A Neuronal Glutamate Transporter Contributes to Neurotransmitter GABA Synthesis and Epilepsy

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The Journal of Neuroscience, August 1, 2002, 22(15):6372-6379

A Neuronal Glutamate Transporter Contributes to Neurotransmitter GABA Synthesis and Epilepsy
Jehuda P. Sepkuty¹, Akiva S. Cohen², Christine Eccles¹, Azhar Rafiq³, Kevin Behar⁴, Raquelli Ganel¹, Douglas A. Coulter², and Jeffrey D. Rothstein¹
¹ Departments of Neurology and Neuroscience, Johns Hopkins University, Baltimore, Maryland 21287, ² Departments of Pediatrics and Neuroscience, University of Pennsylvania School of Medicine and the Stokes Research Institute of Children's Hospital of Philadelphia, Philadelphia, Pennsylvania 19104, ³ Medical College of Virginia of Virginia Commonwealth University, Richmond, Virginia 23284, and ⁴ Department of Psychiatry, Yale University, New Haven, Connecticut 06520

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The predominant neuronal glutamate transporter, EAAC1 (for excitatory amino acid carrier-1), is localized to the dendritesand somata of many neurons. Rare presynaptic localization is restrictedto GABA terminals. Because glutamate is a precursor for GABA synthesis,we hypothesized that EAAC1 may play a role in regulating GABAsynthesis and, thus, could cause epilepsy in rats when inactivated.Reduced expression of EAAC1 by antisense treatment led to behavioralabnormalities, including staring-freezing episodes and electrographic(EEG) seizures. Extracellular hippocampal and thalamocorticalslice recordings showed excessive excitability in antisense-treatedrats. Patch-clamp recordings of miniature IPSCs (mIPSCs) conductedin CA1 pyramidal neurons in slices from EAAC1 antisense-treatedanimals demonstrated a significant decrease in mIPSC amplitude,indicating decreased tonic inhibition. There was a 50% loss ofhippocampal GABA levels associated with knockdown of EAAC1, andnewly synthesized GABA from extracellular glutamate was significantlyimpaired by reduction of EAAC1 expression. EAAC1 may participatein normal GABA neurosynthesis and limbic hyperexcitability, whereasepilepsy can result from a disruption of the interaction betweenEAAC1 and GABAmetabolism.

Key words: EAAC1; transport; antisense; GABA; metabolism; epilepsy

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Glutamate transport is the major mechanism controlling extracellular glutamate levels, preventing excitotoxicity, and avertingneural damage associated with epilepsy. (McBean and Roberts, 1985;Rothstein et al., 1992, 1993, 1994, 1996; Robinson et al., 1993a,b;Tanaka et al., 1997). Glutamate transporters are localized tothe membranes of synaptic terminals and astroglial processes thatensheath synaptic complexes (Hertz, 1979; Kanner and Schuldiner,1987; Danbolt et al., 1992; Kanai et al., 1993; Rothstein et al.,1994, 1996; Conti et al., 1998; He et al., 2000). GLAST (for glutamate-aspartatetransporter [EAAT-1 (for excitatory amino acid transporter-1)](Storck et al., 1992; Arriza et al., 1994) and GLT-1 (for glutamatetransporter-1) (EAAT-2) (Pines et al., 1992; Arriza et al., 1994)are astroglial glutamate transporters, and EAAC1 (for excitatoryamino acid carrier-1) (EAAT-3) (Kanai and Hediger, 1992; Arrizaet al., 1994; Shashidharan et al., 1994; Kanai et al., 1995; Bjoraset al., 1996; Nakayama et al., 1996; Velaz-Faircloth et al., 1996;Eskandari et al., 2000), EAAT-4 (Fairman et al., 1995), and EAAT-5(Arriza et al., 1997) are neuronal proteins. Astroglial glutamatetransporters are responsible for at least 80% of the high-affinityglutamate transport and the majority of synapticinactivation.

EAAC1 is highly concentrated in the somata and dendrites of many neurons, especially those in the hippocampus, striatum, cerebellum,and olfactory bulb. There is little evidence for glutamate transporterproteins in the presynaptic terminal, with one exception. EAAC1has been localized to inhibitory GABAergic neurons, includingcerebellar Purkinje cells (Rothstein et al., 1994; Conti et al.,1998; He et al., 2000), which are highly concentrated in presynapticGABAergic terminals. Because of its unusual localization to GABAterminals, we hypothesized that the loss of EAAC1 could alterpresynaptic GABA metabolism, perhaps by altering a precursor supplyof glutamate. In this study, we now show that EAAC1 contributesto new synthesis of inhibitory neurotransmitter GABA and thatloss of EAAC1 produces "staring"epilepsy.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Intraventricular antisense administration. All animal experiments were performed with approval by the Johns Hopkins AnimalCare and Use Committee. Male Sprague Dawley rats (250-350 gm)were anesthetized with 4% chloral hydrate (1 ml/100 gm). Antisenseoligonucleotides (oligodeoxynucleotides) were infused intraventricularlyby mini-osmotic pumps as described previously, including oligonucleotidesto EAAC1, GLAST, and GLT-1 (Rothstein et al., 1996). Lyophilizedoligonucleotides were reconstituted in artificial CSF (ACSF) (Wagner,1994; Wahlestedt, 1994; Rothstein et al., 1996) at a concentrationof 2.5 mg/ml, dialyzed (Rothstein et al., 1996), and then filtered(0.22 µm) before use. Four EEG screw electrodes were placed onthe skull during the same procedure (one frontal and one parietalon each side). Antisense and sense oligodeoxynucleotides weredelivered at a rate of 1-10 µg/hr over a 9-12 dperiod.

