Presynaptic Depression at a Calyx Synapse: The Small Contribution of Metabotropic Glutamate Receptors

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Volume 17, Number 21, Issue of November 1, 1997 pp. 8137-8146
Copyright ©1997 Society for Neuroscience

Presynaptic Depression at a Calyx Synapse: The Small Contribution of Metabotropic Glutamate Receptors

Henrique von Gersdorff, Ralf Schneggenburger, Sibylle Weis, and Erwin Neher
Department of Membrane Biophysics, Max Planck Institute for Biophysical Chemistry, D-37077 Göttingen, Germany

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Synaptic depression of evoked EPSCs was quantified with stimulation frequencies ranging from 0.2 to 100 Hz at the single CNSsynapse formed by the calyx of Held in the rat brainstem. Half-maximaldepression occurred at $approx$ 1 Hz, with 10 and 100 Hz stimulation frequenciesreducing EPSC amplitudes to $approx$ 30% and $approx$ 10% of their initial magnitude,respectively. The time constant of recovery from depression elicitedby 10 Hz afferent fiber stimulation was 4.2 sec. AMPA and NMDAreceptor-mediated EPSCs depressed in parallel at 1-5 Hz stimulationfrequencies, suggesting that depression was induced by presynapticmechanism(s) that reduced glutamate release. To determine thecontribution of autoreceptors to depression, we studied the inhibitoryeffects of the metabotropic glutamate receptor (mGluR) agonists(1S, 3S)-ACPD and L-AP4 and found them to be reversed in a dose-dependentmanner by (RS)- $alpha$ -cyclopropyl-4-phosphonophenylglycine (CPPG),a novel and potent competitive antagonist of mGluRs. At 300 µM,CPPG completely reversed the effects of L-AP4 and (1S, 3S)-ACPD,but reduced 5-10 Hz elicited depression by only $approx$ 6%. CPPG-sensitivemGluRs, presumably activated by glutamate spillover during physiologicalsynaptic transmission, thus contribute on the order of only 10%to short-term synaptic depression. We therefore suggest that themain mechanism contributing to the robust depression elicitedby 5-10 Hz afferent fiber stimulation of the calyx of Held synapseis synaptic vesicle pool depletion.
Key words: EPSCs; NMDA; AMPA; competitive antagonist; synaptic transmission; auditory brainstem slices; secretion; short-term plasticity

INTRODUCTION

Use-dependent synaptic depression is a ubiquitous phenomenon observed in a wide variety of synapses from invertebrates (Kusanoand Landau, 1975; Charlton et al., 1982; Atwood et al., 1994)to mammals (Debanne et al., 1996; Rosenmund and Stevens, 1996).In the mammalian neocortex, for example, synaptic depression isthe predominant form of short-term synaptic plasticity observedbetween pyramidal cell pairs that have a high release probability(Thomson et al., 1993; Abbott et al., 1997; Tsodyks and Markram,1997). Understanding the properties and underlying mechanismsthat generate synaptic depression therefore is vital for an understandingof how neural networks operate in the brain. Multiple cellularmechanisms, perhaps acting simultaneously, may be responsiblefor the generation of synaptic depression. Some proposed mechanismsare autoreceptor activation (e.g., metabotropic glutamate receptor,mGluR; Forsythe and Clements, 1990; Baskys and Malenka, 1991;Nakanishi, 1994; Takahashi et al., 1996), presynaptic calciumcurrent inactivation (Wu and Saggau, 1997), depletion of the readilyreleasable pool of synaptic vesicles at active zones (Thies, 1965;Liu and Tsien, 1995; Stevens and Tsujimoto, 1995), postsynapticreceptor desensitization (Magleby and Pallotta, 1981; Trussellet al., 1993; Otis et al., 1996), and adaptation of the calciumsensor for exocytosis (Hsu et al., 1996). To study and quantifyhow much each of these different processes contributes to depression,a CNS synapse preparation that expresses robust synaptic depressionis necessary.

A model CNS synapse is the calyx of Held, where a single large calyciform terminal synapses onto each principal neuron ofthe medial nucleus of the trapezoid body (MNTB) in the mammalianbrainstem (Forsythe and Barnes-Davies, 1993; Borst et al., 1995).This axo-somatic glutamatergic synapse is involved in computingsound localization, and the calyx structure, with its multipleactive zones, ensures fast, reliable synaptic transmission. Wehave characterized short-term plasticity (Magleby, 1987) at thissynapse by recording EPSCs evoked by trains of presynaptic actionpotentials delivered at various frequencies (0.2-100 Hz). We showthat AMPA and NMDA receptor-mediated EPSCs depress in a parallelmanner for 1-5 Hz stimulation frequencies. This suggests thatglutamate release is reduced during stimulation trains at thesefrequencies and that depression is attributable to presynapticmechanism(s) and is not a consequence of postsynaptic receptordesensitization.

Recently, evidence was reported that use-dependent spillover of glutamate from the synaptic cleft (Asztely et al., 1997) canactivate presynaptic mGluRs (Scanziani et al., 1997) and thuslead to depression. By using a potent antagonist of group II andIII mGluRs, (RS)- $alpha$ -cyclopropyl-4-phosphonophenylglycine (CPPG)(Jane et al., 1996), we have investigated whether the activationof presynaptic mGluRs sensitive to L-AP4 and ACPD is involvedin producing short-term synaptic depression at the calyx of Held.We conclude that they contribute on the order of only 10% to theoverall depression elicited by 5-10 Hz stimulation.

