Block of Glutamate-Glutamine Cycle Between Astrocytes and Neurons Inhibits Epileptiform Activity in Hippocampus

doi:10.1152/jn.00665.2001

Block of Glutamate-Glutamine Cycle Between Astrocytes and Neurons Inhibits Epileptiform Activity in Hippocampus

Alberto Bacci,¹^,^* Giulio Sancini,²^,^* Claudia Verderio,¹ Simona Armano,¹ Elena Pravettoni,¹ Riccardo Fesce,³ Silvana Franceschetti,² and Michela Matteoli¹

¹Consiglio Nazionale delle Ricerche Institute of Neuroscience, Cellular and Molecular Pharmacology, Department of Medical Pharmacology, 20129 Milano; ²Istituto Neurologico C. Besta, 20100 Milano; and ³Università Degli Studi Dell'insubria, 21100 Varese, Italy

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Bacci, Alberto, Giulio Sancini, Claudia Verderio, Simona Armano, Elena Pravettoni, Riccardo Fesce, Silvana Franceschetti, and Michela Matteoli. Block of Glutamate-Glutamine Cycle Between Astrocytes and Neurons Inhibits Epileptiform Activity in Hippocampus. J. Neurophysiol. 88: 2302-2310, 2002. Recurrent epileptiform activity occurs spontaneously in cultured CNS neurons and in brain slices in which GABA inhibitionhas been blocked. We demonstrate here that pharmacological treatmentsresulting in either the block of glutamine production by astrocytesor the inhibition of glutamine uptake by neurons suppress or markedlydecrease the frequency of spontaneous epileptiform dischargesboth in primary hippocampal cultures and in disinhibited hippocampalslices. These data point to an important role for the neuron-astrocytemetabolic interaction in sustaining episodes of intense rhythmicactivity in the CNS, and thereby reveal a new potential targetfor antiepileptictreatments.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Enhanced activity of excitatory synapses, produced by an imbalance of excitation and inhibition, has been considered as apossible mechanism for sustained epileptic hyperexcitability.In particular, evidence from experimental models of epilepsy andfrom patients indicates that glutamate and aspartate play an importantrole in the initiation, spread, and maintenance of epileptic dischargesand that compounds that modify glutamate release alter seizureexpression (Chapman 1998; Lee and Hablitz 1989; Loscher 1998;Malouf et al. 1990; McBain et al. 1988; Meldrum 1994). Whereasconsiderable attention has been focused on the involvement ofglutamatergic neurotransmission in epilepsy, little is known aboutthe mechanisms sustaining the spontaneous synaptic activitiesallowing recurrent seizures. In this scenario, one may expectthat neurons, during epileptiform activity, require a strong metabolicsupport, in the form of precursors and proper energy substrates,to fill the rapid-turnover neurotransmitter pool and to continuouslyadjust the ionic gradients which tend to be altered by the increasedneuronalactivity.

In the CNS, neurons are metabolically coupled to astrocytes and the key-site of this neuron-glia interaction is the synapse(Bacci et al. 1999a; Haydon 2001; Pfrieger and Barres 1996; Tsacopoulosand Magistretti 1996), which is the most specialized structureresponsible for transmitting and processing information betweenneurons. Among other functions, astrocytes are responsible forremoving potassium ions (Cooper 1995) and glutamate (Bergles etal. 1999) accumulating in the synaptic microenvironment duringsynaptic activity. Glial cells also provide the presynaptic terminalwith the glutamate precursor glutamine and with lactate, whichis used by neuronal cells as a preferential energy substrate (forreviews see Bacci et al. 1999a; Deitmer 2001; Patel et al. 1982;Pfrieger and Barres 1996; Rothman et al. 1999; Tsacopoulos andMagistretti 1996). One might therefore hypothesize that astrocytesplay a role in supporting an efficient neuronal functionality,via these multiple processes, during prolonged synaptic activity.In agreement with this possibility, it has been previously demonstratedthat the glial-specific metabolic blocker fluoroacetate, whichselectively inhibits glial cell function, decreases spontaneousand evoked synaptic transmission (Keyser and Pellmar 1994).

