Short-Term Plasticity of Kainate Receptor-Mediated EPSCs Induced by NMDA Receptors at Hippocampal Mossy Fiber Synapses

doi:10.1523/JNEUROSCI.5182-06.2007

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The Journal of Neuroscience, April 11, 2007, 27(15):3987-3993; doi:10.1523/JNEUROSCI.5182-06.2007

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Cellular/Molecular
Short-Term Plasticity of Kainate Receptor-Mediated EPSCs Induced by NMDA Receptors at Hippocampal Mossy Fiber Synapses
Nelson Rebola,¹^,2 Shankar Sachidhanandam,¹ David Perrais,¹ Rodrigo A. Cunha,² and Christophe Mulle¹
¹Laboratoire "Physiologie Cellulaire de la Synapse," Centre National de la Recherche Scientifique Unité Mixte de Recherche 5091, Bordeaux Neuroscience Institute, University of Bordeaux 2, 33077 Bordeaux, France, and ²Faculty of Medicine, Institute of Biochemistry, Center for Neuroscience and Cell Biology of Coimbra, University of Coimbra, 3004-504 Coimbra, Portugal

   Abstract

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Kainate receptors (KARs) are heteromeric ionotropic glutamatereceptors that play a variety of functions in the regulationof the activity of synaptic networks. Little is known aboutthe regulation of the function of synaptic KARs in the brain.In the present study, we found that a conditioning activationof synaptic NMDA receptors (NMDARs) induces short-term depressionof KAR–EPSCs but not of AMPA receptor–EPSCs at synapsesbetween mossy fibers and CA3 pyramidal cells. Short-term depressionof KAR–EPSCs by synaptic NMDARs peaked at 1 s and reversedwithin 20 s, was likely induced and expressed postsynaptically,and was homosynaptic. It depended on a rise of Ca²⁺ in the postsynapticcell and on the activation of the phosphatase calcineurin thatlikely binds to the GluR6b (glutamate receptor subunit 6b) subunitsplice variant allowing the dephosphorylation of KARs and inhibitionof activity. Finally, we show in the current-clamp mode thatshort-term depression of KAR–EPSPs is induced by the coincidentdischarge of action potentials in the postsynaptic cell togetherwith synaptic stimulation. Hence, this study describes a formof short-term synaptic plasticity that is postsynaptic, dependson the temporal order of presynaptic and postsynaptic spiking,and likely affects the summation properties of mossy fiber EPSPs.

Key words: kainate receptors; short-term synaptic plasticity; NMDA receptors; mossy fiber; hippocampus

   Introduction

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Glutamatergic synaptic transmission is mediated by AMPA receptors(AMPARs) and NMDA receptors (NMDARs) that are found colocalizedin the postsynaptic density of the vast majority of glutamatergicsynapses in the brain and are activated concomitantly afterrelease of glutamate from the presynaptic terminal. Postsynaptickainate receptors (KARs) show restricted cellular and subcellularexpression. Kainate receptor-mediated EPSCs (KAR–EPSCs)have been best characterized at synapses between mossy fibersand CA3 pyramidal cells in the hippocampus (Castillo et al.,1997; Vignes and Collingridge, 1997; Mulle et al., 1998; Contractoret al., 2003), although they have also been observed in a varietyof other synapses (Huettner, 2003; Lerma, 2003; Pinheiro andMulle, 2006). A single stimulation of mossy fibers is sufficientto activate synaptic KARs (Castillo et al., 1997), which onlyyields EPSCs of small amplitude and slow kinetics. The analysisof KAR mutant mice has further demonstrated that 1-(4-aminophenyl)-4-methyl-7,8-methylenedioxy-5H-2,3-benzodiazepine(GYKI 53655)-resistant EPSCs were mediated by KARs composedof the glutamate receptor subunit 6 (GluR6) and KA2 subunits(Mulle et al., 1998; Contractor et al., 2003; Ruiz et al., 2005).
Compared with AMPA and NMDA receptor-mediated synaptic transmission,little is known about the plasticity of KAR–EPSCs. Earlyduring postnatal development, long-term potentiation expressionat thalamocortical synapses is associated with a reduction ofKAR–EPSCs (Kidd and Isaac, 1999). In perirhinal cortexneurons, activation of PKC by stimulation of mGluR5 enhancesKAR–EPSCs (Cho et al., 2003; Park et al., 2006). In theseneurons, a train of 200 stimuli at 5 Hz results in long-termdepression of KAR–EPSCs via a mechanism involving mGluR5,PKC, and PICK1 (protein interacting with C kinase-1) PDZ (postsynapticdensity-95/Discs large/zona occludens-1) domain interactions(Park et al., 2006), and possibly a change in the number ofsynaptic KARs (Hirbec et al., 2003). At hippocampal mossy fibersynapses, KAR–EPSCs are regulated as a consequence ofpresynaptic changes in glutamate release properties (Ito etal., 2004), but no form of synaptic plasticity specific forKAR–EPSCs has yet been described. However, the functionalproperties of recombinant KARs can be regulated on a shortertime scale by direct cAMP-dependent phosphorylation (Traynelisand Wahl, 1997). In cultured hippocampal neurons, a conditioningactivation of NMDARs depresses native KAR-mediated responsesin a rapid and reversible manner (Ghetti and Heinemann, 2000).This depression depends on Ca²⁺ influx through NMDA receptoror voltage-gated calcium channels and on the activation of calcineurin(Ghetti and Heinemann, 2000). It also requires the heteromericassembly of GluR6a and GluR6b and the association of calcineurinwith the C-terminal domain of GluR6b in the KAR complex (Coussenet al., 2005). The present experiments were designed to examinewhether synaptic KARs at hippocampal mossy fiber synapses wereprone to a phos-phorylation-dependent regulation and to definewhether this resulted in postsynaptic plasticity of KAR–EPSCs.