Video-EEG recording. Four EEG electrodes (Plastics One, Roanoke,VA) were mounted on the skull with cranioplastic cement duringthe stereotaxic placement of the cannula (one frontal and oneparietal on each side, 2 and 3 mm from the midline skull suture,respectively). Rats underwent daily EEG recording in a chamberthat allowed unrestrained movement while recording. Signals wererecorded using Grass EEG machine model 8-16 with amplifiers witha bandpass filter set between 1 and 70 Hz. Sensitivity was setto 7 µV/mm, and paper speed was set to 30 cm/sec. Two channelswere recorded. Bipolar and referential recordings were performedwhile the rat was awake and mobile in the chamber. EEG was sampledfor 20 min or until seizure activity occurred. If seizure activityoccurred, observation was continued until 5 min of non-epileptiformEEG activity had been recorded. Clinical behavior was monitoredby video camera during the EEG recording. EEG recording and interpretationwas done with the recorder-interpreter blinded to thetreatment.

Extracellular thalamocortical and hippocampal entorhinal cortical field potential slice recording. Four antisense EAAC1 experimentaland four sense EAAC1 control rats were decapitated 10 d afterinfusion. Thirteen antisense and 10 sense thalamocortical sliceswere recorded. Rat thalamocortical slices were prepared usingthe slice angle developed by Agmon and Connors (1991) (Coulterand Lee, 1993). Connections were verified by microscopic examinationof slices. Once cut and visualized, slices were transferred toan incubator, in which they were kept submerged in warmed (35°C)oxygenated medium until use. The slice medium was composed of(in mM): 130 NaCl, 3 KCl 3, 1.25 NaH₂PO₄, 0 MgCl₂, 26 NaHCO₃,and 10 dextrose. A separate incubator allowed preexposure of individualslices to low Mg²⁺ medium before recording. Slices were incubated for at least 1hr after dissection and for 1 hr or more in low Mg²⁺ medium before recording. Before recording, slices were transferredto an interface-type recording chamber, in which they were maintainedat 35°C. Differential AC-coupled extracellular recordings wereconducted using 2 M $Omega$ insulated tungsten electrodes (bandpass filteredat 10-3000 Hz). Recording was conducted from cortex in one channeland thalamus in the secondchannel.

Five antisense EAAC1 experimental and three sense EAAC1 control rats were decapitated 10 d after infusion for hippocampalentorhinal cortex (HEC) slice experiments, and eight antisenseand five sense slices were recorded. In brief, brain slices wereprepared using previously reported methods (Rafiq et al., 1993).Rats were anesthetized with halothane and decapitated, and thebrain was quickly removed and chilled for 1-2 min in a modifiedsucrose-based ACSF (SACSF) composed of (in mM): 200 sucrose, 3KCl, 1.25 NA₂PO₄, 0.9 MgCl₂, 2 CaCl₂, 26 NaHCO₃, and 10 glucose(equilibrated with 95% O₂-5% CO₂). After a 1 min wash in coldSACSF, the two hemispheres were dissected by midsagittal dissection.Hemispheres were immediately returned to oxygenated, cold SACSFuntil needed for slicing. Each hemisphere was individually blockedand sectioned in an inclined 12° transverse plane, modified fromJones and Heinemann (1988), with the use of a vibratome (Lancer1000; Vibratome, St. Louis, MO). Brain slices were subsequentlytransferred to a holding chamber in which they were kept submergedin ACSF containing (in mM): 130 NaCl, 3 KCl, 1.25 NA₂PO₄, 0.9MgCl₂, 2 CaCl₂, 26 NaHCO₃, and 10 glucose (warmed to 32°C andvigorously bubbled with 95% O₂-5% CO₂ for a period of 1-2 hr).Before recording, slices were transferred to an interface-typerecording chamber, in which they were perfused with 35°C ACSFat 1-1.5 ml/min for extracellular recording experiments. Extracellularfield potential recordings were made with the use of insulatedtungsten electrodes, placed in the pyramidal cell body layersof area CA1, CA3, and the dentate gyrus of each slice (Jones andHeinemann, 1988; Coulter and Lee, 1993; Rafiq et al., 1993). Allslice recordings and interpretation was done with the recorder-interpreterblinded to thetreatment.

Quantification of excitability. EEG and hippocampal slice recordings were analyzed by manually counting spikes (Daly and Pedley,1990) during the whole record for each rat and slice on the 10thtreatment day. Spike count in the EEG recordings of all EAAC1antisense-treated rats were compared with spike count in the EEGrecordings of three controls: EAAC1 sense-, GLT-1 antisense-,and GLAST antisense-treated rats. The average number of spikesper minute in each group was compared [ANOVA, followed by Fisher'sprotected least significant difference (PLSD) for spikes per minute].All of the spontaneous interictal spikes (SISs) in the hippocampalslice recordings were counted and compared between the EAAC1 antisense-and EAAC1 sense-treated rats (Student's t test). The thalamocorticalslice recordings were analyzed by manual measurement of the durationof discharges in seconds and calculating the average durationof discharges (seconds discharge per minute recording) in eachslice and then comparing the averages of EAAC1 antisense- andEAAC1 sense-treated rats (Student's ttest).

