Extracellular Signal-Regulated Kinase (ERK) Controls Immediate Early Gene Induction on Corticostriatal Stimulation

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The Journal of Neuroscience, November 1, 1998, 18(21):8814-8825

Extracellular Signal-Regulated Kinase (ERK) Controls Immediate Early Gene Induction on Corticostriatal Stimulation
Véronique Sgambato, Christiane Pagès, Monique Rogard, Marie-Jo Besson, and Jocelyne Caboche
Laboratoire Neurochimie-Anatomie, Institut des Neurosciences, Unité Mixte de Recherche 7624, Université Pierre et Marie Curie, 75005 Paris, France

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Activity-dependent changes in neuronal structure and synaptic remodeling depend critically on gene regulation. In an attemptto understand how glutamate receptor stimulation at the membraneleads to gene regulation in the nucleus, we traced intracellularsignaling pathways targeting DNA regulatory elements of immediateearly genes (IEGs). For this purpose we used an in vivo electricalstimulation of the glutamatergic corticostriatal pathway. We showthat a transient activation of extracellular signal-regulatedkinase (ERK) proteins (detected by immunocytochemistry with ananti-active antibody) is spatially coincident with the onset ofIEG induction [c-fos, zif 268, and map kinase phosphatase-1 (MKP-1)detected by in situ hybridization] in the striatum, bilaterally.Both Elk-1 and CREB transcription factors (targeting SRE and CREDNA regulatory elements, respectively) were hyperphosphorylatedin register with ERK activation and IEG mRNA induction. However,their hyperphosphorylation occurred in different subcellular compartments:the cytoplasm and the nucleus for Elk-1 and the nucleus for CREB.The role of the ERK signaling cascade in gene regulation was confirmedafter intrastriatal and unilateral injection of the specific ERKinhibitor PD 98059, which completely abolished c-fos, zif 268,and MKP-1 mRNA induction in the injected side. Of interest, bothElk-1 and CREB hyperphosphorylation also was impaired after PD98059 injection. Thus two different ERK modules, one dependingon the cytoplasmic activation of Elk-1 and the other one dependingon the nuclear activation of CREB, control IEG transcriptionalregulation in our model. Our findings provide significant insightsinto intracellular mechanisms underlying synaptic plasticity inthe striatum.

Key words: motor cortex; striatum; c-fos; zif 268; transcription factors; Elk-1; CREB; phosphorylation; ERK; kinases; phosphatases

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

In the CNS, activity-dependent changes in gene expression can elicit long-term adaptive responses underlying synaptic plasticity(Sheng and Greenberg, 1990; Ginty et al., 1992; Ghosh and Greenberg,1995; Ginty, 1997). Glutamate, which is involved in long-termpotentiation (LTP), regulates the transcription of immediate earlygenes (IEGs) such as c-fos. Two DNA regulatory elements, at least,are crucial for this transcriptional regulation: the cAMP/calcium-responsiveelement (CRE) and the serum-responsive element (SRE) (Bading etal., 1993; Miranti et al., 1995; Xia et al., 1996; Johnson etal., 1997). The CRE site is controlled by the phosphorylationof the CRE binding protein (CREB) on residue Ser¹³³ by cAMP-dependent kinase (PKA) (Gonzalez and Montminy, 1989)and calcium/calmodulin-dependent protein kinases (CaMKs) (Dashet al., 1991; Sheng et al., 1991; Matthews et al., 1994; Sun etal., 1994).

