Intracellular Calcium Transients and Potassium Current Oscillations Evoked by Glutamate in Cultured Rat Astrocytes

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Volume 17, Number 19, Issue of October 1, 1997 pp. 7278-7287
Copyright ©1997 Society for Neuroscience

Intracellular Calcium Transients and Potassium Current Oscillations Evoked by Glutamate in Cultured Rat Astrocytes

Jianguo Chen, Kurt H. Backus, and Joachim W. Deitmer
Abteilung für Allgemeine Zoologie, FB Biologie, Universität Kaiserslautern, D-67653 Kaiserslautern, Germany

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Glutamate responses in cultured rat astrocytes from cerebella of neonatal rats were investigated using the perforated-patchconfiguration to record membrane currents without rundown of intracellularmessenger cascades, and microfluorometric measurements to measurethe intracellular Ca²⁺ concentration ([Ca²⁺]_i) and intracellular pH (pH_i) with fura-2 AM and 2 $'$ ,7 $'$ -bis-(2-carboxyethyl)-5,6-carboxyfluoresceinacetoxy methylester respectively. In the perforated-patch mode,glutamate evoked single or multiple outward current transientsin 82% of the cells, which disappeared when the recording techniquewas converted into a conventional whole-cell mode. The outwardcurrent transients were accompanied by [Ca²⁺]_i transients, whereas pH_i fell monophasically, without any signof oscillation. Pharmacological analysis of the glutamate-inducedresponses indicated that ionotropic receptor activation evokedan inward current but no outward current transients, and metabotropicreceptor activation (of the mGluR1/5 type) elicited outward currenttransients but no inward current. The outward current transientswere reduced in frequency, or even abolished, after depletionof the intracellular Ca²⁺-stores by the Ca²⁺-ATPase inhibitor cyclopiaconic acid (10 µM). They reversed near $-$ 85 mV and were reduced by tetraethylammonium (10 mM), suggestingthat they were caused by K⁺ channel activation. It is concluded that glutamate evoked theseK⁺ outward current transients by oscillatory Ca²⁺ release mediated by mGluR activation. The corresponding membranepotential waves across the astroglial syncytium could providespatial and temporal dynamics to the glial K⁺ uptake capacity and other voltage-dependent processes.
Key words: glutamate; perforated patch-clamp; gramicidin; current oscillation; [Ca²⁺]_i oscillations; Ca²⁺-activated K⁺ channels; rat

INTRODUCTION

Changes in the intracellular Ca²⁺ concentration ([Ca²⁺]_i) play a crucial role in many processes involved in the modulation ofsignal transduction, development, and plasticity in the CNS. Atpresent, multiple pathways have been demonstrated that can leadto [Ca²⁺]_i changes. The involvement of glutamate receptors appears toplay a key role. The activation of glutamate receptors can change[Ca²⁺]_i by two distinct mechanisms. First, receptors of the ionotropicsubclass, namely NMDA and a subpopulation of Ca²⁺-permeable AMPA/kainate receptors, directly mediate a Ca²⁺ influx. Second, receptors of the metabotropic glutamate receptorsubclass (mGluR), e.g., the mGluR1 and mGluR5, induce the hydrolysisof phosphatidylinositol that leads to the inositol triphosphate(IP₃)-mediated release of Ca²⁺ from intracellular stores. In addition, the membrane depolarizationmediated by ionotropic glutamate receptors could activate voltage-dependentCa²⁺-channels that allow Ca²⁺ influx.

Glial cells express ionotropic glutamate receptors in culture (Bowman and Kimelberg, 1984; Kettenmann et al., 1984) and insitu (Berger et al., 1992; Müller et al., 1992; Seifert and Steinhäuser,1995). In cultured cerebellar fusiform cells (Burnashev et al.,1992), in cerebellar Bergmann glial cells in situ (Müller etal., 1992), in hippocampal glial cells in the CA1 region of thestratum radiatum (Jabs et al., 1994), and in hilar glial precursorcells (Backus and Berger, 1995), evidence was found that the activationof AMPA/kainate receptors can also result in a Ca²⁺ influx.

Monophasic and multiple intracellular Ca²⁺ transients were observed in cultured astrocytes after the application of glutamatereceptor agonists (Glaum et al., 1990; Jensen and Chiu, 1990,1991; de Barry et al., 1991; Holzwarth et al., 1994; Brune andDeitmer, 1995). The pharmacological profile of these responsesrevealed that both Ca²⁺ influx and intracellular Ca²⁺ release were responsible for the Ca²⁺ transients. Recent results suggested that glial cells might communicatewith each other, or with neurons, using waves of Ca²⁺ elevation that spread via gap junctions through the astrocyticsyncytium. Ca²⁺ waves were propagated between glutamate-stimulated cells (Cornell-Bellet al., 1990; Charles et al., 1991), indicating the occurrenceof a long-range oscillatory signaling mechanism in glial cells.In hippocampal astrocytes, waves of [Ca²⁺]_i could be induced by the activity of neighboring neurons (Daniet al., 1992). Focal electrical stimulation of astrocytes in mixedcultures of rat forebrain cells induced intercellular Ca²⁺ waves and large increases in [Ca²⁺]_i in neighboring neurons, suggesting the existence of glial-neuronalsignaling pathways (Nedergaard, 1994).

