Control of Synaptic Depression by Glutamate Transporters

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The Journal of Neuroscience, March 1, 2000, 20(5):2054-2063

Control of Synaptic Depression by Glutamate Transporters
Rostislav Ture $c$ ek and Laurence O. Trussell
Oregon Hearing Research Center and Vollum Institute, Oregon Health Sciences University, Portland, Oregon 97201

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The role of glutamate transporters in the regulation of synaptic depression was examined in the avian nucleus magnocellularis.Repetitive stimulation of presynaptic auditory nerve fibers resultedin acute depression of EPSCs. Pharmacological blockade of glutamatetransport in glial cells enhanced residual glutamate in the synapticcleft and markedly increased the extent of depression at stimulusfrequencies above 20 Hz via a postsynaptic mechanism. Glutamatepyruvate transaminase, a glutamate scavenger, accelerated thedecay of the EPSC and reduced synaptic depression, indicatingthat transporters are not completely effective in rapid removalof glutamate. Regulation of residual transmitter by glia may thusserve to control synaptic strength in a frequency-dependentmanner.

Key words: AMPA; auditory; plasticity; depression; synapse; cochlear nucleus

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The removal of glutamate from the synaptic cleft is accomplished through passive diffusion of transmitter and its subsequentuptake by glutamate transporters located in glial cells and neurons(Gegelashvili and Schousboe, 1998). Such uptake ultimately recyclestransmitter and prevents excitotoxic damage (Rothstein et al.,1996; Tanaka et al., 1997). What immediate effect the activityof transporters has on low-frequency EPSCs depends on the density,location, and affinity of the transporters, as well as factorsrelated to the sites and amount of transmitter release (Trussell,1998). These factors are clearly not constant at all synapsesin the CNS, because block of uptake by selective antagonists haswidely varying effects in different brain regions and preparations(Trussell, 1998). Moreover, the role of transporters during activationof the synapse at physiological firing rates is not well understood.One might expect, for example, that repetitive stimulation would,in the absence of transport, result in rapid accumulation of transmitter.Such build-up of glutamate could then inhibit synaptic function,either presynaptically through metabotropic glutamate receptors(Maki et al., 1994; Scanziani et al., 1997) or postsynapticallyby desensitization of glutamate receptors (Otis et al., 1996a).

In neurons of the cochlear nucleus magnocellularis (nMag) of the chick, end-bulb synaptic terminations of the auditory nerveproduce large EPSCs mediated by AMPA receptors (Zhang and Trussell,1994a,b). Repetitive activation of these synapses results in strongsynaptic depression because of both presynaptic and postsynapticfactors, the latter representing receptor desensitization (Trussellet al., 1993; Otis et al., 1996a). In a previous study of thispreparation, block of glutamate transport at room temperatureusing selective antagonists was observed to have little effecton the time course of the EPSC, only prolonging a small slow phaseof the EPSC (Otis et al., 1996b). This slow component of the EPSCwas proposed to reflect the slow removal of residual transmitterfrom the synaptic cleft. Here, we report the effects of increasingor decreasing the clearance rate of glutamate on synaptic depression.We found that transporters acted primarily to minimize, but couldnot eliminate, the short-term accumulation of glutamate and subsequentdesensitization of AMPA receptors and that enhancement of glutamateremoval increased synapticstrength.

Parts of this work have been published previously in abstract form (Ture $c$ ek and Trussell, 1998).

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

These experiments were performed at the Department of Physiology, University of Wisconsin-Madison; all experimental proceduresfollowed the guidelines of the Animal Care and Use Committee ofthat institution. Brainstem slices (300 µm) prepared from embryonicday 18 (E18) to E19 chick embryos (Zhang and Trussell, 1994b;Otis et al., 1996b) were stored in and, during recordings, perfusedat 3 ml/min with an oxygenated extracellular solution (35-37°C)composed of (in mM): 140 NaCl, 20 glucose, 5 KCl, 1 MgCl₂, 3 CaCl₂,and 10 HEPES (315 mOsm) at pH 7.3 with NaOH. Slices were bathedin antagonists of NMDA, GABA_A, and glycine receptors [20 µM (±)-3-(2-carboxypiperazin-4-yl)propyl-1-phosphonicacid] 20 µM 7-Cl-kynurenic acid, 15 µM SR-95531, and 2 µM strychnineto isolate AMPA receptor-mediated EPSCs. Recording pipettes forwhole-cell recording of EPSCs contained (in mM): 125 CsMeSO₃,15 CsCl, 5 EGTA, 1 MgCl₂, and 10 HEPES (290 mOsm) at pH 7.2 withCsOH. For recordings of orthodromic action potential activity,pipettes contained (in mM): 107.5 K-gluconate, 32.5 KCl, 5 EGTA,1 MgCl_2, and 10 HEPES (285 mOsm) at pH 7.3 with KOH. For recordingsof transporter-evoked currents, the bath solution given abovewas supplemented with 50 µM 6,7-dinitroquinoxaline-2,3-dione,40 µM GYKI-52466, 10 mM TEA, 1 mM 4-aminopyridine, and 1 µM tetrodotoxin,and the pipette fill contained (in mM): 110 KNO₃, 30 KCl, 1 MgCl_2,5 EGTA, and 10 HEPES (280 mOsm) at pH 7.3 with KOH. Voltages arecorrected for junction potentials of $-$ 11.7 (K-gluconate-basedfilling solution), $-$ 6.5 (KNO₃) and $-$ 8.8 (CsMeSO₃) mV. Glutamatepyruvate transaminase (GPT) was applied by pressure ejection (0.12-0.42psi, diameter of mouth of an application pipette was 30 µm; distancefrom cell, 40-50 µm) (Picospritzer II; General Valve, Fairfield,NJ) or by bath perfusion. Concentration of GPT was 5-60 U/ml,as indicated, and enzyme applied in the presence of 2-20 mM pyruvicacid. Osmolality of all extracellular solutions was checked andadjusted with water to ~320 mOsm. Viscosity of extracellular solutionswas not measurably changed by addition of GPT (60 U/ml) when assayedusing a falling-ball viscometer (Gilmont, Barrington, IL). Insome cases, pyridoxal 5-phosphate (10 µM) was added to perfusionsolution.

