Glutamate Induces Rapid Upregulation of Astrocyte Glutamate Transport and Cell-Surface Expression of GLAST

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The Journal of Neuroscience, December 1, 1999, 19(23):10193-10200

Glutamate Induces Rapid Upregulation of Astrocyte Glutamate Transport and Cell-Surface Expression of GLAST
Shumin Duan, Christopher M. Anderson, Becky A. Stein, and Raymond A. Swanson
Department of Neurology, University of California, San Francisco, and Veterans Affairs Medical Center, San Francisco, California 94121

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Glutamate transporters clear glutamate from the extracellular space by high-affinity binding and uptake. Factors that regulateglutamate transporter expression and activity can thereby influenceexcitatory neurotransmission. Transporter function in GABAergicand other systems has been shown to be regulated by transportersubstrates. Here, glutamate regulation of glutamate transportwas studied using primary murine astrocyte cultures that expressthe GLAST (EAAT1) and GLT-1 (EAAT2) transporter subtypes. Glutamatewas found to stimulate glutamate transport capacity (V_max) ina dose- and time-dependent manner. The maximal increase was 100%,with an ED₅₀ of 40 µM glutamate and with onset beginning ~15 minafter onset of glutamate exposure. The uptake stimulation wasreproduced by D-aspartate, which is also a transporter substrate,but not by nontransported glutamate receptor agonists. Moreover,glutamate incubation did not stimulate transport when performedin a sodium-free medium, suggesting that the stimulatory effectof glutamate is triggered by increased transporter activity ratherthan receptor activation. Treatment with the actin-disruptingagents cytochalasin B or cytochalasin D prevented the glutamate-inducedincrease in glutamate uptake. Biotinylation labeling of membranesurface proteins showed that glutamate incubation produced anincrease in GLAST expression at the astrocyte cell surface. Theseresults suggest that cell-surface expression of GLAST can be rapidlyregulated by glutamate through a process triggered by GLAST activityand involving the actin cytoskeleton. This feedback loop providesa mechanism by which changes in extracellular glutamate concentrationscould rapidly modulate astrocyte glutamate transportcapacity.

Key words: EAAT1; EAAT2; GLT-1; GLAST; actin; cytochalasin; glutamate uptake; trafficking

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Glutamate is the major excitatory neurotransmitter of the mammalian CNS (Fonnum, 1984). Glutamatergic transmission is ultimatelyterminated by binding of glutamate to its transporters and subsequentglutamate uptake (Robinson and Dowd, 1997). Glutamate uptake isaccomplished primarily by a family of Na⁺-dependent, high-affinity glutamate transporters. Five subtypesof these transporters have been identified, EAAT1-EAAT5, and thesehave differing regional, cellular, and developmental distributions(Robinson and Dowd, 1997; Gegelashvili and Schousboe, 1998). Althoughglutamate transporters are present on both neurons and astrocytes,uptake by astrocytes appears to dominate in brain (McLennan, 1976;Rothstein et al., 1996). Astrocytes in mammalian forebrain expressonly the EAAT1 (GLAST) and EAAT2 (GLT-1) subtypes, with GLASTand GLT-1 denoting the rat homologs that were first cloned anddescribed (Rothstein et al., 1994; Swanson et al., 1997; Gegelashviliand Schousboe, 1998).

Glutamate uptake is regulated at several levels. Expression of transporter protein is regulated by cAMP, neuronal factors,and in response to various brain injuries (Gegelashvili et al.,1996; Robinson and Dowd, 1997; Swanson et al., 1997; Gegelashviliand Schousboe, 1998; Schlag et al., 1998). The activity of expressedtransporters can be regulated by phosphorylation (Casado et al.,1993), sulfhydryl oxidation (Trotti et al., 1997), Zn²⁺ (Vandenberg et al., 1998), arachidonic acid (Zerangue et al.,1995), and other factors. In addition, at least some glutamatetransporter subtypes can transit between the intracellular compartmentand the membrane surface. EAAT3 has been shown to move to themembrane surface in C6 glioma cells after phorbol ester-mediatedprotein kinase C (PKC) activation (Davis et al., 1998), whereasastrocyte GLAST accumulation at the membrane may be inhibitedby phorbol ester (Correale et al., 1998). In both instances, thechanges in membrane localization of transporter correlate withchanges in glutamate transportactivity.

