Expression of the GLT-1 Subtype of Na+-Dependent Glutamate Transporter: Pharmacological Characterization and Lack of Regulation by Protein Kinase C

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Vol. 289, Issue 3, 1600-1610, June 1999

Expression of the GLT-1 Subtype of Na⁺-Dependent Glutamate Transporter: Pharmacological Characterization and Lack of Regulation by Protein Kinase C¹

Jue Tan, Olga Zelenaia, Dana Correale, Jeffrey D. Rothstein and Michael B. Robinson

Departments of Pediatrics and Pharmacology, Children's Hospital of Philadelphia, University of Pennsylvania, Philadelphia, Pennsylvania (J.T., O.Z., D.C., M.B.R) and Department of Neurology, The Johns Hopkins University, Baltimore, Maryland (J.D.R.)

	Abstract

Top Abstract Introduction Experimental Procedures Results Discussion References

Several subtypes of Na⁺-dependent glutamate transporters have been pharmacologically differentiated in brain tissues. Fivedistinct cDNA clones that express Na⁺-dependent glutamate transport activity have been isolated. Onegoal of the current study was to compare the pharmacological propertiesof the rat GLT-1 subtype of transporter to those identified previouslyusing rat brain tissues. To accomplish this goal, GLT-1 was stablytransfected into two different cell lines that express low levelsof endogenous transport activity (MCB and L-M (TK-)). Severalclones stably transfected with GLT-1 were isolated. In each cellline, Na⁺-dependent glutamate transport activity was saturable with similarK_m values (19 and 37 µM). The pharmacological properties of GLT-1-mediatedtransport in these cell lines paralleled those observed for thepredominant pharmacology observed in cortical crude synaptosomes.These data are consistent with other lines of evidence that suggestthat GLT-1 may be sufficient to explain most of the Na⁺-dependent glutamate transport activity in cortical synaptosomes.Although recent studies using HeLa cells have suggested that GLT-1can be rapidly up-regulated by activation of protein kinase C(PKC), modulation of PKC or phosphatase activity had no effecton GLT-1-mediated activity in these transfected cell lines. Todetermine if GLT-1 regulation by PKC is cell-specific, HeLa cells,which endogenously express the EAAC1 subtype of transporter, werestably transfected with GLT-1. Although EAAC1-mediated activitywas increased by activation of PKC, we found no evidence for regulationof GLT-1. Despite the present findings, GLT-1 activity may beregulated by PKC under certainconditions.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

The acidic amino acids, glutamate and aspartate, are the predominant excitatory neurotransmitters in the mammalian centralnervous system (for review, see Mayer and Westbrook, 1987). Inaddition to their essential role as mediators of rapid signaling,these excitatory amino acids (EAAs) also contribute to brain damageobserved in acute insults to the nervous system, including hypoxemia,head trauma, and seizure disorders (for review, see Choi, 1992).The levels of EAAs approach 10 mmol/kg in the brain whereas extracellularlevels are maintained at micromolar or submicromolar concentrations(for review, see Schousboe, 1981). Because there is no evidencefor extracellular metabolism, it is generally assumed that lowextracellular concentrations of the EAAs are maintained by Na⁺-dependent transport activity (Schousboe, 1981). Malfunction and/orreverse operation of transporter proteins results in an accumulationof extracellular EAAs and excessive activation of EAA receptorscontributing to excitotoxicity (for review, see Attwell et al.,1993).

In the early 1990s, three cDNA clones that express Na⁺-dependent glutamate transport in heterologous expression systems wereidentified and named GLAST (Storck et al., 1992), GLT-1 (Pineset al., 1992), and EAAC1 (Kanai and Hediger, 1992). Using strategiesbased on the homology of these transporters, three human homologswere identified and named EAAT1-3 (Arriza et al., 1994) and thensubsequently two additional glutamate transporters (neuronal EAAT4and retinal EAAT5) were identified (Fairman et al., 1995; Arrizaet al., 1997).

Before the cloning of individual transporters, pharmacological studies provided evidence for multiple subtypes of transportersthat are differentially expressed in various brain regions (forreview, see Robinson and Dowd, 1997). For example, transport incrude synaptosomal membranes prepared from forebrain (cortex,hippocampus, or striatum) regions and midbrain is inhibited bydihydrokainate (DHK) with IC₅₀ values of approximately 100 µM,whereas transport in cerebellar preparations is essentially insensitiveto inhibition by DHK. L- $alpha$ -aminoadipate (L-AAD) displays the oppositepattern of inhibition. The cloning of transporter subtypes ledto studies of their pharmacological properties and localization.Based on its sensitivity to inhibition by L-AAD and cerebellarlocalization, it is assumed that EAAT4 may be sufficient to explainthe predominant transport activity observed in cerebellar crudesynaptosomes (Fairman et al., 1995). The other neuronal transporter,EAAC1, has pharmacological properties that differ from those observedfor cortical crude synaptosomes (Dowd et al., 1996). The glialtransporter, GLAST, has pharmacological properties that are dramaticallydifferent from those observed in crude cortical synaptosomes andare similar to those of transport observed in undifferentiatedastrocyte cultures that express GLAST (Arriza et al., 1994; Stoffeland Blau, 1995; for review, see Robinson and Dowd, 1997). Theonly other cloned transporter that could explain the forebrainpharmacology is the glial transporter GLT-1 (corresponding tothe human homolog EAAT2). The pharmacological properties of thehuman homolog appear to agree with those observed in forebrain/corticalcrude synaptosomes (Arriza et al., 1994), but the pharmacologicalcharacterization of the rat homolog is limited and is not consistentbetween studies (Pines et al., 1992; Wang et al., 1998).

The availability of cDNA clones and specific antibodies has also facilitated studies of the regulation of these glutamatetransporters. There is evidence that GLAST-mediated transportcan be rapidly down-regulated by activation of protein kinaseC (PKC) and subsequent phosphorylation of the transporter (Conradtand Stoffel, 1997). Recent studies suggest that EAAC1-mediatedtransport is increased by activation of PKC or decreased by aninhibitor of phosphatidylinositol 3-kinase (Davis et al., 1998).These effects on activity are correlated with altered cell surfaceexpression and are consistent with regulation of activity throughtrafficking to and from the cell surface. There is also evidencethat GLT-1 may be rapidly regulated by activation of PKC (Casadoet al., 1993; Ganel and Crosson, 1998). In the earlier study,PKC activation increased glutamate transport; in the later study,PKC activation decreased transport activity by increasing theK_mvalue.

