The Concentration of Synaptically Released Glutamate Outside of the Climbing Fiber-Purkinje Cell Synaptic Cleft

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The Journal of Neuroscience, July 1, 1999, 19(13):5265-5274

The Concentration of Synaptically Released Glutamate Outside of the Climbing Fiber-Purkinje Cell Synaptic Cleft
Jeffrey A. Dzubay and Craig E. Jahr
Vollum Institute, Neuroscience Graduate Program, Oregon Health Sciences University, Portland, Oregon 97201

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

AMPA receptors and glutamate transporters expressed by cerebellar Bergmann glial cells are activated by neurotransmitter releasedfrom climbing fibers (Bergles et al., 1997). Based on anatomicalevidence, this is most likely the result of glutamate diffusingout of the climbing fiber-Purkinje cell synaptic clefts (Palayand Chan-Palay, 1974). We used the change in the EC₅₀ of the Bergmannglia AMPA receptors produced by cyclothiazide (CTZ) to estimatethe concentration of glutamate reached at the glial membrane.The decrease of the EC₅₀ gives rise to a concentration-dependentpotentiation of the AMPA receptor-mediated responses (Patneauet al., 1993). By comparing the increase in amplitude of the AMPAreceptor response in the Bergmann glia (840 ± 240%; n = 8) withthe shift in the glutamate dose-response curve measured in excisedpatches (EC₅₀, 1810 µM in control vs 304 µM in CTZ), we estimatethat the extrasynaptic transmitter concentration reaches 160-190µM. This contrasts with the concentration in the synaptic cleft,thought to rapidly rise above 1 mM, but is still high enough toactivate glutamate receptors. These results indicate that thesphere of influence of synaptically released glutamate can extendbeyond the synapticcleft.

Key words: ion channels; AMPA receptors; glutamate transporters; glutamate; extrasynaptic; glia

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Vesicular release of the neurotransmitter glutamate from presynaptic terminals results in millimolar levels of glutamate inthe synaptic cleft (Clements et al., 1992; Clements, 1996; Diamondand Jahr, 1997). The close apposition of the presynaptic and postsynapticmembranes limits the dilution of neurotransmitter before reachingthe postsynaptic receptors and thereby ensures that a high concentrationof glutamate activates these receptors. The actions of the glutamatethat diffuses out of the synaptic cleft are less clear. Eventually,high affinity Na⁺-dependent transporters in the surrounding membranes take up theglutamate (Nicholls and Attwell, 1990; Kanai et al., 1993). Althoughglutamate transporters are capable of reducing extracellular glutamateto submicromolar levels, attaining such low concentrations isnot instantaneous (Zerangue and Kavanaugh, 1996). For example,release of glutamate at excitatory synapses in both cerebellumand hippocampus results in transporter activation in surroundingglia for >10 msec (Bergles and Jahr, 1997; Bergles et al., 1997;Clark and Barbour, 1997). The concentration reached outside ofparallel and climbing fiber synapses on cerebellar Purkinje cellsis sufficient to activate low-affinity AMPA receptors on the surroundingBergmann glia (Bergles et al., 1997; Clark and Barbour, 1997).

The emerging picture of the perisynaptic space is that of a region in which the concentration of transmitter can be transientlyelevated with synaptic activity. These increases in extrasynapticglutamate can result in modulation of synaptic transmission viaactivation of both metabotropic (Scanziani et al., 1997) and ionotropic(Clarke et al., 1997) receptors. The concentration of glutamatereached outside of the cleft after synaptic release is criticalin determining the extent of extrasynaptic receptor activation.Recent estimates based on the concentration dependence of thekinetics of AMPA receptor responses in outside-out patches indicatedthat the glutamate concentration peaks at <250 µM at the Bergmannglia membranes (Bergles et al., 1997). However, the responsesbelow this concentration were too small to analyze, limiting themeasurement. By using cyclothiazide (CTZ) to alter the dose-responserelationship of glutamate at Bergmann glia AMPA receptors, wereport that the glutamate concentration transiently peaks at 160-190µM in the extrasynaptic space. This concentration is sufficientfor activation of perisynaptic glutamatereceptors.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Slices and solutions. Parasagittal slices of 13- to 15-d-old rat cerebella were cut at a thickness of 300 µm using a vibratomein an ice-cold external solution containing (in mM): 119 NaCl,2.5 KCl, 2.5 CaCl₂, 1.3 MgCl₂, 1 NaH₂PO₄, 26.2 NaHCO₃, and 11glucose, bubbled with 95% O₂-5% CO₂. The slices were placed inthe same solution warmed to 34°C for 15-30 min and then storedat room temperature. During recordings, the slices were perfusedwith the above solution with the addition of 100 µM picrotoxinand 5 µM (DL)-3-(2-carboxypiperazin-4-yl)-propyl-1-phosphonicacid (CPP). Patch experiments were performed in the presence of200 µM DL-threo- $beta$ -hydroxy-aspartic acid (THA) to isolate the AMPAreceptor response, with an extracellular solution containing (inmM): 135 NaCl, 5.4 KCl, 5 HEPES, 1.8 CaCl₂, and 1.3 MgCl₂, pH7.4. THA has been shown previously to have no direct effect onAMPA receptors (Tong and Jahr, 1994). For the synaptic and dose-responseexperiments in Bergmann glia, the pipette solutions contained(in mM): 130 KNO₃, 20 HEPES, 10 EGTA, and 1 MgCl₂, pH 7.2. Forthe voltage jump experiments, the internal solution had (in mM):100 Cs-methanesulfonate, 20 TEA-Cl, 20 HEPES, 10 EGTA, 1 MgCl₂,3.1 Mg-ATP, 0.3 Na₂-GTP, and 4 phosphocreatine, pH 7.2; this solutionapproximately doubled the input resistance (28 ± 14 M $Omega$ with KNO₃to 58 ± 18 M $Omega$ with Cs-methanesulfonate). For the synaptic andpatch experiments in Purkinje cells, the pipette solution contained(in mM): 107.5 Cs-gluconate, 10 TEA-Cl, 20 HEPES, 10 EGTA, 0.3Na2-GTP, 4 Mg-ATP, and 8 NaCl, pH 7.2. The sources of the chemicalsare as follows: L-glutamate, HEPES, EGTA, Mg-ATP, phosphocreatine,THA, CaCl₂, and MgCl₂ (Sigma, St. Louis, MO); NaCl, KCl, NaH₂PO₄,NaHCO₃, and glucose (Mallinckrodt, Paris, Kentucky); Na₂-GTP (BoehringerMannheim, Mannheim, Germany); 6-nitro-7-sulfamoylbenzo[f]quinoxaline-2,3-dione(NBQX) (Tocris, Ballwin, MO); CPP, CTZ, and picrotoxin, (ResearchBiochemicals, Natick,MA).

