Metabotropic Glutamate Receptor Activation Modulates Kainate and Serotonin Calcium Response in Astrocytes

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Volume 17, Number 5, Issue of March 1, 1997 pp. 1825-1837
Copyright ©1997 Society for Neuroscience

Metabotropic Glutamate Receptor Activation Modulates Kainate and Serotonin Calcium Response in Astrocytes

Laurel L. Haak¹, H. Craig Heller¹, and Anthony N. van den Pol²
¹ Department of Biological Sciences, Stanford University, Stanford, California 94305-5020, and ² Section of Neurosurgery, Yale University School of Medicine, New Haven, Connecticut 06520

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Although metabotropic glutamate receptor (mGluR) modulation has been studied extensively in neurons, it has not been investigatedin astrocytes. We studied modulation of glutamate-evoked calciumrises in primary astrocyte cultures using fura-2 ratiometric digitalcalcium imaging. Calcium plays a key role as a second messengersystem in astrocytes, both in regulation of many subcellular processesand in long distance intercellular signaling. Suprachiasmaticnucleus (SCN) and cortical astrocytes showed striking differencesin sensitivity to glutamate and to mGluR agonists, even afterseveral weeks in culture. Kainate-evoked intracellular calciumrises were inhibited by concurrent application of the type I andII mGluR agonists quisqualate (10 µM), trans-(±)-1-amino-1,3-cyclopentanedicarboxylate(100-500 µM), and (2S-1 $'$ S-2 $'$ S)-2-(carboxycyclopropyl)glycine (L-CCG-I)(10 µM). Inhibition mediated by L-CCG-I had long-lasting effects(>45 min) in ~30% of the SCN astrocytes tested. The inhibitioncould be mimicked by the L-type calcium channel blocker nimodipine(1 µM) as well as by protein kinase C (PKC) activators phorbol12,13-dibutyrate (10 µM) and phorbol 12-myristate 13-acetate (500nM), and blocked by the PKC inactivator (±)-1-(5-isoquinolinesulfonyl)-2-methylpiperazine(200 µM), suggesting a mechanism involving PKC modulation of L-typecalcium channels. In contrast, mGluRs modulated serotonin (5HT)-evokedcalcium rises through a different mechanism. The type III mGluRagonist L-2-amino-4-phosphonobutyrate consistently inhibited 5HT-evokedcalcium rises, whereas in a smaller number of cells quisqualateand L-CCG-I showed both inhibitory and additive effects. Unlikethe mGluR-kainate interaction, which required a pretreatment withan mGluR agonist and was insensitive to pertussis toxin (PTx),the mGluR modulation of 5HT actions was rapid and was blockedby PTx. These data suggest that glutamate, acting at several metabotropicreceptors expressed by astrocytes, could modulate glial activityevoked by neurotransmitters and thereby influence the ongoingmodulation of neurons by astrocytes.
Key words: astrocytes; suprachiasmatic nucleus; calcium; serotonin; kainate; metabotropic glutamate receptors; ionotropic glutamate receptor; digital imaging; cortex

INTRODUCTION

Astrocytes are an integral part of signal processing in the nervous system. They express functional receptors for severalneurotransmitters and modulators and show stereotyped calciumresponses from internal or external sources (Murphy and Pearce,1987; Barres et al., 1988; Barres et al. 1990; McCarthy and Salm,1991; Hösli and Hösli, 1993; Sontheimer, 1994). Changes in intracellularcalcium not only modify glial physiology, but they also seem tobe involved in complex intercellular communication networks (forreview, see Finkbeiner, 1993). Astrocytes can control neuronalexcitability directly (Nedergaard, 1994; Parpura et al., 1994)or indirectly through modulation of extracellular potassium (Barres,1991) or glutamate levels (Shao and McCarthy, 1994; Gallo andRussell, 1995).

Astrocytes have been studied in regard to their function in various physiological states, including development (LaMantia,1995), glucocorticoid neurotoxicity (Horner et al., 1990; Virginet al., 1991), and ischemia (Tombaugh and Sapolsky, 1990; Duganet al., 1995; Papadopoulos et al., 1996), and in psychiatric disorders,including anxiety and depression (Whitaker-Azmitia et al., 1993).Glutamate and serotonin (5HT) play critical roles in several ofthese states (LaMantia, 1995; Saxena, 1995). In addition, resultsfrom several labs have suggested that astrocytes may play a rolein the control of circadian rhythmicity (Ewer et al., 1992; vanden Pol et al., 1992; Lavialle and Servière, 1993, 1995; vanden Pol and Dudek, 1993; Bennett and Schwartz, 1994; Prosser etal., 1994).

Glutamate is the major excitatory neurotransmitter in the CNS, including the cortex and the suprachiasmatic nucleus (SCN).In the SCN it acts as the primary excitatory transmitter conveyingthe photic signal from the retina that entrains the circadianclock. Modulation of glutamate transmission has been studied extensivelyin neurons in the CNS. In hypothalamic neurons, modulators suchas neuropeptide Y (NPY) and adenosine depress glutamatergic transmissionby either a pertussis toxin (PTx)-sensitive G-protein-coupledpathway or by inhibition of voltage-activated calcium channels(VACCs). In neurons, glutamate-evoked calcium rises were depressedby adenosine, whereas in astrocytes calcium responses were potentiatedby adenosine (Obrietan et al., 1995).

Interactions between ionotropic and metabotropic receptors have been shown in several neuronal systems (Glaum and Miller,1993; Nakanishi, 1994; Schoepp, 1994; Gereau and Conn, 1995; Gormanet al., 1995). Modulation may occur by downregulation of ion channelreceptor sensitivity directly or by cross-regulation through anothertransmitter system or second messenger pathway. mGluRs have beenshown in neurons to modulate potassium channel function (Gerberand Gähwiler, 1994) and calcium channel currents (Sahara andWestbrook, 1993; Chavis et al., 1995). This interaction is sometimessensitive to G-protein inhibitors such as PTx but not to secondmessenger blockade, raising the possibility of a direct actionof the G-protein in neurons (Lester and Jahr, 1990; Swartz andBean, 1992; Chavis et al., 1994; Ikeda et al., 1995; Choi andLovinger, 1996).

Metabotropic glutamate receptors (mGluRs) are divided into three groups based on sequence homology of the cloned receptorsand on group-selective agonists and second messenger pathways(Nakanishi, 1992, 1994; Nakanishi and Masu, 1994). All three groupsof mGluRs are expressed in SCN cells (van den Pol, 1994; van denPol et al., 1995, 1996a). Modulatory interactions between ionotropicand mGluRs have not been studied in astrocytes.