In a previous study, we reported that synchronous epileptiform activity in hippocampal cultures is dependent on the presenceof adjacent glial cells (Verderio et al. 1999). Here we show thatthe maintenance of epileptiform activity in cultured hippocampalneurons and in hippocampal slices in which GABA-inhibition hasbeen blocked crucially depends on the delivery of glutamine fromastrocytes to neurons. These results reveal a novel function ofglial cells in supporting the long term feeding of neuronal cellsduring enhanced neuronalactivity.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Hippocampal cell culture

Primary neuronal cultures were prepared from the hippocampi of 18-day-old fetal rats as previously described (Bartlett andBanker 1984; Verderio et al. 1999). In some experiments, to warrantthe strict proximity with glial cells, neurons were plated oncoverslips already containing monolayers of hippocampal astrocytes,prepared as described (Calegari et al. 1999).

Fura-2 videomicroscopy and patch-clamp recordings from hippocampal neurons in culture

Cultures were loaded for 40 min at 37°C with 2-4 mM Fura-2 pentacetoxy-methylester in Krebs-Ringer solution buffered withHEPES (KRH) with the following composition (in mM): 150 NaCl,5 KCl, 1.2 MgSO₄, 2 CaCl₂, 10 glucose, and 10 HEPES/NaOH; pH 7.4)and transferred to the recording chamber of an inverted microscope(Axiovert 100; Zeiss) equipped with a calcium imaging unit. Amodified CAM-230 dual wavelength microfluorimeter (Jasco, Tokyo,Japan) was used as a light source for the assays. The experimentswere performed at room temperature (24-25°C) using an Axon ImagingWorkbench 2.2 equipped with a PCO Super VGA SensiCam (Axon Instruments).Conventional whole cell patch clamping was employed using an Axopatch200B amplifier (Axon Instruments) controlled by a PC computer.During acquisition and data analysis, pClamp (Axon Instruments)and Origin (Microcal) software was routinely used. The patch pipette(3-5 MOhm resistance) contained the following (in mM): 140 potassiumgluconate, 2 MgCl₂, 10 HEPES, 1 EGTA, and 4 MgATP. Miniature EPSCs(mEPSCs) were recorded in 1 µM tetrodotoxin (TTX) and 100 µM APV.All the data are reported as mean ± SE. Error bars represent SE.Statistical comparisons were done by using Student's t-test. Differenceswere considered significant if P < 0.05.

Extracellular field potential recordings from hippocampal slices

Wistar rats (adult, both sexes) were deeply anesthetized by ether inhalation and decapitated. The brain was removed and placedin ice-cold artificial cerebrospinal fluid (ACSF) of the followingcomposition (in mM): 126 NaCl, 3.5 KCl, 2 CaCl₂, 2 MgSO₄, 1.2NaH₂PO₄, 26 NaHCO₃, and 10 glucose (pH 7.3-7.4) and was bubbledwith 95% O₂-5% CO₂. Transverse hippocampal slices 400- to 450-µmthick were cut from dorsal hippocampus using a vibratome, transferredto an interface chamber, and perfused with ACSF. The temperaturewas maintained at 35°C, and the slices were allowed to equilibratefor 1-1.5 h before the electrophysiological recordings were started.Bicuculline methiodide (5-10 µM), picrotoxin (25-50 µM), methioninesulfoximine (MSO; 1-3 mM), glutamine (0.1-0.2 mM), CNQX (10 µM,dissolved in 0.1% DMSO), and $alpha$ -(methylamino) isobutiric acid (MeAIB;12.5 mM) were freshly added to standard ACSF. Moreover, in someexperiments, MeAIB 12.5 mM was equimolar substituted to NaCl.Glucose 12.5 mM was added to ACSF in control experiments aimedat excluding a putative osmotic effect of MeAIB on spontaneousepileptic discharge (SED)frequency.

Spontaneous field potentials were recorded from CA1 region (pyramidal layer and/or stratum radiatum). Series of field responseswere evoked by low frequency (0.2 Hz) electrical stimulation ofthe Schaffer collaterals. Signals were continuously monitoredby means of chart recording, stored on a magnetic tape, and digitizedoff-line on a PC (sampling frequency of 2-4 kHz). The frequencyof SEDs was calculated as the reciprocal of the mean inter-SEDinterval from recordings samples of 16 min. The slope of the descendingportion of the population EPSP was extracted by a computer homemade program using linear regression. Paired t-test or Wilcoxontest were used for statisticalanalysis.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Epileptiform activity in cultured hippocampal neurons relies on metabolically intact astrocytes