Recording and perfusion techniques. Bergmann glia were identified by their size (~10 µm soma diameter) and location (nearthe Purkinje cell bodies) using a 40× water-immersion objectiveon an upright microscope (Axioskop; Zeiss, Oberkochen, Germany)equipped with infrared-differential interference contrast optics.Further confirmation of their identity was provided by their largenegative membrane potential ( $-$ 90 to $-$ 80 mV), low input resistance(28 ± 14 M $Omega$ with KNO₃), and lack of action potentials. Bergmannglia currents were recorded at their resting potential. Purkinjecell bodies were identified by their large size (20-30 µm), layeredarrangement, and large dendritic tree. Purkinje cell EPSCs wererecorded at approximately $-$ 10 mV to minimize the current amplitude.Patch pipettes were pulled from World Precision Instruments (Sarasota,FL) glass number PG10165-4 and had resistances of 1.5-3 M $Omega$ . Climbingfibers were stimulated with a theta glass pipette (catalog #TGC150-10;Warner Instruments, Hamden, CT) pulled to a 4-6 µm tip and filledwith external solution. The stimulating electrode was placed inthe granule cell layer between 10 and 50 µm from the Purkinjecell layer. A constant current stimulator (Weco, Millbrae, CA)was used to supply a 100 µsec pulse of 10-100 µA. The pipettewas repositioned, and stimulus intensity was adjusted until thecurrent required to elicit an all or none response was minimized.This was done to eliminate any significant parallel fiber activation.We tested for parallel fiber activation by stimulating at an intensitynear threshold that produced some climbing fiber failures andonly proceeded when the failures were complete; that is, whenno residual response was evident. Synaptic currents were filteredat 1 kHz and sampled at 10 kHz, and outside-out patch currentswere filtered at 2-5 kHz and sampled at 50 kHz. A theta glassflow-pipe mounted on a piezoelectric bimorph (Vernitron, Bedford,OH) was used for agonist applications to outside-out patches asdescribed previously (Lester and Jahr, 1992; Tong and Jahr, 1994).The ability to change the solution flowing through both sidesof the flow-pipe was added via miniature manifolds (Warner Instruments).The solutions were allowed to flow for at least 2 min betweenconditions to allow complete exchange through the manifold andtubing. Two to three concentrations with and without CTZ presentwere tested in each patch, and the amplitudes were normalizedto the response to 3 mM glutamate without CTZ. Data were acquired,and some analysis was done using AXOBASIC software (Axon Instruments,Foster City, CA), and further analysis was preformed using Origin5.0 (Microcal Software, Northampton, MA), Igor Pro (Wavemetrics,Lake Oswego, OR), and InStat (Graph Pad Software, San Diego, CA).Most experiments were performed at room temperature (22-24°C).In some experiments, the bath temperature was elevated with anin-line heating device (Warner Instruments). Values are givenas mean ± SD, and p values are for paired Student's t tests unlessnotedotherwise.

Voltage jump protocol. A novel method to estimate the time course of synaptic conductances introduced by Pearce (1993) hasbeen formalized by Häusser and Roth (1997), and the experimentsillustrated in Figure 6 were based on that method. Each trialconsisted of a single climbing fiber stimulation combined witha voltage step from $-$ 50 to $-$ 80 mV. There were 32 trials in a singlerun through the experiment, and the voltage was stepped at a differenttime in each trial; 1 msec increments were used at times nearthe climbing fiber stimulus, and 4 msec increments were used atearlier and later times. The process was repeated several times(5-14) for averaging purposes, and 200 µM CTZ was used to increasethe size of the currents. Interleaved voltage jump trials withoutsynaptic stimulation were subtracted, and the charge transferwas calculated by integration. The recovered charge was plottedversus time relative to the stimulation. The resulting curve wasfitted with the following equation, where s is the time of thejump relative to the stimulus, $tau$ _epscrise and $tau$ _epscdecay are thetime constants of the conductance approximated by the sum of twoexponentials, $tau$ _v is the time constant of the voltage change atthe conductance, A is a constant, and Q is the recoveredcharge.

