Glutamate, But Not Dopamine, Stimulates Stress-Activated Protein Kinase and AP-1-Mediated Transcription in Striatal Neurons

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Volume 17, Number 10, Issue of May 15, 1997 pp. 3455-3466
Copyright ©1997 Society for Neuroscience

Glutamate, But Not Dopamine, Stimulates Stress-Activated Protein Kinase and AP-1-Mediated Transcription in Striatal Neurons

Michael A. Schwarzschild¹^,²^,^a, Rebecca L. Cole¹^,⁴^,^a, and Steven E. Hyman¹^,³^,⁴
¹ Laboratory of Molecular and Developmental Neuroscience, Massachusetts General Hospital, Charlestown, Massachusetts 02129, Departments of ² Neurology and ³ Psychiatry, Massachusetts General Hospital and Harvard Medical School, Boston, Massachusetts 02115, and ⁴ Program in Neuroscience, Harvard Medical School, Boston, Massachusetts 02115

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Drugs that stimulate dopamine and glutamate receptors have been shown to induce the expression of AP-1 proteins (such as c-Fosand c-Jun) in the striatum and to induce binding of these proteinsto AP-1 sites on DNA, leading to the hypothesis that AP-1-mediatedtranscription contributes to the long-term effects of these drugs.To examine this hypothesis, we compared the regulation of AP-1-mediatedtranscription to the inductions of AP-1-binding activity and genesencoding AP-1 proteins in primary cultures of striatal neurons.Although glutamate, dopamine, and forskolin (an activator of adenylatecyclase) all induce c-fos mRNA and AP-1 binding, we found, surprisingly,that only glutamate induces transcription of a transfected AP-1-drivenfusion gene. To explore the basis for this discrepancy, we investigatedthe possibility that the phosphorylation of c-Jun may also berequired for AP-1-mediated transcription in striatal neurons.Glutamate, but neither dopamine nor forskolin, raises the levelsof phosphorylated c-Jun as well as the activity of a Jun kinase(SAPK/JNK) in striatal cultures. Both the glutamatergic inductionof AP-1-mediated transcription and activation of SAPK/JNK appearto be mediated, at least in part, via NMDA receptors. In striatalneurons, the phosphorylation of AP-1 proteins produced by glutamatemay be required to convert AP-1 protein expression and bindingto transcriptional activation.
Key words: glutamate; NMDA; SAPK; JNK; c-fos; c-jun; AP-1; transcription; striatum; cell culture

INTRODUCTION

Corticostriatal glutamate projections and mesostriatal dopamine projections are the predominant afferents innervating themedium spiny neurons of the striatum. Medium spiny neurons, whichmake up >90% of all striatal neurons, project out of the striatumvia two major pathways, the striatonigral and striatopallidalpathways. Medium spiny neurons giving rise to the striatonigralpathway express largely D1 dopamine receptors (Gerfen et al.,1990; Le Moine et al., 1991), which are positively coupled toadenylate cyclase; those giving rise to the striatopallidal pathwayexpress largely D2 dopamine receptors (Gerfen et al., 1990; LeMoine et al., 1990), which are negatively coupled to adenylatecyclase. Medium spiny neurons in both output pathways also expressa variety of NMDA (Standaert et al., 1994; Landwehrmeyer et al.,1995) and non-NMDA (Martin et al., 1993; Tallaksen-Greene andAlbin, 1994) ionotropic glutamate receptors as well as metabotropicglutamate receptors (Testa et al., 1994, 1995).

Stimulation of dopaminergic or glutamatergic receptors on striatal neurons elicits not only short-term physiological responses,but also long-term responses that result from second messengerregulation with subsequent alterations in gene expression. Regulationof gene expression in striatum by dopaminergic drugs has beenwidely reported, with many groups describing induction of bothimmediate early genes and neuropeptide genes. For example, theindirect dopamine agonists amphetamine and cocaine have been shownto induce expression of c-fos mRNA and its protein product instriatum in a D1 dopamine receptor-dependent manner (Graybielet al., 1990; Young et al., 1991; Nguyen et al., 1992; Konradiet al., 1994). Both amphetamine (Nguyen et al., 1992) and cocaine(Hope et al., 1992, 1994) also induce AP-1-binding activity, ofwhich c-Fos is a component, in striatal cell extracts.

Glutamatergic stimulation has been shown to induce mRNAs encoding AP-1 proteins in a variety of neuronal systems, includingcultured hippocampal neurons (Lerea et al., 1992, 1993; Badinget al., 1993, 1995) and cultured cerebellar granule cells (Szekely,1989). In primary cultures of cortical and striatal neurons, activationof NMDA receptors results in induction of c-fos, fosB, c-jun,and junB mRNA (Vaccarino et al., 1992; Condorelli et al., 1994).Glutamate stimulation also results in an NMDA receptor-dependentincrease in AP-1-binding activity in cultured neurons (Condorelliet al., 1994). In vivo stimulation of NMDA receptors by intrastriatalinjection of quinolinic acid results in the induction of Fos proteinin the majority of striatal projection neurons (Berretta et al.,1992).

Overall, there now exists a body of data on the induction of c-Fos and other AP-1 proteins, as well as on AP-1-binding activityby dopaminergic and glutamatergic stimuli in striatum. It hasbeen hypothesized that induction of c-Fos and AP-1 binding instriatal neurons would lead to significant alterations in transcriptionof AP-1-regulated target genes. However, this hypothesis has notbeen tested directly. We have undertaken the present study toinvestigate the mechanisms and transcriptional consequences ofthose inductions in a primary neuronal culture model system thatpermits transfection analysis. We report that although glutamate,dopamine, and forskolin all induce c-fos expression and AP-1 binding,only glutamate activates AP-1-mediated transcription. We identifythe activation of a Jun kinase (SAPK/JNK) and the phosphorylationof c-Jun as a potential mechanism for the glutamatergic inductionof AP-1-mediated transcription. The specificity of the SAPK/JNKsignaling cascade for glutamate versus dopamine may have implicationsfor drug action in the striatum in vivo. Moreover, our data raisenew questions regarding the involvement of SAPK/JNK pathways inglutamate-regulated developmental, neurodegenerative, and neurotoxicprocesses in the CNS.

MATERIALS AND METHODS
Primary striatal culture. Primary striatal cell cultures were prepared as described (Konradi et al., 1994), with the modificationthat cells were placed in defined media just 4 hr after platingto further curb proliferation of glial cells. The defined medium(DMEM/F12 with B-27 supplementation, Life Technologies, Gaithersburg,MD) includes 1.0 mM calcium, 0.7 mM magnesium, 4.2 mM potassium,and 40 µM glutamate. However, as determined by HPLC analysis,glutamate levels in the medium just before drug treatment rangedfrom 1 to 5 µM (Konradi et al., 1996). Experiments were performedwith cells after 5 d in culture. Drugs for treatment of culturesincluded dopamine (RBI, Natick, MA), glutamate (Sigma, St. Louis,MO; all other glutamatergic agents from RBI), forskolin (Sigma),and 12-O-tetradecanoylphorbol-13-acetate (TPA, Sigma). Glial cellcultures were prepared as with the standard neuronal cultures,except that striatal cell suspensions were seeded onto uncoatedsix-well tissue culture plates (Costar, Cambridge MA), and cultureswere maintained in 10% Nu-serum (Collaborative Biomedical Products,Bedford, MA) media to allow glial growth from sparse (~1% surfacecoverage) on day 1 in culture to near confluence on day 9 in culture.