MATERIALS AND METHODS
Slice preparation. The preparation of brainstem slices from 8- to 11-d-old Wistar rats followed the procedure described byForsythe and Barnes-Davies (1993) and Borst et al. (1995). Ratswere decapitated, and the brainstem was immersed in ice-cold low-calciumartificial CSF (aCSF) containing (in mM): NaCl 125, KCl 2.5, MgCl₂3.0, CaCl₂ 0.1, glucose 25, NaHCO₃ 25, NaH₂PO₄ 1.25, ascorbicacid 0.4, myo-inositol 3, and Na-pyruvate 2, pH 7.4, when bubbledwith carbogen (95% O₂/5% CO₂), with osmolarity $approx$ 320 mOsm. Alternatively,a low-sodium (0 NaCl), high-sucrose (250 mM) aCSF was used sometimes.The brainstem, with cerebellum, was glued with cyanoacrylate glueonto the stage of a vibratome slicer (Campden Instruments), and200-µm-thick transverse slices were cut proceeding from a caudalto rostral direction. Three to four slices containing the MNTBand the presynaptic axons of the calyx of Held thus were obtained.Slices were transferred rapidly to an incubation chamber containingnormal aCSF gently bubbled with carbogen and maintained at 37°Cfor 30-60 min and were used for experiments during the next 5-6hr. The normal aCSF was the same as the low-calcium aCSF describedabove except that 1.0 mM MgCl₂ and 2.0 mM CaCl₂ were used.

Electrophysiology and optics. All recordings were done in normal aCSF at room temperature (21-25°C). The standard patch pipettesolution consisted of (in mM): K-gluconate 115, KCl 20, Na₂-phosphocreatine10, HEPES 10, EGTA-K₄ 5, ATP-Mg 4, and GTP 0.3, pH 7.2 with KOH.The final osmolarity was $approx$ 295 mOsm. Some experiments also weredone with Cs-gluconate or CsCl instead of K-gluconate. Sliceswere placed in a recording chamber and held in place by a platinumgrid while normal aCSF solution was perfused at a rate of $approx$ 1 ml/minby a gravity-fed system of syringes and Teflon tubing. The levelof solution was kept constant by a negative feedback pressure-sensitivesystem. Slices were visualized by IR-DIC microscopy (Stuart etal., 1993) through a 40× or 63× water immersion Zeiss objectiveon an upright Zeiss microscope (Axioskop, Zeiss, Oberkochen, Germany).A bipolar stimulation electrode made from Teflon-coated platinum-iridiumwire (50 µm thickness) was placed gently on the midline of thetransverse slices. The space between the two stimulation wireswas $approx$ 0.5 mm so as to stimulate the presynaptic fiber bundles innervatingthe MNTB. This arrangement avoided the generation of postsynapticantidromic action potentials. A preselection of cells within theMNTB was done by using a patch pipette for extracellular recordingof action potentials elicited by afferent fiber stimulation. Onlythose cells that showed extracellularly recorded pre- and postsynapticaction potentials (Wu and Kelly, 1993; Borst et al., 1995) werechosen for whole-cell recordings. Extracellularly recorded postsynapticaction potentials displayed an increasing synaptic delay in therange of 0.5-3 msec during 5-10 Hz stimulation trains. Whole-cellfast current-clamp (EPC-9 feature; data not shown) recordingsof postsynaptic action potentials showed that this increase indelay is attributable to a progressively less steep rise in successiveEPSPs because of synaptic depression (see Swandulla et al., 1991).Cells recorded from were situated on the slice surface or oneto two cell layers ( $approx$ 50 µm) deep within the slice.