Calcium signaling at the SRE DNA regulatory element is still an enigma. This site is required for serum-induced c-fos expression(Treisman, 1992) in the context of mitotic cell regulation. Togetherwith flanking DNA sequences, it serves as sites for the assemblyof multiprotein complexes that include a dimer of serum responsefactor (SRF) (Treisman, 1986; Norman et al., 1988; Schröter etal., 1990) and a ternary complex factor (TCF) (Shaw et al., 1989)(for review, see Treisman, 1992, 1995). Although SRF is phosphorylatedrapidly in response to mitogenic stimulation and phosphorylationaffects its DNA binding properties (Rivera et al., 1993), a majorregulatory input received by the SRE is attributed to TCF phosphorylation(Hill et al., 1993). Elk-1, the first TCF to be identified (Hipskindet al., 1991), is phosphorylated rapidly on Ser³⁸³ and Ser³⁸⁹ in its C-terminal region in response to the activation of extracellularsignal-regulated kinase (ERK) proteins (Marais et al., 1993; Hipskindet al., 1994a,b). This increases its ability to form a ternarycomplex with SRF and SRE (Gille et al., 1992, 1995) and to activatec-fos transcription (Hill et al., 1993; Marais et al., 1993; Zincket al., 1993; Hipskind et al., 1994a,b; Janknecht et al., 1994).

In postmitotic neurons, ERK proteins are expressed abundantly (Boulton and Cobb, 1991; Fiore et al., 1993a). They can be activatedin response to increases in intracellular calcium levels or glutamatereceptor stimulation (Bading and Greenberg, 1991; Fiore et al.,1993b; Rosen et al., 1994; Kurino et al., 1995), and this activationis critically required for LTP in rat hippocampus (English andSweat, 1996, 1997). However, whether ERK activation is requiredfor glutamate-induced gene regulation remains to be established.

We chose the in vivo stimulation of the corticostriatal pathway as a promising model for studying ERK implication in glutamate-inducedIEG regulation (Sgambato et al., 1998). Stimulation of glutamatergiccortical afferents (Reubi and Cuenod, 1979) can elicit LTP instriatal neurons in vivo (Charpier and Deniau, 1997). We showhere that a transient activation of ERK targeting both Elk-1 andCREB transcription factors in distinct subcellular compartmentsis critically involved in IEG [c-fos, zif 268, and map kinasephosphatase-1 (MKP-1)] mRNA induction.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Corticostriatal stimulations
After anesthesia with pentobarbital (6 mg/kg, i.p.; Sanofi, Paris, France), cortical electrical stimulations were appliedin animals placed in a conventional stereotaxic apparatus. Carewas taken to minimize uncontrolled sources of stimulation; theskin around the points of stereotaxic contention and areas ofincision were numbed with Xylocaine. Body temperature was monitoredthroughout the experiment and kept at 37-38°C with a homeothermicblanket. A small craniotomy was made over the orofacial area ofthe motor cortex according to previously described stereotaxiccoordinates (Paxinos and Watson, 1986). Orofacial cortical stimulationswere applied through pairs of wires (Ni-Chrome, 0.2 mm diameter)1.5 mm apart and inserted at a depth of 1.5 mm from the corticalsurface. Electrical stimuli consisted of trains of pulses of 200µA intensity and 50 msec duration delivered at frequencies of250 Hz, repeated at 4 Hz for a period varying from 15 to 60 min.The localization of the jaw area was identified precisely by observingthe motor effects evoked by these electrical pulses. The polarityof electrodes was reversed every 30 sec to avoid lesion of corticaltissue. Sham-stimulated rats were treated identically except thatno electrical stimulation was delivered. At the end of stimulation,brains were processed for either neuroanatomical (in vivo perfusionwith PFA 4%) or biochemical (rapid extraction of lateral or medialparts of the striatum) studies (see below).

Tissue preparation for in situ hybridization and immunocytochemistry
Rat brains were fixed by intracardiac perfusion of 4% paraformaldehyde (PFA) in 0.1 M Na₂HPO₄/NaH₂PO₄ buffer, pH 7.5 (phosphatebuffer), delivered with a peristaltic pump at 50 ml/min during10 min. Brains were removed and post-fixed in the same fixativesolution for 2 hr, washed overnight in 0.1 M phosphate buffercontaining 15% sucrose, and then frozen in isopentane (for 1 minat $-$ 25°C). Sections (20 µm) were cut on a microtome and then keptin a solution containing 30% ethylene glycol, 30% glycerol, 0.1M phosphate buffer, and 0.1% diethyl pyrocarbonate (DEPC; Sigma,Deisenhofen, Germany) at $-$ 20°C until they were processed for insitu hybridization or immunohistochemistry.