Calcium phosphate transfection. A construct containing four consecutive AP-1 elements fused to the luciferase reporter genewas transfected into primary striatal cultures using a serum-freecalcium phosphate transfection protocol. The AP-1 core consensussequence is identical to that described below for the substanceP (SP) AP-1 oligonucleotide. Briefly, on day 5 in culture cellswere fed with DMEM (Life Technologies) and the conditioned mediumwas saved and stored at 4°C. To transfect, 5 µg of DNA in 80 µlof total calcium phosphate precipitate was added to each 35 mmwell for 1 hr, at which time cells were washed twice with DMEM,and 1.5 ml of conditioned medium was added back and the cellswere returned to the incubator. Drugs were added ~36 hr aftertransfection, and cells were harvested 6 hr after the drug treatmentsand assayed for luciferase activity. All experiments were performedin triplicate. Overall transfection efficiency ranged between1 and 5%, determined by cytochemistry after transfection of anRSV- $beta$ gal expression plasmid (data not shown).

Electrophoretic mobility shift assay. Electrophoretic mobility shift assays (EMSA) were performed as described previously(Korner et al., 1989). Cells were lysed in EMSA buffer containingNP-40 (1%) and the phosphatase inhibitors sodium fluoride (1 µM,Sigma) and microcystin (5 µM, Life Technologies). Approximately5 µg of protein was loaded per lane. Oligonucleotides were synthesizedwith an overhang and annealed in the presence of 20 mM NaPO₄,1 mM EDTA, and 100 mM KCl. The overhangs of the double-strandedoligonucleotides were then filled in, using Superscript ReverseTranscriptase (Life Technologies), with ³²P-labeled dCTP. All experiments were performed in an excess ofprobe. The sequence of oligonucleotide used in electrophoreticmobility shift assays was AP-1-human SP promoter or human metallothionein(hMT) promotor, 5 $'$ -GATCAGCATGAGTCACTTC-3 $'$ or 5 $'$ -GATCCGCGTGACTCAGCGC-3 $'$ ,respectively (Konradi et al., 1994); CRE, 5 $'$ -GATCGCTGACGTCAGGG-3 $'$ (Hoeffler et al., 1988; Hai et al., 1989); AP-4 (human proenkephalingene), 5 $'$ -GATCGTCAGCTGCGGG-3 $'$ (Comb et al., 1988); jun2TRE(rat c-jun promoter), 5 $'$ -AGCTAGCATTACCTCATCCC-3 $'$ (Morookaet al., 1995). The overhang is shown in italics, core consensussequences in bold. Note that the core AP-1 motifs within the SPand hMT promoters are identical on their opposite DNA strandsand, thus, the two AP-1 oligonucleotides differ only in flankingsequence. Although the binding patterns of the two AP-1 probesare virtually identical for the experiments described here andpreviously (Konradi et al., 1993), the difference in flankingsequence does promote the binding of an additional protein complexto the hMT AP-1 element. This binding complex is nonspecific,because it is not altered by drug treatment or competition withat least 10-fold excess unlabeled probe (Konradi et al., 1995).

For competition assays, the unlabeled and labeled probes were combined before the addition of lysates, after which incubationwas performed at 4°C for 10 min and then at room temperature for10 min before loading the reaction mixture on a gel. For supershiftanalysis, antibodies (1 µg) together with whole-cell extract proteins(5 µg) were incubated in a 30 µl volume at 4°C for 10 min, followedby incubation with labeled probe (1 ng) at 4°C for 10 min andthen at room temperature for 10 min before loading (25 µl). Antibodiesused in supershift analysis include those directed against c-Jun(sc-45 X, Santa Cruz Biotechnology, Santa Cruz, CA), ATF-2 (sc-187X, Santa Cruz Biotechnology), and c-Fos (Ab-5, Oncogene Science,Uniondale, NY).

Northern blot analysis. Northern blot analysis was performed as described (Cole et al., 1995). Briefly, cells were lysed in400 µl of NP-40 lysis buffer, and phenol-chloroform extractionwas used to isolate the RNA. Equal amounts of RNA (2 µg) wereloaded per lane. Blots were hybridized with a c-fos or c-jun riboprobe(Gemini system, Promega, Madison, WI). Hybridization of a cyclophilincDNA probe (Danielson et al., 1988) was used as an internal control.

Western blot analysis. Cells were lysed in their wells as they were thawed on ice in 100 µl of a 1× Laemmli buffer. Lysateswere sonicated, boiled, separated on polyacrylamide gels, andthen electroblotted onto Immobilon-P membranes (Millipore, Bedford,MA). After blocking in 5% milk/0.05% Tween 20 in PBS, the membraneswere probed with primary antibody in otherwise identical bufferexcept with 0.5% milk and 1:10,000 polyclonal anti-SAPK $beta$ (whichcross-reacts with $alpha$ and $gamma$ forms) (Kyriakis et al., 1994) and/oranti-JNK1 (C-17, Santa Cruz Biotechnology), 1:1000 anti-phospho(Ser73)-c-Jun(New England Biolabs, Beverly, MA), 1:2000 anti-c-Jun [Santa Cruz'sH-79 was used as NEB's anti-c-Jun antibody (#9162)] did not detectany inducible immunoreactivity), 1:500 anti-phospho-CREB (UBI,Lake Placid, NY), and 1:1000 anti-CREB (New England Biolabs) for1 hr. After multiple washes membranes, were treated with 1:5000donkey anti-rabbit IgG (Amersham, Arlington Heights, IL) in thesame buffer for 1 hr. After multiple additional washes in thesame buffer, except without milk, membranes were processed withECL reagents per the manufacturer's protocol (Amersham).

For the Western blots with phosphatase pretreatment, each striatal lysate was prepared using 40 µl of the immune-complex kinaseassay's lysis buffer (see below), except that 400 mM NaCl and5 µM microcystin were included, and that the other phosphataseinhibitors (sodium vanadate and $beta$ -glycerophosphate) were presentat 1/100th their standard concentrations. Calf intestinal alkalinephosphatase (Sigma P-0405, 20 U in 1 µl with or without heat inactivationby boiling for 15 min) was added to 20 µl of the lysate supernatant,and the mixture was incubated at 37°C for 30 min before stoppingthe reaction with 6× Laemmli buffer. The Western blot analysiswas completed using anti-phospho(Ser73)-c-Jun, as above.