For s $<=$ 0

For s > 0

The fits were performed using custom Igor macros written by Dr. Michael Häusser (Department of Physiology, University CollegeLondon, London, UK). Two controls were performed to confirm thelinearity of the membrane between $-$ 50 and $-$ 80 mV. Holding at $-$ 70mV and stepping ±5, 10, 15, and 20 mV resulted in currents thatoverlapped exactly when scaled by the command voltage (data notshown). In addition, Bergmann glia AMPA receptor responses recordedat 50 mV had the same time course as those recorded at $-$ 80 mV(see Fig. 6C).

NEURON simulation. Using the Windows version of the program NEURON (Hines, 1993), a template for a Bergmann glial cell wasconstructed with the following parameters: soma, 10 µm long, 10µm diameter, 10 segments; 12 processes, 300 µm long, 0.5 µm diameter,100 segments; and end feet, 5 µm long, 5 µm diameter, 10 segments(Palay and Chan-Palay, 1974; de Blas, 1984; Bergles et al., 1997).Two identical neighboring cells were connected to the recordedcell via cylinders 1 µm long and 1 µm in diameter. The electricalparameters were R_a = 150 $Omega$ · cm, C_m = 1 µF/cm², and g_m = 100 µS/cm² in the soma and processes, and g_m = 500 µS/cm² in the end feet for simulations of recordings using the Cs-methanesulfonate-basedinternal solution. For the KNO₃-based internal solution, the passivemembrane conductances were made four times higher. The reversalpotential for the passive conductances was set at $-$ 90mV.

The model parameters above were determined by an iterative process. In addition to the general morphology of the Bergmannglial cell (Palay and Chan-Palay, 1974; de Blas, 1984; Bergleset al., 1997), the passive response of the Bergmann glia to asquare 1 nA current injection was reproduced along with the amountof filtering estimated by the Häusser voltage jump analysis.The simulated passive response was constrained to an input resistanceof 28 M $Omega$ and a single exponential rise of 1.4 msec using the KNO₃internal solution. With the Cs-methanesulfonate solution, therise was 5.8 msec, and the input resistance was 59 M $Omega$ . The simulationwas further constrained to filter a synaptic conductance thatdecays with a tau of 5.9 msec such that the EPSC recorded at thesoma decays with a tau of 8.4 msec, using the Cs-methanesulfonateinternal solution. The synaptic conductance was simulated witha point process consisting of a sum of one rising and one decayingexponential placed on each process. The location of the synapsewas one of the parameters altered in the development of the model,and in the final model each synapse was located 210 µm from thesoma.

This model was used to estimate the error in the peak amplitude of the Bergmann glia AMPA receptor response to climbing fiberstimulation in the presence and absence of CTZ. To reproduce theexperimental data, the synaptic conductance parameters were setas follows: in CTZ, $tau$ _rise = 1.22 msec, $tau$ _decay = 8.34 msec, andg_max = 570 pS; and in control, $tau$ _rise = 0.4 and 0.7 msec, $tau$ _decay= 3.85 msec, and g_max = 67 and 64 pS. A range of values was usedfor the rise time in control because it was not uniquely definedby the system; values down to 100 µsec were slowed by cable filteringto near the 0.83 ± 0.27 msec 20-80% rise time measured at thesoma. In patches from Bergmann glia somata, the 20-80% rise timeof a response to 250 µM glutamate was 0.6 msec (Bergles et al.,1997). Thus, a range at approximately this value was used forthe synaptic conductance to account for differences in concentrationand speed of agonistapplication.

AMPA receptor kinetic model. To simulate the activation of the AMPA receptor by glutamate, a kinetic model of the AMPA receptor(see Fig. 8A) was developed using Simulation Control Program (SimulationResources, Berrien Springs, MI). Details of the model are givenin Results and in the legend of Figure 8.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

CTZ increases the Bergmann glia AMPA receptor response

CTZ increases the apparent affinity of AMPA receptors (Patneau et al., 1993; Yamada and Tang, 1993; Partin et al., 1994, 1996).We used this property of CTZ to measure the concentration of glutamatereaching the AMPA receptors in the Bergmann glial cellmembrane.

As reported previously (Bergles et al., 1997), climbing fiber stimulation in cerebellar slices activates currents in Bergmannglia mediated by both AMPA receptors and glutamate transporters.After establishing a stable baseline of the combined AMPA receptor-transportercurrent for 5 min (stimulating every 15-20 sec), a saturatingconcentration of CTZ (200 µM) was applied while continuing tostimulate. Over a period of minutes, the amplitude of the responseincreased dramatically (Fig. 1A,B). After the response stabilized,the AMPA receptor antagonist NBQX (10 µM) was applied to isolatethe transporter current (Fig. 1A,B) (Bergles et al., 1997; Clarkand Barbour, 1997). Separation of the AMPA receptor-mediated responsein the presence and absence of CTZ was achieved by subtractingthe transporter current from the combined responses (Fig. 1C).For this subtraction to be valid, the transporter current mustbe unaffected by CTZ, as will be shown below.

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Figure 1. The effects of CTZ and temperature on the response of the Bergmann glial cell to climbing fiber activation. A, A plot of the peak amplitude of the Bergmann response to climbing fiber stimulation every 20 sec. After 5 min of stable baseline, 200 µM CTZ was applied in the perfusate, followed 10 min later by 10 µM NBQX. The resting-holding potential of the cell was $-$ 88 mV. B, Averages of five sweeps under control conditions, in CTZ, and in NBQX. C, Comparison of the time course of the different components of the response isolated by subtraction of the synaptically activated transporter current (STC), the current remaining in NBQX. Averages of five sweeps were scaled to their peaks. D, The AMPA receptor-mediated response in CTZ at 35°C, at 25°C, and again at 35°C. E, The AMPA receptor-mediated response (STC subtracted) at 35°C under control (CONT) conditions and with 200 µM CTZ present (CTZ). The responses in D and E are from a different cell than in A-C and are averages of five responses. This resting-holding potential of the cell was $-$ 82 mV.