Cultured hippocampal neurons (12-20 days old) were loaded with the calcium indicator Fura-2 and recorded in physiologicalmedium (KRH) by means of calcium imaging and whole cell current-clamptechniques. We have previously demonstrated that neurons undergospontaneous [Ca²⁺]_i oscillations coupled to long-lasting bursts of action potentials(Fig. 1A; Bacci et al. 1999b; Verderio et al. 1999). This spontaneoushyperexcitability, which resembles epileptiform activity producedin vitro by various experimental manipulations (De Lorenzo etal. 1998; Furshpan and Potter 1989; Segal 1994; Segal and Furshpan1990; Verderio et al. 1999), has been found to rely on glutamatergicneurotransmission (Bacci et al. 1999b). Furthermore, epileptiformactivity selectively occurred in those neurons that were growingwith adjacent glial cells (Verderio et al. 1999).

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Fig. 1. Fluoroacetate blocks neuronal epileptiform activity in cultured neurons. A: simultaneous current-clamp and calcium-imaging recordings from the same neuron. Long bursts of action potentials, resembling epileptiform activity, coincide with calcium transients. B and C: the gliotoxic drug fluoroacetate (FAc; 200 µM) gradually reduces the frequency of [Ca²⁺]_i oscillations. B: plot of oscillation frequency in control and in FAc-treated neurons calculated in 10-min intervals and normalized to control (10 min before FAc application). C: temporal analysis of [Ca²⁺]_i oscillations measured from a neuron in a fura-2-loaded culture. FAc reduces oscillations with a latency to onset approximately 10 min following addition (arrow), up to a complete block of the activity after approximately 40 min. The 2 traces are continuous in time. Application of 30 µM glutamate at the end of the experiment, induces a calcium response in the FAc-treated neuron. D: calcium responses elicited by 30 µM glutamate application before and after 30 min of FAc application in the same neuron. E: histogram quantifying the responses to glutamate before and after FAc application. F: current-clamp recordings from a neuron in control solution (top), from a neuron exposed for 1 h to 200 µM FAc (middle), and from a neuron exposed for 1 h to 200 µM FAc in the simultaneous presence of 100 µM glutamine (bottom). In FAc-treated cultures, spontaneous postsynaptic potentials are still present. Glutamine prevents the FAc-induced inhibition of the oscillatory activity. G: plot showing the percentage of oscillating cells in control conditions, after FAc intoxication and after FAc plus glutamine treatment.

To define whether astrocytes actively contribute to the neuronal epileptiform activity, the selective gliotoxic drug fluoroacetate(FAc 200 µM) (Clarke et al. 1970; Hassel et al. 1992; Hulsmannet al. 2000; Keyser and Pellmar 1994; Muir et al. 1986; Paulsenet al. 1987; Waniewski and Martin 1998) was applied to oscillatingcultures. FAc gradually depressed the oscillatory activity witha latency to onset of approximately 10 min following addition(Fig. 1C, arrow), up to complete block of [Ca²⁺]_i fluctuations in about 40-50 min (Fig. 1, B and C, n = 32).Several pieces of evidence indicate that the effects of FAc werenot due to changes in neuronal intrinsic responsiveness and excitability.FAc-treated neurons did not display any change in basal calciumlevels (Fig. 1, C and D), in resting potentials (control: $-$ 73± 0.58 mV, n = 8; FAc-treated: $-$ 71.45 ± 1.21 mV, n = 6; P = 0.3)or in the threshold for the action potential initiation (control: $-$ 40.5 ± 0.5 mV, n = 8; FAc-treated: $-$ 38.18 ± 1.31 mV, n = 6; P= 0.26). Furthermore, FAc-treated neurons were able to respondto the application of exogenous glutamate (30 µM) without significativerundown of [Ca²⁺]_i response (amplitude of the calcium response after FAc treatmentwas 99.75 ± 1.81% with respect to controls (mean ± SE, n = 8,P < 0.05) (Fig. 1, D and E). In addition, 30-45 min after incubationwith FAc, neurons were still able to fire action potentials eitherspontaneously or in response to a depolarizing stimulus (datanot shown, n = 9) and to generate transient changes in [Ca²⁺]_i when exposed to a Mg ²⁺-free medium, a treatment which facilitates N-methyl-D-aspartate(NMDA)-receptor activation by endogenous glutamate (data not shown;Abele et al. 1990; Verderio et al. 1995).