Immune-complex kinase assays. Treatment of striatal cultures was terminated by aspirating off medium, washing once with chilledPBS, aspirating off the wash, and freezing plates in liquid nitrogenfollowed by storage at $-$ 80°C. The kinase assay was modified fromKyriakis et al. (1994). Lysis buffer (1 ml/well; 20 mM HEPES,pH 7.4, 2 mM EGTA, 1 mM sodium vanadate, 50 mM $beta$ -glycerophosphate,10% glycerol, 1% Triton X-100, 2 µM leupeptin, 400 µM phenylmethylsulfonylfluoride, 10 KIU/ml aprotinin, 400 µM diisopropyl fluorophosphate,and 1 mM dithiothreitol) was added to the frozen cells, whichwere thawed and lysed on ice for 15 min. The lysate was spun ina microfuge (15,000 g) for 5 min at 4°C, and the supernatant wastransferred to 40 µl of 1:1 lysis buffer/swollen protein A-SepharoseCL-4B beads (Sigma) to which an anti-kinase antibody had beenadded. Polyclonal anti-SAPK $beta$ , anti-JNK1(C-17), or anti-p38 (anti-XMpk2)(Rouse et al., 1994) antibodies at 1:1000 final concentrationwere used. Immunoprecipitation was performed at 4°C, with rotationof samples for 2-12 hr. Beads were washed once in lysis buffer,twice in high ionic strength buffer (500 mM lithium chloride,100 mM Tris, pH 7.8, 0.1% Triton X-100, and 1 mM dithiothreitol),and three times in kinase buffer (20 mM MOPS, pH 7.2, 10 mM magnesiumchloride, 2 mM EGTA, 0.1% Triton X-100, and 1 mM dithiothreitol).To the 20 µl of beads with 20 µl of overlying kinase buffer wasadded 20 µl of substrate [0.3 mg/ml c-Jun(1-135)-GST or 0.2 mg/mlmyelin basic protein (Sigma)] in kinase buffer. The kinase reactionwas initiated by adding 15 µl of 50 mM magnesium chloride and125 µM total ATP including 4-10 µCi $gamma$ ³²P-ATP per sample. After 20 min at 30°C with frequent mixings,the reactions were stopped by the addition of 20 µl 6× Laemmlibuffer. Samples were boiled 5 min before running on a 12% polyacrylamidegel. Radiolabeled (phosphorylated) Jun substrate was detectedin a band corresponding to the predicted 40 kDa using a Phosphorimagerdetection system (Molecular Dynamics, Sunnyvale, CA; used forall radioassays).

In-gel kinase assay. Striatal Jun kinase activity was characterized by immunoprecipitating SAPK/JNK (with anti-JNK1[C-17]at 1:1000 as in the immune complex kinase assay above). The immunoprecipitatedkinase was then resolved electrophoretically under denaturingconditions in a polyacrylamide gel polymerized with 40 µg/ml c-Jun(1-135)-GST,renatured, and then incubated in the gel with 100 µCi/ml $gamma$ ³²P-ATP, as described previously (Cano et al., 1994).

RESULTS

Glutamate, but not dopamine or forskolin, induces AP-1-mediated transcription
We compared the effects of known inducers of AP-1 binding on transcription of a transfected 4× AP-1 luciferase construct inneuron-enriched striatal cultures derived from embryonic day 18(E18) rats. The AP-1 sequence used is a consensus sequence foundwithin the promoter of the preprotachykinin gene, which is expressedin D1 dopamine receptor-expressing striatal neurons. Like thephorbol ester TPA (the classic activator of AP-1-mediated transcription),glutamate (100 µM) stimulates the activity of the luciferase reportergene 7- to 10-fold (Fig. 1A,B). This glutamate-induced transcriptionalactivation is blocked by pretreatment with the NMDA receptor antagonistMK-801 (Fig. 1B). In contrast, dopamine (100 µM) and forskolin(a direct activator of adenylate cyclase, 10 µM) do not inducetranscriptional activation of this AP-1-driven construct. In fact,dopamine and forskolin result in a slight, but reproducible, decreaseof luciferase activity to levels below basal (Fig. 1A) (data notshown).
Fig. 1. Glutamate, but not dopamine or forskolin, induces expression of a transfected 4× AP-1-luciferase fusion construct. A, Glutamate(Glu, 100 µM) and TPA (100 nM), but not dopamine (DA, 100 µM)or forskolin (F, 10 µM), activate transcription of a 4× AP-1 luciferaseconstruct. Values for luciferase activity are given as fold induction,and data are represented as mean ± SEM percentage of transfectedcontrol values (n = 3). Background luciferase activity determinedfrom untransfected controls was subtracted; *p < 0.05 comparedwith control group. B, The glutamate activation of AP-1 transcriptionis blocked by MK-801 (1 µM, added 10 min before glutamate); *p< 0.05 compared with control or glutamate plus MK-801 groups.
[View Larger Version of this Image (9K GIF file)]

Glutamate, dopamine, and forskolin all increase AP-1-binding activity in extracts of the striatal cultures
To investigate whether the inability of dopamine and forskolin to induce Ap-1-mediated transcription results from an inabilityto induce AP-1 binding in the striatal cultures used here, wemeasured AP-1-binding activity using EMSA. Glutamate (100 µM)induces binding to the consensus AP-1 sequence with peak bindingactivity occurring after 2 hr of treatment (Fig. 2A-C). The specificityof binding and the relative affinities of the bound proteins forthe AP-1 element compared with other DNA binding sites were examinedusing competition with unlabeled oligonucleotides (Fig. 2B). Aftera 2 hr glutamate stimulation, unlabeled AP-1 (self) competes forthe inducible binding at 5- and 10-fold molar excess, whereasthe related jun2TRE element and consensus ATF element only competefor binding at 100-fold molar excess. The unrelated AP-4 elementdoes not compete for AP-1 binding, even at 100-fold molar excess(Fig. 2B). Formation of the glutamate-induced AP-1 complex isblocked by pretreatment with the NMDA receptor antagonist MK-801(Fig. 2D).
Fig. 2. AP-1 binding after glutamate, dopamine, and forskolin stimulation in primary striatal cultures. A, AP-1 binding in striatalextracts after stimulation with dopamine (DA, 100 µM), glutamate(Glu, 100 µM), forskolin (Forsk, 10 µM), and TPA (100 nM) for2 hr. Controls (dash) are from untreated cells. B, The specificityof AP-1-binding activity was determined by gel-shift competitionexperiments with striatal extracts 2 hr after glutamate stimulation.Unlabeled AP-1 (self), the related oligonucleotides for jun2TREand CRE, and the unrelated AP-4 element display decreasing potencies,respectively, in their abilities to compete for the upper bindingcomplex (specific band). In addition to the specific band, twoless-specific, faster-migrating complexes can be observed (arrowheads).These binding complexes are present in untreated cell extractsand are not glutamate-inducible (see Fig. 3). These complexesare not competed effectively by addition of unlabeled self butcan be competed by all the oligonucleotides, including the unrelatedAP-4 element, at 100-fold molar excess. C, Time courses of glutamate-and forskolin-induced AP-1 protein binding. After glutamate stimulation,AP-1 binding is induced with a peak at 2-4 hr. Forskolin inductionof AP-1 binding is more robust and peaks at 2 hr. D, The inductionof AP-1 binding by glutamate stimulation can be blocked by theNMDA receptor antagonist MK-801 (1 µM, added 10 min before glutamate).All data are representative of at least three independent experiments.All experiments were performed with the SP AP-1 oligonucleotideprobe.
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Stimulation by dopamine results in a small but reproducible induction of AP-1 binding, with an increase that also peaks at2 hr (Fig. 2A). In other experiments, it was observed that dopaminecan also induce a modest increase in a slightly more slowly migratingAP-1 complex (data not shown). Many D1 dopamine receptor actionsare mediated by the cAMP pathway. In striatum in vivo, ~50% ofmedium spiny neurons express D1 receptors (Gerfen et al., 1990).Thus, dopamine would only stimulate adenylate cyclase in a subsetof the cells in the cultures and perhaps not fully stimulate adenylatecyclase, even in those cells. Forskolin, which directly stimulatesadenylate cyclase in a receptor-independent manner and presumablyin all cells, thus would be expected to produce a greater activationof the cAMP pathway than would dopamine. Indeed, forskolin (10µM), like glutamate and TPA, results in a robust increase in AP-1binding that also peaks at 2 hr (Fig. 2A,C).

