Reduced Excitatory Drive onto Interneurons in the Dentate Gyrus after Status Epilepticus

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The Journal of Neuroscience, March 15, 2001, 21(6):2048-2057

Reduced Excitatory Drive onto Interneurons in the Dentate Gyrus after Status Epilepticus
James Doherty and Raymond Dingledine
Department of Pharmacology, Emory University Medical School, Atlanta, Georgia 30322

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Impaired GABAergic inhibition may contribute to the development of hyperexcitability in epilepsy. We used the pilocarpinemodel of epilepsy to demonstrate that regulation of excitatorysynaptic drive onto GABAergic interneurons is impaired duringepileptogenesis. Synaptic input from granule cells (GCs), perforantpath, and CA3 inputs onto hilar border interneurons of the dentategyrus were examined in rat hippocampal slices during the latentperiod (1-8 d) after induction of status epilepticus (SE). Short-termdepression (STD) of GC inputs to interneurons induced by brief(500-800 msec), repetitive (5-20 Hz) stimulation, as well as paired-pulsedepression at both GC and CA3 inputs to interneurons, were significantly(p < 0.05) enhanced in SE-experienced rats. In contrast, we foundno significant differences between SE-experienced and age-matchedcontrol rats in the properties of minimal EPSCs evoked at lowfrequency (0.3 Hz). Consistent with reduced GABAergic inhibitiononto granule cells, paired-pulse depression of perforant path-evokedgranule cell population spikes was lost in SE-experienced rats.Enhanced STD was partially mediated by group II metabotropic glutamatereceptors, because the selective antagonist, 2S-2-amino-2-(1S,2S-2-carboxycyclopropyl-1-yl)-3-(xanth-9-yl)propanoicacid, attenuated STD in SE-experienced rats but had no effecton STD of GC inputs in the normal adult rat. The group II mGluRagonist, (2S',1R',2R',3R')-2-(2,3-dicarboxylcyclopropyl) glycine(1 µM), produced a greater depression of GC input to hilar borderinterneurons in SE-experienced rats than in controls. These resultsindicate that, in the SE-experienced rat, excitatory drive tohilar border inhibitory interneurons is weakened through a use-dependentmechanism involving group II metabotropic glutamatereceptors.

Key words: hippocampus; seizure; granule cell; short-term depression; metabotropic glutamate receptor; status epilepticus

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

GABAergic neurotransmission regulates cortical functions such as synaptic plasticity (Wigström and Gustafsson, 1983; Groverand Yan, 1999; Steele and Mauk, 1999), processing of sensory information(Dykes, 1997; Zheng and Knudsen, 1999), and learning and memory(Keverne and Brennan, 1996; Paulsen and Moser, 1998). A linkagebetween GABAergic neurotransmission and epilepsy has long beenrecognized (Olsen and Avoli, 1997). Inhibition of GABA_A receptorstriggers acute seizures (Prince, 1978), and drugs that potentiateGABAergic inhibition are typically anticonvulsant (George andKulkarni, 1996; Olsen and Avoli, 1997; Bleck, 1999). However,it is not clear whether the anticonvulsant effect of GABA receptorpotentiation reflects a general dampening of cortical excitabilityor a selective compensation for a specific deficit in GABAergicinhibition.

Disruptions in the strength of GABAergic inhibition occur in the epileptic hippocampus. However, both a loss or reduction(Sloviter, 1991; Bekenstein and Lothman, 1993; Merlin and Wong,1993; Whittington and Jefferys, 1994; Rice et al., 1996; Hirschet al., 1999; Williamson et al., 1999) or an increase (King etal., 1985; Haas et al., 1996; Swanson et al., 1998; Wilson etal., 1998) in synaptic inhibition have been reported. Depressedsynaptic inhibition occurs in experimental epilepsy models, includingthe pilocarpine (Rice et al., 1996; Bausch and Chavkin, 1997),tetanus toxin (Empson and Jeffreys, 1993; Whittington and Jeffreys,1994), and self-sustaining limbic status epilepticus (SE) (Manganand Lothman, 1996) models. GABA_A receptor antagonists also unmaskepileptiform activity in chronic experimental models of epilepsy(Patrylo and Dudek, 1998; Smith et al., 1998).

Numerous alterations occur in hippocampal circuitry after SE, producing remodeled networks with properties significantly differentfrom normal brain (Coulter, 1999; Sloviter, 1999). Many pathologicalalterations produced during epileptogenesis might disinhibit hippocampalcircuitry, including changes in GABA_A receptor subunit compositionor properties (Bühl et al., 1996; Kapur and Macdonald, 1997;Brooks-Kayal et al., 1998; Macdonald and Kapur, 1999), death ofGABAergic interneurons (Obenaus et al., 1993; Houser and Escaplez,1996), changes in receptor-mediated regulation of GABAergic neurotransmission(Haas et al., 1996; Mangan and Lothman, 1996; Bausch and Chavkin,1997), or loss of excitatory synaptic input onto GABAergic interneurons(Sloviter, 1991; Bekenstein and Lothman, 1993).

Excitatory synaptic inputs onto hilar border interneurons undergo short-term plasticity that is partially mediated by metabotropicglutamate receptors (mGluRs) (J. Doherty, D. Mott, S. Alagarsamy,P. J. Conn, and R. Dingledine, unpublished observations). HippocampalGABAergic interneurons undergo both short-term (Galarreta andHestrin, 1998) and long-term (McMahon and Kauer, 1997; Laezzaet al., 1999) forms of synaptic plasticity. Small deficits inthe regulation or strength of excitatory synaptic drive onto GABAergicinterneurons during epileptogenesis can have significant consequencesfor local excitability, because individual interneurons typicallysynapse onto large numbers of principal neurons (Freund and Buzáski,1996). Small reductions in the strength of inhibitory neurotransmissioncan trigger acute seizure-like activity (Miles and Wong, 1987;Chagnac-Amitai and Connors, 1989).

We demonstrated that short-term depression (STD) of excitatory afferents onto dentate hilar border interneurons is enhancedin SE-experienced rats. Diminished drive onto interneurons ispartially mediated by enhanced mGluR-mediated depression of transmitterrelease.

Some of these data have appeared previously in preliminary form (Doherty and Dingledine, 1997b, 1998).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Pilocarpine-induced status epilepticus. The pilocarpine-induced model of chronic epilepsy in rats (Turski et al., 1983, 1989;Cavalheiro et al., 1991; Mello et al., 1993) was chosen becauseit replicates several features of human temporal lobe epilepsy.Male Sprague Dawley rats (36-60 d old; 102-210 gm) were injectedwith methylscopolamine and terbutaline (2 mg/kg, i.p.). Thirtyminutes later, experimental rats received a single injection ofpilocarpine HCl, whereas sham-treated rats received saline injections.Although a range of pilocarpine doses (315-350 mg/kg, i.p.) wastested with the aim to produce the highest proportion of ratsexperiencing status epilepticus with the lowest mortality rate,a concentration of 335 mg/kg was used for >90% of the experiments.Seizure duration and frequency progressively increased until astate of SE characterized by rearing and falling was achieved.SE was allowed to proceed for 75-90 min and then was terminatedwith sodium pentobarbital (25-50 mg/kg, i.p.). Rats were allowedto recover for 1-8 d before hippocampal slices were prepared forelectrophysiological recordings. A single intraperitoneal injectionof pilocarpine evoked seizures in 94% (92 of 98) of treated rats.Typically, intermittent seizures characterized by head bobbingand forelimb clonus appeared 5-15 min after pilocarpine injection.Seizure severity and frequency increased progressively over 5-15min, culminating in a state of SE in 84% (82 of 98) of treatedrats. Slices taken from SE-experienced rats, defined as thoseundergoing >75 min of SE (n = 48), were examined for changes insynaptic inhibition in the dentategyrus.