Patch recording in brain slices. Male Sprague Dawley rats were used in all experiments. Recordings were obtained from visuallyidentified pyramidal neurons in stratum pyramidale of area CA1of the rat hippocampus. For the purpose of this study, animalswere divided into four groups: EAAC1 antisense-treated rats, controls(sense-treated rats and naive rat controls), and GLAST antisense-treatedrats. Brain slices were prepared using previously reported methods(Rafiq et al., 1993). In brief, rats were anesthetized with halothaneand decapitated, and the brain was quickly removed and chilledfor 1-2 min in a modified SACSF) composed of (in mM): 201 sucrose,3.2 KCl, 1.25 NaHPO₄, 2 MgCl₂, 2 CaCl₂, 26 NaHCO₃, and 10 glucose10 (equilibrated with 95% O₂-5% CO₂ at 32.5°C). The brain wasglued, frontal side down, to a glass platform with cyanoacrylatecement, and coronal whole brain slices (225 µm) were sectionedusing a vibratome (Lancer 1000). Brain slices were subsequentlyhemisected, transferred to a holding chamber, and incubated inwarm (35°C) normal ACSF containing 126 mM NaCl substituted forsucrose and allowed to equilibrate for at least 2 hr before beingtransferred to the recordingchamber.

Whole-cell voltage-clamp recordings were conducted at room temperature from visually identified CA1 pyramidal neurons usinginfrared differential interference contrast or Hoffman modulationcontrast video microscopy (Stuart et al., 1993; Cohen et al.,2000). Cells were voltage clamped at $-$ 60 mV, and signals wererecorded and amplified with an Axopatch 1D (Axon Instruments,Foster City, CA), filtered at 2 kHz, digitized, sampled at 44kHz with a pulse code modulator digitizer (Neuro-Corder DR-890;Neurodata Instruments, New York, NY), and stored on videotapefor off-line analysis. Electrodes were fabricated from thick-walledborosilicate glass (World Precision Instruments, Sarasota, FL)and pulled to a resistance between 2 and 6 M $Omega$ when filled withan internal solution composed of (in mM): 135 CsCl, 10 HEPES,2 MgCl₂, and 4 MgATP, pH 7.25 (CsOH) on a two-stage puller (modelPP-83, Narishige, East Meadow, NY). To isolate GABA_A-mediatedevents, tetrodotoxin (TTX) (400 nM) and the excitatory amino acidantagonists D-2-amino-5-phosphonopentanoic acid (D-AP-5) (50 µM)and 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX) (6 µM) were addedto the superfusingACSF.

Recorded miniature IPSCs (mIPSCs) were reacquired using Dempster software (Strathclyde, Glasgow, UK), which collects eventsusing a manually controlled threshold detector and is capableof detecting events as small as 2-3× the baseline noise. To attemptto minimize cases of inadequate space clamp, neurons were usedfor analysis only when series resistance (R_s) was <20 M $Omega$ , andat least 80% series resistance compensation was achieved. R_s waschecked frequently throughout experiments, and neurons in whichR_s increased >20% were discarded. The kinetics of mIPSCs, i.e.,amplitude, rise, and decay times, were analyzed using cumulativeprobability histograms. mIPSC frequency was determined using Mini-Analysissoftware (Synaptosoft, Leonia, NJ). Reagents were purchased fromthe following vendors: all salts and diazepam were from Sigma(St. Louis, MO); D-AP-5 and CNQX were from Research Biochemicals(Natick, MA); and TTX was from Calbiochem (La Jolla, CA). Alldrugs were made as stock solutions and then diluted to their finalconcentration in the bathing medium. Statistical significancebetween cumulative probability distributions in control and drugconditions in individual neurons was assessed at the p < 0.05confidence level using the Kolmogorov-Smirnov nonparametric statisticaltest. Two-tailed unpaired Student's t tests were performed todetermine statistical significance at the p < 0.05 confidencelevel when comparing different treatment groups. All mIPSCs recordingsand interpretation was done with the recorder-interpreter blindedto thetreatment.

GABA levels. Dissected brain regions were homogenized in 0.1N perchloric acid. After thiol derivatization, levels of GABAwere determined using HPLC (0.18 M sodium acetate and 41% acetonitrilebuffer, pH 5.0; mobile phase at a flow rate of 2.5 ml/min) usinga 5 nm reverse-phase column (ODS Biocal; Bio-Rad, Hercules, CA)coupled with electrochemical detection (BioAnalytical Systems,West Lafayette, IN). Retention time for GABA was ~6.5 min as confirmedwith [¹⁴C]GABA standard. Tissue protein levels were determined by a Coomassieblue assay. Levels of total GABA are expressed as nanomoles permilligram ofprotein.

GABA metabolism. Supernatants (30 µl) from [¹⁴C]glutamate uptake experiments were mixed with 0.1N perchloric acid (165 µl),5 µl of 5-aminovaleric acid (45 µM solution in 0.1N perchloricacid), and 800 µl of "working reagent" [opthaldialdehyde (OPA)solution], and the solution was incubated at room temperaturefor 6 min. The working reagent was prepared by dissolving 67.1mg of OPA in 50 ml of methanol, 56 µl of t-butylthiol, and 15ml of 1 M carbonate buffer, pH 9.6, and the mixture was broughtto a final volume of 100 ml with ~30 ml of water. Exactly 6 minafter the addition of the OPA solution to the sample, 50 µl ofthe derivatized sample was analyzed by HPLC. Authentic GABA standardsallowed quantification of total GABA levels in the samples. Fractionsof each sample were collected (30 sec/fraction), and 300 µl aliquotswere mixed with 3 ml of scintillation cocktail and [¹⁴C] activity was analyzed by liquid scintillation spectroscopy(Wallac, Turku, Finland). Specific activity of [¹⁴C]GABA was calculated for each sample. Tissue protein levels weredetermined by a Coomassie blue assay with bovine serum albuminas standard. [¹⁴C]GABA-specific activities were compared in antisense- and sense-treatedsamples, in experiments of naive rats with and without DL-threo- $beta$ -hydroxy-asparticacid (THA) and in experiments of naive rats treated with 6-diazo-5-oxo-l-norleucine(DON) and dihydrokainate (DHK) at times t = 0 min and t = 30min.