   Materials and Methods

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Transverse hippocampal slices (350 µm thick) were obtainedfrom 15- to 21-d-old C57BL/6 mice. Slices were transferred toa recording chamber and continuously superfused with an oxygenatedextracellular medium (95% O₂ and 5% CO₂) containing (in mM):125 NaCl, 2.5 KCl, 2 CaCl₂, 0.6 MgCl₂, 1.25 NaH₂PO₄, 26 NaHCO₃,16 glucose, pH 7.4. Whole-cell voltage-clamp recordings weremade at room temperature from CA3 pyramidal cells. The intracellularsolution contained the following (in mM): 140 cesium methanesulfonate,2 MgC₂, 4 NaCl, 5 phospho-creatine, 2 Na₂ATP, 1 EGTA, 10 HEPES,0.33 GTP, pH 7.3. For current-clamp recordings, the followingintracellular solution was used (in mM): 130 potassium gluconate,2 MgCl₂, 4 NaCl, 5 phospho-creatine, 2 Na₂ATP, 1 EGTA, 10 HEPES,0.33 GTP, pH 7.3. In some experiments, 1 mM EGTA was replacedby 20 mM BAPTA, and in others, 100 µM peptide correspondingto the last 15 aa of GluR6b or to a 15 aa scramble sequence(Coussen et al., 2005) was added to the intracellular solutiontogether with a cocktail of anti-proteases (pepstatin, aprotinin,leupeptin, and pefabloc, 10 µg/ml each). Neurons werevoltage clamped at –80 mV, unless otherwise indicated,and bicuculline (10 µM) was present in the superfusateof all experiments. The access resistance was <20 M ${Omega}$ , andresults were discarded if it changed by >20%.
Mossy fiber (Mf)–EPSCs were evoked by minimal intensitystimulation (Marchal and Mulle, 2004) and were characterizedby a marked facilitation after switching stimulus frequencyfrom 0.1 to 1 Hz and by their sensitivity to group 2/3 mGluRagonist LCCG-1 [(2S,1S,2S)-2-(carboxycyclopropyl)glycine] (10µM). Recordings were made using an EPC 9 amplifier (HEKAElektronik, Lambrecht/Pfalz, Germany) and were filtered at 0.5–1kHz, digitized at 5 kHz, and stored on a personal computer foradditional analysis (IGOR PRO 5.0; WaveMetrics, Lake Oswego,OR). Values are presented as mean ± SEM. Either a pairedor unpaired Student's t test was used to define statisticaldifferences between values.
All drugs were obtained from Tocris Bioscience (Ballwin, MO)or Sigma (St. Louis, MO). SR141716A [N-piperidino-5-(4-chlorophenyl)-1-(2,4-dichlorophenyl)-4-methyl-pyrazole-3-carboxamide]was kindly provided by Olivier Manzoni (INSERM, University ofBordeaux 2).