Interneuron recordings. All recordings from SE-experienced rats were made at 1-8 d after SE, before the appearance of extensivesupragranular mossy fiber sprouting (Mello et al., 1993). Theprocedures for recording from interneurons in hippocampal sliceswere essentially as previously described (Doherty and Dingledine,1997). Thin (225 µm) hippocampal slices were prepared from bothpilocarpine- and sham-treated rats. Rats were first anesthetizedwith isoflurane, then brains were rapidly removed into ice-coldartificial CSF (ACSF) containing (in mM): 120 NaCl, 3.5 KCl, 0.75CaCl₂ · 2 H₂O, 2.25 MgSO₄ · 7 H₂O, 24 NaHCO₃, 1.25 NaH₂PO₄, 1Na pyruvate, 10 glucose, pH 7.4 (295-305 mOsm). Slices from thedorsal half of the hippocampus were cut with a vibratome, incubatedat room temperature (24-25°C) for 5-60 min, and finally transferredto a submerged recording chamber. Once in the recording chamber,slices were perfused with a room temperature ACSF containing (inmM): 130 NaCl, 3.5 KCl, 1.5 CaCl₂ · 2 H₂O, 1.5 MgSO₄ · 7 H₂O,24 NaHCO₃, 1.25 NaH₂PO₄, 10 glucose, pH 7.4 (295-305 mOsm), ata rate of 2-3 ml/min. Individual interneurons located at the borderof the hilus and the granule cell (GC) layer were visually selectedfor whole-cell patch-clamp recording using Hoffman modulationcontrast optics (600×) and previously established criteria (Dohertyand Dingledine, 1997, 1998). Interneurons in this study includebasket cells, which synapse on the somata of granule cells, aswell as interneurons that project into the molecular layer (Freundand Buzáski, 1996). No differences in the electrophysiologicalproperties of excitatory synaptic inputs were detected betweensubsets of hilar border interneurons with different axonal projections;therefore results from all interneurons were consideredtogether.

Field potential and whole-cell patch recordings were performed using an Axopatch 1D electrometer (Axon Instruments, FosterCity, CA). Field potential responses were acquired with an ACSF-containingpatch electrode placed in the granule cell layer. Sharpened tungstenmicroelectrodes placed in the outer molecular layer to a depthof 5-50 µm were used to evoke field potentials. Stimulus intensitywas adjusted to produce a response at 40% of maximal populationspike amplitude. All stimuli were triggered by Clampex protocols(Axon Instruments) and delivered through photoelectric stimulusisolation units (World Precision Instruments, Sarasota, FL). Sealformation and whole-cell configuration of patch-clamp recordingswere achieved in current-clamp mode; passive membrane propertieswere measured before switching to voltage-clamp mode. Whole-cellresponses were filtered at 3 kHz, digitized at 10-30 kHz, andcollected directly to a computer using pClamp 7.0. Patch electrodes(5-7 M $Omega$ ) were pulled from borosilicate glass using a two-stagevertical puller and filled with solution containing (in mM) 130CsOH, 140 methanesulfonic acid, 10 HEPES, 2 MgCl₂, and biocytin(0.5-1%). Intracellular solution was buffered to pH 7.3 with CsOHand adjusted to 275-280 mOsm with H₂O. Voltage-clamp experimentswere performed at a holding potential of $-$ 70 mV in hilar borderinterneurons and 0 mV in granule cells. Series resistance, inputresistance, and holding current were periodically monitored throughoutexperiments; only neurons with stable electrophysiological parameterswere included. Glass micropipettes were used to deliver stimuli(0.3 Hz, 10-80 µA; 300-400 µsec) in the stratum granulosum (granulecells) 10-50 µm from the recording site or in the stratum pyramidaleof the CA3b and CA3c regions. For minimal stimulation experiments,stimulus intensities were adjusted to the lowest level necessaryto evoke visually identifiable EPSCs. Multiple sites were testedin each region to isolate a single reliable EPSC, as well as toprevent antidromic activation of interneurons in response to stimulationin the GC. Minimally evoked EPSCs were visually differentiatedfrom synaptic failures as previously described (Doherty and Dingledine,1997). Briefly, evoked events were required to meet several criteriato be accepted for analysis. These included a short mean latency(2-7 msec) from the stimulus artifact, characteristic fast risingand exponential decay phases, and peak amplitudes that exceeded2 SD of the mean amplitude of the baseline electrical noise. Eventschosen for analysis were confined to a 2 msec window centeredaround the mean latency to minimize the possibility of countingspontaneous EPSCs as evoked events. Stimulus trials that did notproduce events meeting these criteria were designated as synapticfailures and were not included in the calculation of EPSC parameters.The failure rate in synaptic transmission for each excitatoryinput was defined as the percentage of failures over the totalnumber of stimulus trials. Individual inputs were not consideredfor further analysis if the mean failure rate was >90% duringcontrol stimulation. Transmission rate was defined as 100% $-$ failurerate.

Drugs. Pilocarpine HCl (315-350 mg/kg), methylscopolamine (10 mg/kg), terbutaline (10 mg/kg), and sodium pentobarbital (25mg/kg) (Sigma, St. Louis, MO) were dissolved in 0.9% sterile saline.Bicuculline methobromide (10 µM), (+)- $alpha$ -methyl-4-carboxyphenylglycine(500 µM), (2S',1R',2R',3R')-2-(2,3-dicarboxylcyclopropyl) glycine(DCG-IV; 1 µM) (Tocris Cookson, Ballwin, MO), and 2S-2-amino-2-(1S,2S-2-carboxycyclopropyl-1-yl)-3-(xanth-9-yl)propanoicacid (LY341495; 500 nM) were dissolved in ACSF and delivered bybathperfusion.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Depressed synaptic inhibition in the dentate gyrus

Field potential recordings of perforant path input to dentate granule cells were used to assess the strength of feedback andfeedforward synaptic inhibition in the dentate gyrus from 1 to28 d after pilocarpine-induced SE. Population spikes were recordedin the granule cell layer in response to paired stimuli deliveredto the perforant path in hippocampal slices from both controland pilocarpine-treated rats (Fig. 1A). In control rats, paired-pulseinhibition, determined by measuring the amplitude of the secondpopulation spike amplitude as a percentage of the first, was observedover an interstimulus interval ranging from 10 to 30 msec. Paired-pulseinhibition was replaced by facilitation in slices taken from SE-experiencedrats when compared with control rats (Fig. 1A,B), indicating asignificant (p < 0.001, one-way ANOVA) loss of synaptic inhibitionduring paired stimulation. Paired-pulse facilitation of perforantpath-evoked population spikes (224 ± 65%; n = 3) was observedwithin 1-2 d after induction of SE. However, the magnitude ofthe facilitation continued to increase for 4-5 d, reaching a peakat 305 ± 22% (Fig. 1C; n = 6). The establishment of SE was requiredto produce the loss of paired-pulse inhibition in granule cells.In four pilocarpine-treated rats that experienced intermittentseizures, but not SE, paired-pulse inhibition remained normal,reducing the second population spike to 43 ± 13% of the firstpopulation spike amplitude at an interstimulus interval of 10msec. This level of inhibition was not significantly different(p = 0.6, one-way ANOVA with post hoc Bonferroni test) from controlslices (24 ± 9%; n = 9). Multiple population spikes were not observedin the dentate gyrus after either single or paired stimulationof the perforant path in slices taken from normal or SE-experiencedrats.