CTZ increased the peak amplitude of the AMPA receptor component 840 ± 240% (p < 0.0001; n = 8) and slowed the time course.The 20-80% rise time of the response in CTZ was 1.6 ± 0.5 mseccompared with 0.8 ± 0.3 msec for the control response, and thehalf-decay time was 9.4 ± 2.8 msec in CTZ versus 4.3 ± 2.9 msecin control (n = 8). This slowing is caused by, at least in part,the relief of desensitization that, under control conditions,is likely to truncate the rising phase and speed the decay ofthe response. An increased affinity would also prolong the response,as receptors may remain occupied longer and be sensitive to lowerconcentrations of glutamate diffusing to more remotereceptors.

There is evidence that the effects of extrasynaptic glutamate are reduced at physiological temperatures (Asztely et al., 1997;Kullmann and Asztely, 1998). The strong temperature dependenceof transport (Wadiche et al., 1995) and the expression of glutamatetransporters in the postsynaptic Purkinje cells (Rothstein etal., 1994) may decrease the glutamate diffusing to the Bergmannglia membranes at physiological temperatures. However, consistentwith the hippocampal astrocyte recordings of Bergles and Jahr(1998), the glial transporter and AMPA receptor-mediated currentswere present in the Bergmann astrocytes at elevated temperatures.Raising the bath temperature from 25 to 35°C slightly increasedthe amplitude and speeded the kinetics of the Bergmann glia responses(Fig. 1D). At 35°C, the 20-80% rise time and half-decay time forthe control AMPA receptor-mediated responses were 0.6 ± 0.2 and3.0 ± 1.9 msec respectively, and in 200 µM, CTZ they were 0.8± 0.1 and 5.5 ± 0.3 msec (n = 3). The effect of CTZ on the amplitudeof the AMPA receptor-mediated response at 35°C was not significantlydifferent from that seen at room temperature (740 ± 150% increase;p = 0.53; unpaired t test) (Fig. 1E). The remainder of the experimentswere performed at roomtemperature.

The Bergmann glia transporter current as a monitor of climbing fiber release probability

There is evidence that, at some synapses, CTZ can increase the probability of release (Barnes-Davies and Forsythe, 1995; Diamondand Jahr, 1995), which would complicate our analysis of transmitterconcentration. Several findings indicate that CTZ alters climbingfiber release probability very little. First, the paired-pulseratio (30 msec interval) of the Bergmann glia AMPA receptor-mediatedresponse to climbing fiber activation was unaffected by CTZ (0.15± 0.08 in control vs 0.14 ± 0.06 in CTZ; p = 0.60; n = 7). Second,the transporter currents recorded at the end of experiments inwhich CTZ was present were the same proportion of the initialcontrol dual-component response as those recorded at the end ofexperiments in the absence of CTZ (40.4 ± 18.3%; n = 8; vs 44.3± 13.4%; n = 17; p = 0.55; unpaired t test). Third, the transportercurrent isolated with NBQX was not affected by the addition of200 µM CTZ (101 ± 10% of control p = 0.94; n = 3) (Fig. 2A). Theseresults suggest that the probability of release is not alteredby CTZ at this synapse. However, it is possible that the transportercurrent is insensitive to changes in release because of saturationof the transporters. To demonstrate that they are sensitive tosuch changes, the release probability was altered while monitoringthe transporter current (Fig. 2B). Transporter currents were reducedto 63 ± 12% of control (p < 0.0001; n = 8) by adding 5 µM CdCl₂and increased to 116 ± 3% of control (p < 0.003; n = 4) by raisingexternal Ca⁺² to 7.5 mM. A large increase was not expected because the probabilityof release at this synapse is already very high (Dittman and Regehr,1998; Silver et al., 1998).

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Figure 2. The Bergmann glia transporter current indicates no effect of CTZ on climbing fiber release. A, Top, Peak amplitude plot of the Bergmann glia response. The AMPA response was blocked with 10 µM NBQX, and no increase in amplitude of the remaining transport current was seen after application of 200 µM CTZ. Bottom, Averages of 10 traces, with the last trace located at the time points indicated in the amplitude plot. The membrane potential of the cell was $-$ 80 mV. B, The transporter current (isolated with 10 µM NBQX) of a different cell showing the effects of adding 5 µM Cd⁺² or 5 mM Ca⁺² to the external solution. Averages of 5-15 traces. The membrane potential of this cell was $-$ 78 mV.

Purkinje cell AMPA receptor response as a monitor of climbing fiber release probability

CTZ was also ineffective in altering the climbing fiber release probability as measured by Purkinje cell responses. The amplitudeof the Purkinje cell EPSC resulting from climbing fiber stimulationwas unchanged by application of 200 µM CTZ (100 ± 7% of control;p = 0.96; n = 5) (Fig. 3). The paired-pulse ratio of the climbingfiber-Purkinje cell EPSC was also not altered by CTZ (0.44 ± 0.16in control vs 0.38 ± 0.06 in CTZ; p = 0.46; n = 4) (Fig. 3C).Consistent with the lack of a CTZ effect on the amplitude of thePurkinje cell EPSCs, the amplitude of patch responses to a saturatingdose (3 mM) of glutamate were also unaffected by CTZ (109 ± 10%of control; p = 0.55; n = 4). These results argue that the largeincrease in amplitude of the Bergmann glia AMPA receptor responsecaused by CTZ is not the result of an increase in climbing fiberrelease probability but rather is caused by a direct effect ofCTZ on the apparent affinity of the AMPA receptors.