Tissue preparation and [C¹⁴]glutamate uptake. Antisense- and sense-treated rats were decapitated 10 d after antisense infusion,and brains were rapidly removed and placed into chilled, oxygenated(95% O₂-5% CO₂) Krebs'-Ringer's bicarbonate (KRB) buffer (in mM:119 NaCl, 4.8 KCl, 1.7 CaCl₂, 1.2 MgCl₂, 1.2 KH₂PO₄, 23.8 NaHCO₃,and 5.5 glucose, pH 7.4). After 30 sec, the brain was placed ona chilled aluminum block (4°C), and hippocampus and thalamus weredissected from 1 mm coronal sections, followed by slicing into0.25 mm prisms (McIlwain tissue chopper; Brinkman Instruments).Prisms were suspended in chilled fresh KRB buffer in microvials(Eppendorf) on ice. DON, an inhibitor of phosphate-activated glutaminase(Sigma), was added to the microvial to a final concentration of10 mM. The microvials containing antisense- and sense (control)-treatedhippocampi and thalami were incubated with shaking at 37°C for15 min. The vials were then centrifuged (500 rpm, 5 min), andDON was washed out using the chilled KRB buffer. In some experiments,after washing out DON, THA was added to hippocampal prisms inthe microvials to a final concentration of 1 mM. The vials wereincubated for 15 min in 37°C, and the reaction was stopped onice. While on ice in chilled fresh KRB oxygenated buffer, glutamate(20 µM final concentration), [¹⁴C]glutamate (~1 µCi), and DL-gabaculline (20 µM final concentration)were added and incubated at 37°C for 30 min (Behar and Boehm,1994; Sibson et al., 1998). The reaction was terminated by chillingon ice and adding 0.4N perchloric acid. Some tissue was reservedfor the HPLC assay of GABA. The tissue was homogenized, frozen,and thawed at 37°C twice to break the cell membranes, and thehomogenate was centrifuged at 14,000 rpm for 20 min at 4°C. Theremaining pellet was dissolved in 200 µl of 1N NaOH for proteinassay. The supernatant fraction was filtered through 0.45 µm poresyringe filter and stored in $-$ 70°C until GABAanalysis.

Immunoblots. Antisense- and sense-treated rats were decapitated after 10 d of intraventricular treatment, and the brains wererapidly removed and placed on a chilled aluminum block (4°C).Coronal sections of brain were sliced at 1-2 mm intervals fromthe occipital pole to the olfactory bulbs. Immunoblots of thetissue homogenates were prepared with affinity-purified polyclonaloligopeptide antibodies to EAAC1 as described previously (Rothsteinet al., 1994, 1996)

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Antisense knockdown of EAAC1

Previous studies have demonstrated reliable and specific knockdown of EAAC1 expression after chronic intraventricular administrationof antisense oligonucleotides (Rothstein et al., 1996). By 8-10d after administration of EAAC1 antisense oligonucleotides, expressionof EAAC1 was reduced by >60% (Fig. 1a). Sense oligonucleotides(Fig. 1a) had no effect on EAAC1 expression and neither did randomoligonucleotides or antisense to other glutamate transporters:GLT-1 or GLAST (Rothstein et al., 1996). Loss of EAAC1 leads toa small loss in total tissue glutamate transporter activity (Rothsteinet al., 1996).

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Figure 1. Antisense EAAC1 treatment leads to loss of hippocampal EAAC1 expression and epilepsy. a, Immunoblots from hippocampal tissue of three antisense-treated rats (4, 5, 6) have reduced expression of EAAC1 by 60-70% compared with the hippocampus of three sense controls (1, 2, 3). b, e, EEG of an awake ambulating adult rat 1 or 2 d after infusion of antisense (b) or sense (e). A normal mixture of frequencies without spikes was seen in both animals. c, f, Recordings of the same rats (as in b and e, respectively) on day 4 or 5. Runs of high-voltage polyspike discharges for ~2.5 sec, with return to baseline background EEG, can be seen in the antisense-treated rat (c) but not in the sense-treated rat (f). d, g, On days 9 or 10, the maximal antisense effect was seen as prolonged continuous high-voltage spikes, spike and wave complexes, background slowing, and decreased mixture of frequencies in the antisense-treated rat (d) but not in the sense-treated rat (g). h, The mean number of spikes per minute on days 9 or 10 in antisense EAAC1 compared with three controls (GLT-1 antisense-, GLAST antisense-, and EAAC1 sense-treated animals) is significantly increased. *p < 0.005 between the study group and each of the control groups but not between the different controls; ANOVA with Fisher's PLSD for mean spikes per minute.