   Results

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

We examined the possibility that synaptic NMDARs could regulatethe function of KARs at synapses between mossy fibers and CA3pyramidal cells. Mf–EPSCs were evoked in CA3 pyramidalcells at minimal stimulation intensity in the presence of bicuculline(10 µM) to block GABA_A receptors, and unless otherwiseindicated, GYKI 53655 (50 µM) to block AMPARs. Under theseconditions (with 0.6 mM Mg²⁺ in the extracellular medium), Mf–EPSCsrecorded at –80 mV were blocked (>95% inhibition) byCNQX (25 µM; data not shown). In GluR6^–/–mice in which KAR–EPSCs are abolished (Mulle et al., 1998),residual Mf–EPSCs of small amplitude could be recordedat –80 mV. These residual EPSCs that corresponded to theNMDA receptor component of the Mf synaptic response only represented7.5 ± 1.8% (n = 8) of the amplitude of Mf–EPSCsrecorded in wild-type mice. Thus, at this membrane potentialin the presence of GYKI 53655, Mf–EPSCs are in great partmediated by KARs. In response to a train of five pulses at 20Hz, the amplitude of KAR–EPSCs during the train increasedand remained potentiated 500 ms after the train because of presynapticfacilitation (Salin et al., 1996; Ito et al., 2004) (Fig. 1A).

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Figure 1. Short-term depression of KAR–EPSCs at mossy fiber synapses. A, Representative traces illustrating short-term depression of mossy fiber KAR–EPSCs in CA3 pyramidal cells. A train of five stimulation pulses at 20 Hz was delivered to mossy fibers, followed by a test stimulation ( ${Delta}$ t = 500 ms). The train was either given with the cell membrane potential being held at –80 mV [control train (ctr)] or at –40 mV [conditioning train (cond)]. The amplitudes of test KAR–EPSCs after a control (EPSC_ctr) or a conditioning (EPSC_cond) train were compared (enlarged traces are superimposed in inset). B, Average time course of normalized mossy fiber KAR–EPSCs in response to the test stimulus. The KAR–EPSC value was normalized to the average of the amplitudes of KAR–EPSCs obtained in control conditions for the first four KAR–EPSCs in each recording. Arrows indicate the time when the conditioning train was applied. C, Time course of depression of KAR–EPSCs by the conditioning train of mossy fiber stimulation. Time between the end of the train and the control stimulus ( ${Delta}$ t) was varied between 0.2 and 20 s.

To examine the consequences of synaptic activation of NMDARson KAR–EPSCs, we depolarized the membrane to –40mV while applying the train of five stimulation pulses at 20Hz (conditioning train). The membrane potential was set backto –80 mV 50 ms after the last stimulus in the train,and a test stimulus was given 500 ms thereafter (Fig. 1A, bottom).At –40 mV, Mf–EPSCs were only inhibited by 25 ±10% (n = 3) by CNQX, indicating that NMDARs largely contributeto Mf–EPSCs under these conditions. We compared the amplitudeof KAR–EPSCs in response to a test stimulus given 500ms after a control train (membrane potential held at –80mV) or after a conditioning train. The conditioning train ledto the decrease of KAR–EPSC amplitude by 32 ± 3%(n = 11) (Fig. 1A,B). The depression of KAR–EPSCs wastransient and highly reproducible during repetition of the conditioningtrain (Fig. 1B). Depolarization of the cell membrane to –40mV in the absence of synaptic stimulation did not significantlyaffect the amplitude of KAR–EPSCs (102 ± 6% ofcontrol; n = 8). By varying the interval between the train andthe test stimulus, we observed that depression of KAR–EPSCsby a conditioned train developed progressively from almost noeffect at 0.2 s to a peak at 1 s (Fig. 1C). KAR–EPSCsreturned to control levels with an interval of 20 s. Changingthe parameters of the conditioning protocol by increasing thenumber of stimulation pulses to 10 or increasing the rate ofstimulation within the train to 50 Hz did not further increasethe extent or time course of KAR–EPSC depression (10 stimulationpulses at 20 Hz, 25 ± 4%, n = 7; 5 stimulation pulsesat 50 Hz, 28 ± 2%, n = 4).
Short-term depression of KAR–EPSCs requires changes inthe membrane potential of the postsynaptic neuron. This couldresult in changes in the properties of postsynaptic KARs. Alternatively,depression could be induced postsynaptically and expressed presynapticallythrough the release of a retrograde messenger, such as whatis observed for depolarization-induced suppression of excitation(Diana and Marty, 2004). In this case, depression should affectsimilarly both AMPAR- and KAR-mediated EPSCs. We thus examinedthe effect of a conditioning train on AMPAR–EPSCs (inthe absence of GYKI 53655) (Fig. 2A). A control train inducedpost-tetanic potentiation of AMPAR–EPSCs (increase by434 ± 81%, n = 8) when comparing the first EPSC in thetrain and the test EPSC (EPSC_ctr). The amplitude of the testAMPAR–EPSC was not significantly different (p > 0.05)in response to a conditioning train (Fig. 2A,B), indicatingthat the conditioning protocol selectively affects KAR functionand strongly suggesting that the mechanisms of depression donot involve an alteration of glutamate release. In support ofthis notion, pharmacological manipulations that are known toincrease or decrease mossy fiber synaptic transmission at apresynaptic level did not affect the extent of KAR–EPSCdepression (supplemental Fig. 1, available at www.jneurosci.orgas supplemental material). For instance, activation of adenosineA₁ receptors tonically depresses Mf–EPSCs by acting ata presynaptic level (Nicoll and Schmitz, 2005). Accordingly,bath application of the A₁ receptor antagonist 8-cyclopentyl-1,3-dipropylxanthine(100 nM) increased Mf–EPSC amplitude (153 ± 17%of control Mf–EPSC amplitude; n = 5), without affectingthe extent of depression of KAR–EPSCs (29 ± 5%;n = 5). Conversely, the A₁ receptor agonist CADO (1 µM)decreased Mf–EPSC amplitude (to 39 ± 9% of controlMf–EPSC amplitude; n = 7) but did not change the depressionof KAR–EPSCs (30 ± 3%; n = 7). Finally, forskolin(10 µM), which is known to increase mossy fiber synaptictransmission by acting at a presynaptic level (Nicoll and Schmitz,2005) (236 ± 15 of control Mf–EPSC amplitude; n= 4), did not affect the depression of KAR–EPSCs (27 ±5%; n = 7).