Patch pipettes were pulled from borosilicate glass (Hilgenberg, Malsfeld, Germany) and were coated with low-melting-pointdental wax or Sylgard, followed by brief fire polishing. The opentip resistance was 3-5 M $Omega$ , and uncompensated access resistancewas 5-10 M $Omega$ after whole-cell break-in. Seal resistances were inthe range of 1-10 G $Omega$ in the cell-attached mode, whereas in whole-cellthe leak currents varied from 100 pA to 1 nA in the data set acceptedfor analysis. However, the large majority of the cells that wereanalyzed had leak currents of 100-400 pA with the K-gluconate-basedpipette solution. Cells were voltage-clamped at a holding potentialof $-$ 80 mV if not stated otherwise. During many whole-cell recordingsthe series resistance (R_s) tended to increase gradually. For pharmacologicalexperiments for which stable EPSC had to be recorded over prolongedtimes ( $>=$ 30 min; see Fig. 5A), R_s was monitored by a 3 msec hyperpolarizing( $-$ 5 mV) prepulse applied before each stimulus. In the event ofa change in R_s, the R_s compensation of the EPC-9 amplifier waschanged such that the compensated value was kept constant ( $approx$ 5M $Omega$ ). In other experiments that did not require comparing EPSCamplitudes over prolonged times, R_s compensation was switchedto maximal values (up to 90% with a 10 µsec delay), giving compensatedseries resistances of 1-2 M $Omega$ . For these values and EPSC amplitudesof 8 nA (e.g., see Fig. 1), we estimate that the error in theclamp voltage at the peak of an EPSC is $approx$ 10-20 mV. No correctionswere made for liquid junction potentials.
Fig. 5. CPPG effectively antagonizes the depressing effects of L-AP4. A, Peak amplitudes of AMPA EPSCs elicited at 0.2 Hz plottedas a function of time. L-AP4 (50 µM) was applied during the timesindicated by the solid bars. In three instances during this experiment,30 or 100 µM CPPG (hatched bars) was applied to the slice duringthe continued presence of 50 µM L-AP4. Note that the depressingeffect of 50 µM L-AP4 was partially recovered by 30 µM CPPG andwas recovered more completely by 100 µM CPPG. B, An example fromanother cell in which 300 µM CPPG reversed completely the effectof 50 µM L-AP4. C, EPSCs (average traces of n = 5 single sweeps)corresponding to the control condition, to the presence of 50µM L-AP4, and to 50 µM L-AP4 in the presence of 300 µM CPPG. Samecell as shown in B.
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Fig. 1. Synaptic depression in principal neurons of the rat MNTB. A, An example of EPSCs elicited by afferent fiber stimulation trainsof 30 stimuli at 0.5 Hz. Voltage-clamp recordings were made ata holding potential of $-$ 80 mV in 2 mM [Ca]_o and 1 mM [Mg]_o. Notethat the first EPSC in the train is the largest and that the onsetof the EPSCs was $approx$ 1.5 msec after the stimulus artifact. B, Inthe same cell as in A, EPSCs were elicited by 30 stimuli at 10Hz. C, The peak EPSC amplitude of examples A and B are plottedfor 0.5 Hz (open symbols) and 10 Hz (closed symbols). These AMPAreceptor-mediated EPSCs depressed from the initial amplitude (I₀)to a new steady-state value (I_ss), which was obtained from thesteady-state value of an exponential fit (solid line; $tau$ = 2.47sec for 0.5 Hz and $tau$ = 159 msec for 10 Hz).
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Stimulation pulses applied through a Master-8 Stimulator (AMPI, Jerusalem, Israel) had a duration of 100 µsec and amplitudesof 2-20 V. Stimulation pulses were controlled by a Macintosh computer(Quadra 960) running Pulse software (HEKA Electronics, Lambrecht/Pfalz,Germany), and signals were recorded via an EPC-9 (HEKA) patch-clampamplifier. Sampling rates and filter settings were 50 and 5 kHzand 10 and 2 kHz for AMPA and NMDA receptor-mediated EPSCs, respectively.To induce synaptic depression, we applied trains of n = 30 stimuliat different frequencies, and peak EPSC amplitudes were measuredafter leak correction with the Pulse program. The peak amplitudeswere plotted as a function of time and fit with an exponentialfunction by IgorPro software (Wavemetrics, Lake Oswego, OR). Thesteady-state value of the exponential fit was taken as the EPSCamplitude at the end of the trains (I_ss; see Fig. 1C, for an example).To calculate the amount of depression, we divided I_ss by I_o, thepeak amplitude of the first EPSC in a train. For the NMDA componentof the EPSCs measured at +60 or +80 mV, peak amplitudes were measuredin a time window between 10 and 20 msec after the stimulus artifact(see Fig. 4A). Because of the slow decay kinetics of the NMDAreceptor-mediated EPSC, a residual current of 5 ± 4% (n = 6 cells),7 ± 3% (n = 3 cells), and 33 ± 8% (n = 4 cells) of I_o was observedat the onset of the second EPSC with stimulation intervals of1 sec (1 Hz), 0.5 sec (2 Hz), and 200 msec (5 Hz), respectively.Average data are reported as mean ± SD values.
Fig. 4. Depression of NMDA receptor-mediated EPSCs. A, EPSCs were elicited at 1 Hz at a holding potential of +60 mV. The first seventraces in a train of 30 stimuli are shown. A Cs-gluconate-basedinternal pipette solution was used (see Materials and Methods),and 100 µM glycine plus 2 µM strychnine were added to the externalsolution. Inset shows the initial part of the same data on anexpanded time scale (time bar = 20 msec). The horizontal arrowheadsindicate the peak amplitude of the first and the depressed AMPAreceptor-mediated component of the EPSCs at a holding potentialof +60 mV. The vertical dotted lines on the inset indicate thetime window from which the peak NMDA receptor-mediated componentof the EPSC was obtained. B, Time course of depression of NMDAEPSC (closed symbols) and AMPA EPSCs (open symbols; recorded at $-$ 80 mV) for a 1 Hz train recorded from the same cell as shownin A. EPSC amplitude values were normalized to I₀.
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Drugs. D( $-$ )-2-Amino-5-phosphonopentanoic acid (D-AP5), 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX), (1S,3S)-1-aminocyclopentane-1,3-dicarboxylicacid (ACPD), L(+)-2-amino-4-phosphonobutyric acid (L-AP4), (2S,1 $'$ R,2 $'$ R,3 $'$ R)-2-(2 $'$ ,3 $'$ -dicarboxycyclopropyl)-glycine(DCG-IV), and CPPG were purchased from Tocris Cookson (Bristol,UK). Strychnine was obtained from Research Biochemicals (Natick,MA), and all other drugs and chemicals were from Sigma (Deisenhofen,Germany) except purified Cs-gluconate salt, which was kindly providedby Dr. J. G. G. Borst (Max-Planck-Institute, Heidelberg, Germany).