Astrocytes express a large repertoire of voltage- and ligand-gated ion channels, e.g., Ca²⁺-activated K⁺ channels (Quandt and MacVicar, 1986) or GABA_A-receptors (Stelzeret al., 1988), which are sensitive to changes in [Ca²⁺]_i. Because the cytosol is dialyzed rapidly during conventionalwhole-cell clamp recordings, we used the perforated patch-clamptechnique to characterize the membrane responses evoked by glutamatereceptor agonists. In combination with the fluorescent imagingtechnique to measure [Ca²⁺]_i and pH_i, we could show in single cells that the applicationof agonists of glutamate receptors evoked oscillations of membranecurrents associated with multiple [Ca²⁺]_i transients.

A preliminary report of some of the results has been published previously in abstract form (Chen et al., 1997).

MATERIALS AND METHODS
Cell culture. For preparing primary cultured astrocytes, the cerebellar hemispheres of newborn rats (P0-P1) were rapidly removed.Cells were isolated and cultured according to the method describedby Fischer (1984). Immunohistochemical staining confirmed thatthe cultures consisted of enriched (>95%) glial fibrillary acidicprotein-positive astrocytes (Brune et al., 1994). After the cellshad reached confluence, oligodendrocytes and macrophages wereremoved by a shaking procedure, and the remaining cells were dissociated,plated on glass coverslips coated with poly-D-lysine, and incubatedin 7% CO₂ at 37°C. The experiments were performed between 2 and15 d after plating of the astrocytes at room temperature (~22-24°C).

Experimental setup. For perforated patch-clamp recordings, the culture dish was mounted on the stage of an inverted microscope(Zeiss). For the combined electrophysiological and microfluorometricexperiments, the culture dish was mounted on an inverted fluorescencemicroscope (Diaphot, Nikon, Tokyo, Japan) equipped with a NikonCF-Fluor 20× objective. Recording patch pipettes were pulled fromborosilicate glass, and the tips were fire-polished (resistance4-6 M $Omega$ , when filled with the pipette solution). Gramicidin-perforated-patchrecordings were performed following the method of Kyrozis andReichling (1995). Briefly, the electrode tip was filled for 1-40sec with the gramicidin-free pipette solution (see below) to avoidproblems with seal formation, and then back-filled with the gramicidin-containingpipette solution. After the formation of a gigaseal (on-cell recording)(Hamill et al., 1981), short steps in holding potential were appliedcontinuously at 2 min intervals to monitor the gradual decreasein series resistance. Drug application was not started until theseries resistance decreased below 50 M $Omega$ , which usually lasted20-30 min. The reference potential for all measurements was thezero-current potential of the pipette in the bath before establishmentof the gigaseal.

Currents were recorded by an EPC-7 (List, Darmstadt, Germany) patch-clamp amplifier. Before digitization (sampling rate 0.5-1kHz), currents were filtered at 3 kHz with a three-pole low-passBessel filter. Data were stored and evaluated with the aid ofthe PCLAMP hardware and software package (Axon Instruments, FosterCity, CA) for a personal computer. To determine the agonist-inducedcurrent amplitudes, the maximal deflection from the baseline wasused. The difference of two samples was tested using the two-tailedt test.

Microfluorometric recordings. The fluorescence microscope was equipped with a dual excitation fluorometric imaging system(PTI, Wedel, Germany). The illumination was generated by a 75W xenon bulb. Monochromator settings, chopper frequency, and completedata acquisition were controlled by software (PTI) for microcomputersystems. Astrocytes were loaded by incubating the cell culturesin 2 $'$ ,7 $'$ -bis-(2-carboxyethyl)-5,6-carboxyfluorescein-acetoxy-methylester(BCECF-AM; 25 µM) for 20 min or fura-2 AM (5 µM) for 60 min atroom temperature. Dye-loaded astrocytes were excited by monochromaticlight at wavelengths 350 and 380 nm (fura-2 AM) to measure [Ca²⁺]_i or at 440 and 495 nm (BCECF-AM) to measure pH_i. The fluorescenceemission of the cell under perforated-patch control, of anothersingle cell, and the emission of a selected area with a groupof 5-10 cells on the coverslip was recorded simultaneously witha video camera (SIT C-2400, Hamamatsu, Garching, Germany), usinga 495 nm longpass filter for fura-2 AM and a 520 nm longpass filterfor BCECF-AM. The signals were sampled at 3 Hz and computed intorelative ratio units. Drug-induced changes of [Ca²⁺]_i were measured by determining the changes of the fluorescenceratio of 350 nm: 380 nm. The BCECF-AM ratio of 440 nm: 495 nmwas converted into pH units according to calibration describedby Brune et al. (1994).