Neurons were viewed using a Zeiss (Oberkochen, Germany) Axioskop FS with differential interference contrast optics and a 60×water immersion objective. Borosilicate glass electrodes for whole-cellrecording had resistances of 3-4 M $Omega$ , and series resistances duringrecordings were <7 M $Omega$ and were compensated electronically by >90%.Neurons were voltage clamped to $-$ 30 mV and glial cells to $-$ 70mV, unless otherwise indicated. For recordings from glial cells,the electrodes were 6-7 M $Omega$ , with series resistances of 13-25 M $Omega$ ,compensated by 80%. EPSCs were elicited (100 µsec, 40-50 V ofstimuli) with an extracellular glass pipette. Zhang and Trussell(1994a) discussed evidence that this method of stimulation activatesa single axonal input in nMag. EPSCs and EPSPs were recorded withan Axopatch 200B (Axon Instruments, Foster City, CA), filteredat 5 kHz, and were digitized at 20 kHz and analyzed using pClampsoftware (Axon Instruments). Transporter currents were filteredat 1 kHz and sampled at 2 kHz. Reagents were obtained from Sigma(St. Louis, MO), Tocris-Cookson (St. Louis, MO), Research Biochemicals(Natick, MA), and ICN Biochemicals (Costa Mesa, CA). Cyclothiazidewas a gift from Lilly Corp. Neurons were identified by their typicalmorphology (spherical round cells of diameter ~20 µm, only oneapparent process), their ability to generate an EPSC and an actionpotential, and their typical current responses evoked by voltagesteps (Zhang and Trussell, 1994a,b). Glia were identified as smallcells (6-8 µm, flat oval or irregular shape, several tiny processes)with no spontaneous EPSCs, incapable of action potential generation,and a characteristic profile of outward current responses evokedby depolarizing voltagepulses.

Exponential current decays were fitted using the Chebyshev algorithm in pClamp 6.0. In initial experiments, the fitting resultswere checked by refitting the data using the slower Simplex algorithm(fractional error criterion 10⁵), which showed excellent agreement. In measuring the amplitudeof EPSCs in a train, the peak of each EPSC was determined relativeto a baseline established by fitting a double exponential to thedecay of the previous EPSC in the train. Means are reported ±1 SD. Populations were compared using paired and unpaired ttests.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Role of transporters during low-frequency synaptic activity

Glutamate transport was inhibited by bath application of extracellular solution containing 300 µM D,L-threo- $beta$ -hydroxyasparticacid (THA) and 300 µM dihydrokainic acid (DHK), termed THA+DHK.In a later section, we show that this mixture effectively inhibitsionic currents generated by glutamate transporters. THA was observedto activate weakly NMDA receptors in neurons (see Fig. 8F), whereasDHK did not activate ionotropic glutamate receptors (Tong andJahr, 1994) or modify their responses to exogenously applied glutamate(data not shown). Thus, in the presence of NMDA receptor antagonists,THA+DHK was adequate for examining the effect of transportersonEPSCs.

Figure 1 shows the action of THA+DHK on EPSCs evoked by stimulation of a single presynaptic axon at 0.03 Hz. No effect wasseen on the amplitude of the EPSCs (Fig. 1A,B,E), even after 20min exposure to the antagonists. Although the EPSCs decayed almostcompletely within a few milliseconds, there was a small, slow"tail" after the EPSC; this current tail was prolonged by THA+DHK,as shown in Figure 1A-D. To quantify this effect, the decay phaseof EPSCs was fitted with a sum of three exponentials (Fig. 1C,D)(Otis et al., 1996a). Figure 1, F and G, shows that only the timeconstant of the third, slowest exponential was slowed by the uptakeblockers, although the relative weights of all three componentsremained the same as in control solutions. As discussed previously(Otis and Trussell, 1996; Otis et al., 1996b), the faster twocomponents are related to the kinetics of AMPA receptors and theasynchrony of vesicle release, whereas the slow phase reflectsslow clearance of low levels of glutamate. The selective prolongationof the slow phase is consistent with the hypothesis that transportersact only fast enough to remove glutamate over a period of tensof milliseconds, although diffusion is rapid enough to clear themajority of transmitter from the cleft within milliseconds.

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Figure 1. Action of transporter blockers on time course of single EPSCs. A, B, Control EPSC and EPSC in THA+DHK (300 µM each) in one cell. Holding potential of $-$ 30 mV. Inset, overlay of traces in A and B, emphasizing late phase of decay. C, D, EPSCs in control and THA+DHK, as indicated, with three-exponential curves (gray) superimposed on the decay phase. Insets emphasize the fit of the curve to the late phases of decay. Arrows indicate times after onset of the response. E, Average change in peak of low-frequency EPSCs induced by THA+DHK (n = 11). F, Values of the time constants in control and uptake blockers for three-exponential fits to decay of low-frequency EPSCs (n = 12). G, Relative magnitudes of each component in the fitted curves.

Repetitive EPSCs during transport block

At higher synaptic stimulus rates, block of transport resulted in larger changes in EPSC amplitude. Figure 2, A and B, showsa response to a 100 Hz train of 10 synaptic stimuli in controlsolution and in THA+DHK. Although the size of the first EPSC inthe train was unchanged, subsequent EPSCs were smaller after blockinguptake. This effect was quantified by measuring the extent ofdepression, expressed as the amplitude of the 10th divided bythe amplitude of the first EPSC in a train (P₁₀/P₁), as a functionof stimulus frequency. Data were collected over a range from 0.03to 600 Hz to determine the frequency-dependence of the actionof transporters. As shown in Figure 2, C and D, no effect on depressionwas evident until the stimulus rate exceeded 10 Hz. Above thisfrequency, blockade of transporters significantly enhanced depression,with the largest effects seen at the highest stimulus rates atwhich measurable responses could be obtained (Fig. 2E, gray bars).For comparison, we also measured the effect of antagonists onthe paired-pulse depression (P2/P1). The second EPSC also showedgreater depression in the presence of uptake blockers but lessthan that observed during lengthier stimulus trains (Fig. 2E,open bars).

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Figure 2. Effect of transport blockers on frequency-dependent depression. A, B, Train of 10 EPSCs elicited at 100 Hz before and during application of THA+DHK. Data from one cell. C, Ratio of the average amplitude of 10th and 1st EPSCs in a train, elicited at different frequencies. Control, n = 10; THA, n = 9. D, The region of data in C in which blockers altered depression. Asterisk indicates significant difference from control solutions (p < 0.01). E, Ratios of the relative amplitude (normalized to first EPSC) of the 10th and 2nd EPSCs in a train in control and blocker solution at different stimulus frequencies (solid bars). At 300 Hz, EPSCs were nearly six times larger in control solutions. Open bars show ratio of second EPSCs in control and blockers, indicating that a greater effect of blockers is seen with longer trains.