In this paper, we describe a difference in glutamate sensitivity in astrocytes derived from SCN and cortex. We investigatedhow agonists for specific classes of mGluRs modulated astrocyteresponsiveness to 5HT and to the ionotropic GluR (iGluR) agonistkainate. We show that mGluR agonists not only acutely enhanceor depress transmitter-elicited calcium rises, but also may inducea depression in kainate responsiveness that lasts even after themGluR agonist is gone. We also demonstrate transmitter-specificmodulatory transduction pathways within astrocytes.

Some of these data have been published previously in abstract form (Haak et al., 1995).

MATERIALS AND METHODS
Tissue culture Neonatal (E22-P2) Sprague Dawley rat brains (Simonsen, Gilroy, CA) were washed three times in ice-cold HEPES-buffered salinesolution (HBSS) (Life Technologies, Grand Island, NY). Coronalslices (525 µM) were prepared using a tissue chopper and washedin ice-cold HBSS. A polished flat 20 gauge stainless steel needlewas used to punch the SCN (see Fig. 1A) and medial pieces of theneocortex from the same slice. Individual tissue punches wereplaced into 0.5 ml thin-walled microcentrifuge tubes containing10 µl of cold HBSS and washed twice with 100 µl of HBSS lackingcalcium and magnesium (HBSS). Punches were incubated overnight at 4°C in 100 µl of HBSS containing 0.2× trypsin-EDTA (Life Technologies). After incubationfor 30 min at 37°C, trypsin was removed, and 100 µl of warm growthmedium was added. Each punch was triturated gently to create asingle-cell suspension and then was plated on a 22 mm² poly-D-lysine-coated glass coverslip in a single well of a 6-welltissue culture plate. Coverslips had been soaked previously overnightin Cleaning Concentrate (Bio-Rad, Richmond, CA), rinsed for 1hr in deionized water, and then dried and autoclaved. To increasecell density, dispersed punches were plated within a 7-mm-diameterglass cloning ring placed on the coverslip. Two hours after plating,3 ml of growth medium was added per well, and rings were removed.Cultures were maintained in a Napco 6100 incubator at 37°C and5% CO₂ in growth medium: glutamate- and glutamine-free MEM (LifeTechnologies) supplemented with heat-inactivated 10% bovine calfserum (Hyclone, Logan, UT), 100 U/ml penicillin/streptomycin (LifeTechnologies), and 1 mM kynurenate (RBI, Natick, MA) (Finkbeinerand Stevens, 1988). Growth medium was replaced weekly. Cells wereused after at least 14 d in vitro.
Fig. 1. Immunocytochemistry. A, Confocal image of a propidium iodide-stained brain slice from a neonatal rat containing the bilateralSCN. The SCN has been punched out of the right side for use intissue culture, and this micrograph shows the remaining tissueslice. Bar, 50 µm. B, D, GFAP immunoreactivity was found in SCNand cortical astrocytes. C, E, In contrast, both cultures werenegative for the neuronal marker MAP2. Bar, 25 µm.
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Histology Verification of SCN cultures. Slices and punches were made as described above. Chilled slices were fixed overnight at 4°Cin 4% paraformaldehyde and 0.3% glutaraldehyde and then incubatedfor 20 min with 2 µg/ml propidium iodide (Molecular Probes, Eugene,OR). Staining was visualized using a Molecular Dynamics Multiprobe2010 confocal microscope. Excitation wavelength (Argon/Kryptonlaser) was 488 nm; the emission wavelength was attenuated below590 nm. Laser illumination was attenuated to 10% maximum intensityby neutral density filters. An example of a slice from which theSCN was punched out for culture is seen in Figure 1A.

Immunocytochemistry. Cells growing on coverslips were rinsed once in 100 mM PBS [containing (in gm/l): 8 NaCl, 0.2 KCl, 1.44Na₂HPO₄, 0.24 KH₂PO₄] and then fixed in ice-cold anhydrous methanol.After cells were fixed, they were washed with four rinses in PBSand then stained, following the protocol included in the VectastainElite ABC Kit (Vector Labs, Burlingame, CA). In brief, cells wereincubated with 1.5% goat serum diluted in PBS. After 30 min, serumwas removed and primary mouse monoclonal antibody diluted in 1.5%goat serum was added as follows: microtubule-associated protein(MAP2) (Sigma, St. Louis, MO) 1:500 dilution, glial fibrillaryacidic protein (GFAP) (Novocastra/Vector Labs) 1:100 dilution.Cells were incubated with primary antibody for at least 1-6 hrand then washed with three rinses of PBS, at which time the secondarygoat anti-mouse antibody (ABC Kit) was added for 30 min. Thencells were washed with three rinses of PBS, incubated with ABCcomplex (ABC Kit) for 30 min, and again washed three times withPBS. Finally, staining was visualized with diaminobenzidine intensifiedwith NiCl₂, added to the cells for 1-2 min. To stop the peroxidasereaction, cells were rinsed in PBS.
Calcium digital imaging Before imaging, cells were incubated for 30 min at 37°C with 5 µM fura-2 acetoxymethylester (Molecular Probes) in a HEPES-bufferedperfusion solution (137 mM NaCl, 25 mM glucose, 5 mM KCl, 1 mMMgCl₂, 3 mM CaCl₂, 10 mM HEPES, pH 7.4). Cells were then washed,loaded into a 180 µl laminar flow perfusion chamber (Forscheret al., 1987), and perfused with HEPES buffer at a constant rateof 1 ml/min. For experiments using zero-calcium HEPES buffer,we omitted CaCl₂ from the perfusion solution and added 1 mM EGTAand a total of 10 mM MgCl₂. Perfusion solutions were applied fromreservoirs using individual capillary lines abutting the laminarflow cell surface. Switching between solutions was accomplishedby opening and closing stopcock valves on individual lines. Solutionsmoved uniformly and rapidly across the perfusion chamber, withcomplete washout in ~5 sec. All experiments were performed atroom temperature. In the course of these experiments and the preliminarywork leading to them, we tested 9360 SCN astrocytes and 4700 corticalastrocytes from 35 separate sets of cultures, with 8-18 coverslipcultures per set.