Solutions and drug application. The pipette solution for perforated patch-clamp recordings contained (in mM): KCl 140, NaCl5, CaCl₂ 0.5, MgCl₂ 1, EGTA 5, HEPES 10; pH adjusted to 7.2 withKOH. Gramicidin (Sigma, St. Louis, MO), 5 mg/ml, was dissolvedin dimethylsulfoxide (DMSO), vortexed for 1 min, sonicated for20 sec, and then added to the pipette solution to give a finalconcentration of 25-50 µg/ml. In some cells the conventional whole-cellconfiguration was established after recording in the gramicidin-perforated-patchconfiguration. This resulted in a dialysis of the cell interiorwith the pipette solution listed above.

During the experiments the cell cultures were superfused continuously with a HEPES-buffered saline containing (in mM): NaCl145, KCl 5, CaCl₂ 2, MgCl₂ 1, glucose 10, HEPES 10; pH adjustedto 7.4 with NaOH. In a few experiments we used a Ca²⁺-free salt solution in which CaCl₂ was replaced by EGTA (1 mM).Stock solutions of glutamate, quisqualate (100 mM in aqua bidest;both from Sigma), and kainate (100 mM in 100 mM NaOH; Sigma) wereprepared. Stock solutions of cyclopiazonic acid (CPA, 50 mM; Sigma)and 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX, 50 mM; TocrisCookson, Bristol, UK) were dissolved in DMSO and stored at $-$ 20°C.Kynurenic acid (Sigma) was dissolved in the saline in the finalconcentration. Stock solutions of trans-(±)-1-aminocyclopentane-1S,3R-dicarboxylicacid (t-ACPD; 20 mM in 50 mM NaOH), (s) 3,5 dihydroxyphenyl-glycine(DHPG; 100 mM in aqua bidest), and L-2-amino-4-phosphonobutyricacid (L-AP4; 20 mM in 50 mM NaOH) were prepared. t-ACPD, DHPG,and L-AP4 were purchased from Tocris Cookson. All other drugswere obtained from Sigma. Drugs were added to the saline shortlybefore use in defined concentrations. Fura-2 AM and BCECF-AM wereobtained from Molecular Probes (Eugene, OR).

RESULTS

Glutamate evokes membrane current oscillations
The whole-cell membrane current of cultured cerebellar astrocytes was recorded in the gramicidin-perforated-patch configurationat a holding potential (V_h) of $-$ 70 mV. In these cells 1 mM glutamate,applied by bath superfusion for 10 sec, evoked different currentresponse patterns (Fig. 1). All of them showed a distinct inwardcurrent (100% of the cells; n = 62), but they differed in thefrequency, shape, and time course of oscillating outward currenttransients (Fig. 1A-C, E) that were superimposed in most cells(82%; n = 51).
Fig. 1. Glutamate-induced current response patterns in cultured cerebellar astrocytes. A-C, The membrane current was recorded in thegramicidin-perforated-patch configuration (PPC), and glutamate(Glu, 1 mM) was applied by bath application for 10 sec as indicated.Glutamate evoked an inward current that was superimposed by multiple(A), a single (B), or no outward current transients (C). D, Inthe conventional whole-cell clamp configuration (WCC), glutamateexclusively induced an inward current without showing any outwardcurrent transients. E, Gramicidin-perforated-patch recording thatdemonstrates the persistency of outward current transients intime.
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In 29 cells, multiple outward current transients (2-8) (Fig. 1A,E) were observed after glutamate application. Although thefirst outward current transient usually had the largest amplitude(41 ± 25 pA; mean ± SD), the subsequent transients showed a continuousbut slow decrease in amplitude with time. When the glutamate applicationwas prolonged until up to 3 min, the outward current transientspersisted for several minutes (data not shown). In some cells(16 of 62), only a single outward current transient with a meanamplitude of 22 ± 14 pA was superimposed onto the rising phaseof the inward current component (Fig. 1B). No outward currenttransients were present in 11 of 62 cells, i.e., in 18% of theastrocytes (Fig. 1C). A few astrocytes (n = 6) showed a mixedresponse where single and multiple outward current transientscould change from one to the next glutamate application and viceversa. The presence of multiple current oscillations in astrocytesshowed a remarkable persistency, because they could be observedfor up to 1 hr without any major changes in shape, number, andamplitude of the current transients (Fig. 1E).