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Figure 2. Short-term depression of KAR–EPSCs involves NMDA activation, postsynaptic calcium rise, and calcineurin activation. A, Effects of the conditioning train on AMPAR–EPSCs. Enlarged traces for EPSC_ctr and EPSC_cond are superimposed in inset. ctr, Control train; cond, conditioning train. B, Summary of the effects of the conditioning train in different experimental conditions. The conditioning train depressed KAR–EPSCs (Control), but not AMPAR–EPSCs, and was abolished in presence of the NMDAR antagonist D-AP5 (50 µM), or when BAPTA (20 mM) or the phosphatase calcineurin inhibitor deltamethrin (100 µM) were included in the patch pipette. **p < 0.01.

Short-term depression of KAR–EPSCs was not observed inconditions in which NMDARs were blocked by D-AP5 (50 µM)(depression by 7 ± 2%, n = 7) and in conditions in whichintracellular Ca²⁺ rise in the postsynaptic cell was preventedby the fast Ca²⁺ chelator BAPTA (20 mM) (depression of KAR–EPSCby 3 ± 6%; n = 4) (Fig. 2B). It was reported that NMDAapplication on cultured neurons decreases KAR-mediated inwardcurrents by the activation of the phosphatase calcineurin (Ghettiand Heinemann, 2000). When the calcineurin inhibitor deltamethrin(500 nM) was included in the recording pipette, the conditioningprotocol did not significantly affect KAR–EPSCs (depressionby 1 ± 6%; n = 6) (Fig. 2B). Recovery from depressionwas strongly reduced when the calcium/calmodulin-dependent proteinkinase II (CaMKII) antagonist KN-62 (50 µM), was presentin the patch pipette (at ${Delta}$ t = 20 s after the train of stimulation,depression of KAR–EPSC by 21 ± 7%; n = 4). Thus,synaptic activation of NMDARs leads to short-term depressionof KAR–EPSCs that appears to depend on the influx of Ca²⁺in the postsynaptic pyramidal cell and on the activation ofthe phosphatase calcineurin.
We recently proposed that binding of calcineurin to GluR6b wasnecessary for the inhibition of kainate-evoked currents by activationof NMDARs in cultured hippocampal neurons (Coussen et al., 2005).Assuming that postsynaptic KARs at mossy fiber synapses mightbe composed of both GluR6a and GluR6b, we tested whether GluR6bwas also determinant for the NMDAR-induced short-term depressionof KAR–EPSCs. We first tested the effects of blockingGluR6b interaction with calcineurin by inclusion of a GluR6bC-terminal peptide (pepR6b) (Coussen et al., 2005) in the recordingpipette (Fig. 3A). Dialysis of pepR6b in CA3 pyramidal cellsdid not affect the average amplitude of KAR–EPSCs duringthe time of the experiment (Fig. 3C,D). Short-term depressionof KAR–EPSCs by a conditioning train was significantlyattenuated in the presence of pepR6b (Fig. 3A,E) (depressionby 11 ± 3%; n = 8; p < 0.05) but not in the presenceof a scramble peptide (see experimental procedures) (depressionof 30 ± 2%; n = 6) (Fig. 3E). We also tested the effectsof synaptic NMDAR activation on KAR–EPSC depression inmice expressing GluR6a but not GluR6b. For this, we used transgenicmice that express myc-GluR6a in hippocampal neurons on a GluR6^–/–background (Coussen et al., 2002). As previously shown, themyc-GluR6a transgene rescued the loss of functional synapticKARs that is observed in GluR6^–/– mice (Fig. 3B).The conditioning train failed to induce a significant depressionof KAR–EPSCs in CA3 pyramidal cells from mycGluR6a x GluR6^–/–mice (9 ± 9%, n = 6) (Fig. 3B,E). This set of experimentslends additional support to the notion that binding of calcineurinto the C-terminal domain of GluR6b subunit is essential forphosphatase activity on the KAR complex that leads to short-termdepression of KAR–EPSCs.