RESULTS

Properties of synaptic depression at the calyx of Held
A single presynaptic action potential elicits a large and rapidly decaying EPSC in the principal cells of the rat MNTB underwhole-cell voltage clamp (Forsythe and Barnes-Davies, 1993; Borstet al., 1995). Such large EPSCs are typical of calyx-type synapses(Trussell et al., 1993; Yawo and Momiyama, 1993; Isaacson andWalmsley, 1995; Zhang et al., 1996). Examples of EPSCs elicitedby afferent fiber stimulation are shown in Figure 1, A and B.Successive EPSCs recorded in 2 mM [Ca]_o and 1 mM [Mg]_o under voltageclamp at a holding potential of $-$ 80 mV decreased in amplitudeduring 0.5 and 10 Hz stimulation trains. The degree of synapticdepression was larger for 10 Hz than for 0.5 Hz, as is indicatedin Figure 1C. EPSCs had a fast decay time (exponential time constant $tau$ $approx$ 1.1 msec) and were blocked by CNQX (5 µM; data not shown),identifying them as AMPA/kainate receptor-mediated EPSCs. Fromhere onward, these fast EPSCs will be termed AMPA EPSCs.

After trains of presynaptic stimuli at frequencies varying from 0.2 to 100 Hz, AMPA EPSCs strongly depressed with the firstEPSCs I_o in a train of stimuli decaying to a new steady-statevalue, I_ss (Fig. 1C). The amount of AMPA EPSC depression, expressedas the ratio I_ss/I_o, was dependent on the frequency of stimulation(Fig. 2A, open symbols). In the example of Figure 1C, I_ss/I_o was0.67 and 0.23 for stimulation frequencies of 0.5 and 10 Hz, respectively.At 100 Hz, depression was found to be 0.08 ± 0.03 for I_ss/I_o (n= 5 cells; see also Fig. 11 in Borst et al., 1995). The frequencyat which half-maximal depression is observed therefore was closeto 1 Hz (see Fig. 2A). This contrasts with the chick magnocellulariscalyx synapse, where half-maximal depression was observed at $approx$ 50Hz (Zhang and Trussell, 1994). The solid line in Figure 2A isa two-exponential function best fit, which includes the 100 Hzdata point. A single exponential function could not fit the datapoints from 0.2 to 10 Hz very well, especially when the 100 Hzdata were included (data not shown). It also should be noted thatthe amount of depression, analyzed at frequencies of 5 and 10Hz (n = 24 cells; Fig. 2B), was correlated with the amplitudeof the first EPSC in a train. Thus, different cells had differentinitial EPSC amplitudes (range 1-11 nA), and for large initialEPSCs we observed a larger degree of depression than for smallinitial EPSC amplitudes (Fig. 2B).
Fig. 2. Frequency dependence of synaptic depression. A, The amount of depression of AMPA EPSCs, expressed as I_ss/I₀, as a functionof stimulus frequency in a range of 0.2-10 Hz (open symbols).The number of cells for each frequency is indicated in parentheses;the total number of cells was n = 36. Note that the average datafor the depression of NMDA EPSC obtained at 1, 2, and 5 Hz areadded also (closed symbols). The solid line is a fit to a doubleexponential function, which included the value of I_ss/I₀ at 100Hz. B, Correlation of the amount of depression I_ss/I₀ and theinitial peak EPSC amplitude I₀. Data for 10 Hz (n = 13; closedsymbols) and 5 Hz (n = 11; open symbols) were pooled and fit bylinear regression.
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The finding that a robust form of synaptic depression can be induced at intermediate stimulation frequencies of 1-10 Hz suggeststhat the recovery rate from depression is slow. Interestingly,a strong depression of AMPA receptor-mediated EPSCs with a fasttime course of recovery ( $approx$ 15 msec at 30°C; Trussell et al., 1993)has been described in a chick calyx synapse, and this form ofsynaptic depression has been linked to desensitization of postsynapticAMPA receptors. We therefore measured the recovery time constantfor synaptic depression elicited at intermediate stimulation frequencies.A conditioning train of 30 pulses at 10 Hz was followed by a singletest pulse given at a variable time interval after the end ofthe stimulus train. A waiting period of 30 sec was used betweenthe single test pulse and a subsequent conditioning train. Anexample of depression at 10 Hz, followed by recovery measuredat time intervals $Delta$ t in the range of 0.5-16 sec, is shown in Figure3A. After a recovery time of 0.5 sec, only $approx$ 10% of the depressionhas recovered, and the complete time course of recovery was wellfit by a single exponential with a time constant $tau$ = 4.2 sec (Fig.3B). This time constant of recovery was independent of the amplitudeof the initial EPSC in the 10 Hz train or the amount of overalldepression.
Fig. 3. Recovery time course from depression induced at 10 Hz. Conditioning trains of 30 stimuli at 10 Hz were followed by singletest stimuli at varying intervals from 0.5 to 16 sec. Aa, A representativeexample of AMPA EPSCs recorded at a holding potential of $-$ 80 mVduring a conditioning train. Ab, Five AMPA EPSCs recorded in thesame cell as for Aa after recovery intervals $Delta$ t varying between0.5 and 16 sec. Note that after 0.5 sec only $approx$ 15% of the decrementin EPSC amplitude induced by depression has recovered. B, Recoverytime course from depression, expressed as the percentage of EPSCdecrement (I_d = I₀ $-$ I_ss; see also Fig. 7B). Data from five cellswere fit by a single exponential function with a time constant $tau$ = 4.2 sec.
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Depression of NMDA receptor-mediated EPSCs
The recovery from synaptic depression at 10 Hz is significantly slower than the recovery from AMPA receptor desensitization,which is in the range of 10-300 msec for various native and recombinantAMPA receptors (Colquhoun et al., 1992; Trussell et al., 1993;Lomeli et al., 1994). We therefore studied NMDA receptor-mediatedEPSCs (Forsythe and Westbrook, 1988) to determine whether depressionresults from a reduction in glutamate release. It has been shownpreviously that manipulations that reduce the amount of presynapticglutamate release lead to a parallel reduction of the AMPA andthe NMDA components of the EPSC [see Perkel and Nicoll (1993)and Tong and Jahr (1994a) and references therein]. Therefore,if depression is attributable to presynaptic mechanism(s), italso should be observable for the NMDA component of the EPSC.