Membrane current oscillations induced by glutamate, however, could be observed only in the gramicidin-perforated-patch configuration.Astrocytes exposed to glutamate (1 mM; 10 sec) in the conventionalwhole-cell clamp configuration responded with an inward currentof 28 ± 7.5 pA (n = 35) (Fig. 1D) that was significantly (p <0.01) larger than that recorded in the gramicidin-perforated-patchconfiguration but never showed any outward current oscillations.In eight cells that showed outward current transients after glutamateapplication in the gramicidin-perforated-patch configuration,the membrane patch was ruptured carefully to establish the conventionalwhole-cell clamp configuration. After this procedure the glutamate-inducedoutward current transients disappeared completely (Figs. 2, 3,top traces), indicating the requirement of a functionally intactcytosol for the occurrence of current oscillations in astrocytesas revealed by the gramicidin-perforated-patch configuration.
Fig. 2. Simultaneous recording of membrane current and [Ca²⁺]_i using the digital imaging technique in fura-2 AM-loaded cerebellar astrocytesshowing multiple outward current transients. Left column, Gramicidin-perforated-patchconfiguration: glutamate (Glu, 1 mM), applied for 10 sec as indicated,induced an inward membrane current that was superimposed by threeoutward current transients (top). Each outward current transientwas preceded by a transient increase in [Ca²⁺]_i (middle). The bottom trace represents the averaged change in[Ca²⁺]_i induced by glutamate recorded from a group of cells in thevicinity of the cell displayed above. Right column, Responsesof the same cells to glutamate after establishment of the conventionalwhole-cell clamp configuration.
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Fig. 3. Simultaneous recording of membrane current and [Ca²⁺]_i using the digital imaging technique in cerebellar astrocytes showinga single outward current transient. Left column, Gramicidin-perforated-patchconfiguration: glutamate (Glu, 1 mM), applied for 10 sec as indicated,induced an inward membrane current that was superimposed by asingle outward current transient (top). A transient increase in[Ca²⁺]_i was followed by a slowly decaying [Ca²⁺]_i decrease (middle). The bottom trace represents the averagedchange in [Ca²⁺]_i induced by glutamate recorded from a group of cells in thevicinity of the cell displayed above. Right column, Responsesof the same cells to glutamate after establishment of the conventionalwhole-cell clamp configuration.
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Simultaneous measurement of [Ca²⁺]_i, pH_i, and membrane current oscillations
Recently it was reported that the application of glutamate on astrocytes could evoke transient and complex oscillatory changesin [Ca²⁺]_i (Cornell-Bell et al., 1990; Glaum et al., 1990; Jensen andChiu, 1990, 1991; de Barry et al., 1991; Dani et al., 1992; Holzwarthet al., 1994; Brune and Deitmer, 1995) and considerable increasesin the intracellular H⁺ concentration (Brune and Deitmer, 1995). Because these experimentswere performed exclusively in intact cells, we supposed that theglutamate-induced current oscillation we observed in the gramicidin-perforated-patchconfiguration could be mediated by changes in [Ca²⁺]_i or pH_i, or both. To examine this issue, the changes in [Ca²⁺]_i or pH_i were recorded simultaneously with the membrane currentin the perforated-patch and conventional whole-cell mode.

Glutamate (1 mM) evoked a large inward current that was superimposed by a number of distinct outward current transients (Fig.2). In the same cell we observed an equal number of transient[Ca²⁺]_i changes that were temporally associated with the outward currenttransients. In addition, a small increase in basal [Ca²⁺]_i was observed that followed roughly the time course of the deactivatinginward current component. In cells that responded only with asingle outward current transient, only a single large Ca²⁺ transient was also apparent (Fig. 3). When the whole-cell clampconfiguration was subsequently established in the same cell (n= 4), both outward current and multiple Ca²⁺ transients disappeared, leaving a strongly reduced single initialCa²⁺ transient and a small tonic increase in basal [Ca²⁺]_i (Figs. 2, 3, top right and middle right traces). Also in twocells in which glutamate failed to induce current oscillationsin the perforated-patch configuration, no Ca²⁺ transients were observed.

Changes in [Ca²⁺]_i in a group of neighboring astrocytes, which were not in contact with the patch pipette, are shown in thebottom traces of Figures 2 and 3. In these cells glutamate alsoinduced changes in [Ca²⁺]_i, but oscillations were not observed, indicating that the fura-2AM fluorescence signal reflected the integrated response of manycells that were not producing oscillations in phase. Rather, thesepresumed [Ca²⁺]_i oscillations showed up as an initial transient and a sustainedrise for >1 min (Fig. 2) or a monophasic [Ca²⁺]_i rise (Fig. 3).

A small decrease in pH_i could be measured in single astrocytes in which 1 mM glutamate evoked outward current transients,but pH oscillations were never observed (Fig. 4). Similar resultswere obtained in single astrocytes or in groups of "unpatched"cells (n = 8), regardless of whether they showed multiple or singleoutward current transients (Fig. 4). These results suggested thatthere was probably no coupling between changes in pH_i and thedifferent current and [Ca²⁺]_i response patterns in these astrocytes.
Fig. 4. Simultaneous recording of membrane current in the gramicidin-perforated-patch configuration and pH_i using the digital imagingtechnique in BCECF-AM-loaded cerebellar astrocytes. Top, Currentresponses induced by glutamate (Glu, 1 mM, applied for 10 secas indicated) of an astrocyte showing multiple outward currenttransients (A) and another showing a single outward current transient(B). Second row from top, Corresponding glutamate-induced pH_ichanges to the current traces on top. Third row from top, Simultaneousmeasurement of the glutamate-induced pH_i change in another singlecell in the vicinity that was not under perforated-patch control.Bottom, Simultaneous measurement of the glutamate-induced pH_ichange averaged over a group of cells in the vicinity. A decreasein pH_i is displayed as an upward deflection.
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Effects of glutamate receptor ligands
The absence of glutamate-induced outward current transients and [Ca²⁺]_i oscillations in the whole-cell clamp configuration suggestedthe involvement of an intracellular messenger system, which wasdialyzed in the conventional whole-cell mode but persisted inthe perforated patch-clamp mode. Because we had observed a correlationin time between [Ca²⁺]_i oscillations and outward current transients, we attempted toidentify the glutamate receptor subtype and the mechanism underlyingthe membrane current oscillations by recording the membrane currentin the gramicidin-perforated-patch configuration. The effectsof different glutamate receptor ligands on [Ca²⁺]_i and pH_i in rat astrocytes had been studied previously (de Barryet al., 1991; Holzwarth et al., 1994; Brune and Deitmer, 1995).