The goal of the present study was to examine the pharmacological properties of the rat homolog, GLT-1, and the possible mechanismsof rapid regulation by PKC. To accomplish these goals, GLT-1 cDNAwas stably transfected into cell lines that express low levelsof endogenous glutamate transport activity. In two separate celllines, the pharmacological properties of GLT-1 parallel thoseobserved in crude cortical synaptosomes. These two cell lineswere used to study the regulation of GLT-1 by PKC. In both celllines, glutamate transport activity was unaffected by activationof PKC. Western blotting and analyses of transport activity suggestthat the previously reported regulation of GLT-1 may be attributedto regulation of endogenously expressed EAAC1 in the cell linesused in earlierstudies.

	Experimental Procedures

Top Abstract Introduction Experimental Procedures Results Discussion References

Materials. L-[³H]Glutamate (40-60 Ci/mmol) was purchased from DuPont (Boston, MA). Nonradioactive L-glutamate (Sigma Chemical Co., St.Louis, MO) was used to dilute the specific activity. The sourcesfor all the EAA analogs are listed in Table 1. MCB 3901 (a Syrianhamster adenovirus type 12-induced tumor, catalog no. CRL-9595),L-M (TK-) (a subline of 5-bromo-2-deoxyuridine-resistant strainof the L-M mouse fibroblast cell line, catalog no. CCL-1.3), andHeLa (epithelioid carcinoma, catalog no. CCL-2) cell lines wereobtained from the American Type Culture Collection (Rockville,MD). The GLT-1 cDNA in pBluescript SK- was a generous gift fromDr. Baruch Kanner (Hebrew University, Jerusalem, Israel). Phorbol12-myristate 13-acetate (PMA) was purchased from Sigma (St. Louis,MO). Forskolin, bisindolylmaleimide II (Bis), okadaic acid (Prorocentrumconcavum), and A23187-free acid (streptomyces chartreusensis)were purchased from Calbiochem (La Jolla, CA).

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TABLE 1
Comparison of potency of EAA analogs for inhibition of GLT-1-mediated transport activity

Subcloning, Stable Transfection, and Maintenance of Cell Lines. L-M (TK-) and MCB cell lines were maintained in Dulbecco's modified Eagle's medium (catalog no. 11960-051, no added glutamine;Gibco BRL, Gaithersburg, MD), 10% heat-inactivated defined fetalbovine serum (catalog no. SH30070.03; Hyclone, Logan, UT), and1% penicillin (100 U/ml)/streptomycin (100 µg/ml; catalog no.15140-122; Gibco BRL) in a 7% CO₂, 37°C incubator. HeLa cellswere maintained in the same media supplemented with 2 mM L-glutamine,and at 5% CO₂.

The GLT-1 cDNA was subcloned into pRC/CMV (Invitrogen) using XhoI and XbaI restrictions sites. After cesium chloride purification,the cDNA was stably transfected into each cell line using calciumphosphate-DNA precipitation as described previously (Ausubel etal., 1995

). 10 µg of pRC/CMV/GLT-1 DNA per 10-cm dish was used.Briefly, cells were incubated with precipitate in 7% CO₂ at 37°Cfor 8 h, then medium containing precipitate was removed, cellswere washed twice with 1× PBS and fed with normal tissue culturemedium. After incubation for 24 h, increasing concentrations ofgeneticin (catalog no. 11811-031, G418, Gibco BRL) were addedto transfected and control cells. Cell culture medium containingG418 was exchanged every 3 to 4 days. After approximately 2 to3 weeks of selection, several apparently clonal colonies wereobserved in plates containing cells that had been transfectedand maintained with 0.5 mg/ml G418. No untransfected cells survivedat this concentration of G418. Several colonies were picked usingsterile filter paper circles (6 mm diameter) soaked in trypsin.These colonies were maintained in cell culture medium containingG418. Shortly after expansion to 10-cm dishes, several colonieswere frozen and maintained in liquid nitrogen. All experimentswere performed with cell lines that had been passaged fewer than30 times. During this time, there was no apparent trend in transporterexpression measured by Western blot oractivity.

Measurement of Na⁺-Dependent Glutamate Transport Activity. Transport assays were performed as described previously (Davis et al., 1998). In a 37°C water bath, cultures (plated in 12-welldishes) were prerinsed two times with 1 ml of prewarmed sodium-or choline-containing buffer (Tris base, 5 mM; HEPES, 10 mM; NaClor choline chloride, 140 mM; KCl, 2.5 mM; CaCl₂, 1.2 mM; MgCl₂,1.2 mM; K₂HPO₄, 1.2 mM; and dextrose, 10 mM). Uptake was initiatedby the addition of 1 ml of prewarmed Na⁺- or choline-containing buffer, which contained L-[³H]-glutamate with or without EAA analogs. After 5 min, cultureswere rinsed three times with 1 ml of ice-cold choline buffer tostop transport activity. Cells were dissolved in 1 ml of 0.1 MNaOH and a 500 µl aliquot was used to quantitate radioactivityby scintillation spectrometry. Protein was also measured in analiquot of solubilized cells using a commercial Bradford kit (Bio-Radprotein assay, Bio-Rad Laboratories, Hercules, CA). Na⁺-dependent transport activity was calculated as the differencein accumulated radioactivity in the Na⁺-containing and choline-containing buffer. In these assays, lessthan 10% of the substrate was accumulated and transport was measuredunder conditions of initial velocity (transport was linear withtime beyond 5min).