EPSCs were elicited in 2 mM [Ca]_o and 1 mM [Mg]_o at positive holding potentials (+60 or +80 mV). Under these conditions adual component EPSC was observed, which consisted of the fastAMPA component as well as of a more slowly rising and decayingcomponent (Hestrin et al., 1990; Forsythe and Barnes-Davies, 1993),which was largely blocked by 50 µM D-AP5 and thus was mediatedby NMDA receptors. Repetitive stimulation at 1 Hz induced depressionof the NMDA component to a value of I_ss/I₀ = 0.59 in the exampleof Figure 4A. The inset in Figure 4A displays the same data onan expanded time scale and shows that the NMDA receptor-mediatedcurrents peaked at $approx$ 16 msec after the peak of the AMPA receptor-mediatedcurrents. In the same cell the amount and the time course of depressionof the peak AMPA component (measured at $-$ 80 mV; Fig. 4B, opensymbols) were found to be similar to the depression of the peakNMDA component (Fig. 4B, closed symbols). In six cells in whichdepression was measured at 1 Hz, I_ss/I_o was 0.47 ± 0.09 for AMPAEPSC and 0.51 ± 0.05 for NMDA EPSC and thus not significantlydifferent (see Fig. 2A). Similar results also were obtained for2 Hz (I_ss/I_o = 0.33 ± 0.05 for NMDA EPSC; n = 3) and 5 Hz (I_ss/I_o= 0.27 ± 0.08 for NMDA EPSC; n = 4) stimulation frequencies. However,at 5 Hz the slowly decaying NMDA baseline current (see Fig. 4A)resulted in a large residual current ( $approx$ 33% of NMDA I_o; see Materialsand Methods) that had to be subtracted systematically. At theshort stimulus intervals during 5 Hz stimulation, a slight overestimationof the degree of depression might occur, because NMDA channelsthat are still open after the first release event might not beactivated (Lester et al., 1990).

NMDA receptors show different forms of desensitization that potentially can contribute to depression of NMDA EPSCs. For example,at subsaturating glycine concentrations (Johnson and Ascher, 1987)a strong form of desensitization has been described (Benvenisteet al., 1990). Therefore, in two cells we added a suprasaturatingglycine concentration to the slice (100 µM glycine in the presenceof 2 µM strychnine), but we found that the depression of NMDAEPSCs was not changed. Also, a Ca-induced desensitization of NMDAreceptors (Legendre et al., 1993) should not be involved, becauseNMDA-mediated Ca influx is negligible at positive membrane potentialsof approximately +60 mV (Schneggenburger et al., 1993), and 5mM EGTA was included in the patch pipette solution (see Materialsand Methods). Thus the simplest interpretation of the findingthat AMPA and NMDA components of the EPSC show similar amountsof depression is that the amount of glutamate release is reducedduring synaptic depression.

CPPG is a potent mGluR antagonist
A possible presynaptic mechanism for depression is the activation of autoreceptors, negatively coupled to release, by spilloverof neurotransmitter from the synaptic cleft (Scanziani et al.,1997). In the calyx of Held, activation of metabotropic glutamatereceptors by synthetic agonists has been shown to inhibit synaptictransmission via a presynaptic mechanism (Barnes-Davies and Forsythe,1995) involving an inhibition of voltage-gated Ca²⁺ currents (Takahashi et al., 1996). However, a potent antagonistfor mGluRs has been lacking for the calyx of Held synapse. Thewidely used antagonist (R, S)- $alpha$ -methyl-4-carboxyphenylglycine(MCPG) (Glaum and Miller, 1993; Bolshakov and Siegelbaum, 1994;Burke and Hablitz, 1994; Maki et al., 1995; Scanziani et al.,1997) was ineffective at the calyx of Held (Barnes-Davies andForsythe, 1995) even at 0.5-1 mM concentrations. We thereforehave studied the actions of a more recently synthesized competitiveantagonist of group II and group III mGluRs, CPPG (Jane et al.,1996).