In the present study we show that in primary mouse astrocyte cultures expressing both GLT-1 and GLAST glutamate transportersubtypes, preincubation with glutamate produces a rapid and dose-dependentincrease in glutamate uptake activity. This effect is triggeredby glutamate transport itself, rather than by activation of glutamatereceptors. The increase in activity is associated with an increasein cell-surface expression of GLAST and is blocked by inhibitorsof actin polymerization. These results suggest a feedback loopwhereby extracellular glutamate concentrations could rapidly influenceastrocyte glutamate uptakecapacity.

Part of this work has been published previously in abstract form (Duan et al., 1998).

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Immunopure immobilized monomeric avidin and sulfo-NHS-biotin were purchased from Pierce (Rockford, IL). Genistein, CF-109203X,trans-(±)-1-amino-1,3-cyclopentanedicarboxylic acid (t-ACPD),L(+)-2-amino-4-phosphonobutyric acid (L-AP4), (S)-4-carboxyphenylglycine(4-CPG), and 1-(5-isoquinolinesulfonyl)-2-methylpiperazine (H7)were purchased from RBI (Natick, MA); 6-cyano-7-nitroquinoxaline-2,3-dione(CNQX), L-trans-pyrrolidine-2,4-dicarboxylate (t-PDC), and $alpha$ -methyl-4-carboxyphenylglycine(MCPG) were purchased from Tocris (Ballwin, MO); and 1,2-bis(2-aminophenoxy)ethane-N,N,N,N-tetra-aceticacid acetoxymethyl ester (BAPTA AM) was purchased from MolecularProbes (Eugene, OR). All other reagents were obtained from Sigma(St. Louis, MO) except wherenoted.

Cell culture preparation. Primary murine cortical astrocyte cultures were prepared as described previously (Swanson and Seid,1998). Tissue harvest was performed in accordance with NationalInstitutes of Health guidelines in a manner that minimized animalsuffering. In brief, cortices were harvested from 1-d-old mice(Simonsen, Gilroy, CA) under deep isofluorane anesthesia. Thecortices were dissociated in papain/DNase, plated in 24-well tissueculture plates in Eagle's MEM containing 10% fetal bovine serum(FBS) (Hyclone, Ogden, UT), and 2 mM glutamine, and maintainedat 37°C in a 5% CO₂ incubator. At confluence (day 12-15), thecultures were treated for 48 hr with 10 µM cytosine arabinosideto prevent proliferation of other cell types, and the medium wasreplaced with MEM containing 2 mM glutamine, 3% FBS, and 0.15mM dibutyryl cAMP to induce differentiation (Sensenbrenner etal., 1980; Swanson et al., 1997). The astrocyte cultures formeda confluent layer of process-bearing, glial fibrillary acidicprotein (GFAP)-positive cells. Each study was repeated on cellsfrom at least two different batches of astrocyte cultures at 28-35d in vitro.

Experimental procedures. Incubations and uptake assays were performed in room air, 37°C, using a balanced salt solution (BSS)containing (in mM): NaCl 135, KCl 3.1, CaCl₂ 1.2, MgSO₄ 1.2, KH₂PO₄0.5, PIPES 5, and glucose 2. pH was adjusted to 7.2 with NaOH.Osmolarity was measured with a vapor pressure osmometer (Wescor,Ogden, UT) and adjusted to 285-315 mOsm with water or NaCl ifneeded. Na⁺-free media was prepared by replacing NaCl with choline chlorideand NaOH with N-methyl-D-glucamine. Ca²⁺-deficient medium was prepared by omitting CaCl₂. All reagentswere diluted into BSS from iso-osmolar stocks prepared in BSSor Na⁺-freeBSS.

Glutamate uptake was determined after preincubation with glutamate or other agents. Preincubations were initiated 6 min afterwashing the cultures into 300 µl of BSS. The preincubations wereterminated by double washes in BSS. The cultures remained in BSSat 37°C until initiation of a glutamate uptake assay (the "washperiod"). The preincubation period was 60 min, and the wash periodwas 6 min except where otherwisenoted.

Glutamate uptake assays were initiated by adding 0.167 µCi/ml ¹⁴C-glutamate (American Radiochemicals, St. Louis, MO) plus 100µM unlabeled glutamate to the culture wells in a final volumeof 300 µl. Uptake was terminated after 7 min by two ice-cold washeswith 500 µl BSS followed by immediate lysis in ice-cold 0.1N NaOH/0.01%lauryl sulfate. Aliquots of lysates were taken for scintillationcounting and protein determinations. In separate experiments,uptake was confirmed to be linear through 10 min incubation (datanotshown).