Probe synthesis for in situ hybridization
The antisense (complementary to cellular mRNA) probes used in this study were ³³P-radiolabeled riboprobes. For c-fos, a 487 bp cDNA subclone correspondingto exon 4 of human cDNA was linearized after HindIII digestionand transcribed with T7 RNA polymerase. For zif 268 riboprobe,a murine zif 268 cDNA subclone corresponding to 1.6 kb was linearizedafter HindIII digestion and transcribed with T7 RNA polymerase.MKP-1 riboprobe was transcribed from a murine MKP-1 cDNA subclonecorresponding to 663 bp with T7 RNA polymerase after linearizationwith PstI. Transcription reactions contained 1 µM [ $alpha$ ³³P]-UTP (3000 Ci/mmol; Isotopchim), 250 µM ATP, CTP, and GTP, andunlabeled UTP (10.5 µM); the reactions were incubated at 39°Cfor 2 hr. After DNase I digestion, the labeled RNA was purifiedby phenol/chloroform/isoamyl alcohol (25:24:1) extraction andethanol precipitation. Gel electrophoresis showed the transcriptsto be predominantly full length.

In situ hybridization
Free-floating sections were mounted on SuperFrost/plus slides (Menzel-Gläser) in RNase-free conditions. Once dried, the mountedsections were rinsed in PBS and treated for 10 min with 0.1 Mglycine in 0.1 M Tris-HCl, pH 7.4. The sections were rinsed for5 min at 37°C in 0.1 M Tris-HCl, pH 8, and 50 mM EDTA, and weretreated for 15 min at 37°C with 1 mg/ml proteinase K in the samebuffer. Before hybridization the sections were subjected to thefollowing treatments: post-fixation for 15 min in 4% PFA, 5 mMMgCl₂ in PBS at room temperature, acetylation for 20 min in aceticanhydride/triethanolamine, pH 8, at room temperature, and stepwisedehydration in alcohol. The following hybridization solution wasapplied on sections, which then were covered with GelBond film(FMC Bioproducts, Rockland, ME). The hybridization mixture contained200 ng/ml (4 ng/section) of ³³P-RNA probe in 20 mM Tris-HCl, pH 8, 300 mM NaCl, 5 mM EDTA, 10%dextran sulfate, 1× Denhardt's solution (0.02% Ficoll, 0.02% polyvinylpyrrolidone, and 10 mg/ml BSA), 0.5 mg/ml Escherichia coli tRNA,0.1 M dithiothreitol (DTT), and 50% formamide. Hybridization wasperformed at 60°C in humid chambers for 16 hr. After the GelBondcoverslips were removed in 4× SSC (1× SSC is 0.15 M NaCl/0.015M Na citrate) and 10 mM DTT, the slides were washed in the samesolution for 1 hr at room temperature and then in 50% formamide,10 mM Tris-HCl, pH 8, 75 mM NaCl, and 2.5 mM EDTA. Sections weretreated with RNase A (20 µg/ml; Sigma) in 400 mM NaCl, 10 mM Tris-HCl,pH 7.5, and 50 mM EDTA for 1 hr at 37°C and then were rinsed for15 min at 60°C in 2× SSC, followed by 0.1× SSC. After dehydration,the sections were air-dried and exposed with Biomax-MR films (Kodak,Rochester, NY) for 3 d (for zif 268) or 6 d (for c-fos and MKP-1probes).