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Figure 1. Synaptic inhibition in the dentate gyrus is impaired at 2-6 d after pilocarpine-induced status epilepticus. A, Field potential recordings evoked in the granule cell layer of the dentate gyrus after paired stimulation of the perforant path in untreated (top) or SE-experienced (bottom) rats. Population spike amplitudes were measured as the difference between the peak amplitude and the midpoint of the field EPSP (dotted lines). Stimulus artifacts (arrows) have been removed for clarity. B, Paired-pulse inhibition was seen at short (10-30 msec) interstimulus intervals (ISI) in untreated rats ( $open circle$ ; n = 9 rats), but was replaced by facilitation in SE-experienced rats ( $triangle$ ; n = 7 rats). C, Paired-pulse facilitation (interpulse interval, 20 msec) peaks at 4-5 d after SE and persists for at least 30 d.

These data indicate an increase in granule cell excitability in SE-experienced rats; however, they alone do not indicate whetherthis results from a loss of inhibition or an increase in synapticfacilitation. Reduction of paired-pulse inhibition was not accompaniedby noticeable deficits in monosynaptic IPSCs evoked at low frequencyby stimulation within the granule cell layer in the presence ofCNQX (3 µM) and D-APV (50 µM). The reliability of synaptic transmissionat monosynaptic GABAergic synapses onto granule cells was highin both untreated (evoked IPSCs in 86 ± 4% of stimulus trialswith minimal stimulation; n = 5 neurons) and SE-experienced (94± 6%; n = 3) rats. IPSC amplitudes in granule cells of SE-experiencedrats produced by a minimally effective stimulus delivered to thegranule cell layer (39 ± 10 pA; n = 3) were not significantlydifferent from IPSCs in granule cells from control rats (27 ±4 pA; n = 5; data notshown).

Excitatory synaptic input to hilar border interneurons in SE-experienced rats

To identify the mechanisms responsible for reduced synaptic inhibition in the dentate gyrus of SE-experienced rats, we studiedthe short-term regulation of excitatory synaptic inputs onto theheterogeneous group of interneurons located at the granule cell-hilarborder in slices from SE-experienced rats. Whole-cell patch recordingswere made from 10 granule cells and 57 visually identified hilarborder interneurons in slices taken from SE-experienced rats.Synaptic responses from interneurons in sham-treated rats (n =12) did not differ from untreated adult rats (n = 34); thus theserecordings were grouped together in the control group. Spontaneousaction potentials were observed at the resting membrane potentialin a slightly larger proportion of hilar border interneurons fromSE-experienced rats (71%) than from control rats (60%). However,there were no significant differences in resting membrane potential,action potential threshold, or input resistance in interneuronsfrom SE-experienced rats when compared with interneurons fromcontrol rats (Table 1). This suggests that changes in interneuronmembrane excitability were not sufficient to explain the observedloss of synaptic inhibition. Spontaneous EPSCs were observed inrecordings from interneurons from both control and SE-experiencedrats. Spontaneous EPSC rise and decay times were slower in interneuronsfrom SE-experienced rats, but there were no changes in amplitudeor frequency (Table 1).


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Table 1. Electrophysiological properties of hilar border dentate interneurons in pilocarpine-treated rats

To determine whether regulation of excitatory synaptic drive to hilar border interneurons is altered in SE-experienced rats,we isolated minimally evoked EPSCs from three different synapticinputs as previously described (Doherty and Dingledine, 1997,1998) (Doherty, Mott, Alagarsamy, Conn, and Dingledine, unpublishedobservations). Stimulation of dentate granule cells (Fig. 2A),CA3 pyramidal cells (Fig. 2B), or perforant path axons evokedminimal inputs to hilar border interneurons from SE-experiencedrats. There were no significant differences in either the reliabilityof synaptic transmission or the kinetics of evoked minimal EPSCsat excitatory inputs to hilar border interneurons in slices fromnormal adult and SE-experienced rats. These data, summarized inTable 2 and the scattergrams in Figure 2, A and B, indicate thatlow-frequency synaptic excitation of hilar border interneuronsappears normal in SE-experienced rats.

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Figure 2. Properties of unitary EPSCs evoked by minimal stimulation onto hilar border interneurons. A, Dentate granule cell inputs to an interneuron from an SE-experienced adult rat. B, Input from stimulation of the CA3 pyramidal cell layer. In each case, the amplitude histogram is unimodally centered on $-$ 10 pA. The scattergrams to the right show the peak of the amplitude histogram for minimally evoked synaptic inputs to interneurons in control and SE-experienced rats. GCL, Granule cell layer; ampl., amplitude; PILO, pilocarpine.


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Table 2. Properties of evoked EPSCs onto hilar border interneurons (measured at $-$ 70 mV)

Enhanced short-term depression in SE-experienced rats

Excitatory inputs to hilar border interneurons in the juvenile and adult rat express synapse-specific forms of short-termplasticity (Doherty, Mott, Alagarsamy, Conn, and Dingledine, unpublishedobservations). Stimulation of granule cell synapses onto interneuronswith brief high-frequency (20 Hz) stimulus trains produces STDin both control (Fig. 3A, top) and SE-experienced (Fig. 3, bottom)rats. STD of GC-evoked inputs to hilar border interneurons wassignificantly potentiated in SE-experienced rats (Fig. 3B). InSE-experienced rats, STD of GC-evoked EPSC amplitudes reacheda plateau at 24 ± 2% of the first EPSC amplitude during 20 Hztrains (n = 16), a significantly (p < 0.001, one-way ANOVA) greaterdepression than was observed during 20 Hz trains in interneuronsfrom control adult rats. The onset of STD was also more rapidat GC inputs to hilar border interneurons in SE-experienced rats.The time constant of the fitted exponential decay function ininterneurons from SE-experienced rats (81 ± 6 msec; n = 16) wassignificantly (p < 0.001, unpaired t test) shorter than was observedfor interneurons in control rats (120 ± 13 msec; n = 13). Therewere no significant changes in the kinetics of evoked EPSCs duringrepetitive stimulation in either control or SE-experienced rats(Fig. 3C).