Subacute loss of EAAC1 leads to epilepsy: video-EEG recording

To evaluate the epileptogenicity of EAAC1 antisense treatment, EEG and video were recorded in awake and ambulating rats (n= 32). Up to 4 d after oligonucleotide treatment, no differencesin behavior or the EEG patterns were noted between the study groupand the control treatments (EAAC1 sense-, GLAST antisense-, andGLT-1 antisense-treated). The EEG consisted of a normal mixtureof frequencies without spikes (Fig. 1b,e) (GLT and GLAST antisensecontrols were not different from untreated or sense treated animals;data not shown). Beginning on the fourth day after EAAC1 antisenseinfusion, brief staring episodes and "freezing"-like postureswere observed that were not seen in EAAC1 sense controls or inGLAST antisense-treated and GLT-1 antisense-treated animals. TheGLT-1 and GLAST antisense-treated animals showed some motor slowingbut no staring-freezing episodes. The behavioral episodes of theEAAC1 antisense-treated rats correlated with EEG changes, markedby brief runs of rhythmic spikes, again not seen in the controls(Fig. 1c,f) (GLT-1 and GLAST antisense controls were not different;data not shown). These behavioral manifestations deteriorateddaily, coupled with worsening EEG. On the 10th day of infusion(a time point corresponding to a maximal 70-90% loss of EAAC1protein) (Rothstein et al., 1996), the behavioral changes consistedof prolonged freezing and staring episodes with occasional tonicposturing of the forepaws. The EAAC1 sense control rats did notshow behavioral changes, and the GLT-1 and GLAST antisense controlsmanifested severe motor weakness without posturing, freezing,or staring episodes. Corresponding to the long staring and freezingepisodes (as recorded by simultaneous video-EEG recording), theEEG recording showed prolonged runs of 4-6 sec spikes and spikeand wave complexes, along with slowing and reduced fast activityof the background. No epileptiform EEG changes were recorded inthe controls. In two of seven GLT-1 antisense controls, therewere a few spikes, but no runs of spikes, rhythmic spikes, orspike and wave complexes were seen (Fig. 1d,g) (GLT-1 and GLASTantisense controls were not different; data not shown). The meannumber of spikes per minute in the EAAC1 antisense-treated group(12.03; n = 6) was significantly higher then the mean number ofspikes per minute in the three other control groups: sense EAAC1(0.98; n = 5), antisense GLT-1 (2.99; n = 6), and antisense GLAST(0.57; n = 4) (Fig. 1h) (ANOVA; p = 0.034). Fisher's PLSD forspikes per minute showed a significant difference between thestudy group antisense EAAC1 and each of the control groups: senseEAAC1 (p = 0.0016), antisense GLT-1 (p = 0.0051), and antisenseGLAST (p = 0.0020), without a difference among the different controlgroups. This finding implies significant and specific epileptiformactivity associated with EAAC1 antisensetreatment.

Extracellular thalamocortical field potential slice recording

To explore the physiological basis of EAAC1 antisense oligonucleotide epileptogenesis, extracellular slice recording and intracellularrecording were used to test the hypothesis that hyperexcitationassociated with the EAAC1 antisense treatment was attributableto decreased inhibition. Extracellular field potentials from thalamocorticaland hippocampal slices of rat brains, relevant to both absenceand partial complex seizures, respectively, were recorded in studyanimals andcontrols.

Extracellular thalamocortical slice recordings showed excessive excitability from the EAAC1 antisense rats compared with sense-treatedcontrols. Recordings from thalamocortical slices in the studygroup showed prolonged runs of spontaneous bursts of spike discharges(as displayed from the thalamic channel) (Fig. 2a), which, atclose scrutiny, showed 6-7 sec spikes and slow-wave complexes(data not shown). Because of the use of magnesium free medium,these runs were occasionally present in sense control slices butwere much less frequent and very short in duration. Typical controlthalamocortical slices showed occasional brief spontaneous burstingspike discharges (Fig. 2b). Quantitative analysis comparing themean duration of these spike discharges (seconds discharges perminute recording) in the thalamocortical slices of antisense-treatedrats (8.1; n = 13) to slices of sense controls (2.8; n = 10) showedsignificant hyperexcitability of the study group (p = 0.013) (Fig.2c).

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Figure 2. Thalamocortical and HEC slices of EAAC1 antisense-treated rats are hyperexcitable. a, b, Thalamocortical slice field potential recordings showing a 10 sec run of spontaneous bursting rhythmic spike discharges (a; + +) in antisense-treated tissue but not in the controls (b) in which occasional spontaneous spike discharges were seen (b; +) (a and b are recorded at 5 mm/sec paper speed). c, The mean duration of spike discharges (seconds per minute) in the antisense-treated thalamocortical slices was significantly increased compared with control (*p < 0.05). d, e, HEC slice field potential recordings showing the occurrence of very frequent SISs in the antisense-treated rat slice (d; + +) and much less frequent SISs (e; +) in the sense-treated rat slice (d and e are recorded at 1 mm/sec). f, Mean number of spikes per minute in the HEC slices of antisense-treated rats was increased.

Extracellular HEC slice recording

Extracellular hippocampal slice recordings showed increased excitability from EAAC1 antisense rats compared with sense controls.The typical recording of HEC slices in the EAAC1 antisense groupshowed very frequent SISs (Fig. 2d), whereas in recordings ofEAAC1 sense-treated rats, such spikes were found much less frequently(Fig. 2e). The mean number of spikes per minute in all of theHEC slices recorded in antisense-treated rats (14.6; n = 5) wasincreased compared with sense-treated controls (1.66; n = 3),but the difference was not statistically significant (p = 0.16)(Fig. 2f). There was a strong correlation between the mean numberof spikes per minute in hippocampal slices and the mean numberof spikes per minute on EEG (r = 0.97; p < 0.0001; data notshown).