Cells were imaged using a 40× Olympus DApo objective with high ultraviolet transmittance on a Nikon Diaphot 300 inverted microscope.Individual cells were tagged with a 5 × 5 pixel square, and 340/380nm Ca²⁺ ratio images were captured every 2 sec and recorded using FLUORsoftware (Universal Imaging, West Chester, PA) running on a 486PC. Switching between 340 and 380 nm wavelengths was accomplishedusing a Sutter (Novato, CA) Lambda 10 controller and filter wheel.Excitation light was provided by a 150 W xenon lamp (Optiquip,Highland Mills, NY) and was attenuated by 90% to minimize photobleaching and photo toxicity and to maximize recording time. Fluorescenceemitted by the cells was passed through a 480 nm filter on themicroscope and into a Hamamatsu 2400 silicon-intensified-targetvideo camera. Between 10 and 40 cells were recorded simultaneouslyin a single experiment. Ratiometric fluorescent values collectedin this way were converted to Ca²⁺ concentrations with the calibration method described by Grynkiewiczet al. (1985) using fura-2 and calcium standard solutions fromMolecular Probes. Calibrated Ca²⁺ data were analyzed on an Apple Macintosh computer using IgorProSoftware (WaveMetrics, Lake Oswego, OR). In the figures presented,each trace represents the ratiometric calcium response of oneastrocyte.

Data for histograms representing peak heights were calculated by subtracting from the peak Ca²⁺ rise an averaged baseline Ca²⁺ level from the 3 min just before the Ca²⁺ rise. Increases of >60 nM over baseline were pooled and averaged.Data are from two to five experiments on different cultures andare presented as the average nanomolar Ca²⁺ rise ± SEM. To determine statistical significance we used a Student'st test, unless mentioned otherwise.

Chemicals. Sodium glutamate and poly-D-lysine hydrobromide (MW >300,000) were purchased from Sigma; kynurenate, trans- (±)-1-amino-1,3-cyclopentanedicarboxylate(t-ACPD), L-2-amino-4-phosphonobutyrate (L-AP4), kainate, quisqualate,serotonin-creatinine complex, PTx, phorbol 12-myristate 13-acetate(PMA), phorbol 12,13-dibutyrate (PDBu), and nimodipine from RBI(Natick, MA); and 2S-1 $'$ S-2 $'$ S)-2-(carboxycyclopropyl)glycine (L-CCG-I)and (±)-1-(5-isoquinolinesulfonyl)-2-methylpiperazine (H-7 dihydrochloride)from Tocris-Cookson (St. Louis, MO).

RESULTS

Glutamate response differs in SCN and cortical astrocytes
Glutamate dose-responses Astrocytes derived from SCN and cortex showed different calcium responses to glutamate. To determine the dose-response relations,astrocyte cultures were tested with a range of GluR agonist concentrations,applied twice for 30 sec each. Each concentration was tested onat least three cultures. Only cells that responded to both applicationswith a calcium rise at least twice that of basal fluctuations(noise) were counted as responders. Results are expressed as apercentage of cells responding per total number of cells testedfor each concentration or as the mean change in cytosolic calciumvalues. The morphology and GFAP staining intensity of astrocytesfrom SCN and cortex appeared similar (Fig. 1B,D). The cultureswere primarily astrocytes; immunostaining with an antibody againstthe neuronal antigen MAP2 did not reveal neurons in these cultures(Fig. 1C,E). Although the morphology of the astrocyte cultureslooked similar, SCN and cortex astrocytes showed marked differencesin glutamate sensitivity (Fig. 2A,B, dotted lines). Although only33% (n = 211) of the SCN astrocytes responded to 100 µM glutamate,almost all cells (95%, n = 151) responded in cortical astrocytecultures.
Fig. 2. GluR agonist dose-response curves in astrocytes. A, B, Dose-response curves for SCN and cortical astrocytes for glutamate(dotted lines), kainate, and t-ACPD. The number of cells thatshowed a repeatable calcium rise to each concentration testedwas plotted, and a curve was fit to the response using the logisticfunction (IgorPro). EC₅₀ for glutamate, kainate, and t-ACPD incortical astrocytes was ~30 µM. In contrast, the EC₅₀ to kainatein SCN astrocytes was ~100 µM. t-ACPD and glutamate evoked a calciumrise in <50% of SCN astrocytes.
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Specific GluR agonist dose-responses Because glutamate stimulates several subtypes of glutamate receptors, we tested agonists for specific GluR subtypes to determinewhether the reduced responsiveness of SCN cells was a result ofcomparatively lowered response at all GluRs. By using the samedose-response protocol described above for glutamate, we foundthat SCN astrocytes were severalfold less sensitive to the ionotropicGluR agonist kainate (n = 263) than were cortical astrocytes.The mGluR agonist t-ACPD rarely evoked calcium rises in SCN astrocytes(n = 241), even at doses up to 1 mM (Fig. 2A). In contrast, corticalastrocytes showed dose-responses to glutamate, kainate (n = 287),and t-ACPD (n = 306) that were very similar to each other (Fig.2B). Although the response to individual agonists was differentbetween cortex and SCN, >90% of the astrocytes from each regionresponded to some glutamate receptor agonist.