Immunocytochemistry
The immunohistochemical procedure was adapted from protocols previously described except that, for the detection of phosphorylatedproteins, 0.1 mM NaF was included in all buffers and incubationsolutions.
Day 1. Free-floating sections were rinsed in Tris-buffered saline (TBS; 0.25 M Tris and 0.5 M NaCl, pH 7.5), incubated for5 min in TBS containing 3% H₂O₂ and 10% methanol, and then rinsedthree times for 10 min each in TBS. After a 15 min incubationin 0.2% Triton X-100 in TBS, the sections were rinsed three timesin TBS. These were incubated with the primary antibody (see below)for 72 hr at 4°C.
Day 2. After three rinses in TBS, the sections were incubated for 48 hr at 4°C with the secondary biotinylated antibody (anti-IgG),using a dilution twice that of the first antibody in TBS.
Day 3. After being washed (three times in TBS), the sections were incubated overnight in avidin-biotin-peroxidase complex(ABC) solution (final dilution, 1:50; Vector Laboratories, Peterborough,UK).
Day 4. The sections were washed two times in TBS and two times in TB (0.25 M Tris, pH 7.5) for 10 min each, placed in a solutionof TB containing 0.1% 3,3'-diaminobenzidine (DAB; 50 mg/100 ml),and developed by H₂O₂ addition (0.02%). After processing, thetissue sections were mounted onto gelatin-coated slides and dehydratedthrough alcohol to xylene for light microscopic examination.

Tissue preparation for Western blot analysis
Day 1. Tissue samples were extracted rapidly from the brain and lysed in solubilization buffer [containing (in mM) 10 Tris-Cl,50 NaCl, 30 sodium pyrophosphate, 50 NaF, 1 DTT, and 0.5 benzamidineplus 1% Triton X-100, 5 µM ZnCl₂, 100 µM Na₃VO₄, 5 nM okadaicacid, 2.5 µg each of aprotinin, pepstatin, and leupeptin, and0.5 µM PMSF]. Insoluble material was removed by centrifugation(13,000 rpm for 20 min at 4°C). Cell lysates (30, 20, or 10 µgper lane for the detection of P-Elk-1, P-CREB, and P-ERK, respectively)were separated by 10% SDS-PAGE before electrophoretic transferonto polyvinylidene difluoride membrane (PVDF; ICN Biochemicals,Paris, France). The blots were saturated (for 1 hr at room temperature)with BSA (Fraction V, Sigma) 8% (for P-Elk-1) or 5% (for P-ERKand P-CREB) and incubated (overnight at 4°C) with the anti-activeantibodies (see below).
Day 2. Subsequently, the blots were incubated for 2 hr at room temperature with goat anti-rabbit horseradish peroxydase-conjugatedantibodies before exposure to the ECL substrate. Then the blotswere stripped (glycine-HCl, pH 2.8, two times for 20 min at 55°C)and saturated overnight in 5% nonfat dry milk.
Day 3. Then the blots were incubated with the nonactive antibodies (see below). The efficacy of the stripping step was assessedby omitting the first antibody and verifying the lack of signalson the blot.

Antibodies
The anti-active antibodies used in this study were polyclonal antibodies raised against the dually phosphorylated Thr/Glu/Tyrregion within the catalytic core of the active form of p44/ERK1and p42/ERK2 [and corresponding to Thr¹⁸³-Tyr¹⁸⁵ in p42/ERK2 (Promega, Paris, France)], a phospho-Ser¹³³ peptide corresponding to residues 129-137 of human CREB (NewEngland Biolabs, Beverly, MA), and a phospho-Ser³⁸³ peptide corresponding to residues 379-392 of human Elk-1 (NewEngland Biolabs). The dilutions used for immunostaining were 1:100for P-ERK and P-CREB antisera and 1:80 for P-Elk-1 antiserum.For Western blot analysis the dilutions were 1:2500 for P-ERKantiserum, 1:500 for P-CREB antiserum, and 1:100 for P-Elk-1 antiserum.
The nonactive antibody used for immunostaining (dilution 1:250) was a rabbit anti-ERK antibody raised against a peptide correspondingto the 345-358 region within the C terminus of the rat ERK2 (SantaCruz Biotechnology). For Western blot analysis the nonactive antibodiesused were anti-ERK antibody (1:4000; Santa Cruz Biotechnology),anti-Elk-1 antibody (1:1000; rabbit polyclonal antibody raisedagainst a recombinant protein corresponding to the C-terminalregion of human Elk-1), and anti-CREB antibody raised againsta peptide corresponding to residues 123-137 of human CREB (1:1000;New England Biolabs).