Fos and Jun, but not ATF-2, are present in induced AP-1 complexes
Antisera directed against AP-1 proteins were used to investigate the composition of glutamate- and forskolin-induced AP-1complexes bound to the consensus AP-1 element (Fig. 3A). Two hoursafter glutamate or forskolin stimulation, the specific AP-1 complexis recognized and supershifted by c-Fos antibodies, indicatingthat c-Fos is present in both complexes. With a specific antiserumdirected against c-Jun, evidence for inclusion of c-Jun in theAP-1 complex was detected reproducibly in extracts of striatalneurons that had been treated with glutamate. A small supershiftedcomplex associated with a diminution in the specific band is observableafter glutamate and, to a lesser extent, after forskolin stimulation.The ability of this antibody to recognize adequately the c-Juncomponent of AP-1 complexes was verified by nearly complete supershiftsof the labeled AP-1 probe incubated in the presence of syntheticc-Jun and c-Fos prepared in reticulocyte lysates (data not shown).
Fig. 3. Supershift analysis of AP-1 and jun2TRE binding complexes after glutamate and forskolin stimulation. A, After 2 hr of glutamate(Glu) and forskolin (F) stimulation, AP-1-binding activity isincreased over control (Con, no drug treatment), as indicatedby the increased intensity of the specific complex (arrowhead).Addition of anti-Fos antibodies ( $alpha$ c-Fos) results in the appearanceof a supershifted band (ss), indicating that Fos protein is presentin the glutamate- and forskolin-induced AP-1-binding complex.The ATF-2 antibody ( $alpha$ ATF) has no effect on AP-1 binding. Thec-Jun antibody ( $alpha$ c-Jun) results in a reduction in the overalllevels of AP-1 binding, suggesting that addition of the antibodyis interfering with formation of the DNA/protein complex. In addition,a minor supershifted band is observable after glutamate and, toa lesser extent, after forskolin stimulation. B, In contrast toAP-1 binding (A), protein binding to the jun2TRE after 2 hr ofglutamate and forskolin stimulation can be supershifted by additionof ATF-2 antibodies, but not by addition of c-Fos antibodies.Arrowheads indicate two specific protein-oligonucleotide complexes.A modest reduction in jun2TRE binding and a minor supershiftedband are also seen after addition of c-Jun antibodies. C, Bindingto the AP-1 element can be disrupted by addition of either a JunD( $alpha$ JunD) or a JunB ( $alpha$ JunB) antibody. Addition of the JunD antibodyreduces basal binding as well as glutamate- and forskolin-inducedbinding. The antibody directed against JunB selectively reducesthe forskolin-induced binding complex. No difference is apparentif 1 µg (1×) or 2 µg (2×) of JunB antibody is included per lane.These reductions in the induced specific complexes (arrowhead)are associated with the appearance of modest probable supershiftbands (asterisk). The SP AP-1 and hMT AP-1 oligonucleotides wereused in A and C, respectively. A nonspecific binding complex isapparent below the specific band in C (not present in A) and isattributable to flanking sequences of the hMT probe, which aredistinct from those of the SP probe (see Materials and Methods).Each experiment is representative and was performed at least fourtimes (A, B) or twice (C).
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Because AP-1 complexes may differ in their abilities to activate transcription depending on which Jun family members theycontain, we also tested antibodies to other members of the Junfamily. Although anti-JunD antibodies disrupt formation of glutamate-and forskolin-induced complexes proportionally, anti-JunB antibodies(at two concentrations) reduce levels of AP-1 complexes inducedby forskolin to a greater extent than those induced by glutamate(Fig. 3C). The diminutions in these specific bands correspondto the appearance of probable supershifted complexes. Althoughfaint, these more slowly migrating complexes appear of increasedintensity after glutamate treatment using anti-JunD antibodiesand after forskolin treatment using either anti-JunD or anti-JunBantibodies. These data suggest that although glutamate and forskolinsimilarly enhance the formation of AP-1 complexes that recruitJunD (which is constitutively present in striatal neurons) (datanot shown), forskolin, to a greater extent than glutamate, inducesJunB as a component of these complexes.

Antibodies specifically directed against another protein, ATF-2, do not recognize the complexes binding the consensus AP-1element (Fig. 3A), although they supershift completely a complexbinding to a jun2TRE oligonucleotide probe (Fig. 3B). The jun2TREis a variant AP-1 promoter element, which binds preferentiallyc-Jun/ATF-2 heterodimers instead of c-Fos/c-Jun heterodimers (vanDam et al., 1993).