Modulation of kainate responses by mGluRs
Using doses of kainate to which 50% of the cells responded (EC₅₀), we investigated the modulation of kainate-evoked calciumrises by mGluR agonists. Repeated application of kainate evokedcalcium rises with <15% variation between peaks (Fig. 3A). InSCN astrocyte cultures, activation of mGluRs inhibited kainate-evokedcalcium rises (Fig. 3B,C). We tested four mGluR agonists: t-ACPD,which stimulates both type I and II mGluRs; quisqualate, whichstimulates both AMPA iGluRs and type I mGluRs; L-CCG-I, whichis fairly specific for type II receptors; and the specific typeIII mGluR agonist L-AP4 (Schoepp, 1994; Pin and Duvoisin, 1995;Roberts, 1995). t-ACPD (500 µM, n = 71/78, $-$ 42.8 ± 1.4%; 100 µM,n = 33/72, $-$ 33.3 ± 3.1%), quisqualate (10 µM, n = 123/145, $-$ 58.3± 2.0%), and L-CCG-I (10 µM, n = 43/52, $-$ 43.7 ± 3.1%) inhibitedkainate-evoked calcium rises by the percentages given and in thenumber (n) of astrocytes indicated. The method used to determinepercentage change is described in the legend to Figure 3. Thetype III agonist L-AP4 (10 µM) was effective in only a few cells(n = 9/53, $-$ 40.2 ± 5.7%).
Fig. 3. mGluR-iGluR modulation in astrocytes. A, Representative astrocyte showing reproducible amplitude of kainate-evoked calciumrises. Kainate (100 µM) was applied at all arrows for 30 sec.There is no significant difference between peak heights. Maximumvariation between peaks was <15%. B, A representative calciumtrace demonstrating the inhibition of kainate calcium rises inone SCN astrocyte tested with four mGluR agonists, demonstratingcomplex modulatory actions in a single astrocyte. mGluR agonists(500 µM t-ACPD, 10 µM quisqualate, 10 µM L-AP4, or 10 µM L-CCG-I)were applied concurrently (large-ended arrows) with 100 µM kainate,or astrocytes were pretreated for 2-3 min with the mGluR agonist(bars) before kainate was applied for 30 sec. This particularcell did not show any apparent long-lasting inhibition by L-CCG-Ithat was seen in other cells (see Fig. 4). C, Kainate-evoked calciumrises were depressed by mGluR agonists in astrocytes. For eachastrocyte, amplitude of kainate-evoked calcium rises was comparedto the calcium rise evoked by kainate plus mGluR agonist. Differencein amplitude was normalized by dividing by the kainate-only amplitudeand multiplying by 100 to obtain a percentage change. Only cellsthat showed a calcium rise to kainate >60 nM over basal levelswere included in the analysis. We used a criterion of a 15% change(+ or $-$ ) in calcium rise amplitude as the low cutoff indicatinga modulatory interaction. Negative numbers indicate an inhibitionof the kainate calcium rise by mGluR agonist. Although both quisqualateand t-ACPD usually depressed calcium rises, in a few cases theyenhanced kainate calcium rises (see text). The number of respondingcells is shown below the bars. The flags represent the SEM.
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In some cases, quisqualate (10 µM, n = 15/45, 280.6 ± 84.4%) and t-ACPD (100 µM, n = 15/72, 189.4 ± 51.9%) increased the kainate-evokedcalcium rise, consistent with their ability to stimulate morethan one glutamate receptor subtype. In cortical glial cultures,100 µM t-ACPD induced calcium rises by itself but decreased themaximal amplitude of the kainate-evoked calcium rises (n = 68/68, $-$ 74.1 ± 1.7%). Thus, the t-ACPD-mediated depression of the kainateresponse was greater in cortical than in SCN astrocytes. Dose-responsecurves to t-ACPD (Fig. 2) suggest that SCN and cortical astrocytecultures contain different populations of functional mGluR receptors.In addition, AMPA and quisqualate show a differential abilityto evoke calcium rises in SCN and cortical cultures. In cortex,most astrocytes show calcium rises in response to AMPA (10 µM,81.8%, n = 154) and quisqualate (10 µM, 99.0%, n = 105). FewerSCN astrocytes showed calcium rises: 43.9% responded to quisqualate(n = 82). Even at 100 µM, only 43.7% showed a calcium responseto AMPA (n = 137), whereas >95% of cortical astrocytes respondedto 100 µM AMPA. Taken together, these results suggest that mGluRmodulation in cortical and SCN astrocytes may involve differentmGluR subtypes.
mGluR agonist treatment evokes long-lasting effects In addition to acute effects, t-ACPD and L-CCG-I evoked a long-lasting depression of subsequent kainate-evoked calcium risesin some SCN and cortex astrocytes (Fig. 4A,B) but had little detectableeffect on others (Fig. 4C). Long-lasting depression was definedas a minimum 15% reduction of kainate-evoked calcium rise by themGluR agonist coupled with subsequent kainate-evoked calcium risesthat did not show recovery to pre-mGluR levels. The post-mGluRkainate rise had to be depressed by within 10% or more of thepercentage decrease found during mGluR application. Long-lastingdepression was seen in 33% (20/60) of SCN astrocytes. L-CCG-Idepressed the mean kainate-evoked cytosolic calcium level by 38.3± 3.4%, from 707 ± 108 to 466 ± 76 nM (p < 0.001; paired t test).Kainate responses 5-20 min after L-CCG-I was removed remaineddepressed by 36.9 ± 2.3%. In contrast, astrocytes that did notrespond to L-CCG-I in the same experiments (n = 40/60) showedlittle decrease in the amplitude of kainate responses over thesame period ( $-$ 8.7 ± 3.9%; p < 0.001 vs cells showing long-lastingdepression; t test). In separate experiments, we demonstratedthat L-CCG-I treatment evoked long-lasting depression of kainate-evokedcalcium rises that extended beyond 45 min (n = 12/55, $-$ 58.4 ±4.2%). This depression was significantly different (p < 0.001;t test) from calcium rises in astrocytes in the same experimentsnot showing an initial depression by L-CCG-I (n = 43/55).