Western Analysis. After washing twice with ice-cold PBS, cells were harvested using 1 ml per 10 cm dish of Na⁺-HEPES buffer (20 mM, pH 7.5), containing MgCl₂ (0.4 mM), EDTA(0.2 mM), phenylmethylsulfonyl fluoride (20 µM), leupeptin (2µg/ml), and aprotinin (0.22 µg/ml). After sonication and centrifugationat 14,000 RPM in a microcentrifuge for 10 min, an aliquot of thesupernatant was used for analysis of protein content and an aliquotwas diluted 1:2 in solubilizing buffer (2% SDS, 10% mercaptoethanol,5% glycerol, 0.005% bromphenol blue, and 50 mM Tris-Cl, pH 7.0).The samples were frozen at $-$ 20°C. Cell culture samples or controlbrain specimens, prepared as described previously (Schlag et al.,1998), were resolved using 10% polyacrylamide gel electrophoresis.After transfer to polyvinylidine fluoride membranes (ImmobilonP, Millipore, Bedford, MA), immunoblots were probed with anti-GLT-1,anti-GLAST, anti-EAAC1, or anti-EAAT4 antibodies (Furuta et al.,1997). Immunoreactivity was visualized by enhanced chemiluminescence(Amersham, Arlington Heights,IL).

Curve Fitting and Statistical Analysis. All values reported are the mean ± S.E.M. of at least three independent observations. Except where noted, IC₅₀ values wereobtained by fitting experimental data to a theoretical curve witha Hill coefficient of one using One Site Competition method inGraphPad Prism software (GraphPad Prism, version 2.0, GraphPadSoftware, Inc., San Diego, CA). When two groups were compared,a Student's unpaired t test was used to compare the values. Multiplegroups were compared by ANOVA with post hoc analysis. A p < .05was consideredsignificant.

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

Selection and Characterization of Cell Lines Stably Transfected with GLT-1. One problem with choosing cell lines for stable expression of glutamate transporters is a high level of endogenous activityobserved in several of the cell types regularly used for stabletransfection, including CHO, COS, or HEK293 (M.B.R., unpublishedobservations). MCB (Desai et al., 1995), and L-M (TK-) (J.D.R.,unpublished observations) express undetectable to low levels ofglutamate transport and HeLa cells were previously used for transienttransfection of GLT-1 (Pines et al., 1992; Casado et al., 1993).To examine endogenous expression of transporter subtypes in thesecell lines, transporter specific antibodies were used for Westernanalysis with cortical or cerebellar protein as a positive control(Fig. 1). A strong immunoreactive band for GLT-1 was observedwith a small amount of cortical membrane homogenate, but no GLT-1immunoreactivity was observed when 80 times more cell line proteinwas analyzed. Similarly, except for HeLa cells, no EAAT4 or GLASTimmunoreactivity was observed in these cell lines; weak immunoreactivebands for these transporters were observed in HeLa cells. No EAAC1immunoreactivity was observed in L-M (TK-) cells, an extremelyfaint immunoreactive band was consistently observed in MCB cells(at approximately 64 kDa), and a robust EAAC1 immunoreactive bandwas observed in HeLa cells (Fig. 1).

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Fig. 1. Western blot analysis of Na⁺-dependent glutamate transporters expressed in untransfected cell lines (L-M (TK-), MCB, and HeLa) and in transfected cell lines (LM-GLT1-8, MCB-GLT1-6, and MCB-GLT1-12). For the GLT-1 immunoblot, 80 µg of protein was loaded in each lane, except for cortical membrane homogenate (1 µg protein), HeLa cells (50 µg protein), and MCB-GLT1-12 cells (20 µg). For the other antibodies, 80 µg of protein was loaded in each lane except for HeLa cells and cortical or cerebellar tissue (50 µg protein). All cell homogenates were harvested from cells grown to 80 to 90% confluence (similar to that used for analyses of transport activity). For each antibody, all of the lanes are from the same gel with the same exposure. Each of these Western blots were repeated in at least two additional independent experiments.

In agreement with the lack of transporter immunoreactivity, essentially no Na⁺-dependent L-[³H]-glutamate transport activity was observed in the L-M (TK-)cells, suggesting that this system would be ideal to study theproperties of GLT-1-mediated transport (Fig. 2). MCB cells expressedmoderate transport activity, which may be attributed to the faintEAAC1 immunoreactive band. Alternatively, this activity may bemediated by EAAT5 or an uncloned transporter, but this was notpursued further. To decrease the possibility that the propertiesof GLT-1 might be artifactually related to a single expressionsystem, we decided to stably transfect both L-M (TK-) and MCBcells with GLT-1.

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Fig. 2. Transport activity in untransfected (stippled bars) and transfected (solid bars) L-M (TK-) and MCB cell lines. The accumulation of L-[³H]-glutamate (0.5 µM) was measured in the presence (+Na⁺) and absence of Na⁺ ( $-$ Na⁺) as described in Experimental Procedures. Na⁺-dependent (Na⁺-dep.) accumulation was calculated as the difference between these two values. Data are the mean ± S.E.M. of at least three independent observations each made in triplicate.

GLT-1 cDNA was subcloned into the pRC/CMV expression vector that confers geneticin (G418) resistance and stably transfectedL-M (TK-) and MCB cells. After transfection, G418-resistant MCBand L-M (TK-) clones were screened for Na⁺-dependent glutamate transport activity and tested for GLT-1 expressionby Western blotting (data not shown). Clones were categorizedinto low, medium, and high levels of expression. The transfectedL-M (TK-) cells chosen for further study are referred to as LM-GLT1-8(Figs. 1 and 2). Compared with other clones identified, LM-GLT1-8expressed moderate levels of transport activity and GLT-1 immunoreactivity,but still expressed nearly 60-fold higher levels of Na⁺-dependent transport activity than untransfected control cells.The MCB clone chosen for further study (referred to as MCB-GLT1-6)expressed moderate levels of GLT-1 protein compared with otherMCB clones. In this cell line, Na⁺-dependent transport activity was 4- to 5-fold that observed inuntransfected MCB cells (Figs. 1 and 2). In both cell lines, theNa⁺-independent accumulation of L-[³H]-glutamate was unaffected by transfection (-Na⁺, Fig. 2).

Kinetic and Pharmacological Properties of L-[³H]-Glutamate Transport Activity in Cell Lines Stably Transfected with GLT-1. The concentration dependence of Na⁺-dependent L-[³H]-glutamate transport activity was examined in both LM-GLT1-8 and MCB-GLT1-6.Between the concentrations of 1 and 1000 µM L-glutamate, transportactivity was consistent with a single saturable process with K_mvalues of 37 ± 4 µM (n = 4) in LM-GLT1-8 cells and 18.6 ± 0.3µM (n = 3) in MCB-GLT1-6 cells (Fig. 3). The V_max values were3.1 ± 0.4 nmol/mg protein per min in LM-GLT1-8 cells and 2.7 ±0.3 nmol/mg protein per min in MCB-GLT1-6 cells, indicating thatboth cell lines express a comparable capacity for transport. Thesecapacities for transport are comparable to those observed in cortical,hippocampal, or striatal crude synaptosomes (Robinson et al.,1991).