Glutamate is a mixed agonist at both ionotropic receptors and mGluRs. Therefore, we tested separately an involvement of ionotropicand metabotropic receptors in the induction of current oscillations.Kainate (400 µM, 10 sec), an agonist of the non-NMDA glutamatereceptor subtype, evoked an inward current, but was unable toelicit outward current oscillations as did glutamate in the samecell (n = 5) (Fig. 5A). Kynurenic acid (1 mM; n = 4) (Fig. 5B),a broad-spectrum glutamate antagonist of ionotropic receptors(Perkins and Stone, 1982), and CNQX (50 µM; n = 4) (Fig. 5C),a selective blocker of the AMPA/kainate receptor subtype (Honoréet al., 1988), reduced the glutamate-evoked inward current butfailed to block the glutamate-induced outward current transients(Fig. 5B,C).
Fig. 5. Effect of ionotropic glutamate receptor ligands. A, Kainate (KA, 400 mM, applied for 10 sec as indicated) did not elicit anycurrent oscillation. B, Kynurenic acid (1 mM, preapplication time:5 min), and C, CNQX (50 µM, preapplication time: 5 min) reducedthe glutamate-induced inward current but not the outward currenttransients.
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Quisqualate, which is known to be an agonist of AMPA/kainate as well as of mGluRs, evoked outward current transients but nodetectable inward current when applied in a concentration of 200µM for 10 sec (n = 5) (Fig. 6A). The metabotropic agonist t-ACPD(30 µM), an agonist reported to activate receptors of the mGluR2/3subtype but that also exerted weak agonistic activity at mGluR1/5receptors (Nakanishi, 1992; Tanabe et al., 1993), failed to evokean inward current but elicited one or multiple outward currenttransients (n = 5) (Fig. 6B). DHPG (100 µM), an agonist reportedto be selective for mGluRs including the mGluR1/5 subtypes, alsomimicked the glutamate-evoked outward current transients (n =5) (Fig. 6C). The agonist of receptors of the mGluR4/6-8 subtypes,L-AP4 (Nakanishi, 1992; Tanabe et al., 1993), however, had noeffect on the membrane current in cultured astrocytes when appliedat 200 µM for 10 sec (n = 5) (Fig. 6D). These results indicatethat the outward current transients evoked by glutamate were attributableto the activation of mGluRs. The pharmacological profile of theglutamate-evoked outward current transients suggested the activationof mGluRs of the mGluR1/5 or mGluR2/3 subtypes.
Fig. 6. The effect of metabotropic glutamate receptor agonists. A, Quisqualate (QQ, 200 µM, applied for 10 sec as indicated), B, t-ACPD(30 µM, 10 sec), and C, DHPG (100 µM, 10 sec) evoked outward currenttransients but no detectable inward currents. D, L-AP4 (200 µM,10 sec) had no effect on the membrane current of cultured cerebellarastrocytes.
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Contribution of intracellular Ca²⁺ mobilization
Glutamate receptors of the mGluR1/5 subtype are coupled via a G-protein to the hydrolysis of phosphatidylinositol, which resultsin the production of IP₃ and the subsequent release of Ca²⁺ from IP₃-sensitive intracellular stores (Berridge and Irvine,1989). To test whether an intracellular Ca²⁺ release was involved in the activation of the glutamate-evokedoutward current transients, intracellular Ca²⁺ stores were depleted using CPA (10 µM), which was preappliedfor 5 min and then in combination with glutamate (1 mM; n = 5).CPA alone elicited a transient [Ca²⁺]_i rise, indicating reversible loss of Ca²⁺ from intracellular stores (n = 6).

