potential). Gray and black traces show corresponding current trace recorded in the basket and Purkinje cell, respectively. C, Average mIPSC frequencies in the Purkinje cell (n = 100 1 sec segments) for each 1 sec segment, plotted against the somatic potential of the basket cell. D, Pooled data from seven pairs. Data in D were normalized to the number of events at a presynaptic holding potential of $-$ 60 mV.

The NMDA component of evoked EPSCs in interneurons is small

The amount of current elicited by bath applications of NMDA in interneurons seemed quite modest, as if few NMDARs residedon the dendritic tree. At all glutamatergic excitatory synapsesinvestigated in the brain so far, with the only exception of parallelfiber EPSCs and climbing fiber EPSCs onto Purkinje cells, NMDAchannels are responsible for a large part of the synaptic currentsat positive potentials. The ratio of the peak current carriedby NMDARs to that carried by AMPA receptors can be estimated bymeasuring at positive potentials the current during two time windows,one positioned 20-30 msec after the response onset, correspondingto the NMDA component, and the other a few msec after the responseonset, corresponding to the AMPA component (Fig. 7). When applyingthis method to evoked EPSCs in interneurons, we found a mean ratioof the NMDA component to the AMPA component of 0.054 ± 0.026 (n= 4). As shown in Figure 7, the identification of both componentswas confirmed by their respective sensitivity to D-APV and NBQX.These experiments show that, at excitatory synapses onto interneurons,the contribution of NMDA receptors to the total current is minimal.From a survey of similar results obtained on a number of mammalianbrain synapses, it appears that the proportion of the NMDA componentis markedly lower at interneurons than at any other preparationexcept for Purkinje cells. In the other synapses, the ratio ofthe NMDA component to the AMPA component ranged from ~0.3 (inmedial septal neurons: Schneggenburger et al., 1992) to ~2.0 (asfor instance in stellate cells of the visual cortex: Stern etal., 1992). Thus, the strength of the NMDA contribution is 6-37times lower at cerebellar interneuron synapses than in other synapses,and the number of NMDA receptors at somatodendritic postsynapticsites appears indeed to be unusually low.

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Figure 7. The NMDA component of interneuron EPSCs is weak. EPSCs were evoked in an interneuron by extracellular stimulation in the granule cell layer. A, At $-$ 60 mV, EPSCs had rapid decay kinetics, fluctuated markedly among trials, and displayed a fair amount of jitter in their onsets. At +60 mV, only hints of a late component could be obtained in single traces. This component was insensitive to NBQX (10 µM) but was blocked by further addition of D-APV (20 µM). All solutions used contained 15 µM bicuculline to block IPSCs. All four panels show five superimposed traces in each condition. B, Average traces at $-$ 60 mV in control conditions (bicuculline alone; thick black line), at +60 mV in control conditions (middle gray line), at +60 mV in the presence of NBQX (thin black line), and at +60 mV after further addition of APV (light gray line). The inset shows the traces at +60 mV with enlarged vertical scale and slow time base. At +60 mV, the peak currents of the AMPA and NMDA components are 59 and 2.4 pA, respectively, with a ratio of 25-fold. Stimulation artifacts have been clipped off.