It is known that FAc inhibits the production of glutamine from glucose in glial cells (Hassel et al. 1992, 1997; Paulsen etal. 1987; Swanson and Graham 1994). We therefore tested whetherthe depletion of the astrocytic glutamine pool might be responsiblefor the inhibition of epileptiform activity in neurons. After1 h of FAc treatment, the percentage of oscillating cells decreaseddramatically (Fig. 1, F and G, from 85 ± 6.3% in control, n =12, to 18 ± 1.3% in FAc-treated cultures, n = 11, P < 0.05). However,when FAc intoxication was carried out in the presence of 100 µMglutamine, the FAc-mediated impairment of epileptiform dischargeswas prevented (oscillating cells: 75 ± 6.1%, n = 12; Fig. 1, Fand G). These data suggest that the astrocytic pool of glutaminemay be relevant in maintaining the oscillatory behavior (see alsoHulsmann et al. 2000).

Block of glutamine production in astrocytes inhibits recurrent epileptiform activity

A relevant source of glutamine in astrocytes derives from synaptically released glutamate, which is taken up by glial transportersand converted into glutamine by the enzyme glutamine synthetase.Glutamine is in turn delivered to neurons, which use it as a precursorfor the synthesis of glutamate (Bacci et al. 1999a; Pfrieger andBarres 1996; Rothman et al. 1999; Fig. 6). To directly test thefunctional significance of the astrocyte-dependent glutamate-glutaminepathway, cultures were exposed to 100 µM methionine sulfoximine(MSO), a selective inhibitor of the enzyme glutamine synthetase,which is specifically expressed by glial cells (Martinez-Hernandezet al. 1977). This experimental treatment has been previouslyfound to result in a block of glutamine production in astrocytes(Derouiche and Rauen 1995; Laake et al. 1995; Ronzio et al. 1969).One hour of treatment with MSO was sufficient to produce eithera complete block of epileptiform activity, leaving basal synapticactivity only (Fig. 2A), or a relevant reduction of the burstfrequency (80.7 ± 4.2% reduction; Fig. 2B; n = 10). The MSO-inducedblock of oscillations was always prevented by the simultaneousexposure of the neuronal cultures to 100 µM glutamine (Fig. 2A;n = 7). Likewise, fluctuations of both membrane potential (Fig.2B; n = 3) and [Ca²⁺]_i (Fig. 2C; n = 11) in MSO-treated cells were partially rescuedby the acute application of 100 µM glutamine. MSO-treated neuronsdid not display any change in resting potential and input resistance(data not shown). Furthermore, MSO application did not changethe receptor responsivity to the application of exogenous glutamate(data not shown).

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Fig. 2. Block of glutamate-to-glutamine conversion in astrocytes reduces epileptiform activity in culture. A: current-clamp recordings before and after 1 h treatment with the astrocyte glutamine synthetase inhibitor methionine sulfoximine (MSO; 100 µM). Note that MSO completely abolishes oscillations without affecting the basal spontaneous excitatory postsynaptic potentials. Simultaneous application of MSO and 100 µM glutamine completely prevents the MSO-induced inhibition of the oscillatory activity. B and C: bursting activity (B) and calcium transients (C) are strongly reduced after MSO treatment and partially rescued by the acute application of 100 µM glutamine.

To investigate whether the block of glutamine synthetase may play a direct role in glutamate release, mEPSCs were recorded,on MSO treatment, from hippocampal neurons growing in cultureon top of astrocytes. A significant reduction of mEPSC frequencywas recorded on MSO treatment (mEPSC frequency recorded 20-30min after MSO application: 47.8 ± 11.8% compared with controls;0-7 min of recording; n = 4; P < 0.05). No significant effectwas produced by MSO, when applied in the concomitant presenceof 100 µM glutamine. In the absence of glial cells, the frequencyof mEPSC recorded 20-30 min after MSO application was 86.58 ±5.05% compared with controls (0-7 min of recording; n = 4; P >0.05) thus indicating that MSO affects miniature activity throughan effect on glialcells.

Spontaneous epileptiform discharges induced in hippocampal slices by GABA-antagonists are reduced by block of glutamine synthesis in astrocytes

We then tested whether the glutamate-glutamine shuttle between neurons and glial cells is able to sustain the long-term maintenanceof recurrent spontaneous epileptiform discharges (SEDs) in hippocampalslices, following induction of long-lasting hyperexcitability.The perfusion with 5-10 µM bicuculline methiodide or 25-50 µMpicrotoxin added to ACSF consistently resulted in hyperexcitabilityphenomena, which occurred spontaneously. SED frequency reacheda steady-state condition after about 30 min from the onset ofGABA-antagonistperfusion.