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Figure 3. Short-term depression of GC-evoked EPSC amplitudes during high-frequency (20 Hz) stimulation was more intense in hilar border interneurons from SE-experienced rats. A, Sample traces demonstrating short-term depression of EPSC amplitudes during high-frequency stimulation of GC inputs in interneurons from untreated (top) and SE-experienced (bottom) rats. The depicted EPSCs represent the average of 12-15 consecutive 20 Hz trains delivered at 3 sec intervals. B, Plot depicting the average depression of EPSC amplitudes produced by 20 Hz stimulation of GC inputs to interneurons from either untreated (; n = 13 interneurons) or pilocarpine-treated ( $triangle$ ; n = 16 interneurons) rats. Each data set was well fit by a single exponential function (solid lines). C, Superimposed first and last EPSCs in a 20 Hz train delivered to GC inputs to interneurons from either an SE-experienced (bottom) or untreated (top) rat. For each pair, the amplitude of the last EPSC in the train was scaled to the amplitude of the first EPSC. The decay kinetics of EPSCs evoked during repetitive activation of GC inputs was not altered during the train in interneurons from either untreated or SE-experienced rats.

Changes in the magnitude of short-term plasticity induced by SE at each of the three excitatory inputs to hilar border interneuronsthat we examined are summarized in Figure 4. At granule cell inputs,STD was significantly enhanced at both 10 Hz (p = 0.03, unpairedt test) and 20 Hz (p < 0.0001, unpaired t test) but not at 5 Hz(Fig. 4A). Enhanced STD of granule cell input to hilar borderinterneurons occurs within 24 hr after induction of SE and persistsfor at least 8 d (Fig. 4B). In contrast, STD of perforant pathinputs to interneurons in SE-experienced rats was not differentfrom STD in control adult rats at any frequency tested (Fig. 4C).

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Figure 4. Short-term depression of evoked EPSCs is enhanced over a range of stimulus frequencies. A, Peak depression of GC-evoked EPSCs was measured at 0.3, 5, 10, and 20 Hz in untreated ( $open circle$ ) and SE-experienced () rats. STD produced a significantly greater depression of EPSC amplitude at both 10 Hz (*p = 0.03, unpaired t test; n = 13) and 20 Hz (*p < 0.001, unpaired t test; n = 17). B, Enhancement of short-term depression at GC inputs to hilar border interneurons persists for at least 8 d after induction of SE. Each point represents the maximal STD achieved during 20 Hz stimulation of GC input for a single interneuron from normal adult ( $open circle$ ; n = 11) and SE-experienced (; n = 16) rats. Maximal depression was calculated to be the amplitude of the plateau current (500-800 msec latency) expressed as a percentage of the first EPSC amplitude. C, STD of perforant path inputs was not enhanced significantly in SE-experienced rats at any frequency tested. D, High-frequency stimulation of CA3 inputs produced a combination of facilitation and depression in the adult rat. In contrast, only HFS-induced depression was observed in SE-experienced rats.

CA3 inputs underwent short-term facilitation during repetitive stimulation at 5 Hz in control adult rats but showed no netplasticity at 10 Hz and depression at 20 Hz (Fig. 4D). In SE-experiencedrats, however, repetitive stimulation of CA3 inputs produced depressionat both frequencies tested (Fig. 4D). Repetitive stimulation ofthe CA3 pyramidal cell layer often produced bursts of EPSCs duringthe trains in both control and SE-experienced rats, likely becauseof synchronized activation of CA3 pyramidal cells (Miles and Wong,1987; Kneisler and Dingledine, 1995). Because this bursting behavioroften obscured the short-term plasticity of evoked inputs, wealso used a paired-pulse protocol to examine the effects of SEon activity-dependent plasticity at evoked inputs to interneurons.This paired stimulation protocol also demonstrated changes inshort-term plasticity at both CA3 and GC inputs to interneuronsin SE-experienced rats (Fig. 5). For example, paired stimulationof GC input to interneurons, delivered at an interpulse intervalof 50 msec, resulted in a depression of the second pulse to 77± 3% of the first EPSC amplitude in control rats (n = 19). InSE-experienced rats, paired stimulation of GC inputs resultedin a significantly greater (p = 0.002, unpaired t test) reductionof the second EPSC (58 ± 5% of the first EPSC amplitude; n = 10).In contrast to the synaptic depression observed at granule cellinputs, paired stimulation of CA3 inputs to hilar border interneuronsat an interval of 50 msec produced facilitation to 225 ± 28% ofthe first EPSC amplitude in control rats (n = 14). In SE-experiencedrats, however, pairing stimuli in CA3 resulted in a depressionof evoked EPSCs onto interneurons (62 ± 21% of the first EPSCamplitude; n = 3). The bursting behavior produced by repetitivehigh-frequency stimulation (HFS) of CA3 inputs was not observedwith paired stimulation.

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Figure 5. Paired-pulse stimulation of evoked inputs to hilar border interneurons in normal adult and SE-experienced rats. A, Paired stimulation to GC inputs delivered at a 50 msec interpulse interval produced a depression of the second EPSC in normal adult rats (top left) that was potentiated in SE-experienced rats (top right). A summary of paired stimulation of GC inputs to interneurons from 19 normal adult ( $triangle$ ) and 10 SE-experienced ( $black-triangle$ ) rats is shown in the bottom panel. Paired-pulse depression was significantly (*p = 0.002, unpaired t test) greater at GC inputs to interneurons in SE-experienced rats. B, Paired stimulation (interpulse interval, 50 msec) at CA3 inputs produced a facilitation in EPSC amplitude in normal adult rats (top left). In contrast, paired stimulation of CA3 inputs in SE-experienced rats produced a depression (top right). Paired stimulation of CA3 inputs to interneurons from 15 normal adult ( $open circle$ ) and three SE-experienced () rats is summarized in the bottom panel. The paired-pulse relationship at CA3 inputs to interneurons in SE-experienced rats was depressed significantly (*p < 0.019, unpaired t test), relative to the strong potentiation in normal adult rats.

Enhanced mGluR-mediated regulation of interneurons in SE-experienced rats

A near maximally effective concentration of the group II mGluR agonist, DCG-IV (1 µM), was significantly (p = 0.004) moreeffective in depressing GC input to hilar border interneuronsin SE-experienced rats at 1-8 d after SE. A comparison of thetime course of the effect of DCG-IV on GC-evoked inputs to hilarborder interneurons is shown in Figure 6A. In control adult rats,GC-evoked EPSCs were reduced by 27 ± 5% (n = 7 neurons). In contrast,DCG-IV produced a 68 ± 5% reduction in GC-evoked EPSCs in SE-experiencedrats (Fig. 6A,B; n = 11 neurons). Enhanced regulation of GC inputsby group II mGluRs was apparent as early as 1 d and persistedfor at least 8 d after the induction of SE (Fig. 6C). The transmissionrate of minimal GC inputs to hilar border interneurons was reducedby DCG-IV to 20 ± 17% of control (n = 3 neurons) in SE-experiencedrats. However, as with GC inputs to hilar border interneuronsin juvenile rats (Doherty and Dingledine, 1998), the amplitudeof minimally evoked EPSCs was unchanged (Fig. 6D). This is consistentwith a presynaptic action of group II mGluRs at GC inputs to hilarborder interneurons in adult control and SE-experienced rats,similar to that in untreated juvenile rats (Doherty and Dingledine,1998).