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Figure 3. The Purkinje cell EPSC shows no increase of climbing fiber release in CTZ. A, Peak amplitude plot of the Purkinje cell EPSC evoked by climbing fiber stimulation. After a stable baseline period, 200 µM CTZ was added to the external solution. The cell was held at $-$ 6 mV. B, Averages of five responses under control conditions and in the presence of 200 µM CTZ. C, The above averages along with the second of a pair of responses isolated by subtraction of the single responses. The paired stimuli were delivered 30 msec apart.

Estimation of transmitter concentration at the Bergmann glia membrane

To estimate the peak transmitter concentration at Bergmann glia AMPA receptors, we have compared the CTZ-induced increasein peak amplitude of the climbing fiber response with the ratioof AMPA receptor dose-response relationships in the presence andabsence of CTZ. Dose-response relationships were determined withrapid applications of glutamate to outside-out patches taken fromBergmann glia somata. CTZ caused a dose-dependent potentiationof the glutamate response, concomitant with a relief of receptordesensitization. As an example of the concentration dependence,the average response to 300 µM glutamate was increased 7.0-fold,whereas the 3 mM response increased by only 2.3-fold (Fig. 4).

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Figure 4. CTZ increased Bergmann glia patch responses to glutamate in a dose-dependent manner. Responses of an outside-out patch to 300 (A) and 3000 (B) µM glutamate (GLU) under control conditions (thin lines) and in the presence of 200 µM CTZ (thick lines). The 300 µM response was increased 9.6-fold by CTZ, whereas the 3000 µM response was only increased 2.5-fold. The responses are averages of 20-40 traces. To account for a small amount of rundown, the conditions were repeated two to three times interleaving the various conditions. The patch was held at $-$ 80 mV. The applications were 10 msec long and separated by 10 sec.

As shown in Figure 5A, there was an increase in both the apparent affinity for glutamate (control, EC₅₀ = 1810 µM; CTZ, EC₅₀= 304 µM) and the maximal response (1.5-fold) in CTZ. Measurementswere made at the peak of the responses. Using the ratio of thetwo dose-response curves, we generated a curve that indicatesthe expected fold increase in the receptor response for concentrationsranging from 3 µM to 30 mM (Fig. 5B). The climbing fiber-evokedBergmann glia response increased 8.4-fold, which corresponds to192 µM on the ratio curve. The 95% confidence interval for thefold increase is 10.4 to 6.4, indicating a range of 80-372 µMglutamate. This estimation of the concentration of glutamate atthe Bergmann glia AMPA receptors (190 µM) is consistent with ourearlier estimates (<250 µM) based on a kinetic analysis (Bergleset al., 1997).

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Figure 5. Quantification of the glutamate reaching the Bergmann glia AMPA receptors. A, Dose-response curves were constructed using data from a total of 18 patches. Two or three concentrations with or without CTZ were tested in each patch. The patch responses, including those in CTZ, were all normalized to 3 mM glutamate under control conditions. The control EC₅₀ for glutamate was 1810 µM, and in the presence of CTZ it was 304 µM. The dotted line is the fit of the control data multiplied by the increase in maximal amplitude (1.5-fold), illustrating what the data would look like with no change in affinity. B, The ratio of the CTZ fit over the control fit plotted against concentration. The average fold increase of the Bergmann glia AMPA response (8.4-fold) falls at 192 µM on the x-axis.

Voltage jump analysis of somatic recordings

In the presence of CTZ, AMPA receptor currents in patches do not desensitize (Fig. 4). If CTZ affects synaptically activatedAMPA receptors on Bergmann glia similarly, the time course ofthe AMPA-mediated conductance should reflect the period over whichclearance of glutamate from the extracellular space occurs. Thisis because the intrinsic kinetics of the receptors, as demonstratedby patch recordings (Fig. 4), are rapid relative to the synapticresponses (Bergles et al., 1997). To determine whether the currentrecorded at the soma accurately reflects the kinetics of the conductance,a voltage jump analysis introduced by Pearce (1993) and formalizedby Häusser and Roth (1997) was used in the presence of CTZ. Thismethod not only extracts information about the amount of filteringof the recorded signals but also gives an indication of the averageelectrotonic distance of the conductances from thesoma.

The method is based on the observation that a change in the driving force will affect the amount of charge transfer only ifit occurs during the active conductance. This is illustrated inFigure 6A, which shows the voltage jump procedure at three separatetime points (relative to the synaptic stimulation) applied toa Bergmann glial cell in the presence of 200 µM CTZ. In Figure6B, the time integral of the AMPA receptor response (the chargetransfer) is plotted versus the time at which the voltage wasjumped. The charge recovery curves were made up of 32 time points;each point was an average of 5-14 measurements in a single cell.The curve was fitted with an analytical function (see Materialsand Methods; Häusser and Roth, 1997) in which the exponentialtime constant for the charging of the membrane (at which the conductanceoccurs) and the decay of the synaptic conductance were allowedto vary. The smallest interval measured was 1 msec, so the timeconstant for the rise time was fixed at 1 msec (a rise time of0.5 or 1.5 msec did not affect the results of the fitting).