In some studies, glutamate uptake was assessed by HPLC measurements of medium glutamate concentrations. Glutamate (100 µM)was added to the wells in a final volume of 300 µl, and the mediumwas harvested 7 min later. Glutamate concentrations were determinedby reversed-phase HPLC of the orthophthaldialdehyde derivativesusing a fluorescence detector. Peak areas were measured with NelsonAnalytical software (Norwalk, CT) and calibrated against BSS sampleswith known glutamateconcentrations.

Biotinylation. Biotinylation of cell surface proteins was performed as described by Qian et al. (1997) and Davis et al. (1998)with some modifications. After a 1 hr preincubation period anda 6 min BSS wash period, the cultures were rinsed twice with PBS/Ca-Mgcontaining (in mM): 138 NaCl, 2.7 KCl, 1.5 KH₂PO₄, 9.6 Na₂HPO₄,1 MgCl2, and 0.1 CaCl₂, pH 7.3. Cultures were then incubated insulfo-NHS-biotin solution (1 mg/ml in with PBS/Ca-Mg) for 20 minat 4°C. Biotinylation was terminated by washing twice in a quenchingsolution of PBS/Ca-Mg in which there was an equimolar substitutionof 100 mM glycine for NaCl (to maintain 300 mOsm). This was followedby an additional 45 min incubation in the quenching solution at4°C. Quenching solution was removed, and the cells were lysedwith 100 µl/well of radioimmunoprecipitation assay (RIPA) bufferwith protease inhibitors (100 mM Tris-HCl, pH 7.4, 150 mM NaCl,1 mM EDTA, 1% Triton X-100, 1% sodium deoxycholate, 0.1% SDS,1 mM iodoacetamide, 1 µg/ml leupeptin, 5 µg/ml aprotinin, and250 µM phenylmethylsulfonyl fluoride) for 1 hr at 4°C with vigorousshaking. The lysates were centrifuged at 14,000 × g for 15 minat 4°C. Three hundred microliters of the supernatant were takenfor Western analysis as the whole cell fraction. The rest of thesupernatant (600 µl) was incubated with 300 µl avidin bead suspensionfor 1 hr at room temperature with gentle shaking. The avidin-lysatesolution was then centrifuged for 15 min at 14,000 × g, and thesupernatant was taken for Western analysis as the intracellularfraction. The pellet was washed four times with 1 ml RIPA bufferand resuspended in 300 µl Laemmli buffer (62.4 mM Tris-HCl, pH7, 2% SDS, 20% glycerol, and 5% 2-mercaptethanol) for 1 hr withgentle shaking at room temperature. After centrifugation for 15min at 14,000 × g, the supernatant was taken for Western analysisas the biotinylated (plasma membrane)fraction.

For Western analysis, the protein samples were loaded and run on a 10% SDS polyacrylamide gel. Samples were electrophoreticallytransferred onto polyvinylidene fluoride membranes (BoehringerMannheim, Indianapolis, IN) and subsequently placed in blockingsolution (5% skim milk/1% bovine serum albumin in 0.1 M phosphatebuffer) for 1 hr at room temperature. The membranes were thentransferred to a blocking solution containing polyclonal anti-actinantibody diluted 1:100 plus either polyclonal anti-GLAST antibody(0.2 ng/ml) or polyclonal anti-GLT-1 antibody (0.02 ng/ml) for12 hr at 22°C. [The affinity-purified antibodies to GLAST andGLT-1 were kindly provided by Dr. Jeffrey Rothstein, Johns HopkinsUniversity, and have been previously characterized (Rothsteinet al., 1994; Swanson et al., 1997; Swanson and Seid, 1998)].The membranes were washed three times in 0.1 M phosphate buffercontaining 0.1% Tween 20 (PB-T) and placed in blocking solutioncontaining a peroxidase-labeled anti-rabbit IgG antibody (BoehringerMannheim), diluted 1:500, for 1 hr. After three additional washesin PB-T, the resulting peroxidase signal was detected using 3,3'-diaminobenzidene.The resulting bands were digitized, and densitometry was performedusing the NIH Image program. The signal for each lane was calculatedby summing the (area × (density-background)) measurements of thediscrete monomer and multimer bands produced by GLAST and GLT-1.