Glutamate, dopamine, and forskolin induce c-fos mRNA
The inductions of Fos-containing AP-1 complexes may be attributable to inductions of c-fos gene expression. We have shownpreviously that dopamine induces c-fos mRNA in primary culturesof striatal neurons in a D1 dopamine receptor-dependent fashion(Konradi et al., 1994; Cole et al., 1995) (Fig. 4C). Forskolin(10 µM) produces an even stronger induction of c-fos mRNA. Glutamate(100 µM) also induces c-fos mRNA in the cultures (Fig. 4A,B).The increase in c-fos mRNA stimulated by glutamate peaks after30-90 min and returns to basal levels by ~6 hr. A similar timecourse of c-fos mRNA induction was observed after dopamine orforskolin stimulation. These inductions of c-fos mRNA, which precedethose of AP-1 binding, support further the possibility that increasedc-Fos levels account, at least in part, for the increased AP-1binding observed in striatal cultures after stimulation of bothglutamatergic and dopaminergic pathways.
Fig. 4. Glutamate, dopamine, and forskolin all induce c-fos mRNA, whereas only glutamate induces c-jun mRNA. A, Northern blot analysisfor c-jun mRNA and c-fos mRNA induced by glutamate (100 µM). c-junmRNA levels peak at an 8.5-fold induction 1.5 hr after glutamatestimulation. The more rapidly and more highly inducible c-fosmRNA peaks at 65-fold induction. Mean values ± SEM represent percentagesof control levels (n = 3). B, C, Time courses for the effectsof glutamate (100 µM), forskolin (10 µM), and dopamine (100 µM)on c-jun, c-fos, and cyclophilin mRNA. Northern blots were firsthybridized with a c-jun riboprobe (3.2 and 2.5 kb transcripts),stripped, rehybridized with a c-fos riboprobe (2.2 kb transcript),and then hybridized for the third time with a cyclophilin cDNAprobe. Cyclophilin (cyclo) mRNA was used as an internal loadingcontrol. All data are representative of at least three independentexperiments.
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Glutamate, but not dopamine or forskolin, increases c-jun mRNA levels
Although the c-fos promoter contains multiple cAMP response elements (CREs) (Berkowitz et al., 1989; Fisch et al., 1989) anda serum response element (SRE), which may account for the inductionsof c-fos mRNA by dopamine, forskolin, and glutamate (see Discussion),the c-jun promoter contains neither a CRE nor an SRE. Rather,major regulatory targets for extracellular signals within thec-jun promoter are two TPA response elements, the jun1TRE andjun2TRE (Angel et al., 1988; van Dam et al., 1995). In contrastto c-fos mRNA, c-jun mRNA is not increased in response to eitherdopamine or forskolin in the striatal cultures (Fig. 4B,C), althoughwe have shown previously that junB mRNA is induced by dopaminein these cultures (Konradi et al., 1996). Unlike dopamine andforskolin, glutamate markedly increased levels of c-jun mRNA witha nearly ninefold induction observed at 60-90 min (Fig. 4A). Thespecificity for glutamate of the induction of c-jun mRNA may accountfor the greater induction of a c-Jun component in the AP-1-bindingcomplex by glutamate compared with forskolin (Fig. 3A).

Glutamate, but not dopamine or forskolin, increases phosphorylated c-Jun
We have demonstrated that in striatal cultures, dopamine, forskolin, and glutamate all induce c-fos expression followed byincreased binding of a Fos-containing AP-1 protein complex toconsensus AP-1 sites. Surprisingly, however, only glutamate increasestranscription through this AP-1 element, indicating that the inductionof AP-1 binding does not suffice to induce AP-1 transcription.In several non-neuronal cell types, AP-1-mediated transcriptionhas been shown to require the phosphorylation of proteins withinAP-1 complexes (Binétruy et al., 1991; Deng and Karin, 1994).Phosphorylation of c-Jun on Ser-63 and Ser-73 within its N-terminalactivation domain has been shown to enhance markedly its abilityto activate transcription without affecting its ability to formdimers or bind DNA (Dérijard et al., 1994; Karin, 1995).

We investigated whether the levels of phosphorylated c-Jun correlate with the inductions of AP-1-mediated transcription instriatal cultures. Using an antiserum that recognizes phospho(Ser73)-c-Jun,but not the dephosphorylated form, Western blot analysis demonstratesthat glutamate increases levels of phospho(Ser73)-c-Jun-like immunoreactivityin three bands with approximate molecular weights of 40, 43, and45 kDa, which correspond to the range of reported molecular weightsof c-Jun (Lamph et al., 1988) (Fig. 5A). The uppermost inducedband (~45 kDa) likely represents phospho-c-Jun, because it coincidesin molecular weight with the major immunoreactive band for total(unphosphorylated and phosphorylated) c-Jun (Fig. 5A,B, bottomblots) and with a similarly induced band of phospho(Ser63)-c-Junimmunoreactivity (data not shown). Furthermore, the induced bandat ~45 kDa (but not at ~43 kDa) was eliminated by phosphatasetreatment of lysates (see Materials and Methods), indicating thatit represents a phospho-antigen. This putative 45 kDa phospho-c-Junband increases within 30 min and peaks after 60-90 min of glutamatetreatment (Fig. 5B, top blot). Increases in total c-Jun proteinwere also induced by glutamate, but did not appear before 1 hrand did not peak until 3 hr of glutamate treatment (Fig. 5B, bottomblot). Thus, although a rise in c-Jun protein may be contributingto increased levels of phospho-c-Jun measured at later time points,it cannot account for the initial increase in phospho-c-Jun levels.
Fig. 5. Elevation of phosphorylated c-Jun levels by glutamate, but not by dopamine or forskolin. A, Western blots probed with anti-phospho(Ser73)-c-Jun(top) and anti-c-Jun (bottom) antibodies performed on the samelysates of striatal cultures treated with or without glutamate(100 µM), dopamine (100 µM), or mannitol (300 mM) for the timesindicated. B, Western blots probed as in A on lysates of striatalcultures treated with glutamate (100 µM) for the times indicated.C, Western blots probed with anti-phospho-CREB (top) and anti-CREB(bottom) antibodies performed on lysates of striatal culturestreated as in A. In A-C, the same blot was probed with antibodiesdirected toward the phosphorylated transcription factor and thenreprobed with the antibodies directed toward the total form. Thepositions of flanking molecular weight markers are indicated onthe right. All results were consistently reproducible in independentexperiments.
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Dopamine and forskolin, which fail to increase AP-1-mediated transcription (see Fig. 1), also fail to elevate levels of phospho-c-Junat 45 or 90 min (Fig. 5A). In these cultures, however, forskolinis capable of raising levels of Ser¹³³ phosphorylated CREB (CRE binding protein), which, like c-Jun,is a member of the superfamily of basic leucine zipper transcriptionfactors (Fig. 5C). Interestingly, glutamate increases levels ofphospho-CREB in striatal cultures, although to a lesser extentthan forskolin. Glutamate-induced phosphorylation of CREB mayreflect the known effects on this transcription factor of calcium/calmodulin-dependentprotein kinases (Sheng et al., 1991) or the Ras-MAPK pathway (Xinget al., 1996).

Glutamate, but not dopamine or forskolin, activates SAPK/JNK
Phosphorylation and activation of c-Jun results from the action of JNK, also called SAPK, because it was shown initially tobe activated by cellular stressors such as ultraviolet radiation,heat shock, and hyperosmolar conditions (Dérijard et al., 1994,Kyriakis et al., 1994). SAPK/JNK is a member of the MAPK/extracellularsignal regulated kinase (ERK) family of protein kinases, the mammalianmembers of which include the ERKs, p38, and SAPK/JNK. SAPK/JNKcomprises several gene products called SAPK $alpha$ , $beta$ , and $gamma$ in therat and JNK1 and JNK2 in humans (Kyriakis and Avruch, 1996). Inaddition to cellular stressors, the inflammatory cytokines IL-1 $beta$ and TNF $alpha$ have been shown to activate both SAPK/JNK and p38 (Freshneyet al., 1994; Han et al., 1994; Rouse et al., 1994). SAPK/JNKalso can be activated by stimulation of muscarinic acetylcholinereceptors expressed by stable transfection of a fibroblast cellline (Mitchell et al., 1995).