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Figure 3. GluR6b subunit is necessary for NMDA-induced short-term depression of KAR–EPSCs. A, Representative traces illustrating short-term depression of mossy fiber KAR–EPSCs in CA3 pyramidal cells obtained when a GluR6b C-terminal peptide (pepR6b), which blocks the GluR6b interaction with calcineurin, was included in the patch pipette. B, Effects of the conditioning train (cond) in slices from transgenic mice expressing GluR6a but not GluR6b (R6a tg x R6^–/–). ctr, Control train. C, Summary plot of the results obtained when interfering with the GluR6b subunit. Blocking GluR6b interaction with calcineurin by inclusion of pepR6b in the recording pipette, but not its scramble version, or working with slices from R6a tg x R6^–/– mice greatly attenuated short-term depression of KAR–EPSCs induced by NMDAR activation. **p < 0.01. D, Summary plot of KAR–EPSCs amplitudes obtained in control conditions and in conditions in which the pepR6b was present in the patch pipette. E, Average time course of normalized mossy fiber KAR–EPSCs obtained when the pepR6b was present in the patch pipette. The KAR–EPSC value was normalized to the average of the amplitudes of KAR–EPSCs obtained in control conditions for the first four KAR–EPSCs in each recording. Arrows indicate the time when the conditioning train was applied. The presence of the pepR6b in the patch pipette did not affect the time course of control KAR–EPSCs, but it strongly reduced the depression induced by the conditioning train.

From a functional point of view, it is important to understandwhether short-term depression is homosynaptic or heterosynaptic.For this, we stimulated with minimal intensity two independentmossy fiber synaptic pathways by using two electrodes positionedin distinct regions of the dentate granule cell region. Thisexperimental setup provides conditions for maximizing the likelihoodthat the two mossy fiber pathways were independent. As a confirmation,we checked that there was no cross-potentiation between thetwo synaptic inputs stimulated (stim 1 or stim 2) as expectedfor two independent inputs: stimulation of input 1 did not causeany increase in the amplitude of Mf–EPSCs triggered bystimulation of input 2 (and vice versa) (Fig. 4A). A conditioningtrain to the first stimulating electrode (stim 1) applied at–40 mV did not induce any significant depression of KAR–EPSCsevoked in response to the second stimulating electrode (stim2) (depression by 1 ± 7%; n = 8) (Fig. 4B, right, C),whereas a similar conditioning protocol in which both the conditioningand the test stimuli were applied to the same mossy fiber pathwayled to the depression of KAR–EPSCs (Fig. 4B, left, C).These data indicate that short-term depression of KAR–EPSCsby synaptic NMDARs can be induced homosynaptically and thusrequires the close localization of these two receptor populations.