In the presence of CPA the outward current transients evoked by glutamate were strongly reduced, usually to a single transient(Fig. 7A), or when it was preapplied for 10 min, they were totallyabolished (Fig. 7B). The inward current component, however, remainedunaffected by CPA (Fig. 7). These results indicate that the currentoscillations were likely mediated by the release of Ca²⁺ from intracellular, CPA-sensitive stores.
Fig. 7. Effect of CPA on glutamate-induced currents in cultured cerebellar astrocytes. CPA (10 µM, preapplied for 5 min) inhibitedthe outward current transients induced by glutamate (1 mM, appliedfor 10 sec as indicated) in cells responding with multiple oscillations(A) or with a single oscillation (B), but had no effect on theinward current component.
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The contribution of an influx of extracellular Ca²⁺ to the glutamate-induced current oscillations was examined by comparingthe current responses evoked in standard saline with those ina Ca²⁺-free saline that contained 1 mM EGTA. The initial outward currenttransient observed in standard salt solution was still prominentwhen glutamate was applied in Ca²⁺-free salt solution (n = 8; not shown). In cells expressing multiplecurrent oscillations, however, no consistent effect of the Ca²⁺-free salt solution was observed. Usually the oscillatory outwardcurrent transients were reduced or disappeared completely (n =6). In these cells, readdition of extracellular Ca²⁺ did not result in a recovery of outward current oscillations.The results suggest that the sustained outward current transientsrequired the presence of extracellular Ca²⁺ to continue, but the large initial transient apparently did notdepend on Ca²⁺ influx and was presumably caused by Ca²⁺ release from intracellular stores.

Identification of the outward current transients
To identify the type of ion channel underlying the glutamate-induced outward current transients we determined their reversalpotential. Therefore, 1 mM glutamate was applied when V_hr wasaltered to more hyperpolarized values during the glutamate-inducedinward current. As shown in Figure 8A,B, the outward current transientsdecreased or reversed their polarity at a holding potential of $-$ 90 or $-$ 100 mV. The current amplitudes were fitted by linear regressionto yield a rough estimate of the reversal potential of these outwardcurrent transients (Fig. 8C). The resulting reversal potentialof $-$ 84.9 mV (n = 4) was close to the calculated K⁺ equilibrium potential (E_K⁺ = $-$ 83 mV), indicatingthe involvement of K⁺ channels during the glutamate-evoked current transients.
Fig. 8. Determination of the reversal potential of glutamate-evoked outward current transients. When the holding potential was changedduring a glutamate-induced current response from $-$ 70 to $-$ 90 mV(A) or from $-$ 70 to $-$ 100 mV (B) as indicated, the outward currenttransients reversed their polarity. C, The current amplitude ofglutamate-induced current oscillations was plotted as a functionof the membrane potential. To estimate the reversal potentialof the current transients, all data points were fitted by linearregression (reversal potential: $-$ 84.9 mV; n = 4; the differentsymbols represent the different cells).
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This was confirmed by the sensitivity to tetraethylammonium (TEA) of the outward current transients. TEA (10 mM; n = 5), aK⁺ channel blocker (Rudy, 1988), reduced the outward current transientsevoked by glutamate in cells showing multiple oscillations (Fig.9A) and also in those with a single outward current transient(Fig. 9B).
Fig. 9. The effect of TEA on glutamate-induced outward current transients. TEA (10 mM, preapplied for 5 min) reduced the glutamate-inducedoutward current transients in cerebellar astrocytes expressingmultiple current oscillations (A) as well as a single currentoscillation (B), indicating that they were mediated by K⁺ channels.
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DISCUSSION

Perforated-patch recordings reveal glutamate-induced current oscillations
To minimize the washout of regulatory molecules that could modulate ion channel activity (Korn et al., 1991), we have usedperforated-patch recordings with gramicidin, which forms poresselective for monovalent cations but impermeable for anions anddivalent cations (Myers and Haydon, 1972). The use of this techniquerevealed that glutamate receptor agonists evoked an inward currentthat was superimposed by a single or multiple outward currenttransients. Many preceding studies on glutamate receptors in glialcells in culture (Sontheimer et al., 1988; Usowicz et al., 1989;Wyllie and Cull-Candy, 1994) and in brain slices (Berger et al.,1992; Müller et al., 1992; Jabs et al., 1994; Backus and Berger,1995; Seifert and Steinhäuser, 1995) missed the current oscillations,presumably because of the use of the conventional whole-cell clampconfiguration. In another study in which the perforated-patchtechnique was used in hilar glial precursor cells, Ca²⁺-dependent K⁺ channels were observed after Ca²⁺ influx through Ca²⁺-permeable AMPA/kainate receptors (Backus et al., 1995).

Identification of the mGluR subtype
The application of the ionotropic agonist kainate evoked an inward current but no superimposed outward current transients,whereas the mixed agonist quisqualate and agonists selective formGluR subtypes, DHPG and t-ACPD, induced outward current transientsbut no inward current component. These findings, together withthe lack of effect of blockers of ionotropic glutamate receptors,kynurenic acid and CNQX, indicate that the outward current transientswere caused by the activation of mGluRs. The inward current componentwas evoked only by glutamate or kainate, in either conventionalor perforated patch-clamp mode, but not by t-ACPD, DHPG, or L-AP4,indicating that it was mediated by ionotropic glutamate receptors,most likely of the AMPA/kainate subtype, which are expressed inastrocytes in culture (Sontheimer et al., 1988; Backus et al.,1989; Usowicz et al., 1989; Burnashev et al., 1992; Wyllie andCull-Candy, 1994; Telgkamp et al., 1996) and in brain slices (Bergeret al., 1992; Müller et al., 1992; Jabs et al., 1994; Backusand Berger, 1995; Seifert and Steinhäuser, 1995).