Fig. 4. Long-lasting depression. L-CCG-I evokes a long-lasting depression of kainate-evoked calcium rises in astrocytes; 10 µM L-CCG-Iwas applied continuously throughout time indicated by horizontalbar. A, B, In these SCN astrocytes, kainate calcium rises weredepressed by L-CCG-I and did not recover to levels seen beforeL-CCG-I was applied. C, In this astrocyte from the same experimentas A and B, little effect of L-CCG-1 was found. Long-lasting depressionwas seen in 20/60 SCN astrocytes. Depressed cells showed a statisticallysignificant difference (p < 0.001) in mean calcium rise when comparedwith all other cells not showing depression and when comparedwith controls in the absence of L-CCG-1.
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Signal transduction pathways: G-proteins To elucidate how mGluR agonists might decrease responsiveness to kainate, we focused on signal transduction pathways. BecausemGluRs act through G-proteins, we asked which G-proteins werenecessary for inhibition. Cultures were treated overnight withthe G_i/G_o protein inhibitor PTx (200 ng/ml). PTx did not blockthe inhibitory effects of 10 µM quisqualate (n = 85), 500 µM t-ACPD(n = 48), or 10 µM L-CCG-I (n = 48), indicating that the inhibitoryactions of these mGluR agonists could not be accounted for solelyby action via a G_i/G_o protein-coupled receptor (Fig. 5). Of interest,PTx treatment dramatically increased the number of cells thatshowed a calcium rise on application of 500 µM t-ACPD from 0/143to 56/108 cells, suggesting that there may be specific signaltransduction systems that are constitutively inactivated or overruledin SCN astrocytes. PTx may block type II mGluRs and thereby uncovera response to PTx-insensitive type I mGluRs. In parallel, theinhibitory effects of quisqualate were potentiated by PTx treatment(without PTx, $-$ 50.9 ± 2.5%; with PTx, $-$ 77.6 ± 2.3%; p < 0.001;t test).
Fig. 5. Effects of PTx on mGluR-mediated depression of kainate calcium rises. Overnight treatment of SCN astrocytes with 200 ng/mlPTx induced little significant effect on the percentage decreaseof kainate-evoked calcium rises mediated by either t-ACPD or L-CCG-I;however, quisqualate-mediated depression seemed to be enhancedby PTx (*p < 0.001). Percentage decrease was calculated as describedin Figure 3.
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Signal transduction pathways: protein kinase C (PKC) Brief exposure (5-30 sec) to 500 µM t-ACPD or 10 µM L-CCG-I had no effect on subsequent kainate responses; however, when cellswere pretreated for at least 2-3 min, a significant depressionof subsequent kainate responses was seen. Modulatory pathwaysthat are limited to membrane components are very rapid (Hille,1994), so the long time course of the mGluR-kainate depressionindicated that a second messenger pathway was involved. One possibleinhibitory transduction pathway involves PKC. Incubation withthe PKC activators PMA (500 nM, n = 61, $-$ 80.9 ± 2.4%) or PDBu(10 µM, n = 57, $-$ 82.8 ± 1.2%) depressed kainate-evoked calciumrises (Fig. 6A-C). The inhibitory effects of L-CCG-I (n = 37)and t-ACPD (n = 68) could be reduced by 30 min pretreatment withthe PKC inactivator H-7 (200 µM). A calcium trace from a representativeSCN astrocyte is shown in Figure 6D1. Before H-7 treatment, t-ACPDdepressed the kainate-mediated calcium rise by $-$ 32.9 ± 2.4%. H-7significantly eliminated the t-ACPD depression of kainate-evokedcalcium rises in 26 of 68 cells (Fig. 6D2) and increased the kainateresponse in the presence of t-ACPD by 55.9 ± 16.5% (p < 0.001;paired t test). These results implicate PKC in the inhibitionof kainate responses by mGluRs.
Fig. 6. Stimulation of PKC mimics effects of mGluR activation in SCN astrocytes. A, PDBu (10 µM) applied for 3 min before 10 µM L-CCG-Ipretreatment further inhibited 100 µM kainate calcium rise (arrows)and also evoked a long-lasting depression of subsequent kainatecalcium rises. B1, B2, PDBu mimicked the depression of kainatecalcium rises mediated by 500 µM t-ACPD. PDBu generated a long-lastingdepression of kainate-evoked calcium rises that did not recoverto pre-PDBu levels. C, Both PDBu (10 µM) and PMA (500 nM) depressedkainate-evoked calcium rises. Astrocytes were tested with 30 seckainate applications, treated with PDBu or PMA for 3 to 5 min,washed for 30 sec, and then retested with kainate. Percentagedecrease was calculated as described in Figure 3. D1, The inhibitoryeffects of t-ACPD could be reduced by the PKC inhibitor H-7. Cellswere treated with 200 µM H-7 for 20 min before cells were retestedwith t-ACPD. D2, Depression of kainate-evoked calcium rises byt-ACPD was reversed significantly by treatment with H-7 in 26/68astrocytes (pre-H-7, $-$ 32.9 ± 2.4%; post H-7, 55.9 ± 16.5; p <0.001; paired t test).
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mGluR agonists modulate VACCs Part of the calcium rise with kainate stimulation may be attributable to activation of voltage-gated calcium channels. Wenext tested the hypothesis that mGluR agonists inhibited kainate-evokedcalcium rises by blocking a calcium channel. Kainate-evoked calciumresponses disappear when cells are incubated in buffer lackingextracellular calcium (Cornell-Bell et al., 1990). In our experiments,kainate-evoked calcium responses were mediated in large part byVACCs, because evoked rises were inhibited by the L-type VACCblockers nimodipine or nickel. Nimodipine (1 µM) inhibited byat least 20% the kainate-evoked calcium rise in 123/146 cells(mean decrease 63.3 ± 1.9%). Nickel (100 µM) showed parallel effectsin 84/93 cells (mean decrease 58.9 ± 2.3%).