Data analysis
Tissue sections of stimulated rats (15, 30, 45, and 60 min), which were processed for immunocytochemistry by using the anti-activeantibodies, were examined under light microscope. P-ERK-, P-Elk-1-,and P-CREB-positive neurons were plotted at 25× magnificationwith a computerized image analyzer (Biocom, Paris, France). Cellcounts were performed for each rat in the ipsilateral striatumto the cortical stimulation in a total surface area of 2.7 mm².

Striatal injection of PD 98059
PD 98059 was dissolved in dimethyl sulfoxide (Me₂SO) to obtain a 10 mM stock solution. Then it was diluted 1:100 in 0.9% NaCl(final concentration, 100 µM). The compound was stereotaxicallydelivered (6 µl), unilaterally, in the lateral part of the striatum[bregma: anterior 9 mm, lateral 3.5 mm, and depth 5.5 mm, accordingto Paxinos and Watson (1986)] by pressure injection through aHamilton syringe fit with a glass micropipette (internal tip diameter,50 µm). The injection was made over a total period of 55 min (45min before stimulation, followed by 10 min during stimulation),and the needle was left in place for 5 min before withdrawal.Then the animals were perfused with 4% PFA as described below.Sham-injected rats were treated identically except that the glassmicropipette contained only the vehicle diluted in 0.9% NaCl.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Kinetics of ERK activation and IEG transcriptional regulation on corticostriatal pathway stimulation

The activation of ERK proteins, detected with an antiserum specifically recognizing their phosphorylated form (anti-phospho-Thr¹⁸³ and -Tyr¹⁸⁵), was not observed in the striatum of sham-stimulated rats (Fig.1A). Similarly, although there was a clear activation in the implantedcerebral cortex, neither c-fos nor zif 268 mRNAs, detected byin situ hybridization, were upregulated in the striatum of theserats (Fig. 1D,G). A short-term electrical stimulation (15 min)applied unilaterally in the motor cortex induced intense P-ERKimmunostaining (Fig. 1B) precisely in the projection area of stimulatedcortical neurons: the lateral striatum (Sgambato et al., 1997).The bilaterality of the corticostriatal afferents (McGeorge andFaull, 1987) was reflected by a bilateral induction of P-ERK immunoreactivityin the lateral striatum. The upregulation of c-fos and zif 268mRNAs, detected on adjacent brain sections, was spatiotemporallycoincident with P-ERK induction at this time point (compare Fig.1B with E and H). Remarkably, after long-term stimulation (60min) P-ERK immunoreactivity clearly was reduced bilaterally inthe lateral striatum (Fig. 1C). This reduction contrasted withthe sustained induction of both messengers in these striatal areas(Fig. 1F,I).

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Figure 1. ERK activation occurs in a tight spatial register with c-fos and zif 268 mRNA induction after unilateral stimulation of the corticostriatal pathway. Brain sections were processed for P-ERK immunoreactivity (A-C) and in situ hybridization of c-fos (D-F) and zif 268 (G-I) mRNAs. Sham-stimulated rats (sham; A, D, G) were electrode-implanted in the right cerebral cortex (arrow in A). Although P-ERK immunostaining (A) is not detectable, c-fos (D) and zif 268 (G) mRNAs are induced slightly in the implanted cortex, with no apparent upregulated signal in the striatum of sham-stimulated rats. Stimulated rats were electrode-implanted in the right cerebral cortex and received electrical cortical stimulation (double arrows in B, C) for either 15 min (15' stim; B, E, H) or 60 min (60' stim; C, F, I). At 15 min of stimulation a strong activation of P-ERK (B) occurred bilaterally in the lateral striatum (lSt), but not in the medial striatum (mSt). Note that this activation occurs in a spatial register with both c-fos (E) and zif 268 (H) mRNA induction. At 60 min of cortical stimulation, although ERK activation (C) decreased in the lateral striatum, c-fos (F) and zif 268 (I) mRNAs remained strongly induced bilaterally.