Suprathreshold transmission

To explore further the effects of the antagonists on synaptic strength, neurons were current clamped, and trains of 20 presynapticstimuli were delivered at different frequencies. Figure 3, A andB, shows that EPSPs remained suprathreshold at 100 Hz, even inthe presence of the uptake blockers, a consequence of the highsafety factor for transmission in nMag (Brenowitz et al., 1998).However, at 173 Hz, EPSPs in THA+DHK immediately fell subthreshold,whereas control EPSPs still evoked action potentials. At stillhigher rates, neither experimental or control EPSPs were consistentlysuprathreshold, although it was evident that the control EPSPswere larger. Figure 3C quantifies the probability of suprathresholdtransmission over the second half of the train, showing that therewas a cutoff frequency above which EPSPs fail to evoke spikesand that block of uptake shifts the cutoff to lower frequencies.Because nMag neurons are innervated by two to three auditory nerveaxons (Jackson and Parks, 1982) and the EPSPs they elicit maysummate (Zhang and Trussell, 1994a), this cutoff presumably occursat higher frequencies in vivo.

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Figure 3. Antagonists of transporters reduce synaptic strength. A, B, Orthodromic action potentials in control and THA+DHK solutions, as indicated. Subthreshold EPSPs become apparent at 173 Hz when uptake is blocked. C, Average action potential probability at different frequencies in control and THA+DHK. Asterisks indicate significant difference from control (p < 0.01). n = 7-16 for different frequencies. Action potential probability was determined by averaging successes (1) or failures (0) for the last 10 responses in trains of 20 stimuli.

Inhibition of glutamate uptake also had effects on the timing of transmission for EPSPs that remained suprathreshold. Figure4A shows that the size and shape of the first orthodromic actionpotential in a 100 Hz train is unaltered by THA+DHK (control shownin gray), whereas the 20th response is smaller and peaks slightlylater. Because the ipsilateral and contralateral nMag must maintainaction potential timing with a precision of hundreds of microseconds(Hyson et al., 1994), we quantified this shift in action potentiallatency in Figure 4B. The difference in timing of the action potentialpeak in control and THA+DHK solutions was measured for the 1stand 20th responses and plotted as a function of stimulus frequency.Although the first response was unaffected by the antagonists,the 20th occurred at progressively later times as frequency wasincreased, such that by 173 Hz, spikes were delayed by nearly200 µsec. This increase in latency was presumably because of thereduction in amplitude of the EPSP and a consequent delay in whenthreshold was reached (Zhang and Trussell, 1994a). The variabilityin the latency of action potentials later in the train was alsohigher in uptake blockers (Fig. 4C); this effect is quantifiedin Figure 4D as the SD of the timing of the peaks of the last10 orthodromic action potentials evoked in the two experimentalconditions.

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Figure 4. Effects of uptake blockers on the timing of orthodromic action potentials. A, First and 20th synaptically driven action potentials in a 100 Hz train, with (black) and without (gray) THA+DHK. Note slight reduction and delay in spike during antagonist application. B, Difference in timing of 1st and 20th action potentials in trains delivered at different rates. At the higher rates, the suprathreshold spikes occurred with a delay nearly 200 µsec longer in the presence of blockers. n = 6-12. C, Jitter in timing of action potentials at the end of trains increased in the presence of antagonists. D, SD of timing of peaks of last 10 orthodromic action potentials in 100 Hz train of 20 stimuli was significantly increased in THA+DHK. n = 6-12 per frequency.

Accumulation of glutamate during trains of stimuli

Evidence that glutamate accumulated in the synaptic cleft during trains of stimuli came from analysis of the amplitude ofcurrents just preceding each response in the train and the currentdecay after the train. As shown in Figure 5A (dashed line), acurrent "plateau" was apparent between each response; this plateauwas increased in the presence of THA+DHK (Fig. 5B). Moreover,after the train, current decayed more gradually when transporterswere blocked (Fig. 5A). This slower decay was not attributableto an enhancement of slow-acting NMDA receptors, because thesereceptors were blocked by competitive and noncompetitive antagonists(see Materials and Methods) and because the amplitude of the slowdecay phase relative to the peak current was not sensitive toholding potential (Fig. 5A, inset). Figure 5C shows that the plateauwas larger at higher stimulus frequencies but that the enhancementproduced by THA+DHK was approximately similar between 30 and 600Hz.

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Figure 5. Evidence for accumulation of glutamate during trains when transporters are blocked. A, Plateau current (marked by dashed line) between EPSCs in a train (100 Hz) is increased in THA+DHK. Average of three traces. Moreover, the current decay after the train is prolonged. Inset, Train recorded at $-$ 60 and $-$ 30 mV was scaled to the amplitude of the first EPSC and superimposed. The overlap of the decay indicates that the slowed decay does not reflect enhanced activation of NMDA receptors by residual glutamate. B, Amplitude of the current plateau versus stimulus number in a 100 Hz train for control and THA+DHK solutions. Amplitudes measured in the 1 msec period just before each stimulus in the train and normalized to the amplitude of the peak of the first EPSC. Asterisk indicates significant difference from control (p < 0.02). C, Increase in current plateau with stimulus frequency. Current level just before final EPSC was measured as in B (p < 0.03). D, E, Comparison of the decay of current after the 10th response in a 100 Hz train to the decay after a single response, for control and uptake blocker solutions. Note that the decay of the single response is slower in control solutions but relatively faster after uptake blockade. F, Decay time after 10th EPSC in a train delivered at the indicated frequencies. Decay was measured as time necessary for 50% decay current amplitude measured 1 msec before the last stimulus in the train. Single asterisks indicate significant difference of THA+DHK solutions from control solution (p < 0.02), and double asterisks indicate significance of control high-frequency responses from responses at 30 Hz (p < 0.01). n = 7-13 cells.