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Fig. 3. Eadie-Hofstee plot of the concentration dependence of Na⁺-dependent L-[³H]-glutamate transport in LM-GLT1-8 (A) and MCB-GLT1-6 (B). Inset: Saturation isotherm of the same data (Michaelis-Menten). Data are the mean ± S.E.M. values of at least three independent observations, each performed in triplicate. For LM-GLT1-8 cells, the V_max value was 3.1 ± 0.4 nmol/mg protein per min and the K_m value was 37 ± 4 µM. For MCB-GLT1-6 cells, the V_max value was 2.7 ± 0.3 nmol/mg protein per min and the K_m value was 18.6 ± 0.3 µM.

Several EAA analogs were tested for inhibition of transport activity in both cell lines and were compared to our previouslypublished data for inhibition of transport activity in crude synaptosomes(Table 1). All of the compounds tested inhibited transport activitywith comparable potencies (within 2.5-fold) in both LM-GLT1-8and MCB-GLT1-6 cell lines. In both cell lines, transport activitywas inhibited by many of the prototypic inhibitors of Na⁺-dependent glutamate transport including D-aspartate, L-cysteate,L-trans-pyrrolidine-2,4-dicarboxylate (L-trans-PDC; Fig. 4A),and DL-threo-hydroxyaspartate (Table 1, Part A). These compoundshave less than 3-fold selectivity for inhibition of transportin either cortex or cerebellum and were 5- to 10-fold more potentas inhibitors of transport in cortical tissue than in GLT-1 transfectedcell lines.

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Fig. 4. Sensitivity of GLT-1-mediated transport to inhibition by L-trans-PDC and DHK. Na⁺-dependent L-[³H]-glutamate transport was measured in the absence and presence of increasing concentrations of inhibitors in MCB-GLT1-6 ( $black-square$ ) and LM-GLT1-8 (

). Data are mean ± S.E.M. values of three independent observations, each performed in triplicate. The solid lines represent the theoretical curves with Hill coefficient of 1. IC₅₀ values are presented in Table 1. The dotted line represents the previously reported sensitivity of cerebellar glutamate transport to the inhibitor and the dashed line represents the previously reported sensitivity of cortical glutamate transport to the inhibitor (Robinson et al., 1991

; 1993

In earlier studies with synaptosomes, we had observed inhibition of transport activity by some compounds that also interactwith EAA receptors (Robinson et al., 1993

). In both LM-GLT1-8and MCB-GLT1-6 cells we observed essentially no inhibition byN-methyl-D-aspartate. In contrast, the ionotropic receptor agonist,(RS)- $alpha$ -amino-3-hydroxy-5-methylisoxazole-4-propionate, inhibitedGLT-1-mediated transport with an IC₅₀ value of 350 µM, suggestingthat at high concentrations some of the effects of this compoundmay be mediated through inhibition of the GLT-1 component of transportactivity. The putative metabotropic glutamate receptor (mGluR)antagonist, L-2-amino-3-phosphonopropionate (L-AP3), inhibitedGLT-1-mediated transport with affinities comparable to those usedto block the mGluRs (for review, see Schoepp et al., 1990

). BecauseL-AP3 also inhibits EAAC1-mediated transport activity (Dowd etal., 1996

), L-AP3 should be used with caution as an mGluRantagonist.

To determine if the pharmacology of GLT-1 correlates with that observed in cortex, inhibitors selective for either corticalor cerebellar transport were tested (Table 1, Part B). DHK, theonly forebrain (hippocampus, cortex, striatum, and midbrain)-selectiveinhibitor available, blocked transport in both MCB-GLT1-6 andLM-GLT1-8 with IC₅₀ values that were within 2-fold of those observedin cortical synaptosomes (Fig. 4B). This contrasts with cerebellaractivity, which is insensitive to DHK. Four compounds with greaterthan 10-fold selectivity for inhibition of cerebellar transportare available (Table 1, Part B). These compounds include: L-AAD, $beta$ -N-oxalyl-L- $alpha$ , $beta$ -diaminopropionate, (2S, 1'S, 2'S)-2-(carboxycyclopropyl)glycine, and $alpha$ -methyl-DL-glutamate. L-AAD blocked GLT-1-mediatedtransport with an IC₅₀ value of 2.5 to 3.5 mM. This potency isapproximately 4-fold lower than the IC₅₀ value for inhibitionof forebrain (cortex, hippocampus, striatum, and midbrain) transport(Robinson et al., 1991

), and is at least 50-fold lower than thatobserved for inhibition of cerebellar transport. In both celllines the other cerebellum-selective inhibitors did not reduceGLT-1-mediated transport activity (<20% inhibition at 1 mM). Thesecompounds inhibit cerebellar transport with IC₅₀ values between100 and 300 µM but do not inhibit cortical transport (Robinsonet al., 1993

). Therefore, the pattern of sensitivity of GLT-1to inhibition by these compounds is most consistent with corticaltransport.

In cortical tissue, data for inhibition of transport by three compounds (kainate, L-homocysteate, and quisqualate) was bestfit to two sites with dramatically different affinities (Table1, Part C). With all three compounds, there was a predominantcomponent that represented approximately 70 to 90% of the sites.The affinities for inhibition of GLT-1 were comparable to thoseobserved for the predominant component in cortex. For example,GLT-1-mediated transport was inhibited by kainate with IC₅₀ values(50-70 µM) similar to the predominant component in cortical synaptosomes(72 µM).