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Figure 6. Voltage jump analysis of the Bergmann glia response. A, Three example time points superimposed to illustrate the voltage jump protocol. Top, Currents resulting from jumping the holding voltage from $-$ 50 to $-$ 80 mV at $-$ 44, 8, and 38 msec relative to the stimulus time point. Middle, The command voltages are the same, and climbing fiber stimulation is added at t = 0. Bottom, Subtractions of the currents in the top panel from the middle panel. These are integrated to calculate the charge transferred. These experiments were performed in the presence of 200 µM CTZ to maximize the amount of charge recovered. B, The resulting charge recovery curve fit with the full analytical function (see Materials and Methods) and with a single exponential fit to the data to the right of 3 msec. The $tau$ _voltage was 3.2 msec, the $tau$ _decay was 6.0 msec, and the single exponential fit gave a $tau$ of 5.5 msec. A single exponential fit to the average response recorded at the soma had a time constant of 6.6 msec. C, Averages of five responses at $-$ 50 and $-$ 80 mV. The response at $-$ 50 mV is also scaled up to the peak of the $-$ 80 mV response to compare their time course.

The average time constant of the decay of the conductance calculated from the full analytical fit of the charge recovery curveswas 5.9 ± 1.6 msec (n = 7). This is not significantly differentfrom single exponential fits to the charge recovery curves starting4 msec after the synaptic stimulation (5.8 ± 1.4 msec; p = 0.657;n = 7). This was significantly faster than the decay of the Bergmannglia AMPA receptor response recorded with a somatic recordingelectrode (8.4 ± 1.0 msec; p = 0.004; n = 7), demonstrating thatthere is some filtering of the conductance (a 42% slowing of thedecay). The average time constant for the charging of the membraneat the active conductance was 4.4 ± 1.9 msec, indicating the averageconductance is electrotonically distant from the soma. This isconsistent with the observation that most of the climbing fibersynaptic contacts are out in the dendritic tree of the Purkinjecell (Palay and Chan-Palay, 1974) and with the filtering of thedecay timecourse.

Our estimation of the transmitter concentration reaching the Bergmann glial membranes depends on our somatic measurement ofthe amplitude ratio of the receptor responses in the presenceand absence of CTZ. Although taking a ratio eliminates concernsof a uniform error in the amplitude measurement, the slowing andlarge increase in amplitude of the AMPA receptor response in CTZmay lead to differential amounts of filtering and voltage escape.We were unable to apply the voltage jump analysis to the Bergmannresponses under control conditions because of their small sizeand variability. Therefore, we used the information on filteringgained from the voltage jump analysis in CTZ to construct a simpleNEURON simulation addressing theseconcerns.

The model was constructed based on the general morphology of Bergmann glial cells (Palay and Chan-Palay, 1974; de Blas, 1984),the passive response of the cells to a square current injection,and the extent of filtering indicated by the voltage jump analysis.The inclusion of end feet with a conductance five times higherthan the rest of the cell (Newman, 1986) was critical in reproducingthe electrical properties of the Bergmann glia. Holding the othermodel parameters constant, the synaptic conductance kinetics andmaximum value were altered so that the simulated AMPA receptorresponses monitored at the soma matched the experimental datain the presence and absence of CTZ (Fig. 7). The unfiltered currentflowing at the conductance under perfect voltage clamp can bycalculated by the NEURON simulation. The perfectly clamped synapticcurrent peaked at 207-217 pA (see Materials and Methods) in control(experimental value recorded at soma, 34 pA) (Fig. 7A) and 1850pA in CTZ (experimental value recorded at soma, 286 pA) (Fig.7B). Accounting for cable filtering and voltage escape, the foldincrease in the amplitude of the AMPA receptor response with CTZshould be adjusted from 8.4-fold (corresponding to 192 µM) to8.5- to 8.9-fold, indicating a range of 160-186 µM glutamate onthe ratio curve.

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Figure 7. Simulation of somatic recordings of the Bergmann glia AMPA receptor responses. A, Simulated recordings under control conditions. Top, Membrane voltage at the synapse. Bottom, Current measured at the soma (thick line), flowing at the synapse (dotted line), and flowing at the synapse under perfect voltage clamp (thin line). B, Simulated recordings in the presence of CTZ. Top, Membrane voltage at the synapse. Bottom, Current measured at the soma (thick line), flowing at the synapse (dotted line), and flowing at the synapse under perfect voltage clamp (thin line).

An AMPA receptor kinetic model

An untested assumption in the preceding analysis is that the dose-response relationships constructed from rapid applicationsof glutamate to outside-out patches accurately represent receptoractivation by synaptically released glutamate in situ. For instance,if the rise time of the synaptic glutamate transient is longerthan that at the patch membrane, the dose-response relationshipin control conditions may be significantly altered by rapid desensitization.To address this issue, we have modified a simple kinetic modelof the AMPA receptor (Diamond and Jahr, 1997) to fit the datafrom Bergmann glia patches and then used the model to determinea driving function representing the synaptic glutamate transientthat produces responses that fit the Bergmann glia climbing fiberresponse. The model replicates both the kinetics (Bergles et al.,1997) and amplitudes of the patch responses over a wide glutamateconcentration range (Fig. 8). To fit the CTZpatch data, the unbindingrate was slowed from 16 to 6 per millisecond, and the rates intoboth desensitized states were zeroed. The ratio of the modeleddose-response curves is in close agreement with the patch data,giving an 8.4-fold increase at 205 µM.