The decay of EPSCs after a train in the presence of THA+DHK was often not exponential but exhibited a slight hump that madeexponential curve fitting imprecise (Fig. 5A, black trace). Therefore,we quantified the decay time after the train by measuring thetime for the current level just preceding the last response inthe train to decay by 50%. This analysis showed that the decaytime of the slow phase of the last EPSC in a train was significantlylonger in THA+DHK. Moreover, whereas the decay after the trainin control solutions was faster for higher frequency trains, inTHA+DHK the decay time was constant between 30 and 600 Hz (Fig.5F). We interpret the acceleration in decay in control solutionto reflect a declining amount of transmitter release on each stimuluswith increasing frequency (Trussell et al., 1993; Zhang and Trussell,1994b); less release would not tax the capacity of transportersas much, and thus clearance would be faster. The fact that onlyafter block of transport was this decay time similar at all frequenciessuggests that a balance was achieved between progressive accumulationof glutamate and a declining release per stimulus, generatinga similar average amount of transmitter after the train. Thisconclusion is supported by comparison of the decay time aftersingle stimuli versus trains, with and without THA+DHK. Figure5, D and E, shows that, whereas in control solutions the slowphase of decay (arrow) was faster after trains compared with singleresponses (gray trace), the slow phase after the train lastedlonger than the single response when uptake was inhibited. Theseresults suggest that reduction in uptake caused a pooling of transmitter,resulting in repeated rebinding of glutamate to AMPAreceptors.

Postsynaptic locus of increased depression

The enhancement of depression and its effects on spike probability and timing could be a result of either the action of glutamateon presynaptic metabotropic glutamate receptors (mGluRs), whichinhibit release in some auditory neurons (Barnes-Davies and Forsythe,1995; von Gersdorff et al., 1997), or the enhancement of desensitizationof postsynaptic AMPA receptors. The former possibility seemedunlikely because previous studies have shown that a selectiveagonist of some mGluRs, (±)-1-aminocyclopentane-trans-1,3-dicarboxylicacid, had little effect on EPSCs in nMag (Otis and Trussell, 1996),at least at room temperature. This was confirmed in the presentstudy using another mGluR agonist, L(+)-2-amino-4-phosphonobutyricacid (L-AP-4). Bath or pressure ejection application of L-AP-4at 100 µM had no effect on either the baseline holding currentor the amplitude of EPSCs (drug/control values, 0.98 ± 0.11 and0.99 ± 0.03, respectively; n = 4 cells). In contrast, the presynapticGABA_B agonist baclofen was able to strongly depress release inthe same preparation (Brenowitz et al., 1998). Because there doesnot appear to be presynaptic control of release by metabotropicglutamate receptors, it seems unlikely that accumulation of glutamatein THA+DHK actedpresynaptically.

This conclusion was confirmed by examining the actions of THA+DHK in the presence of a blocker of AMPA receptor desensitization,cyclothiazide. In nMag, cyclothiazide prolongs the decay of EPSCsand reduces the extent of synaptic depression (Trussell et al.,1993). In five of six neurons, cyclothiazide (100 µM) inhibitedpaired-pulse depression (10 msec stimulus interval), expressedas the response 2/response 1 amplitude ratio, from 0.40 ± 0.20to 0.62 ± 0.20. In these same cells, application of THA+DHK inthe continued presence of cyclothiazide had no significant effecton depression for either the 2nd or 10th response in a 100 Hztrain (p = 0.09 and 0.40, respectively). Figure 6 illustratesthese effects in one cell, showing the decrease in depressionafter application of cyclothiazide (Fig. 6A,B) and the relativelysmall differences between the amplitudes of EPSCs before and afteradding uptake blockers while in a background of cyclothiazide(Fig. 6B,C). Although it has been proposed that cyclothiazidemay have additional presynaptic actions (Diamond and Jahr, 1995;Bellingham and Walmsley, 1999), the postsynaptic action of thedrug on AMPA receptors is well established (Patneau et al., 1993;Yamada and Tang 1993), and our experimental paradigm should notbe sensitive to presynaptic actions of the drug on vesicle releasemechanisms. Thus, under these experimental conditions, the proclivityof AMPA receptors to desensitize, the absence of an effect ofTHA+DHK on depression when cyclothiazide was present, and theapparent lack of presynaptic metabotropic glutamate receptorstogether indicate that glutamate accumulation enhances depressionthrough increase in desensitization.

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Figure 6. Effects of uptake blockers in the presence of cyclothiazide. A, Control responses to train of 10 shocks at 100 Hz. B, In the same cell after application of 100 µM cyclothiazide, the first EPSC is only slightly larger, but subsequent EPSCs are markedly enhanced, reflecting the reduction of depression induced by cyclothiazide. C, Addition of THA+DHK did not significantly increase depression over that seen in B.

Action of a glutamate scavenger

GPT has been used in previous studies to scavenge synaptically released glutamate (O'Brien and Fischbach, 1986; Rossi andSlater, 1993; Min et al., 1998). In the present work, GPT wasused to determine whether or not glutamate accumulates duringstimulus trains when transporters are active. The prediction wasthat, if accumulating glutamate contributed to synaptic depression,then lessening this accumulation by GPT should reduce the extentof depression. Application of GPT at 5-10 U/ml in the presenceof 2-4 mM pyruvic acid (see Materials and Methods) had no effecton the amplitude of low-frequency EPSCs (GPT/control amplitudes,0.96 ± 0.11; n = 8 cells) (Fig. 6A,B). However, examination ofthe decay of EPSCs showed that GPT accelerated the slow phaseof decay, as illustrated in Figure 6, C and D, with no effecton the relative weights of the exponential components (data notshown). Because this slow phase was attributed to rebinding ofglutamate and was enhanced by THA+DHK, this action of GPT indicatesthat residual glutamate is present even with normal transporteractivity. We then examined the action of GPT on the response totrains of stimuli at 173 Hz and found that the enzyme significantlyreduced the extent of depression during trains, for both the 2ndand 10th EPSC in a stimulus train, as shown in Figure 7. Althoughthere was no measurable effect of GPT on the plateau current betweenresponses in a train, GPT did reversibly accelerate the decayof current after the train, from 14.42 ± 6.22 msec in controlto 9.56 ± 1.99 msec in GPT (p < 0.05; n = 8). Thus, the activityof glutamate transporters is not adequate to completely removeglutamate in the synaptic cleft sufficiently fast to prevent somedesensitization of AMPA receptors.