Statistics. Statistical differences were determined by Student's t test for two-group comparisons, or by one-way ANOVA withthe Tukey test for multiple comparisons among more than two groups,or by Dunnett's test when multiple groups were compared againsta single controlgroup.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Glutamate stimulates glutamate uptake in a dose- and time-dependent manner

Glutamate uptake under the standard assay condition of 100 µM glutamate was 7.5 ± 0.8 nmol per milligrams of protein per minute(n = 5). Preincubation of the cultures with glutamate produceda dose-dependent increase in glutamate uptake (Fig. 1A). The glutamateED₅₀ was ~40 µM, and the maximal increase in uptake rate variedfrom 40 to 100% among 32 independent experiments using a 60 minglutamate preincubation and a 6 min interval (wash period) beforethe glutamate uptake assays.

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Figure 1. Glutamate-induced stimulation of glutamate uptake. Data are means ± SEM, n $>=$ 6. A, Glutamate preincubation produced a concentration-dependent increase in subsequent glutamate uptake. B, Effect of varying glutamate preincubation periods. The glutamate preincubation concentration was 100 µM, and the wash period (interval before glutamate uptake assay) was 6 min. C, Effect of varying intervals between glutamate preincubation and beginning of glutamate uptake assay (wash periods). The glutamate preincubation concentration was 100 µM, and the preincubation period was 60 min.

The effects of differing preincubation and postincubation periods are shown in Figure 1. A significant increase in uptakewas apparent with preincubation periods as short as 15 min butnot 6 min. These intervals correspond to 21 and 12 min total elapsedtime between the onset of glutamate preincubation and the initiationof glutamate uptake assays. A maximal effect was achieved within60 min (Fig. 1B). The increased uptake was maintained when thewash period was extended from 6 min to 1 hr, but slowly declinedbetween 1 hr and 7 hr (Fig. 1C).

Eadie-Hofstee plots prepared using different glutamate concentrations during the glutamate uptake assay showed that glutamatepreincubation increased the V_max from 13.6 ± 0.3 to 22.4 ± 2.7nmol per milligrams of protein per minute (p < 0.01). There wasalso a small increase in the apparent glutamate K_m, from 72.9+ 0.3 to 91 + 17 µM, which was not statistically significant (Fig.2). These studies and all subsequent studies were performed usinga 60 min preincubation in 100 µM glutamate and a 6 min postincubationinterval before beginning glutamate uptake assays. Uptake ratesin sodium-free medium were <3% of normal medium at both high andlow glutamate concentrations (data not shown), and consequentlyno correction was made for this small contribution of Na⁺-independent uptake.

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Figure 2. A, Glutamate uptake capacity was increased in glutamate-stimulated cultures. Data are means ± SEM, n = 6. B, Data shown as Eadie-Hofstee plot. V_max was increased from 13.6 ± 0.3 to 22.4 ± 2.7 nmol per milligrams of protein per minute by glutamate preincubation (p < 0.01). The small increase in the apparent glutamate K_m was not statistically significant.

HPLC measurements of glutamate in the astrocyte culture medium confirmed an increase in glutamate uptake rate after preincubationin glutamate (Fig. 3). HPLC was used because of the possibilitythat extracellular ¹⁴C-glutamate could enter the astrocytes not only with net glutamateuptake but also by heteroexchange with unlabeled intracellularglutamate (Blitzblau et al., 1996), because intracellular glutamateconcentrations are increased by glutamate preincubation. Bulkuptake of glutamate was measured by serial HPLC determinationsof glutamate in the culture well media, whereas the standard ¹⁴C-glutamate uptake measurements were performed in sister culturewells at the same time. HPLC measurement of the nominally 100µM glutamate BSS used for the uptake assays yielded a value of104.8 ± 4.2 µM (n = 8). The glutamate remaining after 7 min incubationin culture wells preincubated with glutamate was 83.2 ± 2.0 µM,a value significantly lower than the 91.2 ± 2.0 µM glutamate measuredin wells not preincubated with glutamate (n = 12, p < 0.01). Asshown in Figure 3, the glutamate-induced increase in glutamateuptake measured by HPLC was quantitatively similar to that measuredby the ¹⁴C-glutamate method in sister culture wells.

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Figure 3. The HPLC and ¹⁴C-glutamate methods of measuring glutamate uptake produced similar measures of glutamate-induced stimulation of glutamate uptake. Experiments were performed on sister culture wells on the same day. Data are means + SEM; data were pooled from two experiments. n = 12; **p < 0.01.