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Figure 6. Presynaptic inhibition of transmitter release at GC inputs to hilar border interneurons by the selective group II mGluR agonist, DCG-IV, was enhanced in the SE-experienced rat. A, Time course of the reversible depression of GC-evoked EPSC amplitude by DCG-IV (1 µM). GC inputs were more sensitive to DCG-IV in interneurons from SE-experienced rats (; n = 4) than in interneurons from untreated adult rats ( $triangle$ ; n = 5). B, Maximal depression of GC-evoked EPSC amplitude induced by activation of group II mGluRs is significantly (*p = 0.005, unpaired t test) greater in SE-experienced rats (n = 11) than in untreated controls (n = 7). C, The sensitivity of GC inputs to depression by group II mGluRs is enhanced rapidly after induction of SE and persists for at least 8 d after induction. Each point in the scatterplot depicts the maximal effect of DCG-IV on evoked EPSC amplitudes at GC inputs to a single interneuron from either SE-experienced () or untreated adult ( $triangle$ ) rats. D, The mean amplitude of EPSCs evoked with minimal stimulation of a GC input to a hilar border interneuron from an SE-experienced rat was not depressed by DCG-IV (1 µM).

The mGluR antagonist, LY341495, antagonizes group II mGluRs with potencies in the low nanomolar range (Kingston et al., 1998;Schoepp et al., 1999). Thus, LY341495 at 500 nM provides a powerfulinhibition of group II mGluRs; however, LY341495 is also a potentantagonist for mGluR8, and to a lesser degree mGluR7, at thisconcentration (Schoeppe et al., 1999). In SE-experienced rats,however, LY341495 (500 nM) attenuated STD induced by 20 Hz stimulationof GC inputs to hilar border interneurons (Fig. 7A). The plateaureached during STD of GC-evoked EPSCs was significantly greaterin the absence of LY341495 than in its presence (Fig. 7B). Thus,LY341495 produced a small but significant (p < 0.001, paired ttest) attenuation of short-term plasticity at these synapses inSE-experienced rats, reducing the magnitude of STD by 13%. Incontrast, LY341495 had no significant effect on the magnitudeof STD in normal adult rats (Fig. 7B) (Doherty, Mott, Alagarsamy,Conn, and Dingledine, unpublished observations). These data togetherpoint to enhanced group II mGluR function at granule cell inputto hilar border interneurons in the SE-experienced rat.

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Figure 7. The selective group II mGluR antagonist, LY341495, attenuates STD of interneuron inputs in SE-experienced rats. A, Bath application of LY341495 ( $triangle$ , 500 nM) significantly (p < 0.01, one-way ANOVA) attenuated the STD produced during 20 Hz stimulation of GC inputs to hilar border interneurons from SE-experienced rats (). B, Group data illustrating the effect of LY341495 on the magnitude of STD at GC inputs to hilar border interneurons in the SE-experienced, but not control, rat. In control rats (n = 4), LY341495 had no effect on the plateau amplitude of GC-evoked EPSCs reached during 20 Hz trains. In SE-experienced rats (n = 4), LY341495 significantly (p < 0.01, paired t test) attenuated the plateau current reached during 20 Hz trains.

High-frequency stimulation evokes slow EPSCs in interneurons from SE-experienced rats

Stimulation of GC inputs at 5-20 Hz produced slow inward currents during the stimulus trains. Slow evoked currents are obviousin Figure 3A and are shown in more detail in Figure 8A. Slow currentswere observed during high-frequency stimulation of GC inputs in95% of hilar border interneurons in SE-experienced rats. In contrast,similar slow currents were observed in only 40% of hilar borderinterneurons from control adult rats. The mean amplitude of theslow current was $-$ 26 ± 11 pA (n = 20) in SE-experienced rats and $-$ 9 ± 5 pA in control adult rats (n = 20). The amplitude of thiscurrent was dependent on stimulus frequency, with higher stimulusfrequencies producing larger currents (Fig. 8A,B). There was nocorrelation between the amplitude of the slow current and themagnitude of STD in SE-experienced rats (Fig. 8C). Thus, the slowcurrent was unlikely to have had a systematic effect on the short-termdepression of fast AMPA-mediated EPSCs. The current-voltage relationshipfor the slow current is depicted in Figure 8D. Slow currents hadan apparent reversal potential of >0 mV and showed significantrectification at negative membrane potentials. The selective NMDAreceptor antagonist, D-APV (50 µM), significantly (p < 0.05, pairedt test) reduced the amplitude of the slow current (n = 4), suggestingthat it was largely mediated by NMDA receptors activated duringthe train (Fig. 8E).

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Figure 8. Properties of the slow current produced during HFS of afferent input to hilar border interneurons in SE-experienced rats. A, HFS of the GC input produced slow inward currents at a holding potential of $-$ 70 mV in a hilar border interneuron from an SE-experienced rat. The amplitude of the current was dependent on the frequency of stimulation. Each train was 800 msec in duration. B, Group data showing the relationship between STD and slow EPSC amplitude (n = 6 interneurons). Linear regression analysis indicated no significant correlation (r = 0.42; p = 0.91) between these two measurements. C, Plot showing the lack of correlation between the amplitude of the slow current and the amount of STD produced at that input. Each point represents data from a different interneuron from SE-experienced rats. Stimulation was delivered in all cases to GC inputs at a frequency of 20 Hz. D, Current-voltage relationship of the slow current. Note the pronounced rectification of the evoked current at hyperpolarized potentials. E, The selective NMDA receptor antagonist, D-APV (50 µM), significantly reduced the amplitude of the slow EPSC evoked during 20 Hz GC stimulation in four hilar border interneurons (V_h, $-$ 70 mV).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

SE-induced alterations in short-term plasticity at inputs to inhibitory interneurons

Paired-pulse inhibition of granule cell population spikes was progressively impaired after pilocarpine-induced SE; it wasevident at 24 hr after SE and peaked after 4-5 d. This resultindicates that synaptic inhibition was rapidly impaired or excitationwas enhanced after SE. We hypothesized that synaptic inhibitionwas rapidly reduced after SE because of a reduction of excitatorydrive onto hilar border interneurons. Loss of paired-pulse inhibitionmay be partially attributable to a loss of inhibitory interneuronsin the hilus after SE (Obenaus, 1993). In this study, we demonstratedthat use-dependent depression at two different excitatory synapsesonto surviving GABAergic hilar border interneurons is enhancedafter pilocarpine-induced statusepilepticus.

The magnitude of STD onto hilar border interneurons during repetitive stimulus trains at synapses from both dentate granulecell and CA3 pyramidal cell synapses is significantly enhancedin SE-experienced rats. However, enhanced STD after SE was synapse-specificbecause depression of perforant path synapses was not increased.Despite enhanced STD during high-frequency stimulation after SE,neither the probability of transmitter release nor the amplitudeof minimal EPSCs was altered at these synapses during low-frequencystimulation. Thus, enhanced STD during repetitive activation representsa synapse- and context-dependent deficit in excitatory drive ontointerneurons duringepileptogenesis.