Whole-cell visualized slice patch recording

The limbic hyperexcitability observed in extracellular recording in HEC slices from EAAC1 antisense-treated animals (see above)suggests that the reduction of functional levels of EAAC1 transporterprotein may promote seizure generation by a decrease of releasableGABA. To test this hypothesis directly, mIPSCs, which are mediatedby the spontaneous release of single GABA quanta, in hippocampalarea CA1 in EAAC1 antisense-treated, EAAC1 sense-treated, GLASTantisense-treated, and naive animals, were recorded. GLT-1 antisenseoligonucleotide-treated animals were not used in this analysisbecause the hippocampus was severely damaged by this treatment(Rothstein et al., 1996). The median mIPSC amplitude recordedin CA1 pyramidal neurons from EAAC1 antisense oligonucleotide-treatedanimals (n = 10; number of events was 2486) was significantlysmaller ( $-$ 29.8 ± 3 pA; p < 0.05; unpaired t test) than that recordedin EAAC1 sense oligonucleotide-treated ( $-$ 39.4 ± 2 pA; n = 5; numberof events was 1023), GLAST antisense oligonucleotide-treated ( $-$ 38.5± 2 pA; n = 6; number of events was 1140), and naive ( $-$ 37.1 ±1; n = 3; number of events was 879) controls (Fig. 3a1-a3,b1,c1).The 90% decay time (t90) was significantly faster in the EAAC1antisense-treated group compared with both GLAST antisense andEAAC1 sense groups (Fig. 3b2,c2). However, caution should be usedin interpretation of this result because the 50% decay times (t50)were not significant between the three groups (t50 of 8.97 ± 2,10.13 ± 2, 10.5 ± 1 for EAAC1 antisense-, EAAC1 sense-, and GLASTantisense-treated, respectively). The current measured correspondingto the t90 decay time is very close to our limit of detection.Because of our lack of confidence in the t90 decay time measurement,we calculated the weighted decay $tau$ values for EAAC1 antisense-,sense-, and GLAST antisense-treated groups. The weighted decay $tau$ values were calculated by dividing the area of the events bytheir peak amplitudes, and the median values were compared. Insimilar manner to the t90 decay time data, we found that the EAAC1antisense-treated group decayed significantly faster (p < 0.05)than both EAAC1 sense- and GLAST antisense-treated groups. Themedian weighted $tau$ values were 12.75 ± 1.9 (n = 10), 15.25 ± 1.0(n = 5), and 16.83 ± 3.1 (n = 6) for EAAC1 antisense-, EAAC1 sense-,and GLAST antisense-treated groups, respectively. mIPSC mean frequencywas similar in all three groups recorded (3.2 ± 2.1 Hz for GLASTantisense, 3.44 ± 1.7 Hz for EAAC1 sense, and 3.8 ± 1.1 Hz forEAAC1 antisense).

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Figure 3. The hyperexcitability of hippocampal slices of EAAC1 antisense-treated rats may be secondary to decreased inhibition in CA1 pyramidal neurons. a, Representative mIPSCs (average of 50) from EAAC1 sense (a1), EAAC1 antisense (a2), and GLAST antisense (a3) CA1 pyramidal neurons. b, Cumulative frequency amplitude (b1) and t90 decay time (b2) histograms for neurons in a. c, Histogram of mean mIPSC amplitudes (c1) and t90 decay times (c2) for the three populations. *p < 0.05 denotes significant differences between EAAC1 antisense-treated and both EAAC1 sense- and GLAST antisense-treated groups. AS, Antisense; S, sense.

Regional brain GABA

Because of the decreased inhibition demonstrated by the voltage-clamp recording studies described above, total GABA was measuredin the hippocampus and thalamus of antisense-treated animals comparedwith sense controls and also in other brain regions close to andfar from the intraventricular oligonucleotide infusion (Rothsteinet al., 1994). HPLC analysis of selected brain regions indicatedthat GABA levels were decreased 50% (p < 0.05) in the hippocampusand mildly decreased (nonsignificantly) in the thalamus of EAAC1antisense but not in controls (sense, n = 4; antisense, n = 7)(Fig. 4a).

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Figure 4. Total GABA is decreased significantly in the hippocampus (Hipp) and nonsignificantly in the thalamus (Thal) of EAAC1 antisense-treated rats, suggesting a role for EAAC1 in GABA synthesis in normal rat hippocampi. a, Histograms of mean total GABA levels in different brain regions (Crblm) comparing antisense-treated rats (gray) to sense controls (black). Antisense EAAC1 treatment leads to a loss of hippocampal GABA significantly (*p < 0.05) and thalamic GABA nonsignificantly. b, THA significantly decreases the [¹⁴C]GABA-specific activity measured in hippocampal tissue of normal rats (*p < 0.05). c, The addition of the glutaminase inhibitor DON with glutamate to hippocampal tissue produces a nonsignificant increase in [¹⁴C]GABA-specific activity. d, Addition of DON and DHK with glutamate to hippocampal tissue produces a significant increase in [¹⁴C]GABA-specific activity (*p < 0.05).

New [¹⁴C]GABA metabolism in normal rats

To determine whether changes in GABA reflect a coupling of EAAC1-mediated glutamate transport and GABA metabolism, new synthesisof GABA in EAAC1 antisense-treated rats was measured using [U-¹⁴C]glutamate in the presence of selective enzyme inhibitors toblock glutamate repletion from astrocytic glutamine and GABA catabolism.New glutamate synthesis from astrocytic glutamine was blockedwith the glutaminase inhibitor DON, and GABA catabolism was preventedby gabaculine, a potent and irreversible inhibitor of GABA transaminase.Application of the GABA transaminase inhibitor permitted the experimentsto be conducted under conditions of net GABA synthesis. To testwhether any potential GABA labeling from [¹⁴C]glutamate was transporter dependent in the control hippocampaltissue and because no specific pharmacological inhibitor of EAAC1currently exists, it was necessary to use the nonspecific glutamatetransport inhibitorTHA.