We investigated whether the activation of SAPK/JNK might account for the phosphorylation of c-Jun and the activation of AP-1-mediatedtranscription in cultured striatal neurons. Glutamate rapidlyincreases SAPK/JNK activity, as measured by in vitro phosphorylationof a c-Jun N-terminal substrate by anti-SAPK/JNK immunoprecipitatesfrom treated cells (Fig. 6A). The antibodies used to immunoprecipitateSAPK/JNK activity recognize two major bands on Western blots preparedfrom lysates of striatal cultures (Fig. 6B) corresponding to the54 and 46 kDa isoforms of SAPK/JNK (Hibi et al., 1993; Dérijardet al., 1994; Kyriakis et al., 1994). The lack of alteration ofSAPK/JNK protein levels during the period when its activity ismaximally increased suggests that increased activity is attributableto a post-translational modification of the kinase rather thanincreased protein levels. In-gel kinase assays (Fig. 6B) demonstratethat the glutamate-inducible c-Jun kinase activity in lysatesof primary striatal culture corresponds to proteins of the predictedsizes, with the 46 kDa form predominating.
Fig. 6. Rapid and specific activation of SAPK/JNK by glutamate. A, Immune-complex kinase assay for SAPK/JNK activity at differenttimes after treatment of primary striatal cultures with glutamate(100 µM). The bands indicate c-Jun(1-135)-GST substrate (~40 kDa)that was phosphorylated by anti-SAPK/JNK immunoprecipitates beforeseparation in a polyacrylamide gel. The last lane shows the reactionproduct using cells that were treated with an additional 100 µMglutamate for the last 45 min of a 6 hr treatment. Fold increasesare shown above each lane. B, On the left, a Western blot forSAPK/JNK performed on lysates of untreated striatal cultures andthose treated with glutamate (100 µM) for 1 or 2 hr. On the right,an in-gel kinase assay on anti-SAPK/JNK immunoprecipitates fromstriatal cultures. The phosphorylation of c-Jun(1-135)-GST substrate,which had been incorporated into the polyacrylamide gel, was performedin the gel after separation of immunoprecipitate components. Whenparallel in-gel kinase assays were performed without c-Jun substratepolymerized into the gel, kinase activity was reduced >100-fold(data not shown). The positions of flanking molecular weight markersare indicated for A and B. C, Comparison of immune-complex kinaseassays for SAPK/JNK activity (top graph; using c-Jun(1-135)-GSTas substrate) and p38 activity (bottom graph; using myelin basicprotein as substrate) in immunoprecipitates of striatal cultures.In B (right) and C, treatments lasted 45 min with glutamate (Glu),dopamine (DA), and carbachol (Carb) at 100 µM; forskolin (Fors)at 10 µM; and mannitol (Mann) at 300 mM. The data in A and B weretypical of at least three experiments. The data in C were pooledfrom two experiments, with n = 6 (except for the forskolin group,in which n = 3); * greater than control, with p < 0.05; ** lessthan control (by 10%), with p < 0.05.
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SAPK/JNK activation is maximal (typically two- to threefold over basal levels) 45 min after initiation of treatment with glutamate(100 µM) or 15-45 min before the maximal glutamatergic inductionof phospho-c-jun levels (Figs. 5B, 6A). The kinase activationis prolonged, returning to baseline over 6 hr. To address thequestion of whether kinase activation becomes desensitized underthese conditions, the medium was repleted with additional glutamate(100 µM) 45 min before the end of a 6 hr incubation. This secondaddition led to a modest induction of SAPK/JNK activity, closerto the basal than the maximally activated level (Fig. 6A, lastlane). This result suggests that even if the decrease in SAPK/JNKactivity over 6 hr is partly attributable to loss of glutamatefrom the medium, there also appears to be desensitization of theglutamatergic activation of SAPK/JNK.

Among the major neurotransmitters known to act on striatal neurons, only glutamate activated SAPK/JNK. Neither dopamine norcarbachol, an agonist at muscarinic acetylcholine receptors, increasedSAPK/JNK activity (Fig. 6C). In fact, dopamine as well as forskolinslightly but consistently decreased activity in primary striatalcultures to levels below basal (Fig. 6B,C) (data not shown), asthey had for levels of AP-1-mediated transcription (Fig. 1A).To assess the possibility that a neurotransmitter other than dopamineor acetylcholine might be released from cells in the culturesin response to glutamate and then, in turn, activates SAPK/JNK,we also measured the effect of glutamate in cultures treated withtetrodotoxin, at a concentration (1 µM) that prevents action potentialpropagation. Tetrodotoxin had no effect on the glutamatergic activationof SAPK/JNK (data not shown), suggesting that glutamate acts directlyon the cells in which the kinase is activated, rather than byrelying on the release of an intermediary neurotransmitter.

Another proline-directed MAPK family member, p38, is closely related to SAPK/JNK and has been shown to be activated by thesame cellular stresses, proinflammatory cytokines, and intracellularsignaling cascades that activate SAPK/JNK (Freshney et al., 1994;Han et al., 1994; Rouse et al., 1994; Lin et al., 1995; Mindenet al., 1995). Indeed, in primary cultures of striatal neurons,both p38 and SAPK/JNK activities increase three- to fourfold afterexposure to hyperosmolar conditions with 300 mM mannitol (Fig.6C), which also raised phosphorylated c-Jun levels (Fig. 5A).p38 Activity was measured by in vitro phosphorylation of a myelinbasic protein substrate by anti-p38 immunoprecipitates from treatedcells. Surprisingly, p38 activity was not increased by glutamatein striatal neurons, even when measured in the same lysates thatcontained elevated SAPK/JNK activity.