Given that the patterns of sensitivity of GLT-1 to inhibition by several compounds were similar to that observed in cortex,the pharmacological properties of GLT-1 were compared to thoseobserved in both cerebellar and cortical synaptosomal preparations.To facilitate this comparison, the Log IC₅₀ values for inhibitionof GLT-1-mediated transport were plotted against the Log IC₅₀values for inhibition of cortical or cerebellar synaptosomal transportactivity (Fig. 5). If one assumes that the compounds interactthrough a competitive interaction and use the Cheng and Prusoffequation to convert IC₅₀ values to K_i values (for original reference,see Dowd et al., 1996

), the graphs are essentially identical (notshown). These graphs reveal a significant correlation betweenthe potencies of compounds for inhibition of GLT-1-mediated transportand cortical synaptosomal transport. The slope of the line drawnthrough this data is 1.000 and the x-intercept is 0.526. The slopeof 1 is consistent with a parallel shift in the potencies of thecompounds and the x-intercept of 0.526 would indicate that compoundsare, on average, 3-fold less potent as inhibitors of GLT-1-mediatedtransport than of cortical synaptosomal transport.

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Fig. 5. Correlation between the potency of EAA analogs for inhibition of Na⁺-dependent GLT-1-mediated transport and their potency for inhibition of Na⁺-dependent glutamate transport in cortical (A) or cerebellar (B) synaphosomes. The log of the IC₅₀ value for inhibition of cortical or cerebellar glutamate transport (see Table 1) was plotted as a function of the log IC₅₀ value for inhibition of GLT-1-mediated transport. The IC₅₀ values used for GLT-1 were the averages of the IC₅₀ values for inhibition of LM-GLT1-8 and MCB-GLT1-6. For compounds with data for inhibition that are best fit to two sites in either cerebellar or cortical tissue, the Log IC₅₀ value for the predominant component was used. For compounds without full inhibition curves, the IC₅₀ values were calculated from the percent inhibition assuming a theoretical curve with a Hill coefficient of 1. The numbers refer to each compound used for this correlation (see Table 1 for the names of each compound).

Effects of Over-Expression of Glutamate Transporters in Cell Lines. One approach to limiting the impact of endogenous glutamate transporter expression in cell lines is to express higher levelsof transfected transporter relative to that observed in untransfectedcells (Matthews et al., 1997). In our initial studies, we decidedto attempt a similar approach with an MCB clone (MCB-GLT-12) thatexpressed much higher levels of GLT-1 protein than MCB-GLT1-6(Fig. 1). In this cell line, the V_max value for L-[³H]-glutamate uptake was 24 ± 5 nmol/mg protein per min (data notshown, n = 4), which was almost 10-fold higher than that observedin MCB-GLT1-6. In this cell line, the K_m value for glutamate transportwas four times higher than that observed in MCB-GLT1-6 even thoughless than 10% of the glutamate was transported from the extracellularspace (K_m = 78 ± 30 µM). Similar shifts in the potencies of compoundscleared by transporters have been observed in brain slices andcells in culture (for a recent discussion, see Speliotes et al.,1994), and have been attributed to the rapid clearance of glutamatefrom the local environment near the transporters. This could explainthe lower apparent affinity of the transporter for glutamate,but the pharmacological properties of transport were also affectedby this high level of expression. The sensitivity of transportto DHK was much lower in MCB-GLT-12 (IC₅₀ = 588 ± 89 µM) thanin MCB-GLT1-6 (IC₅₀ = 32 ± 7 µM) as was the sensitivity to inhibitionby L-trans-PDC (112 ± 42 µM, n = 3), kainate (1140 ± 220 µM, n= 3), and L-anti-endo-3,4-methanopyrrolidine dicarboxylate (108± 9 µM, n = 3). To rule out the possibility that confluent MCB-GLT1-12cells express higher levels of EAAC1, GLAST, or EAAT4, proteinsample were harvested from confluent cultures. We found no evidencefor higher levels of any of these proteins in confluent MCB-GLT1-12cells than in confluent MCB-GLT1-6 (data not shown, n $>=$ 2 independentexperiments). Although we cannot rule out the possibility thatconfluence induces expression of EAAT5 or an uncloned transporter,the observation that all of these inhibition data conform to theoreticalcurves with a Hill slope of 1 suggests that a single populationof sites mediates activity in these confluent cultures. To testthe possibility that high expression might be influencing thepharmacological properties of GLT-1 by changing the local environmentclose to the cells, the sensitivity of transport to DHK was examinedusing MCB-GLT1-12 cells grown to approximately 30% confluence.Under these conditions, the IC₅₀ value for inhibition by DHK was148 µM (n = 2), a value which approaches that observed in 80 to90% confluent LM-GLT1-8 and MCB-GLT1-6 cells. Thus, it appearsthat high levels of activity can influence the pharmacologicalproperties.

To determine if this phenomenon might influence the results of the present study, MCB-GLT1-6 cells were grown to less than40% confluence and the sensitivity to DHK was assessed. Underthese conditions, the IC₅₀ value for DHK was indistinguishablefrom that observed at 80 to 90% confluence (IC₅₀ = 33 µM, n =2). This suggests that the pharmacological properties of MCB-GLT1-6are not likely to be affected by confluence of the cells. Thisalso suggests that the phenomenon observed in MCB-GLT1-12 is relatedto the high levels of GLT-1 expression rather than a generalizedchange in MCB cells that occurs when they are grown to highconfluence.

Effects of Modulation of PKC on GLT-1-Mediated Transport. Using HeLa cells, Casado and her colleagues published a report that suggested that GLT-1-mediated transport could be rapidlyincreased by activation of PKC (Casado et al., 1993). Becausethis type of rapid regulation could have significant implicationsfor the control of extracellular EAAs, we pursued this regulationof GLT-1 in both stably transfected cell lines. In both cell lines,preincubation with the phorbol ester (PMA) for 30 min had no effecton transport activity (Fig. 6A, mean of at least nine independentobservations). As a positive control, each of the stock solutionsof PMA was tested for activation of endogenous EAAC1-mediatedtransport in C6 glioma cells. All stocks used caused an increasein transport activity (data not shown, see Davis et al., 1998for description of assay). Higher concentrations of PMA (up to1 µM) and longer incubations (up to 1 h) were also tested andneither caused an increase in GLT-1-mediated transport activityin transfected cells (data not shown, n = 2).