Glutamate stimulation of glutamate uptake is triggered by glutamate transport rather than by glutamate receptors

Glutamate receptor agonists and transporter substrates were tested for their ability to mimic the stimulating effect of glutamateon glutamate uptake. As shown in Figure 4A, preincubation withthe ionotropic glutamate receptor agonists NMDA and kainate failedto evoke glutamate uptake increase, whereas the transporter substrateD-aspartate (D-ASP) did reproduce the glutamate effect. The apparentK_m for astrocyte D-ASP uptake is higher than that of glutamateuptake (Drejer et al., 1982; R. A. Swanson and K. Farrell, unpublishedobservations). Of note, the maximal effect produced by D-ASP wasequivalent to the maximal effect of glutamate but required highermedium D-ASP concentrations. Preincubation with the metabotropicagonists L-AP4 and t-ACPD also stimulated uptake, but interpretationof these results is complicated by the fact that both of theseagents may themselves serve as substrates for glutamate transporters(Harris et al., 1987; Ye and Sontheimer, 1998). The metabotropicreceptor antagonists MCPG and 4-CPG failed to block the stimulatoryeffect of glutamate when added with glutamate during the preincubationperiod (Fig. 4B and data not shown). A similar negative effectwas seen with CNQX, a non-NMDA ionotropic glutamate receptor antagonist.In contrast, the glutamate transport inhibitor t-PDC did preventthe stimulatory effect of glutamate at a concentration that effectivelyinhibits glutamate uptake. Moreover, glutamate, D-ASP, and t-ACPDall failed to stimulate glutamate uptake activity when preincubatedin Na⁺-free medium (Fig. 4C). Taken together, these studies suggestthat stimulation of glutamate uptake by glutamate preincubationis triggered by glutamate transporter activity rather than byglutamate receptor activation.

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Figure 4. Glutamate stimulation of glutamate uptake is triggered by glutamate transport. Data are means + SEM, n $>=$ 5; **p < 0.01. A, Preincubation with the nontransported glutamate receptor agonists kainate (KA) and NMDA did not stimulate glutamate uptake, whereas the transportable agonists t-ACPD, D-ASP, and glutamate did stimulate uptake. B, The glutamate receptor antagonists CNQX and MCPG failed to block the stimulatory effect of glutamate when added with glutamate during the preincubation period, but the glutamate transport inhibitor t-PDC did block the glutamate effect. C, Preincubations performed in Na⁺-free medium failed to stimulate glutamate uptake.

Mammalian forebrain astrocytes express only the GLAST and GLT-1 transporter subtypes. The contribution of GLT-1-mediated uptakewas assessed in glutamate-stimulated cultures by use of the GLT-1-specificinhibitor dihydrokainate (DHK) (Arriza et al., 1994; Robinsonand Dowd, 1997). As shown in Figure 5A, 1 mM DHK had only a negligibleeffect on uptake under basal conditions, and a similar negligibleeffect was seen in glutamate-stimulated cells. DHK was also usedto determine whether GLT-1 mediates the induction of uptake stimulationby glutamate. The uptake stimulation induced by 0.1 mM glutamatewas not prevented by the presence of 1 mM DHK during the preincubationperiod (Fig. 5B). These results suggest that GLT-1 does not contributeto either the increase in uptake capacity induced by glutamatepreincubation or the signaling mechanism that leads to this increase.

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Figure 5. The GLT-1-specific uptake inhibitor dihydrokainate (DHK) had negligible effects on both basal and glutamate-stimulated glutamate uptake. Glutamate concentrations were 0.1 mM both in the preincubation period and during the glutamate uptake assay. Data are means + SEM, n = 6; **p < 0.01. A, Glutamate preincubation induced a large increase in subsequent glutamate uptake rate. DHK did not attenuate this increase and did not significantly reduce uptake under control conditions. B, The presence of saturating DHK concentrations during the preincubation period similarly had negligible effects on glutamate uptake under both control and glutamate-stimulated conditions.

Signal transduction mechanisms

Glutamate transport has several effects on astrocytes, including membrane depolarization, cell swelling, and increased intracellularNa⁺. Table 1 shows results of studies designed to determine whetherglutamate-induced stimulation of uptake might be signaled throughthese effects. Glutamate uptake was not stimulated by depolarizingK⁺ concentrations, by preincubation in 180 mOsm medium (to inducecell swelling), or by incubation in veratridine, a Na⁺ channel ionophore. In addition, preincubation with 1 mM of otherNa⁺-dependent amino acid transporter substrates, cysteine, glycine,and GABA, also failed to affect the glutamate uptake activity.