EPSCs were elicited every 5 sec (Fig. 5A) and were found to be reversibly reduced by L-AP4 and ACPD. On average, peak AMPAEPSCs were reduced from a 100% control value to 34 ± 6% (n = 9)and 53 ± 11% (n = 4) with L-AP4 (50 µM) and ACPD (50 µM), respectively(Fig. 6B). DCG-IV, a high-affinity group II agonist, reduced EPSCsto 60 ± 7% (n = 5) at the relatively high dose of 5 µM and to39 ± 6% (n = 3) at 10 µM, but it has been reported that DCG-IVmight inhibit EPSCs via activation of NMDA receptors (Breakwellet al., 1997) (see, however, Macek et al., 1996) at $approx$ 10 µM, sowe did not study its effects further. In contrast to MCPG (Barnes-Daviesand Forsythe, 1995), we found that CPPG reversed the agonist actionof L-AP4 in a dose-dependent manner. At concentrations of 10 and30 µM, CPPG partially reversed the effect of 50 µM L-AP4 (seeFig. 5A for an example of 30 µM), whereas at 300 µM CPPG restoredthe EPSC amplitude to 104 ± 4% (n = 2) of control (Figs. 5B, 6B).In the presence of CPPG the EPSC decay kinetics were similar tocontrol conditions (Fig. 5C). The dose-response curve of thisCPPG effect is shown in Figure 6A; the data were fit by a Hillfunction with a half-maximal active concentration of 25 µM anda Hill coefficient of 1.5. CPPG also reversed the inhibition inducedby 50 µM ACPD to a value of 99 ± 11% of control (see Fig. 6B).These findings are in agreement with the competitive antagonismof CPPG at group II and group III mGluRs reported by Jane et al.(1996) in the spinal cord of 1- to 5-d-old rats. CPPG is thusa potent antagonist of mGluRs at the calyx of Held.
Fig. 6. Summary of the antagonistic effects of CPPG. A, Dose-response curve for the effect of CPPG on the L-AP4-induced inhibitionof EPSC amplitudes. In each cell (n = 9), applications of 50 µML-AP4 were followed by coapplications of 50 µM L-AP4, togetherwith the indicated concentration of CPPG. EPSC amplitudes wereanalyzed after stable values had been reached ( $>=$ 1 min after changeof solutions; see Fig. 5). The average inhibition induced by 50µM L-AP4 in the absence of CPPG (n = 9) is indicated by the opensymbol. The solid line is drawn according to a Hill equation witha half-maximal active concentration of 25 µM and a Hill coefficientof 1.5. B, CPPG (300 µM) reversed completely the agonist effectof both L-AP4 (50 µM; n = 2 cells) and ACPD (50 µM; n = 4 cells).
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Effects of CPPG on synaptic depression
We next asked to what extent CPPG-sensitive mGluRs contribute to synaptic depression. Given that the affinities of recombinantlyexpressed group II and group III mGluRs for ACPD and L-AP4, respectively,are comparable or even higher than for the putative transmitterL-glutamate (Tanabe et al., 1993) (for review, see Saugstad etal., 1995), a concentration of 300 µM CPPG should be very effectivein blocking the activation of mGluRs by glutamate spillover fromthe synaptic cleft. To test the action of CPPG on synaptic depression,we applied 5 or 10 Hz trains of n = 30 stimuli at intervals of $approx$ 45 sec to allow for the complete recovery of depression in betweenthe trains. After having obtained a few examples of depressionin control conditions, we applied 300 µM CPPG to the slice. Ascan be seen in Figure 7A in which I_ss and I₀ were plotted normalizedto the average value of the corresponding control group, CPPGinduced a small but significant increase in I_ss (1.25-fold overcontrol; n = 4 cells), whereas I₀ was unaffected. The small effectof CPPG on depression is shown in Figure 7B for one cell in whichthe peak EPSC amplitudes from n = 4 trains were averaged for controlconditions (open symbols) and for 300 µM CPPG (closed symbols).To compare the amount of depression under these two conditions,we calculated the decrement I_d in EPSC amplitude (I_d = I₀ $-$ I_ss;see Fig. 7B). In the cell shown in Figure 7B, the decrement was1.03 nA in control and 0.90 nA in the presence of CPPG and thuswas reduced by 12%. On average, the value of I_d was found to bereduced by 6.2 ± 2.5% (n = 4 cells, with I₀ = 1.8, 2.7, 4, and8 nA) when 300 µM CPPG was applied. These results suggest thatCPPG-sensitive mGluRs contribute on the order of 10% or less tothe overall depression elicited by 5-10 Hz stimulation of thecalyx of Held.
Fig. 7. Depression in the presence of CPPG. Trains of 30 stimuli at 5 or 10 Hz were applied at intervals of $approx$ 45 sec. After four tofive examples of depression in control conditions were obtained,300 µM CPPG was perfused into the slice. A, I₀ and I_ss for eachtrain were normalized to the corresponding average values of thecontrol group and plotted as a function of the number of trains.Note that, after 300 µM CPPG was applied (indicated by the solidbar), I_ss was increased to 1.25-fold over control, whereas I₀was unaffected (n = 4 cells). B, For a single cell the averagedepression under control conditions (n = 4 trains; open symbols)is superimposed on the average depression in the presence of 300µM CPPG (n = 4 trains; closed symbols). Note that I₀ is unchanged,whereas the decrement in EPSC amplitude induced by depression(I_d) is slightly reduced by 300 µM CPPG.
[View Larger Version of this Image (21K GIF file)]