The pharmacological profile of mGluR subtypes (Nakanishi, 1992; Tanabe et al., 1993; Pin and Duvoisin, 1995) suggests thatthe induction of outward current transients by glutamate is mediatedby the mGluR1/5 subtypes, because their selective agonist DHPGwas effective. t-ACPD, an agonist of mGluR2/3 and mGluR1/5 subtypes(Pin and Duvoisin, 1995), was also effective. The selective mGluR4/6-8agonist L-AP4 did not induce any response. Because the depletionof intracellular Ca²⁺-stores by CPA led to a reduction of outward current transients,it is likely that the mGluR subtype involved in the mechanismunderlying the outward current oscillations is coupled to intracellularCa²⁺ release. At present, mGluR1/5 receptors are the only mGluR subtypesthat are linked to the IP₃-mediated intracellular Ca²⁺ mobilization (Abe et al., 1992; Aramori and Nakanishi, 1992).Therefore, mGluR1/5 receptors are likely involved in the inductionof these outward current oscillations.

Glutamate-induced [Ca²⁺]_i changes and oscillations
Glial cells respond to various neurotransmitters with changes of [Ca²⁺]_i. Monophasic changes in [Ca²⁺]_i are caused by an elevation of the extracellular K⁺ concentration or by the activation of ionotropic receptor agonists,e.g., kainate (Jensen and Chiu, 1990; Salm and McCarthy, 1990;Brune and Deitmer, 1995) or GABA (Kirchhoff and Kettenmann, 1992).These responses are thought to be caused by an influx of Ca²⁺ through Ca²⁺-permeable ionotropic receptors or voltage-dependent channels(Finkbeiner, 1995). Polyphasic responses evoked by glutamate receptoragonists are characterized by sustained [Ca²⁺]_i oscillations preceded by an initial transient [Ca²⁺]_i rise that is caused primarily by a release of Ca²⁺ from IP₃-sensitive intracellular stores (cf. Finkbeiner, 1995;Verkhratsky and Kettenmann, 1996).

Gramicidin-perforated-patch recordings in combination with fura-2 AM digital imaging disclosed several types of [Ca²⁺]_i changes in cultured cerebellar astrocytes. In a subpopulationof cells, polyphasic changes in [Ca²⁺]_i were prominent and were characterized by two to eight transientrises in [Ca²⁺]_i and a simultaneous increase in the [Ca²⁺]_i baseline. In a small group of cells (<10) glutamate applicationresulted in an initial transient rise of [Ca²⁺]_i that was followed by a sustained plateau reflecting the averagedoscillatory response of a group of cells that closely resembledthe response pattern reported recently for a large group of cells(>20) (Brune and Deitmer, 1995). The nonoscillatory increase inbaseline Ca²⁺ might be caused by a Ca²⁺ influx through Ca²⁺-permeable AMPA receptors that are expressed in cultured rat cerebellarastrocytes (Telgkamp et al., 1996).

In another subpopulation of cerebellar astrocytes, glutamate induced an initial transient rise that was followed by a plateauwithout showing distinct oscillations (Fig. 3). In these cellsthe initial increase in [Ca²⁺]_i might have been insufficient to induce subsequent oscillations;however, the response type of glutamate-induced [Ca²⁺]_i changes strongly depends on the mGluR subtype. In stably transfectedcell lines expressing recombinant receptors of the mGluR1 $alpha$ subtype,monophasic changes in [Ca²⁺]_i were observed, whereas in cells expressing the mGluR5a subtype,oscillatory responses with an increasing number of [Ca²⁺]_i transients were found (Kawabata et al., 1996). Therefore, differentpopulations of cerebellar astrocytes might exist: one populationexpressing primarily the mGluR1 $alpha$ subtype and another the mGluR5asubtype.

Glutamate-induced changes in pH_i
Intracellular acidifications induced by glutamate were small and non-oscillatory and therefore could not be correlated toeither the current or the [Ca²⁺]_i oscillations. The pH_i measurements might have been impairedby the H⁺ permeability of the gramicidin pores (Myers and Haydon, 1972),which could have caused a dampening of the pH_i changes. The mechanismsof this acidification are discussed elsewhere (Brune and Deitmer,1995; Rose and Ransom, 1996; Deitmer and Schneider, 1997).

Is there a link between [Ca²⁺]_i and outward current oscillations?
The [Ca²⁺]_i oscillations observed in the astrocytes likely induced the outward current oscillations, because (1) the numberof Ca²⁺ oscillations always exactly matched the number of outward currenttransients (Fig. 2) and (2) the Ca²⁺ oscillations always started shortly before the correspondingoutward current transient, suggesting that an increase of [Ca²⁺]_i directly caused the current transients. Because the outwardcurrent transients were blocked by TEA and reversed close to theestimated K⁺ equilibrium potential, we conclude that they were mediated byCa²⁺-dependent K⁺ channels.