We demonstrated that depression of glutamate release at GC inputs by group II mGluRs is enhanced after pilocarpine-inducedSE. This enhancement reverses a decrease in group II mGluR functionat these synapses that occurs during development (Doherty, Mott,Alagarsamy, Conn, and Dingledine, unpublished observations). LY341495,a mGluR antagonist with selectivity for group II mGluRs, significantlyattenuated STD at GC inputs in the SE-experienced rat but hadno effect on STD at GC inputs in the normal adult. Thus, groupII mGluR-mediated reduction of transmitter release contributesto STD in the SE-experienced adultrat.

Thus, some synaptic inputs onto hilar border interneurons are susceptible to a partial, reversible disconnection from theirexcitatory drive via an mGluR-mediated, activity-dependent process.This mGluR-mediated disconnection of inhibitory interneurons leadsto a transient disinhibition of granule cell firing in juvenilerats (Doherty, Mott, Alagarsamy, Conn, and Dingledine, unpublishedobservations) and could therefore contribute to increased excitatorymossy fiber activation of CA3 pyramidal cells. We hypothesizethat feedback inhibition of granule cell activity in the epilepticdentate gyrus is episodically reduced when hilar border interneuronsexperience a transient, presynaptic mGluR-mediated reduction inexcitatory drive during repetitive synaptic activation. Additionalwork is needed to determine whether this shift in the balancebetween excitation and inhibition in the dentate gyrus duringthe latent period before spontaneous seizures appear enables furtheractivity-dependent synaptic reorganization in the hippocampusduring epileptogenesis and contributes to triggering seizure generationin the chronically epilepticbrain.

Functional disconnection of interneuron inputs in SE-experienced rats

The dentate gyrus may act as a filter, resisting the transfer of epileptiform discharges from the entorhinal cortex to thehippocampus (Collins et al., 1983). Sufficiently intense stimulationcan overwhelm this "dentate gate" (Stringer and Lothman, 1989).Synaptically mediated seizure activity can be propagated intothe dentate gyrus through the entorhinal cortex (Barbarosie etal., 2000). Our hypothesis that a transient loss of feedback inhibitionduring high-frequency activation of the dentate gyrus, becauseof a functional disconnection of hilar border interneurons, couldprovide a physiological mechanism to overwhelm the dentate gate,facilitating the development of seizure discharges in downstreamhippocampalcircuitry.

Alterations in short-term plasticity were the only defects in excitatory neurotransmission onto interneurons observed afterSE. We found no significant changes in either the properties ofunitary EPSCs or the probability of transmitter release at thesesynapses after SE. Thus, functional disconnection of interneuronsfrom excitatory inputs is subtle, manifesting only in responseto an appropriate range of stimulus frequencies at affected synapses.Although these data are not consistent with a major deafferentationof hilar border interneurons in the SE-experienced dentate gyrus(Sloviter, 1991; Bekenstein and Lothman, 1993), we cannot ruleout the possibility that some excitatory inputs to interneuronsare lost afterSE.

Changes in group II mGluR function in the SE-experienced dentate gyrus

Increased group II mGluR function during epileptogenesis may represent a return toward a juvenile phenotype. The group IImGluR agonist, DCG-IV, powerfully depresses synaptic transmissionat GC inputs to hilar border interneurons in the juvenile rat(Doherty and Dingledine, 1998), but GC inputs in adult rats havea significantly reduced sensitivity to DCG-IV (Doherty, Mott,Alagarsamy, Conn, and Dingledine, unpublished observations). DCG-IV-mediatedinhibition of GC inputs increases after pilocarpine-induced SE,matching the efficacy of DCG-IV observed in the juvenile hippocampus.Likewise, LY341495 reversibly attenuates STD of GC inputs in SE-experiencedrats. In contrast, LY341495 has no effect on STD of GC inputsto hilar border interneurons in the normal adult rat, althoughit does attenuate STD significantly in the juvenile rat (Doherty,Mott, Alagarsamy, Conn, and Dingledine, unpublished observations).Group II mGluR-mediated function during epileptogenesis increasesto the level seen in juvenile rats (Doherty and Dingledine, 1998),suggesting a recapitulation of a development program in the dentategyrus during epileptogenesis. However, in contrast to the transientcontribution of group II mGluRs to STD in normal juvenile rats(Doherty, Mott, Alagarsamy, Conn, and Dingledine, unpublishedobservations), a persistent mGluR component was revealed in SE-experiencedrats (Fig. 7A).

Modulation of mGluR function in cortical circuitry is likely to be an important feature in the epileptogenic process. mGluRmRNA levels are rapidly modulated in the hippocampus after statusepilepticus (Aronica et al., 1997). Although Klapstein et al.(1999) reported that perforant path sensitivity to group III agonistsis reduced in kindled rats, Friedl et al. (1999) found no significantchange in group III sensitivity at these synapses in the samemodel. In contrast, increased sensitivity to group II mGluR agonistsin the SE-experienced dentate gyrus resembles enhanced group IIsensitivity reported in the epileptic amygdala (Neugebauer etal., 1997). mGluR1a (Blumcke et al., 2000) and mGluR4 (Lie etal., 2000) immunoreactivities are increased in the epileptic humandentate gyrus. Group III mGluR function is reduced in hippocampalslices from surgically resected tissue (Dietrich et al., 1999).

We demonstrated enhanced mGluR-mediated inhibition of glutamatergic neurotransmission at GC synapses after SE contributesto enhanced STD in SE-experienced rats. Although these resultsare most consistent with a group II effect, 500 nM LY341495 partiallyantagonizes mGluR8 and mGluR7 (Schoeppe et al., 1999). Thus, anincrease in group III mGluR function could also contribute tothe enhanced STD at these synapses in SE-experienced rats. LY341495did not completely block the enhanced STD in SE-experienced rats,indicating that other mechanisms must contribute to enhanced STDat these synapses. Perhaps activity-dependent increases in therate of vesicle depletion, reduced vesicle pool replenishment(Stevens and Wesseling, 1999), or changes in the properties ofpostsynaptic AMPA receptors (Rozov and Burnashev, 1999) contributeto enhanced STD in SE-experienced rats. We cannot rule out a selectiveloss of a subpopulation of interneurons with weak STD in SE-experiencedrats. However, the observation that the plateau of STD was typicallygreater in SE-experienced rats than in any of the control cells(Fig. 4B) argues against thispossibility.

Functional implications

Although granule cells in vivo do not typically discharge at frequencies likely to activate presynaptic mGluRs (Jung and McNaughten,1993), high-frequency granule cell discharges in the dentate gyruscan precede seizures in the chronically epileptic brain (Braginet al., 1999; Finnerty and Jefferys, 2000). Moreover, granulecells in slices of human epileptic dentate gyrus can dischargeat high frequencies when GABAergic inhibition is compromised (Francket al., 1995). Transient reduction of inhibitory control duringmGluR-mediated depression of interneuron input may contributeto the development of hyperexcitability in the latent period ofepileptogenesis. Polysynaptic IPSCs onto granule cells undergoa progressive depression during high-frequency (30 Hz) stimulationof the perforant path in pilocarpine-treated rats at 8 weeks afterSE (Isokawa, 1996).