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Figure 4. Short-term depression of KAR–EPSCs is homosynaptic. A, Representative traces of mossy fiber–EPSCs illustrating the protocol used to verify whether two independent mossy fibers were being stimulated. Two glass stimulating electrodes were positioned at different loci in the dentate gyrus [stimulation (stim) 1 and stim 2]. Prominent paired-pulse facilitation is observed for both mossy fiber synaptic inputs applied independently (stim 1 and stim 2). However, no potentiation to stim 1 is observed after stim 2 (and vice versa). The two fibers stimulated by stim 1 and stim 2 were considered to be independent. B, Homosynaptic: the conditioning protocol was applied to the same fiber as the test stimulation leading to short-term depression of KAR–EPSCs. Heterosynaptic: for two independent stimulations, applying the conditioning train to stim 1 was without any effect on KAR–EPSCs evoked in response to stim 2. The corresponding superimposed traces are enlarged in inset. ctr, Control train; cond, conditioning train. C, Summary plot of the results obtained when stimulating two different mossy fibers, testing whether applying the conditioning protocol to one mossy fiber could also induce the short-term depression of KAR–EPSCs recorded from stimulation of a second and independent mossy fiber. *p < 0.05.

To address the physiological relevance of this phenomenon, weperformed experiments in the current-clamp mode. Because influxof Ca²⁺ through NMDARs is needed for short-term depression ofKAR–EPSCs, we used a conditioning protocol whereby synapticNMDARs are relieved from the Mg²⁺ block through transient depolarizationapplied in a timely manner with the synaptic release of glutamate.For this, we paired mossy fiber stimulation to a short depolarizingpulse that triggered action potentials (2 ms, 800 pA) given10 ms after each mossy fiber stimulation in the train. The depolarizationresulting from the action potential during activation of NMDARsby synaptically released glutamate will largely favor the openingof NMDAR channels. We recorded a test EPSP 2 s after this conditioningtrain (at this point the membrane potential was on average –66.7± 2.9 mV, n = 7, in control and –66.8 ±2.8 mV, n = 7, after a conditioning train). This pairing protocoldecreased the amplitude of the test KAR–EPSP comparedwith a control train (no pairing) (depression by 21 ±5%; n = 7; p < 0.05) (Fig. 5A,C). In contrast, if the shortdepolarizing pulse was given 10 ms before depolarization, nochange in the amplitude of the test KAR–EPSP was observed(Fig. 5B,C). Depression of KAR–EPSPs was prevented whenBAPTA (20 mM) was included in the recording pipette (depressionby 5 ± 2%; n = 6) and was inhibited by D-AP5 (3 ±4%, n = 11) (Fig. 5B). Thus, coincidence between action potentialdischarge and synaptic stimulation at mossy fiber synapses leadsto short-term plasticity of KAR–EPSPs through activationof synaptic NMDARs.

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Figure 5. Pairing mossy fiber stimulation with postsynaptic depolarization depresses KAR–EPSPs. A, Current-clamp recordings from CA3 pyramidal cells recorded in the current-clamp mode in the presence of 1.3 mM extracellular Mg⁺². Evoking spikes with short depolarizing pulses (2 ms, 800 pA) 10 ms after mossy fiber stimulation (post depol) induced depression of KAR–EPSPs. B, If the depolarizing pulses were each applied 10 ms before mossy fiber stimulation (pre depol), no significant effect of the protocol on KAR–EPSPs was observed. ctr, Control train; cond, conditioning train. C, Summary of the effects of the protocol used in A on KAR–EPSPs in control conditions, in conditions in which 20 mM BAPTA was included in the patch pipette or after inhibition of NMDARs with 50 µM D-AP5, and with the conditions used in B. *p < 0.05

Although a short train of action potentials alone (five spikes)was ineffective in triggering short-term depression of KAR–EPSPs,influx of Ca²⁺ through voltage-gated channels after a much largertrain of action potentials (30 spikes) similarly led to thedepression of KAR–EPSPs (depression by 31 ± 2%;n = 3) (Fig. 6B,C) in an NMDA-independent manner (depressionby 29 ± 8%; n = 3 in the presence of 50 µM D-AP5).We studied the relevance of this 30% reduction of KAR–EPSPsin more physiological conditions of synaptic transmission, inthe absence of the AMPA receptor antagonist GYKI 53655. We stimulatedmossy fibers with a train of five stimuli and compared EPSPsobtained in control conditions versus EPSPs obtained after applyingthe conditioning protocol that consisted of a train of 30 spikesinduced by current injection, before synaptic stimulation. Thisconditioning protocol did not change the amplitude of the firstEPSP in the train (Fig. 6D,E), suggesting that the train of30 spikes did not have any presynaptic effects, nor did it affectAMPA receptors. However, we observed a clear change in the waveformof Mf–EPSPs evoked by a train of five stimuli (Fig. 6D).The kinetic difference is subtle for a single Mf–EPSP,but for subsequent stimuli, a decrease in the decay of Mf–EPSPsis observed that changes summation properties likely attributableto the 30% decrease in KAR–EPSC amplitude. After fourstimuli, summation of Mf–EPSPs is significantly decreased(decrease of 37 ± 7%; n = 6) (Fig. 6D, parameter "a,"F), leading in several instances to a difference in the capacityto trigger action potentials (data not shown). This effect wasnot attributable to the calcium-dependent inactivation of NMDAreceptors (Tong et al., 1995) because we could observe the samedecrease in Mf–EPSPs summation in the presence of D-AP5(decrease of 40 ± 5%; n = 5; data not shown).