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Figure 7. Actions of GPT. A, B, EPSCs from one cell in control and 10 U/ml GPT solution. Inset in B shows an overlay of these two traces, revealing a faster decay phase in the presence of GPT. C, The time constants obtained for three-exponential fits with and without GPT (asterisk indicates difference from control; p < 0.01; n = 8). The third exponential component was significantly shorter in GPT, although the relative weights of the components were unchanged (data not shown). D, E, Trains in one cell show less depression in GPT. Peak amplitudes of the first EPSC are cutoff. F, Average behavior for degree of depression for 2nd and 10th EPSC in a train delivered at 173 Hz, with and without GPT. n = 8 cells; p < 0.01. In three of these eight cases, the enzyme was washed out and reversibility demonstrated.

In a second set of experiments, a higher concentration of GPT was used to see whether the glutamate transient could be furtheraccelerated. Using GPT at a concentration of 40-60 U/ml in thepresence of 10-20 mM pyruvate, results were obtained that weresimilar to those with the lower GPT concentration, except thatthe amplitude of the first response in a train was reduced to0.81 ± 0.26 of control (p < 0.05; n = 18). In control experiments,GPT at 40 U/ml in the absence of pyruvate (n = 5) or applicationof 16 mM pyruvate alone (n = 5) produced no significant effecton amplitude and decay time course of single EPSCs or on the amountof depression, the plateau current or the decay after a 173 Hztrain.

Finally, we examined the effect of GPT at 40-60 U/ml on the time course of single EPSCs and extent of depression seen in thepresence of THA+DHK. As observed above, THA+DHK significantlyincreased the decay time of the third exponential component ofsingle EPSCs from 17.8 ± 5.3 to 42.5 ± 21.0 msec (p < 0.01), whereasin GPT plus THA+DHK the decay constant was 27.0 ± 17.5 msec, whichwas significantly different from the decay constant in THA+DHK(p < 0.01; n = 8 cells) but not from control. The amplitude ofsingle EPSCs in THA+DHK was 99.5 ± 4.1% of control amplitude,whereas in GPT plus THA+DHK it was 85.1 ± 14.7% of the peak amplitudein THA+DHK (p < 0.01; n = 11). GPT was not able to acceleratethe decay of current after a 173 Hz train of stimuli in the presenceof uptake blockers, nor did it antagonize the effects of blockerson the plateau current during the train beyond the 15-20% inhibition,which was also observed for the peak response. However, GPT didantagonize the effects of blockers on depression. The extent ofdepression (P₁₀/P₁) at 173 Hz was 0.14 ± 0.10 in control, 0.08± 0.07 (p < 0.01) in THA+DHK, but only 0.13 ± 0.09 in GPT plusTHA+DHK (p < 0.02 for difference from THA+DHK; n = 9). Thus, althoughthe apparent effectiveness of GPT diminished when transporterswere blocked, GPT was still able to reduce glutamate enough tooppose postsynapticdepression.

Sites of glutamate uptake

The site of glutamate uptake was identified by taking advantage of the current generated by glutamate transporters, whichis a combination of ionic flux coupled to the transport processand of nonstoichiometric flux through an anion channel gated bythe transporter (Otis and Kavanaugh, 1999). We maximized bothsources of current by loading cells with a KNO₃ solution, whichhas been shown to produce large currents during activation ofcloned and native glutamate transporters (Wadiche et al., 1995;Bergles and Jahr, 1997; Bergles et al., 1997; Otis and Jahr, 1998).Glutamate (1 mM) was pressure applied for 100 msec to cells inthe continuous presence of antagonists of AMPA and NMDA receptors(see Materials and Methods), so that the resulting currents werelikely to be associated with transporter activity. In the firstset of experiments, currents were recorded from small cells adjacentto nMag neurons (see Materials and Methods). In previous studies,many of these cells were immunoreactive for GFAP (Canady et al.,1994), an astrocyte-specific marker. We therefore compared theirresponse with that of neurons with application ofglutamate.

Figure 8A-D shows the response of glial cells held at $-$ 70 mV to brief application of glutamate and the effect of blockersof glutamate transporters. Glutamate evoked a slow inward currentin every glial cell tested (average peak response of $-$ 114 ± 14pA; 23 cells). These currents were reversibly blocked by 300 µMTHA (control, $-$ 119 ± 43 pA; THA, $-$ 8 ± 5 pA; 4 cells) (Fig. 8A),by 300 µM L-trans-pyrollidine-2,4-dicarboxylic acid (t-PDC) (control, $-$ 104 ± 52 pA; t-PDC, $-$ 16 ± 14 pA; 4 cells) (Fig. 8B) and by 300µM DHK (control, $-$ 127 ± 40 pA; DHK, $-$ 83 ± 10 pA; 5 cells) (Fig.8C). These effects were significant for all compounds (p < 0.05).The THA+DHK mixture used above was most effective, reducing >96%of the inward current induced by glutamate (control, $-$ 104 ± 27pA; THA+DHK, $-$ 4 ± 2 pA; 5 cells) (Fig. 8D). As shown in Figure8E, application of 1 mM glutamate to nMag neurons in the presenceof AMPA and NMDA receptor antagonists and internally perfusedwith a KNO₃ solution (see Materials and Methods) produced currents<10 pA, and these were relatively insensitive to THA (n = 10).Unlike cerebellar Purkinje cells (Kataoka et al., 1997; Otis etal., 1997), nMag neurons do not express a significant level offunctional glutamate transporters. Because glial cell processesin nMag are adjacent to, or inserted into, the end-bulb synapse(Parks, 1981), it seems likely that they provide a significantsite of glutamate transport in vivo.

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Figure 8. Responses of neurons and glia to glutamate application. A-D shows glial cell responses to a 100 msec puff of 1 mM glutamate in the presence and absence of the indicated antagonist, all at 300 µM. Holding potential was $-$ 70 mV, and pipette contained a KNO₃ solution (see Materials and Methods). Offsets generated by direct activity of the antagonist on transporters were removed to illustrate reduction in glutamate response. These values were $-$ 240 (A), $-$ 350 (B), +90 (C), and $-$ 50 (D) pA. E, Effect of glutamate application on a KNO₃-filled nMag neuron. Largest response is in control bath solution, and two small responses are after block of ionotropic glutamate receptors as in Materials and Methods. Spike-like transient is caused by rapid desensitization of glutamate receptors. Inset amplifies responses in receptor blockers, showing that the residual response is small and only weakly sensitive to THA. F, THA+DHK cocktail (500 msec puff) alone produced a small inward current in a CsMeSO₃-filled neuron, which was antagonized by NMDA receptor antagonists (n = 4). All panels show data from different cells. All recordings made in 1 µM TTX.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Control of glutamate transients in the synaptic cleft