DISCUSSION

Depression is mediated mainly by presynaptic mechanism(s)
Frequency-dependent depression is a major form of short-term plasticity at the calyx of Held synapse. We have found robustdepression of AMPA and NMDA receptor-mediated EPSCs over a widerange of frequencies (0.2-100 Hz) but have studied mostly thesynaptic depression elicited by 5-10 Hz trains, partly becausethis type of depression can be dissociated from facilitation,whereas at higher stimulation frequencies both phenomena occursimultaneously, complicating an analysis of their underlying mechanisms.At 100 Hz, for example, a facilitated second EPSC sometimes isobserved [see Borst et al. (1995), their Fig. 11A]. Furthermore,recently Helmchen et al. (1997) showed that the [Ca]_i transientwithin the calyx of Held, triggered by a single action potential,returns to resting levels after $approx$ 100 msec, so that a rapid buildupof presynaptic [Ca]_i, which could lead to facilitation (Zucker,1989; Atluri and Regehr, 1996), may not occur for 5-10 Hz stimulationfrequencies. In addition, presynaptic calcium current inactivationcaused by calcium influx (Yawo and Momiyama, 1993; von Gersdorffand Matthews, 1996) is probably not significant at lower stimulationfrequencies, thus simplifying the analysis of synaptic depression.Calcium current inactivation in fact has been ruled out as a factorcausing depression in the giant synaptic terminals of goldfishbipolar neurons (von Gersdorff and Matthews, 1997).

The degree of depression of EPSCs as assayed by the ratio I_ss/I₀ depended strongly on stimulation frequencies ranging from0.2 to 1 Hz (Fig. 2A). Half-maximal depression was observed alreadyat $approx$ 1 Hz. This contrasts with recently reported experiments ondepression of evoked field potentials and EPSPs in pyramidal neuronsof the rat neocortex, where half-maximal depression was observedat 10-15 Hz (Abbott et al., 1997; Tsodyks and Markram, 1997).The initial steep dependence of EPSC depression on frequenciesranging from 0.2 to 1 Hz can be accounted for by the recoverytime constant from depression that we independently measured ( $tau$ = 4.2 sec; Fig. 3B); however, for the depression elicited at frequencieslarger than 2 Hz, this relatively slow recovery rate cannot accountfor the observed degree of depression. The shallow dependenceof depression on frequencies in the range from 2-10 Hz (see Fig.2A) is compatible with the hypothesis of an accelerated recoveryor recruitment process during the stimulation train as proposedby Kusano and Landau (1975) for the squid giant synapse.

We have shown that AMPA and NMDA receptor-mediated EPSCs were depressed in a parallel manner for 1-5 Hz stimulation frequencies.AMPA and NMDA receptors are thought to be colocalized in the synapticcleft (Bekkers and Stevens, 1989; Jones and Baughman, 1991). NMDAreceptors, however, show less complete and slower desensitization(Benveniste et al., 1990; Legendre et al., 1993) than AMPA receptors,and under our recording conditions desensitization of NMDA receptorsshould have been negligible. Thus, the simplest interpretationof the finding that AMPA and NMDA EPSCs are depressed in parallelis that presynaptic mechanism(s) are responsible for depression.

The recovery rate from 5-10 Hz depression for AMPA EPSCs that we measured was $tau$ = 4.2 sec. Similar recovery time constantswere reported in the squid giant synapse ( $tau$ = 4.9 sec; Kusanoand Landau, 1975), the frog neuromuscular junction ( $tau$ = 5 sec;Betz, 1970; Magleby, 1987), and cultured hippocampal neurons ( $tau$ = 8-12 sec; Stevens and Tsujimoto, 1995). Recovery from depressionis, however, faster in pyramidal neurons of the neocortex ( $tau$ =300-960 msec; Abbott et al., 1997; Tsodyks and Markram, 1997).Our time constant of 4.2 sec also contrasts with the recoveryfrom AMPA receptor desensitization in outside-out patches fromthe chick magnocellularis neurons (Trussell et al., 1993), whichwas found to be $approx$ 20 msec at room temperature. Furthermore, oneof the AMPA receptor subunits likely to be expressed in rat MNTBprincipal neurons, GluR-D_flop (Geiger et al., 1995), displaysrapid recovery from desensitization when tested in a recombinantsystem ( $tau$ _rec = 30-50 msec; Lomeli et al., 1994). Recent experimentsusing flash photolysis of caged glutamate in the chick magnocellulariscalyx by Otis et al. (1996) also shows that AMPA receptor-mediatedEPSCs recover completely from desensitization within $approx$ 60 msec.This further suggests that depression at 5-10 Hz is not attributableto postsynaptic receptor desensitization. We emphasize, however,that at higher stimulation frequencies (e.g., at 100 Hz) desensitizationmight become a significant factor in AMPA receptor-mediated EPSCdepression (Trussell et al., 1993). Thus at different stimulusfrequencies different mechanisms may operate to produce synapticdepression.