Newly synthesized [¹⁴C]GABA from [U-¹⁴C]glutamate in hippocampal tissue from normal rats incubated in the presence of DON andgabaculine was significantly lower [specific activity, 2.225 (n= 3) vs 6.072 (n = 6); p = 0.003] in the presence of THA (Fig.4b), suggesting that GABA synthesis is dependent on glutamatetransport. To test the effect of DON alone on GABA synthesis,DON was added to hippocampal tissue acquired from normal ratsat time 0 (without adding glutamate), and this was compared withDON, which was added to other hippocampal tissue from controlrats at time 0 and was followed by addition and incubation withcold and [¹⁴C]glutamate and gabaculine for 30 min. Newly synthesized [¹⁴C]GABA is reflected by the difference in [¹⁴C]GABA-specific activity between the tissue with added glutamatecompared with the tissue with no added glutamate, and there wasa nonsignificant difference [increment from specific activity,0.2733 (n = 6) vs 0.3967 (n = 6); p = 0.19] (Fig. 4c). This differencecould be explained by new GABA synthesis from glutamate takenup into synaptic terminals by EAAC1. Alternatively, the enzymaticinhibition of glutaminase, by DON, may have been incomplete, andthe difference could be explained by astroglial glutamine supply.That is, [¹⁴C]glutamate may have been transported into astrocytes by the astroglialtransporter GLT-1, converted to [¹⁴C]glutamine, and then shuttled to the GABA neuron. However, whenDHK, a specific and potent blocker of GLT-1, in addition to DONwas added to hippocampal tissue from control rats at time 0 (withoutadding glutamate) and this was compared with DHK and DON, whichwere added to other hippocampal tissue from normal rats at time0 and was followed by addition and incubation with cold and [¹⁴C]glutamate and gabaculine for 30 min, there was a significantdifference [increment from specific activity, 0.172 (n = 11) vs0.338 (n = 11); p = 0.01]. Newly synthesized [¹⁴C]GABA is reflected by the difference in [¹⁴C]GABA-specific activity between the tissue with added glutamatecompared with the tissue with no added glutamate, and there wasa significant difference, i.e., increased GABA labeling this time(Fig. 4d).

The opposite result, i.e., decreased GABA labeling, would be expected if GABA was labeled from glutamine synthesized from[¹⁴C]glutamate uptake by astroglia attributable to DHK blockade ofthis uptake. Thus, increased GABA labeling after application ofDHK suggests that inhibition of the astroglial transporter ledto an increase in extracellular glutamate, with more now availablefor transport through EAAC1 and GABA synthesis. This suggeststhat EAAC1 is important for GABA synthesis in normalrats.

New [¹⁴C]GABA metabolism in antisense-treated rats and sense controls

To more fully evaluate the role of EAAC1-mediated transport in GABA metabolism, new GABA synthesis was measured in hippocampalslices prepared from EAAC1 sense- and antisense-treated rats inthe presence of DON and gabaculine. [¹⁴C]GABA-specific activity in hippocampal tissue of antisense-treatedrats was significantly lower (1.65; n = 7) compared with sensecontrols (4.03; n = 6; p = 0.017) (Fig. 5a). The newly formed[¹⁴C]GABA over the 30 min incubation period was increased nonsignificantlyin the antisense-treated tissue [from 1.85 to 2.66 nmol/mg protein(× 10⁵); n = 6 (Fig. 5c)] compared with a significant increase [from1.51 to 5.4 nmol/mg protein (× 10⁵); n = 6; p = 0.02 (Fig. 5b)] in the sense-treated tissue. Furthermore,the rate of [¹⁴C]GABA synthesis was approximately five times slower [0.027 nmol/mgprotein (× 10⁵)/min; n = 6]in the antisense-treated compared with the rate ofsynthesis in the EAAC1 sense-treated [0.13 nmol/mg protein (×10⁵)/min; n = 6 (Fig. 5d)] tissue.

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Figure 5. [¹⁴C]GABA-specific activity and synthesis rate are reduced in EAAC1 antisense-treated rats. a, [¹⁴C]GABA-specific activity after incubation of hippocampal tissue with [¹⁴C]glutamate is significantly decreased in EAAC1 antisense-treated rats (*p < 0.05). b, [¹⁴C]GABA is significantly increased with addition of [¹⁴C]glutamate in EAAC1 sense-treated animals (*p < 0.05). c, [¹⁴C]GABA is not increased significantly with added [¹⁴C]-labeled glutamate in EAAC1 antisense-treated animals. d, The rate of [¹⁴C]GABA synthesis with added [¹⁴C]glutamate is five times faster in tissue of EAAC1 sense-treated rats compared with tissue of EAAC1 antisense-treated rats.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Together, these in vivo and in vitro studies demonstrate that EAAC1 antisense-treated rats develop epilepsy and limbic hyperexcitabilityand that this hyperexcitability may be attributable, in part,to a reduction in new GABA synthesis in the hippocampus. Thesestudies also suggest that glutamate transporters in general, andEAAC1 specifically, have a role in synthesis and release of newneurotransmitter GABA in the hippocampus of normal naiverats.