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Figure 6. Depression of KAR–EPSPs can also be induced by a large train of action potentials and is important for summation properties of mossy fiber EPSPs. A, Applying a train of five spikes without pairing with synaptic stimulation does not change the amplitude of KAR–EPSPs. B, In contrast to what we observed with a train of five spikes, a train of 30 spikes induces a clear reduction in KAR–EPSP amplitude. C, Summary of the effects of trains of 5, 10, or 30 spikes on KAR–EPSPs. The decrease of KAR–EPSPs induced by the train of 30 spikes also occurred in the presence of 50 µM D-AP5. D, Representative traces of Mf–EPSPs obtained without blocking AMPA receptors in control conditions (ctr; black) and after applying a train of 30 spikes (cond; gray). In conditions in which KAR–EPSPs are depressed by $~$ 30%, the train of EPSPs displayed significantly less summation (measured as a) compared with the control train of EPSPs. E, The train of 30 spikes did not significantly change the amplitude of the first stimulus, suggesting that this protocol did not have any presynaptic effects, nor did it affect AMPA receptors. F, Summary plot of the effect of a train of 30 spikes in the summation (measured in A as indicated in D) of EPSPs obtained after stimulating mossy fiber with a train of five stimuli. *p < 0.05.

   Discussion

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Short-term changes in synaptic strength are commonly thoughtto be mediated by presynaptic mechanisms such as Ca²⁺ controlof release probability or presynaptic vesicle replenishment(Zucker and Regehr, 2002). Here we describe a form of short-termplasticity of KAR–EPSCs at mossy fiber synapses that isinduced and expressed postsynaptically, in response to the coincidentactivation of NMDARs during a short burst of afferent mossyfiber stimulation.
Several lines of evidence, such as the requirement for the activityof postsynaptic NMDARs and Ca²⁺ increase in the postsynapticCA3 pyramidal cell, argue in favor of a postsynaptic inductionmechanism for short-term depression of KAR–EPSCs. Nevertheless,it could be argued that short-term plasticity of KAR–EPSCsis expressed presynaptically. Indeed, postsynaptic depolarization(possibly in conjunction with activation of postsynaptic NMDARs)can release retrograde messengers, such as endocannabinoids,that can act presynaptically to cause short-term depressionof transmitter release (Alger, 2002; Diana and Marty, 2004).We do not favor this type of mechanism for several reasons.First, short-term depression does not affect AMPAR–EPSCs,as would be expected if glutamate release was involved in theshort-term depression of KAR–EPSCs. In addition, pharmacologicalmanipulations that alter Mf–EPSCs (including KAR–EPSCs)by acting at a presynaptic level are without any effect on theextent of short-term depression of KAR–EPSCs. Finally,short-term depression of KARs by synaptic NMDARs is not observedin transgenic mice with postsynaptic KARs containing GluR6aand not GluR6b, as well as with a postsynaptic infusion of theGluR6b peptide in pyramidal cells. Thus, this form of short-termdepression of synaptic transmission is both induced and expressedpostsynaptically.
We propose that the mechanism of short-term depression of KAR–EPSCsinvolves the Ca²⁺-dependent activation of the phosphatase calcineurin.Previous studies have shown that kainate-activated currentsin hippocampal cultured neurons are depressed by NMDARs andby voltage-dependent Ca²⁺ channels through activation of calcineurin(Ghetti and Heinemann, 2000). We give additional evidence forsuch a mechanism under physiological conditions of activationof synaptic NMDARs. Our experimental protocol allows to finelydetail the time course of inhibition of KAR–EPSCs, whichappears to develop progressively over the first second afterNMDAR activation and to recover within 20 s. This time courseis reminiscent of the calcineurin-dependent regulation of desensitizationof synaptic NMDARs (Tong et al., 1995), which can thus regulatetheir own activity as well as the activity of KARs. It appearsthat Ca²⁺ influx through the KAR channel itself is not sufficientto activate the calcium-dependent enzyme calcineurin, possiblybecause of the low calcium permeability of synaptic KARs thatmight be predominantly