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Table 1. Effects of preincubation conditions on subsequent glutamate uptake

Glutamate transporters have multiple PKC and protein kinase A (PKA) phosphorylation sites, and PKC activation by phorbol esteris reported to modulate glutamate transporter activity in severalcell systems (Casado et al., 1993; Dowd and Robinson, 1996; Conradtand Stoffel, 1997; Davis et al., 1998; Ganel and Crosson, 1998).However, pretreatment with the PKC inhibitor GF-109203X (Toullecet al., 1991) did not block the stimulatory effect of glutamateon uptake activity (Table 2), suggesting that PKC was not involvedin the glutamate-induced uptake stimulation. The PKA and PKC inhibitorH7 (Lagord et al., 1993) also failed to block glutamate-induceduptake. Negative results were also obtained with pertussis toxin,an inhibitor of G_i/G_o-protein; wortmannin, an inhibitor of phosphatidylinositol3-kinase (PI3K) (Clarke et al., 1994); the tyrosine kinase inhibitorgenistein; Ca²⁺-deficient BSS plus the calcium chelator BAPTA-AM; and calciumchannel blockade with Cd²⁺ (Table 2).


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Table 2. Effects of signal transduction inhibitors on glutamate-stimulated glutamate uptake

Recent studies indicate that cytoskeletal components are involved in several signal transduction pathways, as well as in transportertrafficking. As shown in Figure 6, pretreatment of astrocyte cultureswith cytochalasin B, an inhibitor of actin polymerization (MacLean-Fletcherand Pollard, 1980; Ohmori et al., 1992), did not by itself affectglutamate uptake but did attenuate glutamate stimulation of glutamateuptake in a dose-dependent manner. Cytochalasin D, a similar butmore specific agent (Rampal et al., 1980), had a similar inhibitoryeffect on glutamate-induced uptake increase. Pretreatment withnocodazole, an inhibitor of microtubule formation (Jordan andWilson, 1998), did not inhibit glutamate-induced uptake.

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Figure 6. Cytochalasin B (CytB) and cytochalasin D (CytD) attenuated the glutamate-induced stimulation of glutamate uptake, whereas nocodazole (Nocodz) had no effect. CytB, CytD, and Nocodz were added 1 hr before the studies and maintained during the preincubation period. Data are means + SEM, n = 6; *p < 0.05, **p < 0.01.

Glutamate preincubation increases cell surface expression of GLAST

Transporter trafficking to the cell membrane has been previously shown to regulate EAAC1 (EAAT3) glutamate transporter functionin the C6 glioma cell line (Davis et al., 1998) and other transportersin several cell systems (Tsakiridis et al., 1994; Qian et al.,1997; Quick et al., 1997; Wang et al., 1998; Bernstein and Quick,1999). We therefore used biotinylation labeling of cell surfaceproteins to determine whether the glutamate-stimulated increasein astrocyte glutamate uptake could be mediated by increased cellsurface expression of transporters. Biotinylated proteins wereseparated from nonbiotinylated, intracellular proteins by usingavidin-coated beads. Western blots were prepared from biotinylatedand nonbiotinylated protein fractions, as well as from whole-cellfractions. The blots were probed with anti-actin antibody andwith antibody to GLAST (Fig. 7A) or to GLT-1 (Fig. 7B). The actinband provides an index of intracellular proteins present in eachpreparation. GLAST and GLT-1 bands were present at molecular weightscorresponding to both monomeric and multimeric forms, as reportedpreviously (Haugeto et al., 1996; Davis et al., 1998). The effectof glutamate preincubation is apparent on the Western blots andin the pooled data from five independent studies shown in Figure7C. Glutamate preincubation produced an increase in biotinylated(cell surface) GLAST protein and a decrease in nonbiotinylated(intracellular) GLAST, with no change in total cell GLAST protein.In contrast, glutamate preincubation produced no observable changein cell surface or total cell GLT-1 expression. Glutamate didappear to reduce the nonbiotinylated, intracellular pool in somestudies, but it should be noted that interpretation of changesin the GLT-1 intracellular pool is complicated by the fact thatit is small even under control conditions, and this small poolmay be overestimated to varying degrees by small contaminationsfrom the much larger cell-surface pool of GLT-1.