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Fig. 6. Effect of modulation of PKC on GLT-1-mediated transport in LM-GLT1-8 and MCB-GLT1-6 cells. A, cells were pretreated with vehicle dimethyl sulfoxide (DMSO), 100 nM PMA, or 10 µM Bis for 30 min before measurement of Na⁺-dependent glutamate (0.5 µM) transport. Data are the mean ± S.E.M. of at least nine independent observations with PMA and at least three independent observations with Bis. There was no significant effect of either treatment on Na⁺-dependent glutamate transport activity. B, cells were pretreated with either the phosphatase inhibitor okadaic acid (1 µM) or the Ca²⁺ ionophore A23187 (100 nM) alone and in combination with PMA (100 nM) for 30 min. Data are the mean ± S.E.M. of at least three independent observations. There was no significant effect of any of the treatments.

The absence of an effect of PMA could be a consequence of endogenous activation of PKC in these cell lines and/or high levelsof protein phosphatase activity which could theoretically exceedthe capacity for phosphorylation by PKC. To address these possibilities,the effects of the PKC inhibitor, Bis, on transport activity wasexamined. At concentrations that blocked the effects of PMA inC6 glioma and using stock solutions that were tested in parallel(data not shown, see Davis et al., 1998

for description of assay),preincubation with 10 µM Bis for 30 min had no effect on GLT-1-mediatedtransport activity (Fig. 6A). To block phosphatase activity inthese cell lines, okadaic acid, which blocks both protein phosphatase1 and 2A at 1 µM, was tested (Cohen et al., 1990

). Preincubationwith okadaic acid (1 µM) had no effect on transport activity,nor did the combination of okadaic acid and phorbol ester (Fig.6B). Our observations suggest that neither endogenous activityof PKC nor high protein phosphatase activity can explain the lackof an effect of PMA on GLT-1-mediated transport. In an earlierstudy (Casado et al., 1991

), it was reported that the Ca²⁺ ionophore A23187 potentiates the effects of PMA. We found thatA23187 by itself or in combination with PMA had no effect on transportactivity (Fig. 5B). Together, these data suggest that GLT-1 isnot activated by PKC. We also examined the effects of activationof protein kinase A with forskolin and found no change in transportactivity (data notshown).

HeLa cells were used in the earlier study that suggested that GLT-1 could be regulated by activation of PKC (Casado et al.,1993

). To examine the possibility that regulation of GLT-1 byPKC is cell-specific, HeLa cells were stably transfected withGLT-1. Two clones, HeLa-GLT1-7 and HeLa-GLT1-14, that expressmoderate levels of GLT-1 immunoreactivity (Fig. 7A and B) wereisolated. In both of these cell lines, the expression of EAAC1was also increased (Fig. 7, C and D), but the expression of GLASTand EAAT4 was not affected by stable transfection of GLT-1 (datanot shown, n = 2). The kinetic properties of glutamate transportwere examined in control (untransfected) HeLa and in HeLa-GLT1-7cells (Fig. 8A). In untransfected cells, the K_m value for Na⁺-dependent L-[³H]-glutamate transport was 37 ± 19 µM and the V_max value was 212± 74 pmol/mg protein per min (mean ± S.E.M. of three independentobservations). In HeLa-GLT1-7 cells, the K_m value for Na⁺-dependent L-[³H]-glutamate transport was 16 ± 1 µM and the V_max value was 1300± 230 pmol/mg protein per min (mean ± S.E.M. of three independentobservations).

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Fig. 7. Western blot analysis of EAAC1 and GLT-1 expressed in untransfected and transfected HeLa cells. For the GLT-1 immunoblots (A and B), 50 µg of HeLa protein and 0.25 µg of cortical membrane homogenate protein was loaded in each lane. For the EAAC1 immunoblots (C and D), 50 µg of protein was loaded in each lane. Note that these Western blots were also probed with an antiactin antibody and that the immunoblot for Hela-GLT1-14 is a darker exposure than HeLa-GLT1-7. All cell homogenates were harvested from cells grown to 80 to 90% confluence (similar to that used for analyses of transport activity). For each panel, all of the lanes are from the same gel with the same exposure. Each of these Western blots was repeated with at least two additional independent experiments.

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Fig. 8. Analyses of Na⁺-dependent L-[³H]-glutamate transport activity in HeLa cells stably transfected with GLT-1 cDNA. A, Eadie-Hofstee plot of the concentration dependence of Na⁺-dependent L-[³H]-glutamate transport in untransfected HeLa (O) and HeLa-GLT1-7 cells (

). Data are the mean ± S.E.M. values of at least three independent observations, each performed in triplicate. For untransfected HeLa cells, the V_max value was 212 ± 74 pmol/mg protein per min and the K_m value was 37 ± 20 µM. For HeLa-GLT1-7 cells, the V_max value was 1300 ± 230 pmol/mg protein per min and the K_m value was 16 ± 1 µM. B, sensitivity of glutamate transport activity (0.5 µM) to inhibition by DHK in HeLa-GLT1-7. Transport activity was measured in the absence and presence of increasing concentrations of DHK. Data are mean ± S.E.M. values of three independent observations, each performed in triplicate. Data were fit to two sites using GraphPad Prism. The equation used to fit two sites was constrained such that the sum of the fraction of high-affinity sites and the fraction of low-affinity sites equaled 1. The mean IC₅₀ values were 16 ± 5 and 1,200 ± 100 µM and the mean fraction of the high-affinity component was 0.31 ± 0.04. The solid line represents the theoretical curve for the two-site fit of these data and the dashed line represents a theoretical curve for a one-site fit of these data (IC₅₀ value = 378 µM). C, effect of modulation of PMA on glutamate transport activity in HeLa-GLT1-7. Cells were pretreated with vehicle (DMSO) or 100 nM PMA for 30 min before measurement of Na⁺-dependent glutamate (0.5 µM) transport activity. Transport activity was measured in the absence or presence of 300 µM DHK. Delta represents the difference in activity measured in cells treated with DMSO or PKC. Data are the mean ± S.E.M. of three independent observations each performed in triplicate. Although PMA caused a significant increase in transport activity (*p < .001), the PMA-induced increase in transport activity was not affected by DHK.