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Figure 8. Simulations of AMPA receptor responses to brief applications of glutamate. A, State diagram used to reproduce AMPA receptor kinetics. Rates were as follows [units are micromolar per millisecond (for k_a) or per millisecond]: k_a, 0.009; k_a, 16.0 (6.0 in cyclothiazide); k₁, 0.0025; k₂, 5.0; k₂, 0.006 (0 in cyclothiazide); $alpha$ , 1.3; $beta$ , 13.0. k₁ was set to 2.08 (0 in cyclothiazide) to satisfy microscopic reversibility. B, Simulated responses to 10 msec pulses of glutamate at 0.1, 0.3, 1.0, 3.0, 10.0, and 30.0 mM. C, Simulated responses to 10 msec pulses of glutamate at the same concentrations as in B but with k_a set to 6 msec and k₁ and k₂ set to 0 to mimic the effects of cyclothiazide. D, Simulated dose-response curves superimposed on the data from Figure 5A. E, The amplitude ratio of the CTZ simulation over the control simulation plotted against concentration (solid line). The ratio of the logistic fits to the patch data given in Figure 5 is superimposed (dotted line).

A "synaptic" glutamate transient was approximated using a ramp rising phase to a given concentration and a single exponentialfalling phase. The rise time, peak concentration, and decay timewere altered to fit the climbing fiber responses recorded in controland in the presence of CTZ. First, the rise and decay times ofthe glutamate transient were varied to fit the kinetics of theBergmann glia responses while keeping the peak concentration at190 µM. A rise time (time-to-peak) of 1.2 msec and a decay timeconstant of 10 msec fitted the climbing fiber responses in bothconditions. Both the rising phase of the synaptic responses (Fig.9) and the decay times (simulations not shown) were very sensitiveto alterations in the kinetics of the driving function. Althoughchanging the peak concentration of the glutamate driving functiondid not greatly alter the kinetics of the synaptic responses,the amplitude ratio of 8.4 was obtained with a peak concentrationof 190 µM. The amplitude ratio versus concentration relationshipof the modeled synaptic conductances was less steep than eitherthe ratio of the patch data or the simulated patch data. Nevertheless,300 µM yielded a ratio of 7.8, whereas 100 µM resulted in a ratioof 9. Thus, whereas the sensitivity was lower, the amplitude ratiowas still well defined. Clearly, this model oversimplifies thegating mechanism underlying the AMPA receptor currents. However,the modeling does suggest that the method used to estimate theaverage peak concentration of glutamate at Bergmann glia membranesis not greatly degraded by the ambiguities introduced by desensitization.

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Figure 9. Simulated Bergmann glia responses to synaptically released glutamate. A, Synaptic simulations in control (k_a, 16.0 msec) and cyclothiazide (k_a, 6.0 msec; k₁ and k₂ set to 0) with rise time of the driving function (glutamate transient) set to 0.5, 1, 2, 4, and 8 msec. Decay time constant was set at 10 msec and peak concentration at 190 µM. B, Synaptic simulations in control and cyclothiazide as in A with the peak concentration set to 100, 200, 300, and 500 µM. Decay time constant was 10 msec, and the rise time was 1.2 msec.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Our results, indicating that 160-190 µM glutamate reaches the Bergmann glia membrane after climbing fiber stimulation, dependon the modulation of the Bergmann glia AMPA receptor responseby CTZ. CTZ has been shown to greatly reduce desensitization andto increase the apparent affinity of the AMPA receptors (Patneauet al., 1993; Yamada and Tang, 1993; Partin et al., 1994, 1996).The mechanism of its action is not completely understood but isthought to occur via a destabilization of the desensitized stateor a stabilization of the closed nondesensitized state (Trussellet al., 1993, 1994; Yamada and Tang, 1993; Partin et al., 1994,1996). The important property of the action of CTZ for this studyis that it produced a concentration-dependent increase in theresponse of the receptors. This allowed the quantification ofthe glutamate concentration at the Bergmann glia membrane by comparingthe CTZ-induced increase of the synaptic response with that ofthe patch responses to a range of glutamateconcentrations.

In contrast to Bergmann glia responses, the amplitudes of Purkinje cell EPSC and patch responses were not altered by CTZ.This result is similar to that of Dittman and Regehr (1998), whofound that climbing fiber-EPSC peak amplitudes measured in Purkinjecells were slightly reduced by CTZ. The high concentrations ofglutamate in the Purkinje cell experiments (>1 mM in the cleft,and 3 mM for patches) can partially explain this result, becausean increase in affinity would have less effect near saturation.However, even at the top of the dose-response curve, there wasa fifty percent increase in the Bergmann glia patch response.This difference between Purkinje cell patch and Bergmann gliapatch responses may be caused, in part, by the faster desensitizationkinetics of the Bergmann AMPA receptors leading to more desensitizationat the peak of the response in control conditions. In addition,AMPA receptors are susceptible to channel block by CTZ, the magnitudeof which may be altered by different subunit combinations (Patneauet al., 1993; Stern-Bach et al., 1998).