NMDA inhibits evoked IPSCs in interneurons

The finding of an enhanced rate of mIPSCs suggests that NMDA has a stimulatory action at interneuron synapses. However, pastinvestigations have shown that evoked currents may be regulateddifferently from miniature currents (see Kondo and Marty, 1998,and further references within). The effects of NMDA were thereforeinvestigated on evoked currents in interneuron-interneuron synapses.Evoked IPSCs were obtained after extracellular stimulation withinthe molecular layer in the presence of NBQX. In all cases, NMDAapplication (15 µM) resulted in a large increase in the rate ofspontaneous IPSCs, from 3.1 ± 1.6 Hz to 14.3 ± 2.3 Hz, similarto that previously observed in Purkinje cells (Farrant and Cull-Candy,1991; Llano et al., 1991). Frequency ratios ranged from 2 to 280in individual experiments, with a geometric mean of 17. Becausewe were concerned that the increase in background activity mayhave led to the activation of GABA_B receptors and, hence, to aninhibition of evoked IPSCs, the potent GABA_B antagonist CGP 62349(0.5 µM; it was shown in separate experiments that this dose fullyblocked inhibitory effects of baclofen on Purkinje cell IPSCs)was included in some experiments (four of seven). Results obtainedwith and without the antagonist were similar, and are pooled togetherhereafter. In all experiments, the mean amplitude of the evokedIPSC was reduced, with a mean ratio to the control of 0.29 ± 0.13(n = 7; ratio different from 1 with p < 0.01; test across experiments).Thus, NMDA has a strong inhibitory effect on evoked IPSCs. Thisinhibition was accompanied by a clear and significant increasein the rate of failures, which on average rose from 0.41 ± 0.04in the control to 0.70 ± 0.07 in the presence of 15 µM NMDA (pairedt test; p < 0.02; Fig. 8). Therefore, the inhibition in overallIPSC size results at least in part from a reduced probabilityof release. Nevertheless, there was no systematic effect of NMDAon paired-pulse ratio (Fig. 8). The lack of effect of NMDA onpaired pulse ratio is, however, compatible with a presynapticeffect. It was earlier shown that depolarization-induced suppressionof inhibition (DSI), which is a form of presynaptic inhibition,does not involve any change of paired pulse ratio, and it wassuggested that this reflects axonal conduction block during DSI(Alger et al., 1996).

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Figure 8. NMDA reduces evoked IPSCs in interneurons. A, Superimposed representative traces (three in each top panel) in control conditions (10 µM NBQX; left), and after addition of 15 µM NMDA (right). Each trace represents the response to a stimulation pair (interval, 20 msec; stimulation frequency, 0.33 Hz). Note that addition of NMDA leads to an increase in the frequency of spontaneous IPSCs. Average responses in control conditions and in the presence of NMDA are shown in the bottom panels. Stimulation artifacts have been clipped off. B, Average failure rate results (responses to the first pulse of pairs) for seven experiments such as in A, including four cells in the presence of 0.5 µM CGP 62349 and three cells without the blocker. C, Summary data for paired-pulse ratios in control conditions and in NMDA.

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

NMDA-induced potentiation of mIPSC frequency

The principal result of this study is that NMDA increased the frequency of mIPSCs recorded in both interneurons and Purkinjecells. The frequency of mEPSCs in either cell type was not modified,and the mIPSC frequency increase was considerably larger in interneuronsthan in Purkinje cells, indicating that this action of NMDA isspecific for the nature of both presynaptic and postsynapticneurons.

In Purkinje cells, NMDA preferentially increased the frequency of small mIPSCs. This might reflect a differential NMDA-inducedpotentiation of GABA release at a distinct subset of synapsesthat mediate small synaptic currents, whereas other synapses withlarger mIPSCs are less affected by NMDA. The alternative possibility,that the change of mean mIPSC amplitude would be postsynaptic,is very unlikely because Purkinje cells do not respond to NMDAin the age group examined here (Farrant and Cull-Candy, 1991;Llano et al., 1991; Rosenmund et al., 1992; confirmed by presentstudy).