Cell depolarization caused by application of 55 mM potassium also evoked calcium rises via VACCs. Potassium evoked repeatablecalcium rises with <15% variation between peaks (n = 16) (Fig.7A). In SCN astrocyte cultures, nimodipine (1 µM) transientlyblocked calcium rises evoked by 55 mM potassium in all cells tested(n = 51; pre/post nimodipine, $-$ 13.3 ± 2.0%; during nimodipine, $-$ 79.1 ± 2.2%; p < 0.001; paired t test). Most of the potassium-evokedcalcium rise was blocked by nimodipine; other calcium channelantagonists were not tested. Calcium rises elicited by potassiumwere inhibited by the PKC activator PMA (500 nM, n = 14/18, $-$ 46.0± 5.0%) (Fig. 7D) and mGluR agonists (Fig. 7B). Quisqualate (10µM) evoked long-lasting calcium rises, consistent with its abilityto stimulate type I mGluRs. Quisqualate reduced the amplitudeof potassium-evoked calcium rises in 44 of 47 cells (Fig. 7C1).t-ACPD (500 µM, n = 42/58, $-$ 42.9 ± 2.5%), and L-CCG-I (10 µM,n = 42/58, $-$ 34.8 ± 1.8%) (Fig. 7C) inhibited potassium-evokedcalcium rises. Furthermore, both t-ACPD and L-CCG-I (Fig. 7C3)generated a long-lasting depression of subsequent potassium-evokedcalcium rises to an amplitude (t-ACPD: $-$ 40.5 ± 3.7% from 258.0± 33.0 nM to 154.7 ± 22.48 nM, p < 0.001, paired t test; L-CCG-I: $-$ 32.0 ± 4.4% from 211.3 ± 43.5 nM to 139.8 ± 26.8 nM, p < 0.01,paired t test) and percentage (t-ACPD: 30.3% of cells; L-CCG-I:27.6% of cells) similar to those of the mGluR depression of kainateresponses resulting in long-lasting depression. Together, thesedata showing long-lasting effects of t-ACPD and L-CCG-I on kainate-and potassium-evoked calcium rises suggest that activation oftype II mGluRs depressed kainate-evoked calcium rises by reducingthe conductance of voltage-gated calcium channels.
Fig. 7. mGluR activation depresses potassium-evoked calcium rises. A1, A representative calcium trace from an SCN astrocyte showingrepeatability of 55 mM potassium-evoked calcium rises. A2, Meanpotassium-evoked calcium rise (n = 16). Difference between peakswas not statistically significant and did not exceed 15%. B, t-ACPD(500 µM), quisqualate (10 µM), and L-CCG-I (10 µM) all depressedcalcium rises evoked by depolarizing SCN astrocytes with 30 secpulses of 55 mM potassium. Percentage change in evoked calciumrise was calculated as described in Figure 3. C1, A representativecalcium trace from an SCN astrocyte showing quisqualate coulditself evoke calcium rises, and it reduced the maximal responseto potassium. C2, A calcium trace from an SCN astrocyte showingt-ACPD depressing potassium-evoked calcium rises (arrows). t-ACPDwas applied for the duration indicated by the horizontal bar.C3, Application of L-CCG-I evoked long-lasting depression of subsequentpotassium-evoked calcium rises in this representative SCN astrocyte.D, The PKC activator PMA (500 nM) reduced calcium rises evokedby 55 mM potassium. The cell shown here exhibited one of the mostdramatic responses to PMA seen in these cells.
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mGluR-5HT receptor interactions
5HT receptors are found throughout the brain, and high densities are found in the SCN and cortex. Many 5HT receptors seemto be G-protein-coupled (Chilmonczyk, 1995; Saxena, 1995; Sleightet al., 1995). 5HT receptors have been localized in the SCN (Lovenberget al., 1993), and 5HT agonists have been shown to modulate glutamatergicactivity in the circadian system in vivo (Rea et al., 1994; Srkalovicet al., 1994). To determine which glutamate receptors may be involvedin modulation of 5HT responses, we investigated mGluR modulationof 5HT actions in SCN astrocytes.
Similar 5HT response in SCN and cortex astrocytes Unlike the differential responsiveness to glutamate described above, SCN and cortical astrocytes showed very similar calciumresponsiveness to 5HT (Fig. 8). Almost all SCN (87%, n = 199)and cortical (82%, n = 102) astrocytes showed a calcium rise to1 µM 5HT. The construction of dose-response curves revealed thatthe EC₅₀ was ~100 nM in astrocytes from both areas.
Fig. 8. Dose-response curves for 5HT in SCN and cortical astrocytes. SCN (n = 199) and cortical (n = 102) astrocytes show similarresponses to 5HT. Cultures were tested with a range of duplicatedoses of 5HT. Only astrocytes that showed calcium rises twicethat of basal calcium variation to both 5HT applications wereincluded as responders for that dose. At least three cultureswere tested for each dose. Percentage responders were calculatedas described earlier for glutamate agonist dose-response curves.Standard error bars are shown on the 5HT dose-response curve inSCN astrocytes for the following doses: 10 nM, 100 nM, 1 µM, and10 µM (four experiments each).
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mGluR modulation of 5HT calcium responses Glutamate and 5HT interacted to produce calcium rises different from those produced when each transmitter was applied alone(Fig. 9A). In SCN astrocyte cultures, 100 µM glutamate plus 100nM 5HT showed synergistic (Fig. 9A1, A2) or additive (Fig. 9A3)effects in 31% of cells (n = 128). Synergism between 5HT and glutamatewas found in astrocytes where one of the transmitters had evokedlittle calcium rise by itself but greatly amplified the responseto the other transmitter. Similarly, in 31% of cortical astrocytesthere was also an additive effect on calcium levels when cellswere perfused concurrently with 10 µM glutamate and 100 nM 5HT(n = 84). This additive effect was not attributable to activationof the kainate-sensitive iGluRs because in SCN (n = 64) and cortical(n = 106) cultures, 100 µM kainate did not show significant (>15%difference in peak amplitude) additive effects when applied with100 nM 5HT. Kainate seemed to show averaged (Fig. 9B1,B2) or independent(Fig. 9B3) effects when applied with 5HT; 500 µM t-ACPD (Figs.9C, 10B) inhibited the 5HT-evoked calcium rise in SCN glia (n =36/51; $-$ 37.9 ± 3.9%), indicating a modulatory role for mGluRs.
Fig. 9. Glutamate-5HT interactions. A, Glutamate (100 µM) and 5HT (10 µM) showed additive or synergistic interactions in SCN (shown)and cortical astrocytes. Calcium traces are shown from three representativecells from the same experiment. In all three cells, the 5HT +glutamate calcium rise is larger than the calcium rise evokedby either 5HT or glutamate alone. A1 and A2 show examples of synergy,whereas the cell in A3 shows an example of an additive interaction.B, Kainate (100 µM) showed no additive interaction with 5HT (10µM). B1 and B2 show interactions in two astrocytes in which thecombined application of 5HT and kainate seems to yield an averagedcalcium response. B3 shows a cell in which kainate and 5HT calciumeffects seem to be independent. C1, t-ACPD (500 µM), althoughnot evoking a calcium rise alone, completely blocked the 5HT-evokedcalcium rise in this astrocyte. C2, A cell from the same experimentshowed no effect of t-ACPD on 5HT-evoked calcium responses.
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Fig. 10. mGluR-5HT interactions. SCN and cortex astrocytes showed similar interactions between mGluR agonists and 5HT-evoked calciumrises. A, 5HT evoked repeatable calcium rises in SCN (shown) andcortex astrocytes. Here a typical control astrocyte is shown thatresponds to repeated applications of 5HT with similar amplitudecalcium rises. B, Quisqualate (10 µM), L-AP4 (10 µM), and L-CCG-I(10 µM) were applied with 5HT (100 nM), and the resultant calciumrise amplitude was compared with the rise evoked by 5HT alone.Percentage change in calcium rise was calculated as describedin Figure 3. Negative values indicate depression, and positivevalues indicate enhancement of the 5HT-evoked calcium rise. Unlikethe mGluR-iGluR interaction, quisqualate generally enhanced 5HTcalcium rises, L-CCG-I showed mixed results, and L-AP4 showeda very strong and consistent PTx-sensitive depression of 5HT-evokedcalcium rises. This indicated that different mGluR subtypes canindependently and oppositely modulate 5HT-evoked calcium rises.C1, L-AP4 (10 µM) showed rapid and repeatable depression of a5HT-evoked sustained calcium rise. C2, L-AP4 effects were blockedby overnight application of PTx (200 ng/ml).
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5HT evoked repeatable calcium rises in SCN (Fig. 10A) and cortical astrocytes if an interval of at least 5 min occurred betweenapplications. If shorter intervals were used, the amplitude ofsubsequent responses did not recover fully, resulting in smalleramplitude calcium rises caused by 5HT receptor desensitization.For that reason all tests of mGluR modulation of 5HT were performedat intervals of >5 min. Because the first application of 5HT yieldedcalcium rise amplitudes with >15% variability, this initial peakwas not included in the analysis. Experiments with specific mGluRagonists showed that 10 µM quisqualate, which activates both AMPAiGluRs and type I mGluRs, typically enhanced 5HT-evoked calciumrises (n = 49/97, 81.2 ± 9.1%) (Fig. 10B). The type I/II mGluRagonist L-CCG-I (10 µM) could enhance (n = 23/130, 83.2 ± 2.6%)or inhibit (n = 49/130, $-$ 35.7 ± 2.6%) 5HT-mediated calcium rises.Coupled with the t-ACPD inhibitory effects, these results suggestthat GluRs insensitive to kainate are responsible for the additiveeffect seen between glutamate and 5HT.