To determine the kinetics of ERK activation, we measured P-ERK immunoreactivity after 15, 30, 45, and 60 min of stimulation(Fig. 2A). In the medial striatum, corresponding to the nonactivatedarea, P-ERK immunostaining did not vary regardless of the stimulationduration that was used. In the lateral striatum, the activatedprojection area, the immunoreactive signal was significantly higherthan in the medial striatum after 15, 30, and 45 min of stimulation.However P-ERK induction was transient. The maximal signal wasfound at 15 min; it then slowly declined from 30 to 45 min andreturned to basal levels at 60 min. Contrasting with the transientP-ERK induction, c-fos and zif 268 mRNA levels increased progressivelybetween 15 and 30 min, reached maximal levels at 30 min, and thenremained stable (Fig. 2B,C). In the medial part of the striatum,regardless of the stimulation duration that was used, no hybridizationsignals were detectable for c-fos mRNA, and the constitutive levelsof zif 268 mRNA did not vary (Fig. 2B,C).

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Figure 2. Kinetics of ERK activation and c-fos and zif 268 transcriptional regulation on corticostriatal stimulation. Statistical comparisons were performed from three independent animals for each time point, using an image analyzer (IMSTAR, Paris, France). A, Densitometric measurements of P-ERK immunostaining. Signals were significantly higher in the lateral striatum (lSt) than in the medial striatum (mSt) after 15, 30, and 45 min of stimulation (*p < 0.05, paired Student's t test), but not at 60 min. P-ERK immunoreactivity was maximal at 15 min and then progressively decreased to return to basal levels. B, C, Autoradiographic signals from c-fos (B) and zif 268 (C) mRNA detection. Both mRNA levels were significantly higher in the lSt than in the mSt, regardless of the stimulation period used (**p < 0.01, paired Student's t test). Moreover, messenger levels were significantly higher at 30 than at 15 min of stimulation ( p < 0.05, unpaired Student's t test) and then remained high. Note that the transient activation of ERK correlated with a sustained transcriptional regulation of both messengers.

The progressive dephosphorylation of ERK proteins observed in the activated lateral striatum suggested a possible negativefeedback regulation arising from a specific phosphatase. MKP-1is described in vitro on cell line models as an IEG for whichthe rapid transcription by mitogens and subsequent translationare suggestive of a feedback loop mechanism providing a rapidinactivation of ERK (Charles et al., 1993; Sun et al., 1993).We thus tested whether MKP-1 mRNA could be upregulated in vivoin our model. In sham-stimulated rats, although MKP-1 mRNAs wereinduced in the implanted cortex, no signal was detectable in bothstriata (Fig. 3A). At 15 min of stimulation, MKP-1 mRNAs wereinduced bilaterally and specifically in the lateral striatum,matching the spatial ordering of ERK activation (compare Figs.3B and 1B). By increasing the stimulation from 15 to 60 min, MKP-1mRNA induction was enhanced further in the lateral striatum, whereaslevels of this mRNA remained low in the medial part of the striatum(Fig. 3D). At 60 min, a strong MKP-1 mRNA induction occurred ina tight spatial register with the slight ERK activation (compareFigs. 3C and 1C). Thus, corticostriatal pathway stimulation leadsto a rapid and sustained induction of MKP-1 mRNA, which is likelyto account for a negative feedback loop underlying ERK dephosphorylationafter 45 and 60 min of stimulation.