Because hilar border interneurons synapse onto other inhibitory interneurons (Freund and Buzáski, 1996), enhanced STD atinterneuron inputs might produce a paradoxical increase in feedbackinhibition in the dentate gyrus. Indeed, augmentation of GABAergicinhibition in the hippocampus has also been reported in both humanepilepsy (Swanson et al., 1998; Wilson et al., 1998) and chronicexperimental models (Bühl et al., 1996; Haas et al., 1996). However,our data are most consistent with activity-dependent functionaldisinhibition of granule cells. Evidence for this includes impairedsynaptic inhibition within the first week after SE observed inthis study and the demonstration that a DCG-IV-mediated reductionin excitatory input onto hilar border interneurons results inimpaired feedback inhibition of dentate granule cells (Doherty,Mott, Alagarsamy, Conn, and Dingledine, unpublishedobservations).

In conclusion, SE enhances mGluR-mediated depression of excitatory drive onto dentate hilar border interneurons, a potentiallyimportant regulatory mechanism to dynamically influence the strengthof GABAergic inhibition in the dentate gyrus. This aberrant plasticitymay play an important role in epileptogenesis and may triggeror amplify epileptiform activity in the epileptichippocampus.

  FOOTNOTES

Received Aug. 28, 2000; revised Nov. 20, 2000; accepted Jan. 4, 2001.