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Figure 7. Glutamate preincubation increases cell-surface expression of GLAST. Western blots were probed with antibodies to GLAST and actin (A) or to GLT-1 and actin (B). GLAST and GLT-1 bands were present at molecular weights corresponding to both monomeric and multimeric forms. The actin bands provide an index of intracellular proteins present in each preparation. Actin immunoreactivity in the biotinylated fractions was <10% of that in the total cell fractions, and actin immunoreactivity was approximately equal in preparations from control and glutamate-treated cells. Densitometry measurements of the GLAST and GLT-1 bands were pooled from five independent experiments (C). GLAST, but not GLT-1, immunoreactivity was increased in the biotinylated (cell surface) fraction of astrocytes preincubated in 1 mM glutamate. GLAST immunoreactivity was significantly decreased in the nonbiotinylated, intracellular fraction in glutamate-treated cells. Glutamate preincubation did not affect total cell immunoreactivity of either GLAST or GLT-1. Data are means + SEM, n = 3; *p < 0.05, **p < 0.01.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The primary finding reported here is that glutamate can induce a rapid upregulation of astrocyte glutamate uptake. The studiesfurther suggest that the glutamate-induced upregulation is signaledby increased activity of the GLAST (EAAT1) glutamate transportersubtype, and that the increase in uptake is mediated by increasedcell-surface expression of GLAST. Additionally, a role for theactin cytoskeleton in this process is suggested by the findingthat the increase in uptake activity is inhibited bycytochalasins.

Several factors support the conclusion that the glutamate-induced stimulation of glutamate uptake is triggered by increasedactivity of the glutamate transporters. The glutamate effect wasmimicked by D-aspartate, which is also a transporter substrate,stimulation was blocked if the glutamate preincubation was performedin a Na⁺-free medium, and stimulation was not blocked by glutamate receptorantagonists that are not substrates for the transporters. In addition,maximal stimulation of uptake was observed only at glutamate concentrationsthat saturate glutamate transport, and these concentrations farexceed known receptor affinities forglutamate.

The membrane biotinylation studies provide evidence that the increase in uptake is mediated by transporter translocation to(or decreased removal from) the cell membrane. The observed increasein transport V_max with little or no change in glutamate K_m isconsistent with this mechanism. The time course of the glutamatestimulation also supports a trafficking mechanism, because the12-21 min interval between onset of glutamate preincubation andthe resultant increase in uptake activity shown in Figure 1B istoo fast to involve de novo synthesis of new glutamate transportersbut is typical of the time interval required for changes attributableto membrane trafficking (Davis et al., 1998; Bernstein and Quick,1999; Lissin et al., 1999).

GLAST and GLT-1 are the only glutamate transporter subtypes known to be expressed by mammalian forebrain astrocytes, bothin culture and in situ (Rothstein et al., 1994; Swanson et al.,1997; Gegelashvili and Schousboe, 1998). In the present study,glutamate-induced stimulation of glutamate uptake is attributedto GLAST because the GLT-1 selective inhibitor dihydrokainatehad negligible effect, and because GLAST but not GLT-1 exhibitedincreased cell surface expression. It is possible that different,as yet unrecognized transporters contribute to the stimulateduptake, but this seems unlikely because the magnitude of the increaseis large (~100%).

Glutamate has previously been shown to regulate glutamate transport in other ways. Expression of GLAST protein in culturedastrocytes is stimulated by prolonged exposure (7 d) to glutamateor kainate (Gegelashvili et al., 1996), and this increase is accompaniedby an increase in transport V_max. Glutamate preincubation hasalso been reported to reduce extracellular glutamate concentrationsin astrocyte cultures (Ye and Sontheimer, 1999). Interestingly,this effect displays a time course similar to that observed inthe present studies, occurs in response to metabotropic glutamatereceptor agonists as well as to glutamate itself, but is not blockedby metabotropic receptor antagonists. Because many of the metabotropicagonists can also serve as substrates for the transporters (Harriset al., 1987; Ye and Sontheimer, 1998), it is possible that thiseffect is also mediated by a substrate-stimulated increase intransporteractivity.

Although the present studies suggest an upstream signaling mechanism by which increased extracellular glutamate concentrationsmay trigger the increase in glutamate uptake signal and a downstreameffector mechanism by which the increase is accomplished, theydo not establish an intervening signal transduction pathway. Previousstudies have identified mechanisms controlling membrane traffickingof a predominately neuronal glutamate transporter, EAAC1 (EAAT3).In C6 glioma cells expressing EAAC1, PKC activation by phorbolester leads to transporter movement from the intracellular compartmentto the cell surface, whereas the PI3K inhibitor wortmannin decreasedthe membrane EAAC1 expression both in C6 glioma cells (Davis etal., 1998) and in neurons (Munir et al., 1998). Less is knownabout transporter trafficking in astrocytes, but it has been reportedthat membrane expression of GLAST, but not GLT-1, is inhibitedby phorbol ester (Correale et al., 1998). In the present studyneither the PKC inhibitor GF-109203X nor the PI3K inhibitor wortmanninaffected glutamate-induced stimulation of uptake, and variousother interventions also failed to affect stimulation of uptake(Tables 1, 2). However, translocation of membrane proteins doesnot necessarily require signal transduction pathways. G-protein-coupledreceptors (Grady et al., 1997) and ionotropic glutamate receptors(Lissin et al., 1999) appear to involve the conformation-dependentinteraction of the proteins with cytoplasmic regulatory proteinswithout intervening signal transduction, and this raises the possibilityof a similar mechanism for glutamate transporters. Alternatively,the glutamate transporters themselves may serve as signal transducingunits as proposed by Gegelashvili and Schousboe (1998), who notedthat the third intracellular domains of GLAST, GLT-1, and EAAC1each contain a motif similar to that of the IGF-II and $alpha$ -adrenergicreceptors that bind G $alpha$ -subunits of G-proteins.