mGluRs contribute a small amount to depression
Activation of autoreceptors that negatively regulate presynaptic Ca²⁺ channels or exocytosis is a possible mechanism by which depressionmay be induced after repeated synaptic stimulation. At the frogneuromuscular junction, for example, antagonists of adenosineautoreceptors block completely 1 Hz-elicited short-term depression(Redman and Silinsky, 1994). Activation of mGluRs inhibits EPSCsin hippocampal slices (Baskys and Malenka, 1991; Macek et al.,1996) and in the lamprey giant synapse (Krieger et al., 1996).At the MNTB Barnes-Davies and Forsythe (1995) have shown previouslythat agonists of mGluRs depress EPSCs. In addition, Takahashiet al. (1996) showed that activation of mGluRs by L-AP4 inhibitsthe calyx calcium current, thus making activation of mGluRs anattractive possible mechanism for depression at this synapse.We have shown, however, that CPPG-sensitive mGluRs contribute<10% to 5-10 Hz-induced synaptic depression. Nevertheless, ifthe mGluRs of the calyx of Held are located outside the synapticcleft, as is the case for the mGluR2 receptors on the mossy fiberterminals of the rat hippocampus (Yokoi et al., 1996), our resultsconfirm that glutamate spillover can activate presynaptic mGluRs(Scanziani et al., 1997), but the results argue against a tonicinhibition of release by ambient glutamate (Zorumski et al., 1996),because peak EPSCs (I_o) elicited at intervals of $approx$ 45 sec did notchange in the presence of CPPG (Fig. 7A). It is possible thatafter prolonged activation (e.g., 900 stimuli; Kobayashi et al.,1996) mGluR-dependent long-term plasticity phenomena may be inducedat the calyx of Held synapse, but we did not investigate thispossibility. In addition, we emphasize that our recordings wereperformed at room temperature, when glutamate uptake is sloweddown significantly (Tong and Jahr, 1994b; Asztely et al., 1997),so the contribution of mGluRs to short-term synaptic depressionmay be even smaller at the higher physiological temperature. Furthermore,we have used juvenile rats (postnatal day P8-P11) in our experiments,and certain aspects of synaptic transmission may not be developedfully at this age (Lohmann and Friauf, 1996).

Implications of depression at the calyx of Held synapse
A single synaptic terminal can be stimulated reliably at the calyx of Held. Above the stimulus threshold a single action potentialis triggered through a single large-diameter axon. Dendritic filteringor attenuation of EPSCs is probably absent because of the axo-somaticnature of the synaptic structure. The anomalously large numberof active zones, however, makes this synapse rather unique amongmammalian CNS synapses, which are typically less than a micrometerin size. The quantal content of evoked EPSCs is large ( $approx$ 200 quanta;Borst and Sakmann, 1996), although different active zones mayrelease with different probabilities (Hessler et al., 1993; Rosenmundet al., 1993; Murthy et al., 1997). Despite its pronounced depression,the calyx of Held synapse is capable of reliable synaptic transmissionat 200 Hz in the age range we have studied (Borst et al., 1995;Brew and Forsythe, 1995) at room temperature (25°C); in adultanimals pre- and postsynaptic action potentials can phaselockto an impressive rate of 600 Hz (Smith et al., 1991; Wu and Kelly,1993) at physiological temperatures (37°C). The large number ofrelease sites therefore might be seen as a safety factor thatallows reliable synaptic transmission to take place even at highfrequencies when only a small fraction of synaptic vesicles mightbe available for release. In addition, the particular set of ionchannels expressed in the postsynaptic principal neurons, someof which display rapid activation and strong outward rectification(Brew and Forsythe, 1995), may aid the principal cell in followinghigh stimulation frequencies even when quantal output is low becauseof synaptic depression.

In summary, our data are consistent with a presynaptic locus for synaptic depression induced at 1-10 Hz stimulation frequencies,with a small contribution from presynaptic mGluR activation. Becausethe [Ca]_i transients in the calyx should not summate significantlyat these frequencies (Helmchen et al., 1997), presynaptic calciumcurrent inactivation is an unlikely possibility as a mechanismfor depression. We thus suggest that vesicle pool depletion maybe the main mechanism inducing depression at these lower frequencies.The calyx of Held synapse, stimulated at 1-10 Hz, thus may becomean excellent model system to study synaptic vesicle recruitmentat conventional active zones that have been depleted by depression.

FOOTNOTES

Received June 26, 1997; revised Aug. 8, 1997; accepted Aug. 12, 1997.

This work was supported by the Deutsche Forschungsgemeinschaft (SFB406) and by Alexander von Humboldt and Human Frontier ScienceProgram fellowships to H.v.G. We thank Drs. J. G. G. Borst andI. D. Forsythe for advice on the MNTB brainstem slice preparation.

Correspondence should be addressed to Dr. Henrique von Gersdorff, Max-Planck-Institut für biophysikalische Chemie, AbteilungMembranbiophysik, Am Fassberg D-37077, Göttingen, Germany.

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