This work was supported by an American Epilepsy Society Research Training Fellowship (J.D.), the Charles E. Culpeper Foundation(J.D.), and the National Institutes of Health (R.D.). We thankDr. Y. Ohfune and Tocris Cookson for DCG-IV, Dr. D. Schoepp forLY341495, Dr. V. Nadler for help with the pilocarpine model ofchronic seizures, and Drs. S. Bausch and D. Mott for helpful commentson thismanuscript.
Correspondence should be addressed to James Doherty, 5010 Rollins Research Center, Emory University Medical School, 1510 CliftonRoad, Atlanta, GA 30322. E-mail: jdoherty{at}bimcore.emory.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Aronica EM, Gorter JA, Paupard M-C, Grooms SY, Bennett MVL, Zukin SR (1997) Status epilepticus-induced alterations in metabotropic glutamate receptor expression in young and adult rats. J Neurosci 17:8588-8595[Abstract/Free Full Text].
Ascády L, Kamondi A, Sík A, Freund TF, Buzáki G (1998) GABAergic cells are the major postsynaptic targets of mossy fibers in the rat hippocampus. J Neurosci 18:3386-3404[Abstract/Free Full Text].
Barbarosie M, Louvel J, Kurcewicz I, Avoli M (2000) CA3-released entorhinal seizures disclose dentate gyrus epileptogenicity and unmask a temporoammonic pathway. J Neurophysiol 83:1115-1124[Abstract/Free Full Text].
Bausch SB, Chavkin C (1997) Changes in hippocampal circuitry after pilocarpine-induced seizures as revealed by opioid receptor distribution and activation. J Neurosci 17:477-492[Abstract/Free Full Text].
Bekenstein JW, Lothman EW (1993) Dormancy of inhibitory interneurons in a model of temporal lobe epilepsy. Science 259:97-100[Abstract/Free Full Text].
Bleck TP (1999) Management approaches to prolonged seizures and status epilepticus. Epilepsia 40 [Suppl 1]:S59-63.
Blumcke I, Becker AJ, Klein C, Scheiwe C, Lie AA, Beck H, Waha A, Friedl MG, Kuhn R, Emson P, Elger C, Wiestler OD (2000) Temporal lobe epilepsy associated up-regulation of metabotropic glutamate receptors: correlated changes in mGluR1 mRNA and protein expression in experimental animals and human patients. J Neuropathol Exp Neurol 59:1-10[ISI][Medline].
Bragin A, Engel Jr J, Wilson CL, Fried I, Mathern GW (1999) Hippocampal and entorhinal cortex high-frequency oscillations (100-500 Hz) in human epileptic brain and in kainic acid-treated rats with chronic seizures. Epilepsia 40:127-137[ISI][Medline].
Bragin AG, Jando G, Nadazdy Z, Hetke J, Wise K, Buzsaki G (1995) Gamma (40-100 Hz) oscillations in the hippocampus of the behaving rat. J Neurosci 15:47-60[Abstract].
Breakwell NA, Rowan MJ, Anwyl R (1996) Metabotropic glutamate receptor dependent EPSP and EPSP-spike potentiation in area CA1 of the submerged rat hippocampal slice. J Neurophysiol 76:3126-3135[Abstract/Free Full Text].
Brooks-Kayal A, Shumate MD, Jin H, Rikhter TY, Coulter DA (1998) Selective changes in single cell GABA_A receptor subunit expression and function in temporal lobe epilepsy. Nat Med 4:1166-1172[ISI][Medline].
Bühl EH, Otis TS, Mody I (1996) Zinc-induced collapse of augmented inhibition by GABA in a temporal lobe epilepsy model. Science 271:369-373[Abstract].
Canepari M, Cherubini E (1998) Dynamics of excitatory transmitter release: analysis of synaptic responses in CA3 hippocampal neurons after repetitive stimulation of afferent fibers. J Neurophysiol 79:1977-1988[Abstract/Free Full Text].
Cavalheiro EA, Leite JP, Bortolotto ZA, Turski WA, Ikonomidou C, Turski L (1991) Long-term effects of pilocarpine in rats: structural damage of the brain triggers kindling and spontaneous recurrent seizures. Epilepsia 32:778-782[ISI][Medline].
Chagnac-Amitai Y, Connors BW (1989) Horizontal spread of synchronized activity in neocortex and its control by GABA-mediated inhibition. J Neurophysiol 61:747-758[Abstract/Free Full Text].
Collins RC, Tearse RG, Lothman EW (1983) Functional anatomy of limbic seizures: focal discharges from medial entorhinal cortex in rat. Brain Res 280:25-40[ISI][Medline].
Coulter D (1999) Chronic epileptogenic cellular alterations in the limbic system after status epilepticus. Epilepsia 40 [Suppl 1]:S23-33.
Dietrich D, Kral T, Clusmann H, Friedl M, Schramm J (1999) Reduced function of L-AP4-sensitive metabotropic glutamate receptors in human epileptic sclerotic hippocampus. Eur J Neurosci 11:1109-1113[ISI][Medline].
Dobrunz LE, Stevens CF (1997) Heterogeneity of release probability, facilitation, and depletion at central synapses. Neuron 18:995-1008[ISI][Medline].
Doherty J, Dingledine R (1997a) The regulation of excitatory input to inhibitory interneurons of the dentate gyrus during hypoxia. J Neurophysiol 77:393-404[Abstract/Free Full Text].
Doherty J, Dingledine R (1997b) Excitatory synaptic inputs to dentate interneurons in slices from pilocarpine-treated epileptic rats. Epilepsia 38 [Suppl 8]:124[ISI][Medline].
Doherty J, Dingledine R (1998) Differential regulation of excitatory synaptic inputs to hilar border interneurons in the dentate gyrus by metabotropic glutamate receptors. J Neurophysiol 79:2903-2910[Abstract/Free Full Text].
Dykes RW (1997) Mechanisms controlling neuronal plasticity in somatosensory cortex. Can J Physiol Pharmacol 75:535-545[ISI][Medline].
Empson RM, Jefferys JG (1993) Synaptic inhibition in primary and secondary chronic foci by intrahippocampal tetanus toxin in the rat. J Physiol (Lond) 465:595-614[Abstract/Free Full Text].
Finnerty GT, Jefferys JG (2000) 9-16 Hz oscillation precedes secondary generalization of seizures in the rat tetanus toxin model of epilepsy. J Neurophysiol 83:2217-2226[Abstract/Free Full Text].
Franck JE, Pokorny J, Kunkel DD, Schwartzkroin PA (1995) Physiologic and morphologic characteristics of granule cell circuitry in human epileptic hippocampus. Epilepsia 36:543-558[ISI][Medline].
Freund TF, Busáki G (1996) Interneurons of the hippocampus. Hippocampus 6:347-470[ISI][Medline].
Friedl M, Clusmann H, Kral T, Dietrich D, Schramm J (1999) Analysing metabotropic glutamate group III receptor mediated modulation of synaptic transmission in the amygdala-kindled dentate gyrus of the rat. Brain Res 821:117-123[Medline].
Galarreta M, Hestrin S (1998) Frequency-dependent synaptic depression and the balance between excitation and inhibition in the neocortex. Nat Neurosci 7:587-594.
George B, Kulkarni SK (1996) Protective effects of GABAergic drugs and other anticonvulsants in lithium-pilocarpine-induced status epilepticus. Methods Find Exp Clin Pharmacol 18:335-340[Medline].
Grover LM, Yan C (1999) Blockade of GABA_A-receptors facilitates induction of NMDA receptor-independent long-term potentiation. J Neurophysiol 81:2814-2822[Abstract/Free Full Text].
Haas KZ, Sperber EF, Moshé SL, Stanton PK (1996) Kainic acid-induced seizures enhance dentate gyrus inhibition by downregulation of GABA_B receptors. J Neurosci 16:4250-4260[Abstract/Free Full Text].
Hirsch JC, Agassandian C, Merchán-Pérez A, Ben-Ari Y, DeFelipe J, Esclapez M, Bernard C (1999) Deficit of quantal release of GABA in experimental models of temporal lobe epilepsy. Nat Neurosci 2:499-500[ISI][Medline].
Houser CR, Escaplez M (1996) Vulnerability and plasticity of the GABA system in the pilocarpine model of spontaneous recurrent seizures. J Neurosci 13:4470-4485[Abstract].
Isokawa M (1996) Decrement of GABA_A receptor-mediated inhibitory postsynaptic currents in dentate granule cells in epileptic hippocampus. J Neurophysiol 75:1901-1908[Abstract/Free Full Text].
Jung MW, McNaughten BL (1993) Spatial selectivity of unit activity in the hippocampal granule cell layer. Hippocampus 3:165-182[ISI][Medline].
Kapur J, Macdonald RL (1997) Rapid seizure-induced reduction of benzodiazepine and Zn²⁺ sensitivity of hippocampal dentate granule cell GABA_A receptors. J Neurosci 17:7532-7540[Abstract/Free Full Text].
Keverne EB, Brennan PA (1996) Olfactory recognition memory. J Physiol (Lond) 90:399-401.
King GL, Dingledine R, Giacchino JL, McNamara JO (1985) Abnormal neuronal excitability in hippocampal slices from kindled rats. J Neurophysiol 54:1295-1304[Abstract/Free Full Text].
Kingston AE, Ornstein PL, Wright RA, Johnson BG, Mayne NG, Burnett JP, Belagaje R, Wu S, Schoepp DD (1998) LY341495 is a nanomolar potent and selective antagonist of group II metabotropic glutamate receptors. Neuropharmacology 37:1-12[ISI][Medline].
Klapstein GJ, Meldrum BS, Mody I (1999) Decreased sensitivity to group III mGluR agonists in the lateral perforant path following kindling. Neuropharmacology 38:927-933[ISI][Medline].
Kneisler TB, Dingledine R (1995) Synaptic input from CA3 pyramidal cells to dentate basket cells in the rat hippocampus. J Physiol (Lond) 487:125-146[ISI][Medline].
Laezza F, Doherty J, Dingledine R (1999) Long-term depression in hippocampal interneurons: joint requirement for pre- and postsynaptic events. Science 285:1411-1414[Abstract/Free Full Text].
Lie AA, Becker A, Behle K, Beck H, Malitschek B, Conn PJ, Kuhn R, Nitsch R, Plaschke M, Schramm J, Elger CE, Wiestler OD, Blümcke I (2000) Up-regulation of the metabotropic glutamate receptor mGluR4 in hippocampal neurons with reduced seizure vulnerability. Ann Neurol 47:26-35[ISI][Medline].
MacDonald RL, Kapur J (1999) Acute cellular alterations in the hippocampus after status epilepticus. Epilepsia 40 [Suppl 1]:S9-20.
Mangan PS, Lothman EW (1996) Profound disturbances of pre- and postsynaptic GABA_B-receptor-mediated processes in region CA1 in a chronic model of temporal lobe epilepsy. J Neurophysiol 76:1282-1296[Abstract/Free Full Text].
McMahon LL, Kauer JA (1997) Hippocampal interneurons express a novel form of synaptic plasticity. Neuron 18:295-305[ISI][Medline].
Mello LEAM, Cavalheiro EA, Tan AM, Kupfer WR, Pretorius JK, Babb TL, Finch DM (1993) Circuit mechanisms of seizures in the pilocarpine model of chronic epilepsy: cell loss and mossy fiber sprouting. Epilepsia 34:985-995[ISI][Medline].
Merlin LR, Wong RKS (1993) Synaptic modifications accompanying epileptogenesis in vitro: long-term depression of GABA-mediated inhibition. Brain Res 627:330-340[ISI][Medline].
Miles R, Wong RK (1987) Inhibitory control of local excitatory circuits in the guinea-pig hippocampus. J Physiol (Lond) 388:611-629[Abstract/Free Full Text].
Neugebauer V, Keele NB, Shinnick-Gallagher P (1997) Epileptogenesis in vivo enhances the sensitivity of inhibitory metabotropic glutamate receptors in basolateral amygdala neurons in vitro. J Neurosci 17:983-995[Abstract/Free Full Text].
Obenaus A, Esclapez M, Houser CR (1993) Loss of glutamate decarboxylase mRNA-containing neurons in the rat dentate gyrus following pilocarpine-induced seizures. J Neurosci 13:4470-4485.
Ohfune Y, Shimamoto K, Ishida M, Shinozaki H (1993) Synthesis of L-2-(2,3-dicarboxycyclopropyl)glycine: a novel conformationally restricted glutamate analog. Bioorg Med Chem 3:15-18.
Okazaki MM, Molnár P, Nadler V (1999) Recurrent mossy fiber pathway in rat dentate gyrus: synaptic currents in presence and absence of seizure-induced growth. J Neurophysiol 81:1645-1660[Abstract/Free Full Text].
Olsen RW, Avoli M (1997) GABA and epileptogenesis. Epilepsia 38:399-407[ISI][Medline].
Patrylo PR, Dudek FE (1998) Physiological unmasking of new glutamatergic pathways in the dentate gyrus of hippocampal slices from kainate-induced epileptic rats. J Neurophysiol 79:418-429[Abstract/Free