Synaptic depression has been attributed to a variety of factors, including transmitter depletion (von Gersdorff et al., 1997),refractoriness of release (Bellingham and Walmsley, 1999), inactivationof calcium current (Forsythe et al., 1998), activation of presynapticautoreceptors (Barnes-Davies and Forsythe, 1995; von Gersdorffet al., 1997), postsynaptic receptor desensitization (Trussellet al., 1993; Otis et al., 1996a), and use-dependent inactivationof receptors (Tong et al., 1995). The latter three mechanismsare sensitive to the effectiveness of clearance of transmitter,such that a delay in clearance, and the resultant pooling of transmitterduring repetitive activity, will enhance depression. At the end-bulbsynapse in nMag, the concentration of release sites compoundsthe problems of clearance faced by the glutamatergic synapse (Otiset al., 1996b). Inhibition of glutamate transporters at this synapseimpedes clearance, yet only slightly slows the decay of the EPSC.Presumably, the faster components of the EPSC do not reflect theclearance process itself, but rather the kinetics of gating andunbinding or desensitizing the AMPA receptor-channel complex,as well as the time course of vesicle fusion (Diamond and Jahr,1995; Isaacson and Walmsley, 1995; Otis and Trussell, 1996). Asnoted previously, the slower component is best explained as trackingthe delayed clearance of a low concentration of glutamate fromthe cleft. That the slow decay phase is attributable to rebindingof transmitter to AMPA receptors was demonstrated here and inprevious experiments, which showed block of the slow phase byCNQX (Otis et al., 1996b), the similarity in its current-voltagerelationship to steady-state AMPA responses (Otis et al., 1996b),its persistence in NMDA receptor antagonists, the lack of effectof mGluR agonists, and the comparatively rapid binding and unbindingkinetics of AMPA receptors (Raman and Trussell, 1995a). Althoughthis tail of glutamate is far lower than the peak concentrationsachieved in the synaptic cleft, it is significant that only lowmicromolar levels are needed to desensitize AMPA receptors (Ramanand Trussell, 1992) and therefore that residual glutamate couldplay a significant role in the ongoing regulation of synapticstrength. In the absence of uptake, EPSCs decayed more slowlyafter a train than after a single stimulus, despite the reductionin transmitter release, indicating a progressive accumulationof transmitter and its rebinding to AMPA receptors. However, whentransporters were active, the decay was faster after a high-frequencytrain, suggesting that transporters play a vital role in removingglutamate on a per stimulusbasis.

Our results are similar in part to the recent study of Overstreet et al. (1999), who examined the effect of transport blockersin the large synapse of the unipolar brush cell. Although no effectswere reported in that study on the peaks of EPSCs during trains,t-PDC slowed the decay of current after a train of synaptic stimuli,increasing the total charge transfer significantly. The postsynapticgranule cell then integrated the extra charge, resulting in increasedfiring. In contrast, the auditory neurons we studied here fireonly on the peak of each EPSP; thus, they were more sensitiveto effects on peak depression than on the change in the shapeof each response and so the net effect of transport blockade wasinhibitory. These differences highlight the importance of interpretingtransporter action in the context of membrane specializationscharacteristic of different neuronalpathways.

Role of glial cells

Large glutamate transporter-dependent currents were observed in glial cells attached to nMag neuronal cell bodies. These responseswere blocked only partially by a relatively high concentrationof DHK, suggesting that these cells express both GLAST and GLT-1,glial isoforms of transporter that differ in their pharmacologicalsensitivities (Gegelashvili and Schoesboe, 1998). Initial attemptsto record synaptically induced glial transporter currents, ashas been performed in hippocampus and cerebellum (Bergles andJahr, 1997; Bergles et al., 1997; Clark and Barbour, 1997), wereonly rarely successful, suggesting that only a small fractionof the processes of any individual glial cell enshroud a givenaxon terminal in this preparation. However, it may also be thattransporter activity resides in the presynaptic terminal; if so,such uptake could significantly abbreviate glutamate transientson a fast time scale (Tong and Jahr, 1994).

Although the accumulation of glutamate and its effect on depression depend critically on the frequency of glutamate release,the effects of transporter blockers were maximal in the physiologicalrange of firing. Thus, modulation of transport by glial cellscould be a significant point of regulation of synaptic strengthin vivo. It has been shown that glial cells in nMag respond tocessation of auditory nerve transmission by proliferation of processes(Canady et al., 1994); more subtle, dynamic control of glial processesor transporter efficacy could prove important to auditory signaling.For example, we have shown that downregulation of transport shiftsthe "cutoff" of suprathreshold transmission to lower frequencies.In principle, it might also shift to higher frequencies with enhancementof transport rate. It is important to note that nMag synapsesfire spontaneously, in the quiet, at ~100 Hz, and presynapticfibers are driven briefly by acoustic stimuli to nearly 400 Hz(Warchol and Dallos, 1990; Chen et al., 1996). Thus, consideringthe frequency range over which the uptake blockers exerted theireffect (Fig. 2D), these data indicate that transporters are likelyto maintain significant control over synaptic strength in vivo.

The potential for upregulation of transporter activity to increase synaptic strength is underscored by our observation thatthe glutamate scavenger GPT was able to reduce depression andaccelerate the decay of the EPSC, with only minor effect on theamplitude of the first EPSC in a train. This indicates that, undernormal conditions, at temperatures only slightly below normal(37 vs 41°C), glutamate transporters, although critical for synapticfunction, are not able to eliminate immediately and completelythe large volume of transmitter released from the end-bulb synapse.This point has bearing on the mechanisms of desensitization inducedby synaptically released glutamate. AMPA receptors desensitizeupon repeated binding to glutamate. However, because desensitizationis rapid and can proceed even from partially liganded, closedstates of the channel (Raman and Trussell, 1995b), it has beenuncertain whether the synaptically induced desensitization wehave observed previously requires prolonged glutamate exposureor whether it happens upon its initial exposure to transmitter.The present results indicate that at least some glutamate mustpersist in the cleft and cause desensitization by repeated activationof thereceptor.