The effects of PMA (100 nM for 30 min) were examined in both untransfected and transfected cells. In transfected cells, theabsolute increase in transport activity was greater than thatobserved in untransfected cells (in untransfected cells PMA increasedactivity 1.45 ± 0.5 pmol/mg protein per min and in HeLa-GLT1-7PMA increased activity 11 ± 1 pmol/mg protein per min, mean ±S.E.M. of at least three independent observations). Because theamount of EAAC1 immunoreactivity was greater in HeLa cells transfectedwith GLT-1 than in untransfected cells (2.5 ± 0.4-fold increase,p = .018), it seemed possible that regulation of EAAC1 by PKCmight be sufficient to explain the up-regulation of glutamatetransport activity by PMA in these transfected cells. Becauseprevious studies (and the present pharmacological analyses) suggestthat DHK inhibits GLT-1-mediated transport at lower concentrationsthan are required to inhibit EAAC1-mediated transport, the sensitivityof transport to inhibition by DHK was examined in HeLa-GLT1-7(Fig. 8B). The IC₅₀ value for inhibition of GLT-1 is approximately40 µM (this study) and the IC₅₀ value for inhibition of EAAC1is approximately 1 mM (see Robinson and Dowd, 1997

). In HeLa-GLT1-7cells, the data for inhibition of transport activity by DHK werebest fit to two sites with IC₅₀ values of 16 ± 5 and 1,200 ± 100µM (n = 3). The percentage of the high-affinity site was 31 ±4% of the total. Although the observed up-regulation of EAAC1makes it extremely difficult to directly determine if GLT-1 isactivated by PKC, we utilized this differential sensitivity toDHK to indirectly determine if GLT-1 is regulated by PMA. HeLa-GLT1-7were first preincubated with PMA (100 nM) for 30 min and thentransport activity was measured in the absence or presence of300 µM DHK (Fig. 8C). When transport activity was measured inthe absence of DHK, PMA increased activity from 10.7 ± 0.7 to19 ± 0.6 pmol/mg protein per min. When transport activity wasmeasured in the presence of DHK, PMA increased activity from 6.7± 0.3 to 17 ± 0 pmol/mg protein per min. In fact, the averagePMA-induced increase in transport activity (delta) was not significantlydifferent when activity was measured in the presence or absenceof DHK (300 µM). These data suggest that the transport activitymediated by the component with higher sensitivity to inhibitionby DHK (presumably GLT-1) was not regulated by PMA.

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

In the present study, three different cell lines were stably transfected with the cDNA for the GLT-1 subtype of glutamatetransporter. Stably transfected cell lines have been used as idealmodel systems to study the function, pharmacology, and post-translationalregulation of receptors, channels, and other cell surface proteins.In most cases, the corresponding cDNA is transfected into a cellline that does not endogenously express the protein itself orfunctional homologs. Choosing a cell line to stably express glutamatetransporters presents a challenge because many cells endogenouslyexpress these transporters, presumably to provide glutamate and/oraspartate for metabolic purposes. One approach to overcoming theimpact of endogenous expression might be to select a clone thatexpresses high levels of transport activity. In the present paper,we provide evidence that high expression can affect the kineticand pharmacological properties of transport. To overcome theseproblems, we chose cell lines that express undetectable to lowlevels of endogenous transport activity and characterized transfectedclones that express moderate levels of GLT-1-mediatedactivity.

The properties (K_m and sensitivity to inhibitors) of glutamate transport activity are similar in both the MCB-GLT1-6 and LM-GLT1-8cell lines. This suggests that the low level of endogenous transportin untransfected MCB cells did not significantly affect the propertiesof GLT-1. Some of the compounds tested in the present study havebeen tested as inhibitors of GLT-1 in earlier studies. In theoriginal paper that described the cloning and expression of therat homolog of GLT-1, HeLa cells were used as an expression systemand both DHK and L-AAD were reported to potently inhibit transportactivity (IC₅₀ values < 8 µM; Pines et al., 1992). Arriza andhis colleagues expressed the human homolog of GLT-1 (EAAT2) inCOS-7 cells and found that it is blocked by DHK with an IC₅₀ valueof 23 µM and is not blocked by 1 mM L-AAD (Arriza et al., 1994).While the present study was underway, Wang and colleagues reportedthat the rat homolog of GLT-1 expressed in oocytes is inhibitedby DHK with an IC₅₀ value of 8 µM and that the IC₅₀ value forL-AAD is greater than 1 mM (Wang et al., 1998). Dunlop and hiscolleagues reported that the human homolog of GLT-1 (EAAT2) expressedin Madin Darby Canine kidney cells is inhibited by DHK with anIC₅₀ value of 15 µM and that the IC₅₀ value for L-AAD is greaterthan 1 mM (Dunlop et al., 1998). In the present study, DHK inhibitedGLT-1-mediated transport with an IC₅₀ value of approximately 30to 50 µM and L-AAD inhibited transport with an IC₅₀ value of approximately2 to 3 mM. Thus, the sensitivity to L-AAD observed in the originalstudy has not been observed by four other groups. It is possiblethat this difference is because the transporter was solubilizedand reconstituted in the originalstudy.

The sensitivity of GLT-1-mediated transport to inhibition by a number of compounds is remarkably similar to that observedin cortical tissue. Because the pharmacologies of the brain glutamatetransporters, GLAST, EAAC1, and EAAT4, are different from thoseof cortex (see introduction), the simplest interpretation of theseresults is that GLT-1 mediates the bulk of cortical glutamatetransport activity. Although the pharmacology of transport inhippocampus, striatum, and midbrain has been examined with onlya limited number of compounds, the pharmacological propertiesof GLT-1 are also consistent with transport in these brain regions,suggesting that GLT-1 mediates the bulk of transport activityin forebrain and midbrain. Although one cannot rule out the possibilitythat an uncloned transporter mediates activity in these brainregions, GLT-1 gene deletion and knock-down studies also supportthis conclusion. Infusion (ICV) of antisense oligonucleotidesspecific for GLT-1 decreases protein expression by 60% and causesa 50% decrease in brain transport activity (Rothstein et al.,1996). Genetic deletion of GLT-1 (Tanaka et al., 1997) and pathologicloss of GLT-1 in amyotrophic lateral sclerosis (Rothstein et al.,1995) are also associated with a significant loss (up to 90%)of transport activity in brain tissues. One limitation of thesestudies is that the neurodegeneration that accompanies these decreasesin GLT-1 may lead to an overestimation of the contribution ofGLT-1 to transporteractivity.