The effect of MSO on SED frequency was tested about 60 min following the perfusion of GABA_A-receptor blockers to allow epileptiformdischarges to reach a steady-state frequency. After 30 min ofMSO (2 mM) perfusion, a decline in SED frequency could be observed(Fig. 3, A and B; 41.4 ± 0.1% of reduction; P < 0.01; n = 9),and this decay became more evident during the following 60-90min of MSO perfusion (Fig. 3C; 66.1 ± 4.7% of reduction, P < 0.005,n = 9). The addition of 100-200 µM glutamine invariably recoveredthe frequency of SEDs to values close to those observed beforeMSO perfusion (82.7 ± 10.6%).

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Fig. 3. Block of glutamate-to-glutamine conversion in astrocytes inhibits spontaneous epileptiform discharges in GABA antagonist-treated hippocampal slices. A: continuous field recording obtained from CA1 regions of a representative hippocampal slice in the presence of bicuculline (control) and after 45 or 70 min of 2 mM MSO perfusion. The frequency of spontaneous discharges (SEDs) recovers in the presence of 100 µM glutamine. Representative SEDs (corresponding to the boxed segment of the traces) are displayed at higher speed. B: time course of SEDs throughout the entire experiment. Each data point represents the number of discharges over a sample of 200 s. C: average SED frequency assesses on a 16-min epoch under control conditions (bicuculline), and during MSO and MSO plus glutamine perfusion (n = 9). D: SED frequency does not recover during MSO washout and recovers in the presence of glutamine. E: SED frequency returns to the lowest values found during MSO perfusion in case of glutamine washout. F: in the absence of MSO pretreatment, glutamine does not increase SED frequency.

In some experiments, MSO-resistant SEDs slightly increased in duration, showing a greater number of population spikes (Fig.3A). In the presence of GABA blockers (bicuculline or picrotoxin)the number of population spikes was 4.9 ± 0.8, and remained substantiallyunchanged during the first 30-60 min of MSO perfusion (4.3 ± 0.8),whereas it increased to an average value of 7.9 ± 1.0 during thefollowing 30-60 min (n = 9). This phenomenon was however inconsistentand the difference did not reach a statisticalsignificance.

The action of MSO was irreversible: the recovery of SED frequency to values close to those observed before MSO perfusion didnot occur in case of MSO washout and was found to directly dependon the presence of glutamine in the perfusing medium (Fig. 3D).Glutamine perfusion recovered SED frequency to 50% of controlvalue in 15.9 ± 1.6 min, reaching a steady state frequency after33.9 ± 1.6 min. A subsequent glutamine washout produced againa decrease of epileptiform discharge frequency (Fig. 3E; n = 4).SED frequency was not affected when glutamine was added to thedisinhibited slices not previously treated with MSO (Fig. 3F;n = 3). CNQX quickly abolished SED recurrence (data notshown).

Epileptiform activity in culture and in brain slices is inhibited by impairment of glutamine uptake in neurons

The major carriers for glutamine uptake within the brain are represented by systems A, L, and ASC. System A, a sodium-dependent,unidirectional transporter that exhibits reduced activity at lowpH, primarily mediates glutamine uptake in neurons. As systemA family of transporters, which includes the recently cloned GlnT/SAT1(Varoqui et al. 2000), represents a crucial link in the glutamate-glutaminecycle, playing a role as a possible gateway for the synthesisof glutamate in neuronal cells, we have investigated whether animpairment of its function could affect epileptiform activityin hippocampal neurons. A characteristic feature of system A,which differentiates it from systems L and ASC, is the abilityto transport N-methylated substrates such as the non metabolizableamino acid analog $alpha$ -(methylamino)isobutiric acid (MeAIB), whichcompetes with glutamine for uptake. MeAIB, used at concentrationspreviously shown to inhibit glutamine uptake (10-50 mM) (Varoquiet al. 2000), reduced or completely blocked the occurrence ofspontaneous oscillatory activity in fura-2-loaded cultures ofhippocampal neurons, in a reversible manner (Fig. 4A). MeAIB-treatedneurons did not display any change in resting potential or inputresistance (data not shown). Furthermore, MeAIB did not affectglutamate receptor responsivity (amplitude of the calcium responseto 10 µM glutamate after MeAIB treatment: 97.2 ± 4.8% with respectto controls; n = 6; P > 0.05; Fig. 4, B and C).