Despite abundant morphological evidence for the presence of presynaptic glutamate ionotropic receptors in brain slices, littleattention has been given to the potential functional role of suchreceptors. However, it was recently proposed that presynaptickainate receptors inhibit neurotransmitter release in the hippocampus(Chittajallu et al., 1996; Clarke et al., 1997; Rodríguez-Morenoet al., 1997). Even more recently, in the preparation used inthe present study, Bureau and Mulle (1998) found a potentiatingeffect of AMPA receptors on spontaneous IPSCs, which was resistantto the addition of TTX and which was considered as resulting fromthe activation of axonal AMPA-selective receptors. These findings,together with those of the present work, suggest that both NMDA-selectiveand AMPA-selective subtypes of ionotropic glutamate receptorsare present in the axons of cerebellar interneurons, and thatthe activation of both receptor subtypes leads to enhanced spontaneousGABA release. Interestingly, the effects of AMPA receptor activationare maximal near the age used in the present study, and they waneduring further development (Bureau and Mulle, 1998). We have nottested developmental changes in the presentstudy.

Because addition of D-APV decreases the rate of mIPSCs, the concentration of background glutamate appears sufficient to exerta tonic action on the rate of mIPSCs. Thus, one function of presynapticNMDARs could be to regulate the interneuron-induced inhibitionof Purkinje cells according to the glutamate concentration inthe molecularlayer.

Inhibition of evoked IPSCs

IPSCs evoked in interneurons after extracellular stimulation in the molecular layer were severely inhibited by NMDA (Fig.8). Thus, NMDA has opposite effects on miniature and evoked synapticcurrents, as previously found when analyzing the effects of noradrenalinein interneurons (Kondo and Marty, 1998). In other mammalian brainpreparations, it was found that activation of kainate receptorsinhibits both miniature (Rodríguez-Moreno et al., 1997) and evokedsynaptic currents (Chittajallu et al., 1996; Clarke et al., 1997;Rodríguez-Moreno et al., 1997). In the present experiments, theinhibition of evoked IPSCs was not caused by activation of GABA_Breceptors after enhanced GABA liberation, because it was insensitiveto the GABA_B blocker CGP 62349. Still, the inhibitory effect couldbe indirect, and could be caused by presynaptic GABA_A receptors,or by other neurotransmitters than GABA, such as glutamate, whichmight be liberated by NMDA. Alternatively, the inhibition couldresult directly from the activation of axonal NMDARs, which couldelevate the threshold for action potential firing, increase theprobability of transmission failure in the axon, or reduce theprobability of evoked GABA release by some other mechanisms (whichcould involve a long-lasting elevation in axonal calcium concentration).Sorting out these various possibilities is outside the scope ofthe presentwork.

Mg²⁺ dependence of NMDA effect

A characteristic trait of the NMDAR is that it is blocked by external Mg²⁺ in a voltage-dependent manner. The extent of the block dependson the composition of the NMDAR subunits (Kutsuwada et al., 1992;Monyer et al., 1992; Ishii et al., 1993; Monyer et al., 1994;Kuner and Schoepfer, 1996; Casado et al., 1996). The ratio ofthe increase of mIPSC frequency in the absence of any added Mg²⁺ and in the presence of 1 mM Mg²⁺ was about five in this study (for 10 µM NMDA; Fig. 4). This valuecompares well with the corresponding average ratio of 6.5 of currentsthrough recombinant NMDARs containing the NMDAR2C and D subunit,whereas the average of the ratio of currents through recombinantNMDARs containing the NMDAR2A and B subunit was about 17 (Ishiiet al., 1993; Monyer et al., 1994; Kuner and Schoepfer, 1996).An in situ hybridization study revealed the presence of NMDAR2Dsubunits in cells of the molecular layer that were tentativelyidentified as interneurons (Akazawa et al., 1994). NMDARs containingthe 2D subunit could therefore underlie the increase in synapticactivity that we haveobserved.

TTX-insensitive effects are not necessarily presynaptic

The usual distinction between presynaptic and postsynaptic effects in mammalian brain preparations is based on the use ofTTX, which is considered to uncouple the somatodendritic and theaxonal domains of presynaptic neurons. On this basis, any drugthat changes the frequency of miniatures in the presence of TTXis assumed to act "presynaptically", i.e., in the axonal domainof the presynapticcell.