The EEG and behavioral monitoring have shown that EAAC1 antisense-treated rats develop behavioral changes manifested as staring-freezingepisodes, which occur simultaneously with EEG epileptiform changes.These changes are specific and maximal at the time of maximalEAAC1 knockdown. The phenotype of the rats in this study differsfrom the EAAC1-deficient mice reported by Peghini et al. (1997).EAAC1 null mice have a deficit of the transporter protein duringontological development allowing for compensatory responses, whereasantisense knockdown results in the loss of this transporter duringadulthood. Noteworthy in EAAC1 null mice was the decrease in locomotoractivity with episodes of locomotor arrest (Peghini et al., 1997);however, simultaneous EEG recording to rule out seizures werenot reported in their study. In the present study, extracellularfield potential recordings from both thalamocortical and hippocampalslices of antisense-treated rats showed hyperexcitability. Thehippocampal hyperexcitability was correlated with the EEG hyperexcitability.Based on this finding and because of the large decrease in GABAsynthesis, whole-cell patch-clamp recordings of CA1 pyramidalneurons were performed. The data suggest that EAAC1 antisense-inducedhyperexcitability may be attributed to a decrease in mIPSC amplitude,but not mIPSC frequency, in CA1 pyramidalneurons.

A balance of excitation and inhibition is essential for the maintenance of normal function in the brain. Golan et al. (1996)showed that GABA concentration determines the efficacy of inhibition.In the present study, a decrease in total GABA was observed inthe hippocampus of antisense-treated rats but not in sense controls.This decrease was not significant in other regions, although itwas present in the thalamus also. Inhibiting GABA synthesis causesseizures, and some of the effects of anticonvulsants occur throughinterference with enzymes associated with GABA metabolism (Petroffet al., 1996a,b).

High-affinity glutamate transporter subtypes have been found to be specifically localized to both neuronal and astroglialmembranes. Under normal conditions, these proteins maintain lowextracellular levels of glutamate. A series of studies suggestthat the astroglial transporters, GLT-1 in particular, are primarilyresponsible for the synaptic inactivation of glutamate and forpreventing excitotoxic injury (Bergles and Jahr, 1997; Otis andJahr, 1998; Otis and Kavanaugh, 2000). Nevertheless, EAAC1 isthe predominant neuronal transporter present widely throughoutthe CNS dendrites and somata of large and small pyramidal neurons.However, its function in normal synaptic biology has eluded investigators.Molecular anatomic studies suggested that this protein was unexpectedlylocalized to presynaptic GABA terminals (Rothstein et al., 1994;Conti et al., 1998; He et al., 2000). Subsequently, preliminaryantisense knockdown studies suggested a relationship between thisprotein and tissue GABA levels (Rothstein et al., 1996).

GABA is synthesized primarily from the $alpha$ -decarboxylation of glutamate by glutamate decarboxylase (Martin and Rimvall, 1993).An alternate pathway for GABA synthesis via putrescine has beendescribed previously (Seiler and Al-Therib, 1974). Although thecontribution of this pathway to GABA synthesis appears to be smallin the mature rat brain [~1% of total GABA synthesis (Noto etal., 1986)], putrescine has been shown to be a GABA precursorin the developmentally immature retina (Yamasaki et al., 1999).GABA carbon, which is lost from GABAergic neurons, must be replenishedfrom other cells because mature neurons do not possess the necessaryenzymes for de novo synthesis. Glutamine produced in astrocytesis a major precursor of GABA, although few quantitative studiesof the precursors of GABA in vivo have been reported. Neostriatalmicroinjections of methionine sulfoximine, an inhibitor of glutaminesynthetase, resulted in only a ~50% reduction of GABA synthesis(Paulsen et al., 1988), suggesting that a pathway(s) other thanglutamine may also supply glutamate precursors for GABA synthesisin this brain region. The large decrease in GABA levels and GABAsynthesis from extracellular [¹⁴C]glutamate in the hippocampus after knockdown of EAAC1 indicatethat direct transport of glutamate into GABAergic neurons canprovide precursors for GABA synthesis. Furthermore, the electrophysiologicstudies suggest that the loss of EAAC1 leads to decreased mIPSCs,consistent with decreased presynaptic release ofGABA.

Together, these metabolic and electrophysiologic studies clearly document a relationship between the presynaptic glutamatetransporter and the inhibitory transmitter GABA. In turn, thesemetabolic studies strongly suggest that the mechanism of epilepsyin the EAAC1 antisense knockdown rats is mediated by decreasedGABA synthesis and, therefore, decreased CNS inhibition. The datasuggest that, in normal rat brain, EAAC1 may have an importantrole in regulating GABA synthesis and release synthesis. Recently,GTRAP3-18 (for glutamate transporter-associated protein 3-18),an EAAC1 inhibitory modulator, was described (Lin et al., 2001),suggesting that, under normal conditions, EAAC1 may be modulated,perhaps to regulate presynaptic GABA synthesis. Preliminary studiesalso show that increased GTRAP3-18, through inhibition of EAAC1(like antisense), produces epilepsy (Sepkuty et al., 2001). Overall,these studies suggest a novel interaction between excitatory aminoacid transporters and an inhibitory amino acid neurotransmittersystem. Furthermore, they raise new possibilities of manipulatingGABA metabolism through direct or indirect modulation of EAAC1(e.g., GTRAP3-18) and may provide novel therapeutic modalitiesfor the treatment ofepilepsy.

  FOOTNOTES

Received Dec. 27, 2001; revised May 13, 2002; accepted May 13, 2002.

This work was supported by National Institutes of Health Grants NS 40151, NS36465, and NS33958 (J.D.R.) and NS 32403 and NS38572 (D.A.C.).

Correspondence should be addressed to Jeffrey D. Rothstein, Johns Hopkins University, Department of Neurology, Meyer 6-109,600 North Wolfe Street, Baltimore, MD 21287-7247. E-mail: jrothste{at}jhmi.edu.

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