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Fig. 4. Inhibition of glutamine uptake by neurons inhibits spontaneous epileptiform discharges in culture. A: application of $alpha$ -(methylamino) isobutiric acid (MeAIB) at 2 different concentrations blocks (50 mM) or strongly reduces (25 mM) the frequency of [Ca²⁺]_i oscillations in fura-2-loaded hippocampal neurons. B: calcium responses elicited by 10 µM glutamate application before and after MeAIB treatment in the same neuron. C: histogram quantifying the responses to glutamate before and after MeAIB application.

We then tested the effect of MeAIB on epileptiform discharges in disinhibited hippocampal slices. MeAIB (12.5 mM) reducedSED frequency in few minutes (Fig. 5, A and B), reaching a frequencyof 43.1 ± 7.0% of the control value (n = 8; P < 0.01). MeAIB effectwas completely reversible on wash (87.2 ± 2.2% of the control;Fig. 5C). The decrease of SED frequency was found to be more prominentwhen the experiments were performed by adding MeAIB to ACSF (n= 4, 33.0 ± 4.6% of the control frequency) compared with the experimentsin which MeAIB was equimolarly substituted to NaCl (n = 4, 59.1± 6.4%). To exclude any possible osmotic effect on epileptiformdischarge frequency, we performed similar experiments applying12.5 mM glucose instead of MeAIB. Glucose, which is transportedthrough cell membranes with similar kinetics as MeAIB (Chaudhryet al. 2002; Maher et al. 1996), was found to be ineffective onSED frequency (n = 3, 95.0 ± 5.5% of the control values). As theneuronal glutamine transporter is Na⁺-dependent (Varoqui et al. 2000), these data suggest that thedifference in MeAIB potency may be accounted for by extracellularNa⁺ concentration. To asses the effect of MeAIB on excitatory neurotransmission,we tested the substance on the glutamate-mediated population EPSPs(Collingridge et al. 1983) evoked in slices perfused with standardACSF (n = 4). As shown in Fig. 5D, the peak amplitude of populationEPSPs recorded in stratum radiatum was reversibly depressed inthe presence of MeAIB. The peak amplitude and the slope of populationEPSP were respectively reduced by 27.8 ± 4.0% and 31.8 ± 6.9%with respect to the control values (P < 0.05).

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Fig. 5. Inhibition of glutamine uptake by neurons inhibits spontaneous epileptiform discharges in brain slices. A: continuous field recording obtained from hippocampal CA1 region in the presence of 25 µM of picrotoxin (control), during MeAIB (12.5 mM) perfusion, and after MeAIB washout. Representative SEDs (corresponding to the boxed segment of the traces) are displayed at higher speed. B: time course of SEDs throughout the entire experiment. Each data point represents the number of discharges over a sample of 200 s. MeAIB perfusion (12.5 mM) quickly reduces SED frequency that does not changed during perfusion with glucose (12.5 mM) added to ACSF. C: histogram quantifying SED frequency under control condition (25 µM picrotoxin), during MeAIB (12.5 mM) perfusion, and washout (n = 8, P < 0.05). D: MeAIB reversibly reduces the amplitude of population EPSP (n = 4, P < 0.05).

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

The occurrence of spontaneous synchronous discharges is one of the hallmarks of epileptiform activity. A potentially usefulapproach to study the mechanisms underlying the seizure-like activityis represented by hippocampal neurons in primary culture, dueto their relatively simplified circuitry. In this experimentalmodel, long bursts of action potentials, coincident with calciumoscillations, commonly occur either spontaneously (Bacci et al.1999b; Verderio et al. 1999) or on removal of magnesium ions fromthe external medium (Abele et al. 1990). This activity, whichhas been considered as an "in vitro" model of epilepsy (De Lorenzoet al. 1998; Furshpan and Potter 1989; Segal 1994; Segal and Furshpan1990), relies on glutamatergic neurotransmission (Abele et al.1990; Bacci et al. 1999b; Lawrie et al. 1993; Murphy et al. 1992;Nunez et al. 1996) and requires the removal of glutamate fromthe synaptic environment by adjacent astrocytes (Verderio et al.1999). Once taken up by glial transporters, glutamate is convertedby the enzyme glutamine synthetase into glutamine, which is thensent back to neurons. Glutamine is thought to efflux from astrocytesvia specific carriers belonging to the System N family, whoseexpression is restricted to astrocytes (Chaudhry et al. 1999)and to be accumulated by neurons via specific carriers belongingto the MeAIB-sensitive System A family of neutral amino acid transporters(reviewed in Bode 2001). Glutamine is then used as the major precursorfor the synthesis of glutamate (Bacci et al. 1999a; Pfrieger andBarres 1996; Rothman et al. 1999; Tsacopoulos and Magistretti1996; Fig. 6). Therefore by removing glutamate from the synapticcleft, astrocytes might also replenish the neuronal pool of neurotransmitter(Laake et al. 1995). In this study, we demonstrate that the functionalintegrity of the glutamate-glutamine cycle is indeed requiredfor supporting epileptiform activity in hippocampus.