edited (Castillo et al., 1997). As inhippocampal cultured neurons, the recovery from depression ofKAR–EPSCs could be prevented by an inhibitor of CaMKII.Overall, these data favor a mechanism whereby synaptic KARsexist, at least partly, in a phosphorylated form and can bedephosphorylated by the calcium-dependent activation of calcineurin,leading to decreased receptor channel activity (Traynelis andWahl, 1997). It is not yet clear whether one of the KAR subunitsof postsynaptic KARs at mossy fiber synapses is prone to phosphorylationby Ca²⁺-calmodulin kinase II, or whether it is instead a KAR-associatedprotein. Nevertheless, our data lend further support to thenotion that the regulation of KAR function requires the bindingof calcineurin to GluR6b (Coussen et al., 2005). Because ofits rapid onset and the similarity with studies on recombinantreceptors (Traynelis and Wahl, 1997), which implicate a decreasein the opening probability of KAR channels, short-term depressionof KAR–EPSCs is likely attributable to a decrease in thefunction of synaptic KARs, although the removal of KARs fromthe postsynaptic membrane, a mechanism suggested to occur forlong-term depression of synaptic KARs in the perirhinal cortex(Park et al., 2006), cannot be excluded.
Short-term depression of synaptic KARs can occur through a localand synapse-specific mechanism requiring an increase in intracellularCa²⁺ by synaptic NMDARs that are likely closely localized withsynaptic KARs. However, because mossy fiber synapses have multiplerelease sites, it remains possible that a bulk increase of Ca²⁺in the postsynaptic spine is required for the regulation ofKARs. Short-term depression of KAR–EPSPs is triggeredby the coordinated firing of action potentials and mossy fibersynaptic stimulation only when action potential fires duringthe glutamatergic EPSC. It thus represents a novel form of spike-timing-dependentplasticity (Markram et al., 1997; Dan and Poo, 2004).
Although EPSCs mediated by KARs have a much smaller amplitudethan that mediated by AMPARs, they also display much slowerkinetics and prominent summation properties (Castillo et al.,1997). These features allow KAR–EPSPs to play a prominentrole in information transfer in CA1 interneurons by imposinga substantial depolarization during sustained afferent activity(Frerking and Ohliger-Frerking, 2002). In agreement with theimportant role of kainate receptors for summation propertiesof EPSPs (Frerking and Ohliger-Frerking, 2002), we observedthat a 30% reduction of KAR–EPSPs is sufficient to inducea significant change in the summation of mossy fiber–EPSPs.This indicates that the short-term depression described heremight have important physiological consequences mainly duringsustained afferent activity controlling CA3 pyramidal cell depolarization.The precise role of kainate receptors in signal integrationat mossy fiber–CA3 pyramidal cell synapses is far frombeing completely understood. Nevertheless, short-term depressionof KAR–EPSCs in conditions of high afferent activity leadingto spike discharge is expected to exert a feedback inhibitionon the sustained depolarization induced by KAR–EPSPs.Interestingly, it was reported that KAR–EPSCs show attenuatedforms of presynaptic plasticity compared with AMPAR–EPSCs(Ito et al., 2004). Both mechanisms will concur in preventingthe overactivation of synaptic KARs under conditions of sustainednetwork activity and might thus favor information processingin conditions of short bursts of afferent stimulation.

   Footnotes

Received Aug. 7, 2006; revised Feb. 12, 2007; accepted Feb. 15, 2007.
This work was supported by Fundaçao para a Ciênciae para a Tecnologia Grant POCI/NEU-SAU/59135/2004, by the CentreNational de la Recherche Scientifique, the Ministèrede la Recherche of France, the Conseil Régional d'Aquitaine,the Fondation pour la Recherche Médicale (fellowshipto S.S.), and the European Commission (EUSynapse, contract numberLSH-2004-019055 to C.M.). We thank Paulo Pinheiro for criticialreading of this manuscript.
Correspondence should be addressed to Christophe Mulle at the above address. Email: mulle{at}u-bordeaux2.fr
Copyright © 2007 Society for Neuroscience 0270-6474/07/273987-07$15.00/0

   References

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

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