Glutamate activates SAPK/JNK with a high-potency (EC₅₀ ~ 20 µM) (Fig. 7A) (data not shown) and a pharmacological profile typicalof the NMDA subtype of ionotropic glutamate receptors (Fig. 7B).Although NMDA and the non-NMDA ionotropic glutamate receptor agonistkainate both strongly induce SAPK/JNK activity in the cultures,NMDA antagonists are much more effective than a non-NMDA antagonistin blocking activation by glutamate, the presumed neurotransmitter.Specifically, the noncompetitive NMDA receptor blocker MK-801and the competitive blocker APV almost completely block the glutamate-(and NMDA-) induced activation of SAPK/JNK. DNQX, a competitivenon-NMDA ionotropic glutamate receptor antagonist, has no effecton the NMDA-induced activation and only slightly (but reproducibly)reduced the glutamate-induced activation. Stimulation of SAPK/JNKactivity by kainate, however, is minimally attenuated by the NMDAantagonists and is completely blocked by DNQX. The metabotropicglutamate receptor agonist tACPD has no effect on SAPK/JNK activity.
Fig. 7. Pharmacology of glutamatergic activation of SAPK/JNK and comparison of neuronal and glial cultures. A, Concentration-responsecurve for glutamatergic activation of SAPK/JNK in striatal culturesusing immune-complex kinase assay. Striatal cultures were treatedfor 45 min at the concentrations indicated. B, Effects of glutamateagonists and antagonists on SAPK/JNK activity in striatal cultures.Immune-complex kinase assays were performed on cultures treatedwith glutamate (20 µM), NMDA (500 µM), kainate (50 µM), or tACPD(500 µM). The antagonists MK-801 (1 µM), APV (100 µM), and DNQX(100 µM) were added as indicated 10 min before the 45 min incubationwith agonist. Data in A and B were typical of multiple experiments.NMDA, N-methyl-D-aspartate; tACPD, trans-(1S,3R) $-$ 1-aminocyclopentane-1.3-dicarboxylate;APV, 2-amino-5-phosphonovalerate; DNQX, 6,7-dinitroquinoxaline-2,3-dione.C, The effects of glutamate (100 µM) and mannitol (300 mM) for45 min on SAPK/JNK activity measured by immune-complex kinaseassay in standard (predominantly neuronal) striatal cultures (left)and glial striatal cultures (right). E18 striatal cell suspensionswere seeded onto cell culture plates with or without a precoatingof polyethylenimine for neuronal or glial cultures, respectively.Glial cells were cultured for 9 d in the presence of fetal calfserum until near confluent. Standard neuronal cultures (normallyincubated in the presence of serum-containing medium for <1 dbefore it is replaced with defined medium) that were incubatedinstead in serum-containing medium still displayed a two- to threefoldinduction of SAPK/JNK activity with glutamate (data not shown).
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We considered the possibility that NMDA receptors might be expressed by some glia as well as by neurons under conditions ofculture. Although our cultures are highly neuron-enriched, containing~95% neurons based on staining with neuron-specific enolase andGFAP antisera (Konradi et al., 1996), we investigated the possibilitythat glia might contribute to the SAPK/JNK activation by comparingour standard cultures with pure cultures of striatal glia. Theseglial cultures are grown from the same striatal cell suspensionsused to generate the predominantly neuronal glutamate-responsivecultures. Although SAPK/JNK activity was robustly induced in bothneuron-enriched and glial cultures by mannitol (Fig. 7C), onlythe neuronal cultures responded to glutamate.

DISCUSSION
We provide evidence that in primary cultures of striatal neurons, glutamate increases SAPK/JNK activity, phospho-c-Jun levels,and transcription of both a transfected AP-1-driven reporter constructand an endogenous AP-1 (junTRE)-driven immediate early gene, c-jun.Moreover, the sequential time courses of these events and theirspecificity for glutamate over dopamine or forskolin support arole for the SAPK/JNK pathway in the glutamatergic activationof AP-1-regulated genes. We propose that SAPK/JNK activation andthe associated rise in phosphorylated c-Jun levels may mediatethe glutamatergic induction of AP-1-mediated transcription inthese neurons and, in addition, that glutamatergic stimulationmay convert AP-1 binding induced by other neurotransmitters intoa transcriptionally active form.

Glutamatergic activation of SAPK/JNK
SAPK/JNK, a critical mediator of responses to a variety of cellular stressors and inflammatory cytokines (Kyriakis and Avruch,1996), was first cloned from fetal brain (Dérijard et al., 1994),and at least one isoform appears to be expressed exclusively inthe CNS (Mohit et al., 1995). However, SAPK/JNK regulation hasnot been described previously in the nervous system. Here, wedemonstrate that glutamate, a major excitatory amino acid neurotransmitter,activates SAPK/JNK and several of its transcriptional targetsin neuron-enriched cultures from E18 striatum.

The pharmacological profile of the glutamatergic activation of SAPK/JNK demonstrates prominent involvement of an NMDA receptor.However, this action of glutamate is also mimicked by a non-NMDAionotropic receptor agonist and is partially blocked by a non-NMDAreceptor antagonist, suggesting the involvement of a non-NMDAreceptor component as well. Non-NMDA receptor activation can leadto membrane depolarization that may relieve the voltage-dependentMg²⁺ block of NMDA receptors and, in doing so, may enhance NMDA receptoractivation attributable to low levels of ambient glutamate inthe culture medium. Alternatively, there may be a component ofNMDA receptor-independent glutamate activation of this pathway.In addition, a single hybrid receptor comprising NMDA and non-NMDAreceptor subunits (Henley et al., 1992) could account for theobserved pharmacology (Marin et al., 1993).

The neurotransmitter activation of SAPK/JNK in striatal neurons appears specific for glutamate, with neither dopamine nora muscarinic agonist displaying any stimulatory effect. Indeed,SAPK/JNK regulation provides an opportunity for an antagonisticinteraction between dopamine and glutamate, because dopamine slightlyreduces basal SAPK/JNK activity. Activation of the cAMP pathwaymay mediate this dopaminergic inhibition, because forskolin alsodecreases basal SAPK/JNK activity in striatal cultures and hasbeen shown to inhibit stimulated SAPK/JNK activity in T lymphocytes(Hsueh and Lai, 1995). However, depending on the sequence of events,the possible interactions are complex.

The selectivity of the glutamate stimulation for SAPK/JNK versus p38 in the striatal cultures differs from the parallel activationof these kinases by cell stress or cytokines. The basis for thepreviously reported coordinate regulation of SAPK/JNK and p38may involve upstream kinases that utilize p38 as well as SAPK/JNKas their substrates. Indeed, the best-characterized SAPK/JNK kinase(known as SEK1) phosphorylates p38 as well (Lin et al., 1995).However, Moriguchi et al. (1995) presented biochemical evidencethat SEK1 may make up only a minor component of the total SAPK/JNKkinase activity induced by cellular stress. Moreover, they identifiedseveral distinct kinase activities that show substrate specificityfor SAPK/JNK over p38. Thus, glutamate may activate a unique SAPK/JNKkinase, which, in contrast to SEK1, is selective for SAPK/JNKversus p38.

The known neurotoxic effects of glutamate and NMDA raise the possibility that the SAPK/JNK activation is secondary to membranedamage or metabolic insult. For example, glutamate and NMDA inducemarked swelling of striatal neurons (Colwell et al., 1996), andmembrane stretching has in fact been shown to activate SAPK/JNKin cardiac myocytes (Komuro et al., 1996). However, glutamateat a concentration of 100 µM, which maximally activates SAPK/JNK(Fig. 7A), does not produce signs of cellular toxicity or deathin our striatal cultures (M. Schwarzschild and S. Hyman, unpublishedobservations). Others have also reported minimal or no toxicityof glutamate in similar short-term cultures of striatal neurons(Galarraga et al., 1990). In addition, the selectivity for glutamateat this concentration for SAPK/JNK over p38 argues further fora more discrete mechanism of SAPK/JNK activation by glutamate.Whether this regulation is mediated by cation influx, traditionallyassociated with NMDA receptor signaling, or by more recently identifieddirect coupling of NMDA receptors to potential signaling proteins(Niethammer et al., 1996) remains to be explored.