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Fig. 6. The glutamate-glutamine shuttle between glia and neurons. Simplified scheme illustrating the glutamate-glutamine cycle between glia and neurons. The cartoon also shows the targets of the drugs used in this study. FAc blocks the enzyme aconitase in the astrocyte tricarboxylic acid (TCA) cycle and indirectly promotes the entering of glutamine in the TCA cycle. MSO inhibits the enzyme glutamine synthetase, therefore reducing glutamate conversion to glutamine. MeAIB inhibits the glutamine uptake by neurons.

As a first step, we used the gliotoxic drug FAc, which is selectively taken up by astrocytes in the CNS (Hassel et al. 1992;Waniewski and Martin 1998) and has specific effects on astrocytemetabolism. FAc has been previously used to demonstrate that glialcells play an integral role in hippocampal synaptic transmission,because FAc treatment of astrocytes was found to reduce both spontaneousand evoked synaptic transmission (Keyser and Pellmar 1994). Afterbeing converted to fluorocitrate, FAc inhibits aconitase in thetricarboxylic acid (TCA) cycle (Clarke et al. 1970; Hassel etal. 1992; Muir et al. 1986; Paulsen et al. 1987; Waniewski andMartin 1998). Intoxicated astrocytes use glutamine as an alternativeenergy source, converting it into 2-ketoglutarate, which entersthe TCA cycle, rescuing in part cell metabolism, and maintainingATP levels near normal in the first hours after intoxication (Hasselet al. 1997; Swanson and Graham 1994; Fig. 6). Our finding thatglutamine rescues the block of oscillations produced by FAc supportedthe hypothesis that the astrocyte-dependent glutamine supply toneurons could in fact be relevant in sustaining epileptiformactivity.

To more specifically address this point, we pharmacologically interfered with the glutamate-glutamine cycle at two differentlevels (Fig. 6), either blocking the glutamine synthetase-mediatedproduction of glutamine in astrocytes or inhibiting the GlnT/SAT1-operatedglutamine uptake by neurons. Although the pharmacological approachmay have some intrinsic limitations, due to the complex mechanismssustaining and regulating recurrent epileptic discharges, thefinding that both treatments resulted in a strong reduction ofthe frequency of SEDs occurring in primary cultures of hippocampalneurons, strongly pointed to a crucial role of the glutamate-glutaminecycle between astrocytes and neurons in supporting the enhancedsynaptic activity. To then investigate whether the supply of glutaminefrom astrocytes might also contribute to maintain epileptic dischargesin brain structures preserving their physiological connectivity,we blocked the glutamate-glutamine cycle in hippocampal slicesperfused with GABA antagonists. Blockade of GABA-dependent synapticinhibition is an extensively applied method to induce "in vitro"epileptiform discharges, which substantially depend on the unbalancedglutamatergic neurotransmission (Dingledine et al. 1986; Lee andHablitz 1989; Traub and Wong 1983). The synchronous occurrenceof SEDs in a large neuronal population give rise to complex fieldpotentials composed by multiple population spikes occurring witha periodic time course (Traub and Wong 1983). Either MSO or MeAIBperfusion were capable of significantly decreasing the frequencyofSEDs.