The type III mGluR agonist L-AP4 (10 µM) strongly inhibited the 5HT-evoked calcium rise in SCN astrocytes (n = 104/159, $-$ 51.4± 2.6). Cortical glia showed similar effects. Inhibition was rapid,not requiring extended pretreatment with L-AP4 (Fig. 10C), andcould be blocked completely by overnight incubation with PTx (200ng/ml, n = 77, $-$ 0.1 ± 8.8%). This indicated that a rapid, PTx-sensitivepathway was involved. This is in striking contrast to the slowerPTx-insensitive interaction described above between mGluRs andkainate.

DISCUSSION
Our results demonstrate that mGluR activation modulates calcium rises evoked by kainate and 5HT in astrocytes. Distinct mGluRsubtypes and second messenger pathways were involved in mediatingmodulatory interactions with kainate and 5HT. In addition, a novelform of long-lasting depression was demonstrated by the modulationof kainate responses by type I/II mGluR agonists L-CCG-I and t-ACPD.

Transmitter sensitivity
SCN neurons have been reported to be relatively insensitive to low concentrations of glutamate (Shibata et al., 1986; Cahilland Menaker, 1989). Indeed, in SCN slices and cultured cells,Meijer et al. (1993) found no toxic effects of 1 mM glutamateapplied for 30 min. Our results from dose-response analyses oftransmitter action show that SCN astrocytes were significantlyless sensitive to glutamate than were cortical astrocytes, suggestingthat SCN astrocytes mirror the glutamate sensitivity of neuronsin the same area. In contrast, the 5HT sensitivity of astrocytesfrom SCN and cortex is similar, suggesting that astrocytes fromthese brain regions differentially regulate which transmitterreceptors they express, and these differences are detectable invitro even after several weeks in culture.

mGluR-iGluR inhibitory interactions
Our findings are the first to demonstrate in astrocytes the modulation of glutamate and 5HT calcium responses by mGluR agonists.Glutamate mGluR-iGluR modulation has been studied in neurons.Previous studies using patch-clamp techniques in brain slicesand cultured cells have demonstrated an inhibition of kainateactions by mGluR activation in neurons. Schoepp (1994) suggestedthat type II mGluR activation could decrease postsynaptic sensitivityto kainate. t-ACPD and the type II-specific mGluR agonist DCG-IVhave been shown to inhibit AMPA/kainate neural transmission incortical-striatal cocultures (Tyler and Lovinger, 1995). TypeI and III mGluRs have also been implicated in depression of excitatorysynaptic transmission (Gereau and Conn, 1995; Wan and Cahusac,1995). Type I agonists such as t-ACPD and quisqualate are generallythought to exert their actions by stimulating phosphoinositidehydrolysis, with a consequent rise in cytoplasmic calcium. Activationof type II and III mGluRs inhibits cAMP hydrolysis and thus mightnot be expected to result in an intracellular calcium rise.

In our experiments in SCN astrocytes, quisqualate sometimes stimulated an intracellular calcium rise but often evoked no calciumrise. Similar to t-ACPD and L-CCG-I, quisqualate was effectiveat inhibiting kainate-evoked calcium rises. This may indicatethat type I and II mGluRs are both involved in mediating the mGluR-iGluRinteraction, or that a novel mGluR is involved. Alternatively,quisqualate may not be acting on a type I mGluR but instead mayalter a glutamate uptake mechanism (Littman et al., 1995) or modulatecalcium channels through a pathway not involving phosphoinositidehydrolysis (for review, see Pin and Duvoisin, 1995). We foundthat mGluR activation could generate either a rise or a fall incalcium, depending in part on which brain region the astrocyteswere derived from. Rises in cytoplasmic calcium may come fromintracellular stores in the endoplasmic reticulum. On the otherhand, inhibition of kainate-induced calcium rises indicates aninfluence of mGluRs on calcium influx from extracellular space.The differential response in different cells could be mediatedeither by different combinations of mGluRs or from complex interactionsbetween different mGluRs and their second messenger pathways.In this light, it is interesting that mRNA for all eight clonedmGluRs is expressed by SCN cells (Obreitan and van den Pol, 1996;van den Pol et al., 1996a).

In neurons, mGluR agonists may inhibit kainate-induced excitotoxicity (Bruno et al., 1994; Pin and Duvoisin, 1995). Synapticlong-term depression (LTD) may also involve mGluR modulation ofiGluR-evoked calcium influx. Specifically, induction of cerebellarLTD seems to require the coactivation of mGluRs and kainate/AMPAreceptors (for review, see Linden, 1994). LTD may act to protectcells from high levels of glutamate present perisynaptically,or it may act as a kind of gate providing an increased stimulusthreshold. NPY-mediated LTD has been demonstrated in SCN neuronsusing calcium imaging and whole-cell recording (van den Pol etal., 1996b). In the present study, we show for the first timethat t-ACPD and L-CCG-I can elicit a long-lasting depression ofthe amplitude of subsequent kainate-evoked calcium rises in SCNastrocytes. Other researchers have shown that gliotoxins seemto block cerebellar LTD (Winder et al., 1996), and mice deficientfor the astrocyte-specific intermediate filament GFAP show deficientLTD (Shibuki et al., 1996). Our results suggest that one mechanismfor long-lasting effects may involve mGluR-mediated depressionof astrocyte responses to fast transmitters.