If GLT-1 is indeed the predominant cortical (forebrain) transporter, it raises the possibility that nerve terminals do notaccumulate significant levels of glutamate after release, butthere are early lesioning studies that originally suggested thatthere was significant transport into neurons. In these studies,several groups demonstrated that lesioning of afferents decreasestransport activity in the target area (for review, see Fagg andFoster, 1983). Although the original interpretation of these datawas that transporters were localized to nerve terminals, morerecent studies have demonstrated that these lesions result indecreased expression of the glial transporters (Ginsberg et al.,1995; Levy et al., 1995). This suggests that neurons participatein the regulation of expression of the glial transporters in vivo.In fact, in vitro studies have demonstrated that GLT-1 expressionin astrocytes is dependent on the presence of neurons (Gegelashviliet al., 1997; Swanson et al., 1997; Schlag et al., 1998). Thus,some of the early observations that suggested that neurons maybe important for the clearance of glutamate can be explained byglialtransport.

Still, there are observations that cannot be easily explained. First, GLT-1 protein levels in cerebellar synaptosomes arecomparable to that observed in forebrain synaptosomes (Robinson,1998). Yet, no DHK sensitivity is observed in cerebellar synaptosomalmembrane preparations (for review, see Robinson and Dowd, 1997).Second, transport in neuron-enriched cultures, which express onlylow levels of GLT-1 immunoreactivity, has a pharmacology thatis comparable to that observed in cortical synaptosomes (Wanget al., 1998). Although this suggests that there may be anothertransporter with properties similar to GLT-1, the authors didnot exclude the possibility that this low level of GLT-1 expressionmay explain the observedpharmacology.

In an earlier report, Casado et al. (1993) concluded that GLT-1 can be regulated by activation of PKC. In the present study,we found no evidence for regulation of GLT-1-mediated transportactivity by PKC. Activation of PKC, inhibition of PKC, and activationof PKC in the presence of a phosphatase inhibitor had no detectableeffect in two independent cell lines (LM-GLT1-8 and MCB-GLT1-6).In this earlier report, C6 glioma cells were used to demonstratephosphorylation of an immunoprecipitable band. We have found thatC6 glioma cells express EAAC1 but not GLT-1 or the other transporters(Dowd et al., 1996, Davis et al., 1998). Using reverse transcription-polymerasechain reaction another group (Palos et al., 1996) also has concludedthat C6 glioma express only EAAC1. Because EAAC1 is rapidly increasedin response to activation of PKC (Davis et al., 1998), it is possiblethat either the antibody used for immunoprecipitations cross-reactswith EAAC1 or that different sublines of C6 glioma express differentsubtypes of transporters. Casado and her colleagues also transientlyexpressed GLT-1 in HeLa cells using vaccinia virus. They foundthat phorbol esters increase activity of the wild-type transporter,but not of a mutated GLT-1 (S133N) (Casado et al., 1993). Thisprovides fairly convincing evidence that GLT-1 can be regulatedby PMA. In the present study, the effects of PMA on transportactivity were examined in untransfected HeLa and in GLT-1-transfectedHeLa cells (clone HeLa-GLT1-7). Although the increase in transportactivity caused by PMA was greater in GLT-1-transfected cells,the level of EAAC1 immunoreactivity was higher in this transfectedcell line, making it difficult to directly determine if GLT-1is regulated. We attempted to indirectly examine the possibleregulation of GLT-1 by PMA using a strategy to selectively inhibitGLT-1-mediated transport activity using a concentration of DHKthat would be predicted to inhibit GLT-1-mediated transport upto 90% and inhibit EAAC1-mediated transport approximately 20%.Although this experiment demonstrates that the increase in activitycaused by PMA was not inhibited by 300 µM DHK, we cannot ruleout the possibility that PMA changes the potency of DHK for inhibitionof GLT-1. It is difficult to reconcile the results of the presentstudy and those previously published by Casado and her colleagues.It is possible that regulation by PKC is influenced by the levelof transporter expression and that the higher expression presumedto occur with vaccinia virus may explain the difference. Alternatively,it is possible that vaccinia virus induces expression of a protein(possibly a subtype of PKC) that is required for regulation ofGLT-1.

In conclusion, examination of the properties of the GLT-1 transporter reveals that its pharmacological characteristics aresufficient to explain the majority of activity in crude synaptosomesprepared from cortex and possibly other forebrain regions. BecauseGLT-1 is generally thought to be expressed by mature astrocytesin vivo (for review, see Robinson and Dowd, 1997), this suggeststhat extracellular EAAs released from the nerve terminal recyclethrough the astrocyte rather than through reuptake directly intothe nerve terminal. Although there is substantial evidence forpost-translational regulation of other transporters and cell surfaceproteins by PKC (for references, see Davis et al., 1998), we wereunable to detect any effect of PKC stimulation on GLT-1activity.

	Acknowledgments

We thank Brian Schlag for his help with preparing the transfected cell lines, Dr. Paul Rosenberg for his helpful discussionsregarding the explanation for the effects of overexpression oftransporters on their kinetic and pharmacological properties,and Dr. Baruch Kanner for the GLT-1 cDNA. We also thank AnjaliGupta for her excellent editorialassistance.

	Footnotes

Accepted for publication February 16, 1999.

Received for publication August 26, 1998.

¹ This work was supported by National Institutes of Health Grants NS29868 and HD26979 (M.B.R.) and NS36465 (M.B.R., J.D.R.).

Send reprint requests to: Michael B. Robinson, Abramson Pediatric Research Building, Room 502, 34th and Civic Center Blvd., Philadelphia, PA 19104-4318. E-mail: robinson{at}pharm.med.upenn.edu

	Abbreviations

Bis, bisindolylmaleimide II; DHK, dihydrokainate; EAA, excitatory amino acid; L-AAD, L- $alpha$ -aminoadipate; L-AP3, L-2-amino-3-phosphonopropionate; PMA, phorbol 12-myristate 13-acetate; PKC, protein kinase C; L-trans-PDC, L-trans-pyrrolidine-2,4-dicarboxylate; mGluR, metabotropic glutamate receptor; DMSO, dimethyl sulfoxide.

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Expression of the GLT-1 Subtype of Na⁺-Dependent Glutamate Transporter: Pharmacological Characterization and Lack of Regulation by Protein Kinase C¹