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Figure 3. MKP-1 mRNA induction on corticostriatal stimulation. Brain sections of sham-stimulated and stimulated rats were processed for in situ hybridization of MKP-1 mRNAs (A-C). In sham-stimulated rats (A) MKP-1 mRNA levels were detected in the implanted cortex, with no apparent signal in the striatum. By contrast, at 15 min of stimulation (B), although no signals were detected in the medial striatum, MKP-1 mRNA was strongly induced bilaterally in the lateral striatum. This induction persisted at 60 min of stimulation (C). Note that MKP-1 induction spatiotemporally correlated with the ERK activation and IEG induction shown in Figure 1. B, Statistical comparisons were performed from three independent animals with an image analyzer (IMSTAR) after densitometric measurements of mRNA signals on autoradiograms. MKP-1 mRNA levels were significantly higher in the lateral striatum (lSt) than in the medial striatum (mSt), regardless of the stimulation period used (**p < 0.01, paired Student's t test).

Coincident activation of ERK, Elk-1, and CREB on corticostriatal stimulation

On cell lines after serum activation, ERK phosphorylation leads to SRE-driven gene regulation via the hyperphosphorylationof Elk-1 (Hill et al., 1993; Marais et al., 1993; Zinck et al.,1993; Hipskind et al., 1994a,b; Janknecht et al., 1994). Recentevidence also indicates that, in neurotrophin-activated PC12 cellsor primary cortical neurons, CREB is targeted by ribosomal proteinS6 kinase (RSK) (Xing et al., 1996; Finkbeiner et al., 1997),a substrate of ERK proteins (Strugill et al., 1988) (for review,see Seger and Krebs, 1995). We thus searched to trace whetherERK activation, observed at 15 min, was associated with Elk-1and/or CREB hyperphosphorylation. For this purpose we used anti-activeElk-1 (anti-phospho-Ser³⁸³) and CREB (anti-phospho-Ser¹³³) antibodies, together with the anti-active ERK antibody. Immunocytochemicaldetection of these antibodies was analyzed on sections adjacentto those used for P-ERK and IEG mRNA detection in sham and 15-min-stimulatedrats. In sham animals, although P-ERK immunoreactivity was undetectablein the whole striatum (Fig. 4A,B), low constitutive labeling wasdetectable in the nuclei for P-Elk-1 (Fig. 4E,F) and P-CREB (Fig.4I,J). In the medial striatum of stimulated rats, P-ERK (Fig.4C), P-Elk-1 (Fig. 4G), and P-CREB (Fig. 4K) showed the same patternof immunoreactivity as in sham animals. Thus, phosphorylationevents were not influenced by the surgery and electrode manipulation.

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Figure 4. Hyperphosphorylation of ERK, Elk-1, and CREB after 15 min of corticostriatal stimulation. Adjacent brain sections of sham (left panels) or 15-min-stimulated (15' stim; right panels) rats were processed in parallel for P-ERK (A-D), P-Elk-1 (E-H), and P-CREB (I-L) immunohistochemistry. In the medial striatum (mSt) and lateral striatum (lSt) of sham animals, although no constitutive expression of P-ERK was detectable (A, B), a slight constitutive nuclear expression was visible for P-Elk-1 (E, F) and P-CREB (I, J). In the mSt of 15'-stimulated rats, immunolabeling for P-ERK (C), P-Elk-1 (G), and P-CREB (K) was similar to that in sham. By contrast, a clear increase of P-ERK (D), P-Elk-1 (H), and P-CREB (L) was detectable in the lSt. The activation of ERK (D) occurred in both nuclear (arrowhead) and cytoplasmic (thin arrow) neuronal compartments. Similarly, Elk-1 hyperphosphorylation (H) occurred in the nucleus (arrowhead) as well as in cytoplasmic compartments (thin arrow). Finally, CREB activation (L) was restricted to the nucleus (arrowhead) of striatal cells. Data are representative of three independent rats for each group. Scale bar, 1 cm = 15 µm.