Second messenger pathways
mGluRs depressed not only kainate-evoked calcium rises but also high potassium-evoked calcium rises. L-type VACC blockersnimodipine and nickel blocked this. Taken together, these resultssuggest that mGluR activation depressed kainate-induced calciumrises by blocking VACCs in astrocytes. Parallel studies in neuronshave reported similar mechanisms (Sayer et al., 1992; Chavis etal., 1995; Glaum and Miller, 1995; Choi and Lovinger, 1996). Itis also possible that mGluR activation modulates kainate functionby changing ligand binding or gating properties at the kainate-sensitivereceptor.

Depression of kainate calcium rises by mGluR activation could reflect direct modulation of calcium channels (Swartz, 1993;Chavis et al., 1994) by a G-protein-coupled receptor kinase (Diversé-Pierluissiet al., 1996) or by modulation via a slower pathway involvingsecond messengers (for review, see Anwyl, 1991; Hille, 1992, 1994).The mGluR inhibitory modulation of 5HT we described was rapid,required no pretreatment with the mGluR agonist L-AP4, and wasblocked by PTx. The rapid time course of inhibition suggests thata membrane-delimited, G_i/G_o protein-coupled pathway may be involved.In contrast, because PTx did not block the t-ACPD or L-CCG-I inhibitoryinteraction with kainate, a G_i/G_o protein may not be involvedin the mGluR-iGluR modulatory pathway. Also, astrocytes had tobe pretreated with t-ACPD or L-CCG-I to inhibit kainate calciumrises, suggesting that a slow-acting second messenger pathwaywas involved.

The type II mGluR has been shown to couple to its intracellular transduction system via the PTx-sensitive G_i/G_o protein (Tanabeet al., 1992, 1993). Our findings indicate that the type II mGluRreceptor in astrocytes may be coupled with a different G-protein,perhaps G_q, which is insensitive to PTx but coupled to the samesecond messenger pathway as G_i/G_o. Splice variants of mGluRs havebeen described (Nakanishi and Masu, 1994) and may be one explanationfor this transduction difference. Another possibility is thatL-CCG-I, along with t-ACPD and quisqualate, activated a type ImGluR and thereby inhibited kainate-evoked calcium rises.

mGluR-mediated inhibition did not require pretreatment of cells with quisqualate. This is consistent with work on neuronsby Lester and Jahr (1990), which showed that quisqualate rapidlyand directly inhibited calcium currents through a pathway notinvolving second messengers. Taken together, our results implicateboth type I and II mGluRs in the inhibition of kainate-evokedcalcium rises. The mGluRs could be coupled to the same (Saharaand Westbrook, 1993) or distinct (Ikeda et al., 1995) calciumchannels.

Experiments with PKC activators and inhibitors support the hypothesis that the mGluR inhibition of the kainate-evoked calciumresponse involved a second messenger pathway. The PKC activatorsPMA and PDBu mimicked the inhibition, and the PKC inactivatorH-7 blocked the effects of t-ACPD. Although its substrate is notknown in our system, PKC has been shown to inhibit coupling betweenG_q proteins and downstream second messengers (Willars et al.,1996). It is also possible that PKC acts to modify an astrocyteVACC or phosphorylates some other protein that facilitates VACCaction. PKC has been shown to modulate transmitter inhibitionof VACCs in neurons (Rich et al., 1984; Swartz, 1993; Swartz etal., 1993), and our results suggest that PKC activators may actto inhibit astrocyte VACCs.

Functional considerations
Our data demonstrate that mGluRs can exert a profound effect on kainate- and 5HT-evoked changes in cytosolic calcium in astrocytes.This could have a number of physiological ramifications. Long-distancecommunication between astrocytes, found in the SCN (van den Polet al., 1992) and elsewhere in the brain (Cornell-Bell et al.,1990), could be altered in terms of both the spatial spread ofa calcium wave and the probability of the initiation of calciumwaves. 5HT may be more likely than glutamate to initiate a calciumwave in SCN astrocytes, whereas cortical astrocytes may show agreater relative sensitivity to glutamate. One might also considertransmitter signaling in astrocytes in a spatial context. Steady-statelevels of glutamate, for instance, could activate mGluRs thatmight then act to modulate the responses to glutamate or othertransmitters rapidly and discretely released at high concentrationsfrom specific axonal terminals.

The complex modulation of astrocyte calcium levels by mGluRs could play a significant role in intercellular signaling. Increasesin glial calcium could result in the opening of calcium-activatedpotassium channels (Quandt and MacVicar, 1986; Barres et al.,1988; MacVicar et al., 1988), leading to potassium release andincreased excitability in nearby neurons. Rises in astrocyte calciumcould also increase phospholipase A2. The resulting increase inarachidonic acid would reduce glutamate uptake, resulting in anincreased extracellular glutamate level that would alter neuronalactivity (Axelrod et al., 1988; Barbour et al., 1989; Marin etal., 1991). In the SCN, as in many other areas of the brain, astrocytescan surround axodendritic contacts (van den Pol et al., 1992).The rapid movement of extracellular calcium into an astrocytefrom the extracellular space between neuron and astrocyte mightalter calcium-dependent transmitter release from an axonal boutonthat the astrocyte surrounds.

Glutamate is the primary excitatory transmitter of the cortex. It is the transmitter released by optic nerve axons in theSCN that play an important role in phase-shifting the circadianclock. We demonstrate several novel aspects of mGluR modulationin astrocytes. These reveal a level of complexity of transmitterinteractions, not only between different transmitters but evenin the response of different receptors for the same transmitter.mGluRs, acting on astrocytes, may play a pivotal role in settingthe gain for the response of these cells to transmitters, dependenton both spatially and temporally relevant cues. The long-lastingeffect of brief exposure of astrocytes to specific mGluR agonistssuggests that they may serve as a temporal integrator recordingand integrating transmitter activation over a considerable periodof time.

FOOTNOTES

Received Oct. 8, 1996; revised Dec. 12, 1996; accepted Dec. 16, 1996.

This research was supported by National Institutes of Health Grants NS 10174, NS 31573, NS 30619, and NS 34887, and the AirForce Office of Scientific Research. L.L.H. was the recipientof a National Institute of Mental Health predoctoral NationalResearch Service Award. We thank Drs. K. Obrietan and H. Srerefor helpful suggestions on this manuscript.

Correspondence should be addressed to Anthony N. van den Pol, Section of Neurosurgery, Yale University School of Medicine,333 Cedar Street, New Haven CT 06520.

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