Substrate-induced upregulation of transport activity mediated by membrane translocation of transporters, as described here,has been reported recently in other systems. The binding of substratesto the 5-HT transporter can rapidly increase 5-HT uptake by inhibitingPKC-dependent internalization of the 5-HT transporters (Qian etal., 1997; Ramamoorthy and Blakely, 1999). A substrate-inducedrapid increase in GABA uptake was also observed in primary hippocampalcultures and in a cell line expressing the rat brain GABA transporterGAT1 (Bernstein and Quick, 1999), with the increase in GABA uptakecorrelating with increased membrane GAT1 expression. PKC is alsoinvolved in the regulation of GAT1 activity and trafficking (Quicket al., 1997), but in both the 5-HT and GABAergic systems thesignals linking increased substrate exposure to PKC activity remainunknown.

The inhibitory effects of cytochalasin B and cytochalasin D on glutamate-stimulated glutamate uptake suggest that the actincytoskeleton is important for either signal transduction or transportertranslocation in this process. The cytochalasins impair actinpolymerization and promote disruption of the actin cytoskeleton(MacLean-Fletcher and Pollard, 1980). Cytochalasin B has, in additionto effects on actin polymerization, a direct inhibitory effecton glucose transport (Rampal et al., 1980), but cytochalasin Ddoes not have any known direct effect on glucose transportersor other transporterfunction.

The actin cytoskeleton has been linked to intracellular protein trafficking, transporter function, and signal transductionin several systems (Mills and Mandel 1994; Tsakiridis et al.,1994; Lamaze et al., 1997; Wang et al., 1998). Cytochalasin Dinhibits insulin-stimulated glucose uptake and prevents insulin-inducedtrafficking of glucose transporters to the plasma membrane inL6 rat skeletal muscle cells (Tsakiridis et al., 1994) and 3T3-L1adipocytes (Wang et al., 1998). In this system the actin filamentsare thought to facilitate the insulin-induced relocation of PI3Kto the intracellular glucose transporter compartment, rather thanmovement of the glucose transporters themselves (Wang et al.,1998). One potential link between actin and known signal transductionsystems is that activation of the Rho family of the small G-proteincan induce a reorganization of the actin cytoskeleton (Hall, 1998;Sasaki and Takai, 1998).

It is not known whether the two astrocyte glutamate transporters GLAST and GLT-1 have distinct physiological functions. Genedisruption studies suggest that GLAST, unlike GLT-1, may not berequired for neuronal survival under normal conditions in brain(Tanaka et al., 1997; Watase et al., 1998). The rapid upregulationof GLAST transport capacity in response to elevated extracellularglutamate concentrations observed here suggests that GLAST mayhave a unique function in feedback regulation of extracellularglutamate concentrations and glutamatergic synaptic activity.Studies by Tong and Jahr (1994) and Diamond and Jahr (1997) showthat transporter binding of glutamate contributes to an early,fast reduction in synaptic glutamate concentrations in additionto the slow, later phase attributable to actual glutamate uptake[but also see Otis et al. (1996)]. Translocation of GLAST to theastrocyte cell surface could therefore affect glutamatergic transmissionin two ways: by increasing the number of glutamate binding sitesand by accelerating subsequent glutamateuptake.

  FOOTNOTES

Received March 30, 1999; revised Aug. 6, 1999; accepted Sept. 9, 1999.

This work was supported by National Institutes of Health Grant RO1 NS31914 and the Veterans Affairs Merit Review program (R.A.S.).We thank Dr. Michael B. Robinson for helpful advice on the biotinylationstudies.
Correspondence should be addressed to Dr. Raymond A. Swanson, (127) Neurology, V.A.M.C., 4150 Clement Street, San Francisco,CA 94121. E-mail: ray{at}itsa.ucsf.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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