The withdrawal of extracellular Ca²⁺ did not affect the initial outward current transient in most astrocytes, suggesting thatit was mediated by an intracellular Ca²⁺ release. In addition, maintained oscillatory outward currenttransients required the presence of extracellular Ca²⁺. Recent findings have indeed shown that the initial transientrise in [Ca²⁺]_i was mediated by an intracellular Ca²⁺ release and that the sustained [Ca²⁺]_i oscillations required the presence of extracellular Ca²⁺ (Cornell-Bell et al., 1990; Glaum et al., 1990; Jensen and Chiu,1990; de Barry et al., 1991; Holzwarth et al., 1994; Kim et al.,1994; Brune and Deitmer, 1995). In contrast, nonglutamate-evokedoscillations in [Ca²⁺]_i also persisted in the absence of extracellular Ca²⁺ (mechanical stimulation: Charles et al., 1991; P_2Y-purinergicstimulation: Kastritsis et al., 1992); however, it cannot be discountedthat the reduction of oscillatory outward current transients wasattributable to a depletion of intracellular Ca²⁺ stores caused by the withdrawal of extracellular Ca²⁺.

Kainate did not induce current oscillations, although it did evoke distinct changes in [Ca²⁺]_i in astrocytes (Enkvist et al., 1989; Jensen and Chiu, 1990,1991; Holzwarth et al., 1994; Brune and Deitmer, 1995). A monophasicincrease in [Ca²⁺]_i, however, would give rise to a monophasic Ca²⁺-activated K⁺ current. Therefore, the kainate-induced current represents thesum of a large inward current through kainate-activated AMPA receptor/channelsand a K⁺ outward current. Perforated-patch recordings in hilar glial precursorcells in situ in acute hippocampal slice preparations have shownthat kainate could also induce biphasic current responses thatwere composed of an AMPA receptor/channel-mediated inward currentand a subsequent delayed Ca²⁺-activated K⁺ current (Backus et al., 1995).

This is the first report of glutamate-induced current oscillations in glial cells. Glutamate-induced depolarizations of themembrane potential have been reported previously in cultured ratbrain astrocytes (Bowman and Kimelberg, 1984; Kettenmann et al.,1984) and were attributed to the activation of non-NMDA receptors(Backus et al., 1989). In these studies the changes in membranepotential were measured with sharp intracellular microelectrodes,which should not affect [Ca²⁺]_i transients. Although our experimental conditions are comparable,none of these studies has shown any oscillatory changes in membranepotential after glutamate application. In cultured cortical ratastrocytes, however, quisqualate induced biphasic changes in membranepotential (compare Fig. 1C of Backus et al., 1989), characterizedby an initial transient hyperpolarization and a delayed depolarizationmediated by non-NMDA receptors. Moreover, oscillations of themembrane potential were observed in glial cells of rat hippocampalslices (Walz and MacVicar, 1986) and in astrocytes of kainic acid-lesionedhippocampal slices after the application of a phorbol ester (MacVicaret al., 1987).

Oscillatory changes in [Ca²⁺]_i can spread across the glial syncytium like waves (cf. Finkbeiner, 1995) and thus by activationof Ca²⁺-activated K⁺ channels could give rise to wave-like changes of the glial membranepotential. In astrocytes such potential waves could arise at sitesof increased neuronal activity, where an elevation of the extracellularK⁺ concentration and the exposure to glutamate depolarize the membranepotential and evoke an increase in [Ca²⁺]_i. K⁺ uptake into the astrocytic syncytium could travel in phase witha hyperpolarizing potential wave, thus providing spatial dynamicsto the glial K⁺ buffer capacity.

FOOTNOTES

Received May 21, 1997; revised July 17, 1997; accepted July 18, 1997.

This study was supported by a grant of the Deutsche Forschungsgemeinschaft to J.W.D. and K.H.B. (De 231/11-1). We thank C.Lohr for critically reading this manuscript. We are grateful toSandra Bergstein for her excellent technical assistance.

Reprint requests should be addressed to Dr. J. W. Dietmer, Abteilung für Allgemeine Zoologie, FB Biologie, Universität Kaiserslautern,Postfach 3049, D-67653 Kaiserslautern, Germany.

Dr. Chen's present address: II. Physiologisches Institut de Universität Heidelberg, Im Neuenheimer Feld 326, D-69120 Heidelberg,Germany.

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Volume 17, Number 19, Issue of October 1, 1997 pp. 7278-7287 Copyright ©1997 Society for Neuroscience

Intracellular Calcium Transients and Potassium Current Oscillations Evoked by Glutamate in Cultured Rat Astrocytes

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Volume 17, Number 19, Issue of October 1, 1997 pp. 7278-7287
Copyright ©1997 Society for Neuroscience