The observation that CTZ increased the peak amplitude of the Bergmann glia climbing fiber response to the same degree at 35and 25°C (740 ± 150 vs 840 ± 240%; p = 0.53) suggests that a similarpeak concentration of glutamate reaches the glial AMPA receptorsat the two temperatures. Despite the strong temperature dependenceof transport (Wadiche et al., 1995), it is possible that the initialbolus of glutamate that reaches nearby Bergmann glia AMPA receptorsis relatively unaffected by the faster transport at physiologicaltemperatures. The turnover time for glutamate transporters atelevated temperatures may be as fast as 12 msec (Bergles and Jahr,1998), much slower than the time to peak of the Bergmann gliaAMPA receptor response at 35°C (~2 msec). Therefore, althoughbinding of glutamate by transporters expressed by both Purkinjecells and Bergmann glia undoubtedly lowers the concentration ofglutamate reaching Bergmann glial AMPA receptors, it is unlikelythat the binding capacity during the response rise time will besignificantly altered by the increased transporter cycling rateat higher temperatures. It would appear, then, that the initialwave of glutamate reaching the Bergmann glia AMPA receptors istoo fast to be altered significantly by elevating temperatureto near physiologicalvalues.

The variability in the degree of potentiation by CTZ of the Bergmann glia AMPA response (840 ± 240%; n = 8) may indicate somebiological variability in the concentration of glutamate seenby the Bergmann glia. The spatial arrangement of the receptorsaround the cleft, the degree of synapse envelopment, the maturityof the cell being recorded from, and other factors may vary fromcell to cell and give rise to different average concentrationsseen by a given Bergmann glia. Interestingly, in searching forthe primary all-or-none climbing fiber response in the Bergmannglia, there was occasionally a secondary all-or-none input. BecauseBergmann glia processes are not planar like Purkinje cell dendrites(de Blas, 1984), each Bergmann glial cell may interact with morethan one climbingfiber.

Previously CTZ has been linked to an increase in the probability of release at some synapses (Barnes-Davies and Forsythe,1995; Diamond and Jahr, 1995; but see Mennerick and Zorumski,1995; Isaacson and Walmsley, 1996). In contrast, we show herethat the climbing fiber release probability was not significantlyaltered by CTZ. This difference might be explained by the highrelease probability of the climbing fiber terminal (Dittman andRegehr, 1998; Silver et al., 1998). The strong paired-pulse depressionseen at this synapse, along with little increase in synaptic strengthwith elevated external calcium, indicate that release probabilityis near maximal (Dittman and Regehr, 1998; Silver et al., 1998).Consistent with our results, Dittman and Regehr (1998) recentlyshowed little effect of CTZ on the paired-pulse ratio of climbingfiber-evoked EPSCs recorded in Purkinje cells. The presynapticaction of CTZ on terminals with a low probability of release wasconfirmed in one of our Purkinje cell recordings in which we monitoredthe effects of CTZ on a parallel fiber input. These inputs havea low release probability, as demonstrated by their paired-pulsefacilitation (Atluri and Regehr, 1996). In contrast to the climbingfiber-evoked response in Purkinje cells, the parallel fiber EPSCsincreased approximately sixfold, and the paired-pulse ratio switchedfrom facilitation to depression in CTZ. The variability in thepresynaptic effects of CTZ with different pathways may also reflectdifferential expression of CTZ receptivity in theterminals.

In the presence of CTZ, we estimate that the Bergmann glia AMPA receptor conductance decays with a time constant of 6 msec.This should reflect the decay of the glutamate concentration atthese receptors because there is no desensitization in CTZ andthe intrinsic kinetics of the receptors are rapid. This is fasterbut not inconsistent with our previous report of a 17 msec decayof extrasynaptic glutamate based on the Bergmann glia transportercurrent (Bergles et al., 1997). Our current estimate is in partfaster because it accounts for the cable filtering and voltageescape inherent in somatic voltage-clamp recordings. In addition,the lower apparent affinity of the AMPA receptors would make themless sensitive than the transporters to reduced concentrationsof glutamate diffusing to more distant areas. It is also possiblethat the AMPA receptors may be more localized to the membranessurrounding the synaptic clefts (Baude et al., 1994), whereasthe transporters may cover more surface area of the Bergmannglia.

The main result of this paper is that glutamate escapes from the climbing fiber-Purkinje cell cleft and can reach perisynapticmembranes at concentrations of 160-190 µM. This concentrationis sufficient to activate all classes of glutamate receptors,including metabotropic, NMDA, and non-NMDA receptors. There isa growing body of evidence indicating that synaptic transmissioncan be modulated by glutamate that escapes from the synaptic cleft(Clarke et al., 1997; Forsythe and Barnes-Davies, 1997; Scanzianiet al., 1997). There is also evidence that the high-affinity NMDAreceptors at one synapse may sense glutamate released from neighboringsynapses (Kullmann and Asztely, 1998; Rusakov and Kullmann, 1998).The results presented here demonstrate a basic requirement ofboth of these phenomena, that glutamate can escape the synapticcleft and reach the surrounding membranes at a concentration sufficientto activate glutamate receptors. This alters the standard viewof the actions of glutamate in the CNS, expanding the sphere ofinfluence of synaptically released glutamate beyond the postsynapticmembrane.

  FOOTNOTES

Received Nov. 24, 1998; revised March 29, 1999; accepted April 19, 1999.

This work was supported by National Institutes of Health Grants MH11978 (J.A.D.) and NS21419 (C.E.J.). We thank Drs. DwightBergles, Jeff Diamond, and Jacques Wadiche for a critical readingof this manuscript and their helpful comments. A special thanksto Dr. Tom Otis for initial experimental ideas and to Dr. MichaelHäusser for help with the voltage jump analysis and NEURONsimulation.
Correspondence should be addressed to Craig E. Jahr, Vollum Institute L474, Oregon Health Sciences University, 3181 S.W. SamJackson Park Road, Portland, OR 97201-3098.

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