Effectiveness of GPT

Neither blockade of glutamate transport nor enhancement of glutamate degradation with low concentrations of GPT altered thepeak of single EPSCs; only with high concentrations of GPT wasthe peak slightly reduced. Regarding GPT, this result is not surprisingconsidering the low capacity of GPT to consume glutamate. At aturnover rate of 1100/sec and a concentration of 60 U/ml, GPTshould reduce the glutamate concentration by 14 µM/msec, assuming2 mol of glutamate per GPT molecule (Gatehouse et al., 1967; Jenkinsand Saier, 1970). With a peak glutamate transient of ~6 mM (Otiset al., 1996a), this level should have only a minor effect onthe peak EPSC. GPT also did not reduce the plateau current betweenEPSCs in a train, although this may simply reflect the signal-to-noiseratio; because the largest difference in current between GPT andcontrol single EPSC decay phases was only ~20 pA (Fig. 6), thereduction of the current between ongoing, fluctuating EPSCs wouldnot be easilyresolved.

Another issue is that the nMag EPSC, even at its peak, is influenced by cross-talk among clusters of release sites (Otis etal., 1996a). Thus, factors that influence accessibility of glutamateto adjacent synapses could markedly alter the synaptic response.Although the capacity of our GPT solutions for glutamate degradationis relatively low, it may be sufficient to alter the peak EPSCby impeding or slowing cross-talk. This point is also relevantto why block of transport did not alter the peak of single EPSCs,in contrast to what was observed in hippocampal cultures (Tongand Jahr, 1994). If glutamate transporters located on glial cellprocesses are interposed between clusters of release sites ratherthan between each individual site, then transport blockers wouldonly be effective on glutamate transients generated by the aggregateactivity of multiplesynapses.

In the presence of uptake blockers, GPT was less effective. Although still able to reduce depression, current decay aftertrains was not accelerated. Yet clearly the enzyme was active,because it altered depression, and in the absence of uptake blockershastened current decay. This result may give insight into thelevels of glutamate in the cleft during these experimental conditions.The steady-state dose-response relationship for glutamate in nMagis biphasic, with a peak between 70 and 100 µM (Raman and Trussell,1992). Reduction in glutamate levels through the 70-200 µM rangemight be expected to influence the occupancy of receptors, andso alter desensitization, yet produce little decrease (or evenan increase) in the plateaus and slow phases of EPSCs that wemeasured. That, plus the fact that little desensitization occurswith less than ~1 µM glutamate (Raman and Trussell, 1992), suggeststhat alterations in slow currents observed with GPT and withoutuptake blockers probably reflected actions in the range of 1-70µMglutamate.

  FOOTNOTES

Received Oct. 28, 1999; revised Dec. 9, 1999; accepted Dec. 22, 1999.