In the case of MSO, the effect was irreversible, persisted after long-lasting washout, but was regularly reverted by glutamineaddition to the superfusing medium. The slow and progressive effectof MSO on SED frequency, well agrees with a gradual reductionof the available glial glutamine. This is in agreement with recentdata indicating that the recurrent excitatory bursts, which occurin brain stem and sustain the respiratory rhythm, substantiallydepend from glutamine provided by glial cells, are suppressedby either FAc or MSO and recovered in the presence of exogenousglutamine (Hulsmann et al. 2000). MSO is known to exert a convulsantaction "in vivo" (Cloix and Hevor 1998; Sellinger et al. 1968),through a mechanism which is still debated. This property mightaccount for our observation of an increased duration of individualSEDs remaining during late MSO perfusion. This effect, which wefound to occur in a delayed time window with respect to the earlydecline of SED frequency, is better accounted for by a late influenceon cell excitability mediated by a slow impairment of ammoniumor carbohydrate metabolism (Cloix and Hevor 1998; Sellinger etal. 1968) rather than by a direct effect of the drug on glutamatereceptors (Shaw et al. 1999). On the other hand, no late "excitatoryside effect" could be detected during perfusion with MeAIB, acompetitive inhibitor of the system A family of neutral aminoacid transporters, not active on systems L, ASC, and N (Bode etal. 2001; Varoqui et al. 2000). As expected by a pharmacologicaltreatment not involving an enzymatic step, the inhibitory effectof MeAIB on SED frequency was very fast compared with MSO. MeAIBis actively transported through the neuronal membrane (Chaudhryet al. 2002; Su et al. 1997; Varoqui et al. 2000), so that, atleast at the applied concentrations, it is not expected to exertany significant osmotic effect. In agreement, we did not foundany change by applying equimolar concentrations of glucose, whichis transported through the cell membrane with a Michaelis-Mentenkinetics comparable to that of MeAIB (Maher et al. 1996). Thegreater efficiency of MeAIB in decreasing SED frequency when appliedin the presence of physiological concentrations of extracellularNa⁺ well agrees with the Na⁺ dependence of the efficiency of GlnT/SAT1 (Varoqui et al. 2000).

Our data also indicate that impairment of the glutamate-glutamine shuttle between astrocytes and neurons affects mEPSC activityof neuronal cells. Indeed, MSO was found to significantly reducemEPSC frequency in neurons growing on top of glial cells, withouthaving effects in neurons without astrocytes. As a dramatic decreaseof mEPSC frequency occurs in rat hippocampal slices and culturesfollowing treatment with bafilomycin A1, a potent blocker of thevacuolar-type ATPase, which results in a reduced synaptic vesiclefilling (Zhou et al. 2000), our data open the possibility thatthe glutamate-glutamine cycle plays a role in glutamate replenishmentof synaptic vesicles. In further support of this possibility,MeAIB has been recently found to affect mEPSC frequency and amplitude,selectively in neurons growing on top of glial cells (Armano etal. 2002), thus suggesting the possibility that the glutamate-glutamineshuttle between astrocytes and neurons plays a direct role inglutamate replenishment of synapticvesicles.

In conclusion, our data support the view that the neuron-astrocyte coupling, through the restoration of the presynaptic glutamatepool, could mediate a plastic form of bidirectional communication,eventually leading to an enhancement of synaptic transmissionin the long term range. This aspect of the glia-neuron couplingmay have significative physiopathological implications. Glialglutamine could indeed contribute to the persistence of periodicfragmentary EEG and clinical epileptic activities that are knownto characterize several forms of severe symptomatic epilepsy inhumans (Chatrian et al. 1964; Westmoreland et al. 1986), whichoften persist for a long time despite antiepileptictreatments.

	ACKNOWLEDGMENTS

We thank Profs. F. Clementi and G. Avanzini for discussion, Dr. J. R. Huguenard for critically reading the manuscript, andDr. S. Coco for help with someexperiments.

This work was supported by Istituto Superiore Sanita (Progetto Sclerosi Multipla n. 61), by Italian Ministry of Universityand Scientific and Technological Research (Ministero dell' Universitàe della Ricerca Scientifica e Tecnologica 2000 and 2001), andby European Community (QLGR3-CT-2000-01343, coordinator E. Scarfone)to M.Matteoli.

Present address of A. Bacci: Dept. of Neurology and Neurological Sciences, Stanford University Medical Center, Stanford, CA94035.

	FOOTNOTES

^* A. Bacci and G. Sancini contributed equally to thiswork.

Address for reprint requests: M. Matteoli, CNR-Institute of Neuroscience, Cellular and Molecular Pharmacology, Dept. of MedicalPharmacology, University of Milano, via Vanvitelli 32, 20129 Milano,Italy (E-mail: MichelaM{at}csfic.mi.cnr.it).

REFERENCES

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
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0022-3077/02 $5.00 Copyright © 2002 The American Physiological Society