One important assumption behind this analysis is that TTX effectively blocks the generation of action potentials in the presynapticcell. The concentration of TTX that was used in our experimentsis clearly sufficient to abolish voltage-dependent Na⁺ currents in interneurons (Llano and Gerschenfeld, 1993; presentexperiments). In addition, we verified in current-clamp conditionsthat no sign of regenerative depolarization could be obtainedin somatic recordings of interneurons either in TTX alone or afteraddition of NMDA. Therefore, interneurons are unable to fire eitherNa⁺- or Ca²⁺-dependent action potentials in the presence ofTTX.

A second, usually tacit assumption is that potential changes linked to activation of somatodendritic receptors are not passivelytransmitted to release sites in the presence of TTX. This is areasonable assumption if the distance between soma and presynapticrelease sites is large. However, a large proportion of releasesites of stellate and basket cells are located at <100 µm fromthe soma (Bishop, 1993; Pouzat and Kondo, 1996), raising the possibilityof a passive transfer of depolarization along the axon cable.Here we performed paired recordings of interneuron-Purkinje cellsynapses in TTX, and found that somatic depolarization does influencerelease sites, leading to an increase in the frequency of mIPSCs(Fig. 6). This result calls for caution in the traditional distinctionbetween presynaptic and postsynaptic effects based on the useofTTX.

Is the increase in mIPSC frequency mediated by somatodendritic or axonal NMDARs?

The finding that depolarization can be transmitted from the soma of interneurons to release sites raises the possibility thatsomatodendritic NMDARs could be responsible for the enhancementin mIPSC frequency recorded in interneurons and Purkinje cells.If this were the case, then the effects of NMDA on mIPSC frequencyshould be mimicked by depolarizing the soma of presynaptic neuronsto the same extent as in the presence of NMDA. This possibilitycan be tested by a quantitative evaluation of the results of pairedbasket cell-Purkinje cell recordings. In these experiments, wemeasured the "weight" of individual basket cell-Purkinje cellconnections as explained in Results, to estimate the part of thesynaptic input contributed by a single basket cell. The mean ofthese weights was 13%. Next we found that on average 30 µM NMDAdepolarized interneurons by 11 mV. From the data in Figure 6 thisdepolarization translates to an increase in mIPSC frequency by8%. Therefore, the 11 mV that are measured in the presence ofNMDA should induce an increase by 8/0.13 = 62% of the mIPSC frequency.Experimentally, an increase by 465% is found (Fig. 4), 7.5-foldhigher than this estimate. This discrepancy is unlikely to becaused by cell-to-cell heterogeneity, because responses to NMDAwere homogeneous within interneurons. Furthermore, because interneuron-Purkinjecell distances were minimized in paired experiments, the degreeof electrotonic coupling between soma and terminals that was measuredis certainly higher than that pertaining on average at interneuron-Purkinjecell synapses, so that the actual discrepancy must be larger thanthe estimated 7.5 factor. This indicates that the somatodendriticdepolarization resulting from the activation of NMDARs is notsufficient to account for the effects on mIPSC frequency thatare obtained. Therefore, the receptors responsible for the increasein mIPSC frequency are probably mostly located in the axonal domainof the cell. This proposal is supported by the recent findingof NMDAR immunostaining in the pinceau region of basket cell terminalsonto Purkinje cells (Petralia et al., 1994).

  FOOTNOTES

Received March 19, 1998; revised Oct. 5, 1998; accepted Oct. 19, 1998.

We thank C. Pouzat and P. Vincent for providing analysis software, and A. Fleig, A. B. Parekh, and I. Llano for comments onthismanuscript.
Correspondence should be addressed to Dr. A. Marty, Arbeitsgruppe Zelluläre Neurobiologie, Max-Planck-Institut für biophysikalischeChemie, Göttingen,Germany.

Dr. Glitsch's present address: University Laboratory of Physiology, Parks Road, Oxford OX1 3PT,UK.

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Results
Discussion
References

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