This work was supported by National Institutes of Health Grant NS28901 (L.O.T.) and Grant TW05406-01 from the Fogarty InternationalCenter, National Institutes of Health (R.T.). We thank Craig Jahrand Tom Otis for helpful conversations and a reading of thismanuscript.
Correspondence should be addressed to L. Trussell, L-335A, Oregon Hearing Research Center, Oregon Health Sciences University,3181 SW Sam Jackson Park Road, Portland, OR 97201. E-mail: trussell{at}ohsu.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Barnes-Davies M, Forsythe ID (1995) Pre- and postsynaptic glutamate receptors at a giant excitatory synapse in rat auditory brainstem slices. J Physiol (Lond) 488:387-406[ISI][Medline].
Bellingham MC, Walmsley B (1999) A novel presynaptic inhibitory mechanism underlies paired pulse depression at a fast central synapse. Neuron 23:159-170[ISI][Medline].
Bergles DE, Jahr CE (1997) Synaptic activation of glutamate transporters in hippocampal astrocytes. Neuron 19:1297-1308[ISI][Medline].
Bergles DE, Dzubay JA, Jahr CE (1997) Glutamate transporter currents in bergmann glial cells follow the time course of extrasynaptic glutamate. Proc Natl Acad Sci USA 94:14821-14825[Abstract/Free Full Text].
Brenowitz S, David J, Trussell L (1998) Enhancement of synaptic efficacy by presynaptic GABA(B) receptors. Neuron 20:135-141[ISI][Medline].
Canady KS, Hyson RL, Rubel EW (1994) The astrocytic response to afferent activity blockade in chick nucleus magnocellularis is independent of synaptic activation, age, and neuronal survival. J Neurosci 14:5973-5985[Abstract].
Chen L, Trautwein PG, Shero M, Salvi RJ (1996) Tuning, spontaneous activity and tonotopic map in chicken cochlear ganglion neurons following sound-induced hair cell loss and regeneration. Hear Res 98:152-164[ISI][Medline].
Clark BA, Barbour B (1997) Currents evoked in Bergmann glial cells by parallel fibre stimulation in rat cerebellar slices. J Physiol (Lond) 502:335-350[ISI][Medline].
Diamond JS, Jahr CE (1995) Asynchronous release of synaptic vesicles determines the time course of the AMPA receptor-mediated EPSC. Neuron 15:1097-1107[ISI][Medline].
Forsythe ID, Tsujimoto T, Barnes-Davies M, Cuttle MF, Takahashi T (1998) Inactivation of presynaptic calcium current contributes to synaptic depression at a fast central synapse. Neuron 20:797-807[ISI][Medline].
Gatehouse PW, Hopper S, Schatz L, Segal HL (1967) Further characterization of alanine aminotransferase of rat liver. J Biol Chem 242:2319-2324[Abstract/Free Full Text].
Gegelashvili G, Schousboe A (1998) Cellular distribution and kinetic properties of high-affinity glutamate transporters. Brain Res Bull 45:233-238[ISI][Medline].
Hyson RL, Overholt EM, Lippe WR (1994) Cochlear microphonic measurements of interaural time differences in the chick. Hear Res 81:109-118[ISI][Medline].
Isaacson JS, Walmsley B (1995) Counting quanta: direct measurements of transmitter release at a central synapse. Neuron 15:875-884[ISI][Medline].
Jackson H, Parks TN (1982) Functional synapse elimination in the developing avian cochlear nucleus with simultaneous reduction in cochlear nerve axon branching. J Neurosci 2:1736-1743[Abstract].
Jenkins WT, Saier M (1970) L-Alanine aminotransferase (pig heart). Methods Enzymol 17A:159-163.
Kataoka Y, Morii H, Watanabe Y, Ohmori H (1997) A postsynaptic excitatory amino acid transporter with chloride conductance functionally regulated by neuronal activity in cerebellar Purkinje cells. J Neurosci 17:7017-7024[Abstract/Free Full Text].
Maki R, Robinson MB, Dichter MA (1994) The glutamate uptake inhibitor L-trans-pyrrolidine-2,4-dicarboxylate depresses excitatory synaptic transmission via a presynaptic mechanism in cultured hippocampal neurons. J Neurosci 14:6754-6762[Abstract].
Min M-Y, Rusakov DA, Kullmann DM (1998) Activation of AMPA, kainate, and metabotropic receptors at hippocampal mossy fiber synapses: role of glutamate diffusion. Neuron 21:561-570[ISI][Medline].
O'Brien RJ, Fischbach GD (1986) Modulation of embryonic chick motoneuron glutamate sensitivity by interneurons and agonists. J Neurosci 6:3290-3296[Abstract].
Otis TS, Jahr CE (1998) Anion currents and predicted glutamate flux through a neuronal glutamate transporter. J Neurosci 18:7099-7110[Abstract/Free Full Text].
Otis TS, Kavanaugh MP (1999) Glutamate transporters and their contributions to excitatory synaptic transmission. In: Ionotropic glutamate receptors in the CNS (Jonas P, Monyer H, eds), pp 419-440. Heidelberg, Germany: Springer.
Otis TS, Trussell LO (1996) Inhibition of transmitter release shortens the duration of the excitatory synaptic current at a calyceal synapse. J Neurophysiol 76:3584-3588[Abstract/Free Full Text].
Otis T, Zhang S, Trussell LO (1996a) Direct measurement of AMPA receptor desensitization induced by glutamatergic synaptic transmission. J Neurosci 16:7496-7504[Abstract/Free Full Text].
Otis TS, Wu YC, Trussell LO (1996b) Delayed clearance of transmitter and the role of glutamate transporters at synapses with multiple release sites. J Neurosci 16:1634-1644[Abstract/Free Full Text].
Otis TS, Kavanaugh MP, Jahr CE (1997) Postsynaptic glutamate transport at the climbing fiber-Purkinje cell synapse. Science 277:1515-1518[Abstract/Free Full Text].
Overstreet LS, Kinney GA, Liu YB, Billups D, Slater NT (1999) Glutamate transporters contribute to the time course of synaptic transmission in cerebellar granule cells. J Neurosci 19:9663-9673[Abstract/Free Full Text].
Parks TN (1981) Morphology of axosomatic endings in an avian cochlear nucleus: nucleus magnocellularis of the chicken. J Comp Neurol 203:425-440[ISI][Medline].
Patneau DK, Vyklicky Jr L, Mayer ML (1993) Hippocampal neurons exhibit cyclothiazide-sensitive rapidly desensitizing responses to kainate. J Neurosci 13:3496-3509[Abstract].
Raman IM, Trussell LO (1992) The kinetics of the response to glutamate and kainate in neurons of the avian cochlear nucleus. Neuron 9:173-186[ISI][Medline].
Raman IM, Trussell LO (1995a) Concentration-jump analysis of voltage-dependent conductances activated by glutamate and kainate in neurons of the avian cochlear nucleus. Biophys J 69:1868-1879[Abstract/Free Full Text].
Raman IM, Trussell LO (1995b) The mechanism of alpha-amino-3-hydroxy-5-methyl-4-isoxazolepropionate receptor desensitization after removal of glutamate. Biophys J 68:137-146[Abstract/Free Full Text].
Rossi DJ, Slater NT (1993) The developmental onset of NMDA receptor-channel activity during neuronal migration. Neuropharmacology 32:1239-1248[ISI][Medline].
Rothstein JD, Dykes-Hoberg M, Pardo CA, Bristol LA, Jin L, Kuncl RW, Kanai Y, Hediger MA, Wang Y, Schielke JP, Welty DF (1996) Knockout of glutamate transporters reveals a major role for astroglial transport in excitotoxicity and clearance of glutamate. Neuron 16:675-686[ISI][Medline].
Scanziani M, Salin PA, Vogt KE, Malenka RC, Nicoll RA (1997) Use-dependent increases in glutamate concentration activate presynaptic metabotropic glutamate receptors. Nature 385:630-634[Medline].
Tanaka K, Watase K, Manabe T, Yamada K, Watanabe M, Takahashi K, Iwama H, Nishikawa T, Ichihara N, Kikuchi T, Okuyama S, Kawashima N, Hori S, Takimoto M, Wada K (1997) Epilepsy and exacerbation of brain injury in mice lacking the glutamate transporter GLT-1. Science 276:1699-1702[Abstract/Free Full Text].
Tong G, Jahr CE (1994) Block of glutamate transporters potentiates postsynaptic excitation. Neuron 13:1195-1203[ISI][Medline].
Tong G, Shepherd D, Jahr CE (1995) Synaptic desensitization of NMDA receptors by calcineurin. Science 267:1510-1512[Abstract/Free Full Text].
Trussell L (1998) Control of time course of glutamatergic synaptic currents. Prog Brain Res 116:59-69[ISI][Medline].
Trussell LO, Zhang S, Raman IM (1993) Desensitization of AMPA receptors upon multiquantal neurotransmitter release. Neuron 10:1185-1196[ISI][Medline].
Ture $c$ ek R, Trussell LO (1998) Control of synaptic depression by glutamate transporters. Soc Neurosci Abstr 24:624.
von Gersdorff H, Schneggenburger R, Weis S, Neher E (1997) Presynaptic depression at a calyx synapse: the small contribution of metabotropic glutamate receptors. J Neurosci 17:8137-8146[Abstract/Free Full Text].
Wadiche JI, Amara SG, Kavanaugh MP (1995) Ion fluxes associated with excitatory amino acid transport. Neuron 15:721-728[ISI][Medline].
Warchol ME, Dallos P (1990) Neural coding in the chick cochlear nucleus. J Comp Physiol [A] 166:721-734[Medline].
Yamada KA, Tang CM (1993) Benzothiadiazides inhibit rapid glutamate receptor desensitization and enhance glutamatergic synaptic currents. J Neurosci 13:3904-3915[Abstract].
Zhang S, Trussell LO (1994a) A characterization of excitatory postsynaptic potentials in the avian nucleus magnocellularis. J Neurophysiol 72:705-718[Abstract/Free Full Text].
Zhang S, Trussell LO (1994b) Voltage clamp analysis of excitatory synaptic transmission in the avian nucleus magnocellularis. J Physiol (Lond) 480:123-136[ISI].

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