Regulation of AP-1 proteins and their DNA binding activity
Glutamate and dopamine differentially regulate c-fos and c-jun mRNA in rat striatal neurons in culture. Although both neurotransmittersinduce c-fos mRNA, only glutamate induces c-jun mRNA. This islikely attributable to differences in the cis-regulatory elementslocated in the promoter regions of these genes. The c-fos promotercontains an SRE that can mediate glutamatergic induction of c-fosmRNA (Xia et al., 1996). It also contains several CREs, whichlikely mediate the effects of dopamine and forskolin (Konradiet al., 1994) and may, in addition, contribute to the calcium-dependenteffects of glutamate (Sheng et al., 1990; Xing et al., 1996).

In contrast, c-jun expression appears to be regulated through TREs rather than through a CRE or SRE. The c-jun promoter elementsjun1TRE and jun2TRE share homology with the consensus AP-1 element,bind AP-1 proteins (Angel et al., 1988; Stein et al., 1992; Rozekand Pfeifer, 1993), and are differentially involved in the inductionof c-jun by phorbol esters, E1A protein, and UV irradiation (Angelet al., 1988; Devary et al., 1991; Stein et al., 1992; van Damet al., 1993). Although the proteins binding to jun1TRE have notbeen characterized fully, the jun2TRE has been shown to preferentiallybind a heterodimer composed of c-Jun and ATF-2 proteins (Morookaet al., 1995; van Dam, 1995). Because c-Jun and ATF-2 both canbe phosphorylated and activated by SAPK/JNK (Hibi et al., 1993;Dérijard et al., 1994; Gupta et al., 1995), the glutamate-specificinduction of c-jun mRNA in our cultures may be mediated by theactivation of SAPK/JNK.

Differential regulation of AP-1-mediated transcription
In contrast to glutamate, dopamine and forskolin do not stimulate AP-1-mediated transcription, despite their ability to induceAP-1 binding. These results indicate that in striatal neurons,an induction of AP-1 binding does not necessarily produce transcriptionalactivation. A simple interpretation of this dissociation mightsuggest that the AP-1 binding complexes induced by dopamine orforskolin stimulation are transcriptionally inactive. Increasedtranscription through the AP-1 site may require the phosphorylationof AP-1 complex components, one example of which is provided byglutamate activation of SAPK/JNK and phosphorylation of c-Jun.Alternatively, because supershift analysis suggests that c-Junis not a major component of the AP-1 complex induced by forskolin,acute activation of cAMP pathways may promote pairing of c-Foswith inhibitory partners. For example, dopaminergic stimulationof these cultures has been shown to induce junB mRNA (Konradiet al., 1996), which is not activated by SAPK/JNK (Karin, 1995;Kallunki et al., 1996). Indeed, our data suggest that forskolinpreferentially induces JunB rather than c-Jun in AP-1 complexes,whereas glutamate may induce c-Jun to a greater extent than JunBin these complexes.

Other inhibitory effects of cAMP in striatal cell culture may contribute to their lack of efficacy for stimulating AP-1-mediatedtranscription. Inhibition could occur upstream of AP-1 proteinphosphorylation at the level of SAPK/JNK, where we and othershave identified an inhibitory effect of cAMP signaling (as describedabove). Conversely, cAMP-mediated inhibition of AP-1 transcriptionmay occur downstream of c-Jun phosphorylation at the level ofCREB binding protein, which mediates transcriptional activationthrough AP-1 as well as through CRE sites (Kamei et al., 1996).

The inability of dopamine or forskolin alone to induce AP-1-mediated transcription was observed in primary striatal cultures,which are necessarily devoid of the dopaminergic and glutamatergicafferents that exist in the intact striatum. However, indirectdopamine agonists such as cocaine and amphetamine and dopaminereceptor antagonists such as haloperidol may act in vivo to modulateglutamate-induced AP-1 transcription. Interactions between dopamineand glutamate are suggested by the close anatomic arrangementof corticostriatal and nigrostriatal nerve terminals synapsingon the dendritic spines of striatal neurons (Freund et al., 1984;Smith and Bolam, 1990). In addition, pharmacological evidenceimplicates glutamate receptors in cocaine- and amphetamine-inducedgene expression in the striatum (Snyder-Keller, 1991; Ohno etal., 1994; Wang et al., 1994; Konradi et al., 1996). Thus, ourfindings in culture raise additional questions about the in vivointeractions of excitatory amino acids with endogenous and exogenousdopaminergic signals. For example, dopaminergic psychostimulantand antipsychotic drugs might raise the levels of AP-1 transcriptionfactors in the intact striatum in a manner that primes or amplifiesa subsequent glutamatergic induction of AP-1 transcriptional effects.

Our findings also raise the possibility that SAPK/JNK, as well as its AP-1 targets, plays a role in physiological and pathologicaleffects of glutamate. Recently, SAPK/JNK activation has been shownunder certain circumstances to be essential for apoptotic celldeath (Xia et al., 1995; Verheij et al., 1996). For example, ina cell line bearing similarities to sympathetic neurons, SAPK/JNK-dependentapoptosis is induced by withdrawing neurotrophic factor support(Xia et al., 1995). These results, together with our own, leadto the hypothesis that SAPK/JNK may mediate the glutamate-inducedcell death implicated in both normal neural development and neurodegenerativedisease. Interestingly, riluzole, an antagonist of postsynapticglutamate function used clinically to slow progression of amyotrophiclateral sclerosis (Bensimon et al., 1994), completely blocks theglutamatergic induction of SAPK/JNK and phospho-c-jun in our system(M. Schwarzschild and S. Hyman, unpublished results). Becausecytoskeletal proteins, in addition to transcription factors, canalso serve as substrates for this kinase (Kyriakis and Avruch,1990), the NMDA-dependent glutamatergic activation of SAPK/JNKobserved here in embryonic striatal neuron cultures may also berelevant to NMDA-dependent changes in neuronal connectivity observedduring development (Scheetz and Constantine-Paton, 1994). Finally,more acute NMDA-dependent neuronal damage, such as that seen inischemic stroke, may also involve SAPK/JNK, because renal andcardiac ischemia/reperfusion has been shown to activate SAPK/JNK(Pombo et al., 1994; Knight and Buxton, 1996).

FOOTNOTES

Received Sept. 30, 1996; revised Feb. 26, 1997; accepted Feb. 28, 1997.
^a   M.A.S. and R.L.C. contributed equally to this manuscript.

This work was supported by Public Health Service Grants DA07134, DA00257, and NS01729. We thank John Kyriakis for anti-SAPK $beta$ antibody, c-jun(1-135)-GST construct, and helpful suggestions;Angel Nebreda for anti-XMpk2 antibody; Steve Fink for the AP-1-luciferaseconstruct; and Zhengui Xia and Michael Greenberg for discussionof transfection methods. We also thank Melissa Meyers and AllisonWong for technical assistance and Bruce Hope, Linda Kobierski,Christine Konradi, and Susan Lewis for valuable discussions.

Correspondence should be addressed to Dr. Steven E. Hyman at his current address: National Institute of Mental Health, Room17-99, Parklawn Building, 5600 Fishers Lane, Rockville, MD 20857.

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