By contrast, in the lateral striatum of 15-min-stimulated rats, immunostaining for P-ERK (Fig. 4D), P-Elk-1 (Fig. 4H), andP-CREB (Fig. 4L) was increased markedly, in a tight correspondencewith IEG induction (data not shown). In this striatal part theP-ERK-positive neurons showed immunostaining in cytoplasmic compartments(including the dendrites; Fig. 4D, thin arrow) suggestive of alocal activation of the protein. Moreover, the appearance of strongnuclear staining (Fig. 4D, arrowhead) was in favor of a nucleartranslocation of activated ERK proteins. P-Elk-1 immunostainingwas increased markedly in nuclei (Fig. 4H, arrowhead) but alsoin cytoplasmic (soma and dendrites; Fig. 4H, thin arrow) compartmentsof activated striatal neurons. Thus, in postsynaptic striatalcells, Elk-1 hyperphosphorylation occurred not only in the nucleus,where it can activate the SRE-DNA regulatory element of IEG promoters,but also in the cytoplasm. By contrast, CREB hyperphosphorylationwas observed exclusively in cell nuclei (Fig. 4L, arrowhead),a result in full agreement with previous studies showing its strictlynuclear localization and regulation (Yamamoto et al., 1989).

To confirm biochemically the specificity of anti-active antibodies used in immunocytochemistry, we performed Western blotson extracts prepared from striata of stimulated rats (Fig. 5A-C).P-ERK antibody yielded two bands of 42 and 44 kDa, the expectedsizes for ERKs 1 and 2 (Fig. 5A). The P-ERK immunoreactivity clearlywas increased in extracts from the lateral striatum relative tothose from the medial striatum. This increase reflected ERK activation,because comparable levels of ERKs 1 and 2 were present in bothextracts (Fig. 5A). Similarly, the P-Elk-1 antibody, which yieldedone band of 62 kDa, the expected size for Elk-1, gave increasedsignals in extracts from the lateral striatum relative to thosefrom the medial striatum, whereas comparable levels of total Elk-1were present in both extracts (Fig. 5B). With P-CREB antibody,a 43 kDa band also was induced specifically in extracts from thelateral striatum when compared with those relative to the medialstriatum (Fig. 5C), whereas levels of nonphosphorylated CREB proteins(corresponding to 43 kDa molecular weight) were similar in bothextracts.

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Figure 5. Western blot analysis of P-ERK, P-Elk-1, and P-CREB immunoreactivity in medial and lateral parts of the striatum after 15 min of stimulation. Extracts of medial (mSt) and lateral (lSt) striatum were dissected rapidly and processed for Western blots. Detection of anti-active proteins was analyzed first, and then total proteins were visualized on the same blot after a stripping procedure. Note the increase of P-ERK (A), P-Elk-1 (B), and P-CREB (C) immunoreactivities in the lSt when compared with the mSt and the same level of total ERKs (A), Elk-1 (B), and CREB (C) proteins in both striatal regions. Molecular weights (in kDa) are indicated to the right of each blot.

Long-term stimulation leads to a dephosphorylation of ERK, Elk-1, and CREB

A comparative analysis of P-ERK-, P-Elk-1-, and P-CREB-positive cells was performed after various stimulation time points.We observed a significant decrease in the number of P-ERK-positiveneurons between 30 and 45 min and at 60 min (Fig. 6A). At thistime point only a few neuronal cells remained labeled for P-ERKin the lateral striatum (Fig. 6C). In these cells P-ERK was stilldetectable in cytoplasmic (Fig. 6C, thin arrow) and nuclear (Fig.6C, arrowhead) compartments. For P-Elk-1 and P-CREB, only cellspresenting hyperphosphorylation were counted in this area. Thisshowed a significant decrease between 15 and 30 min, which continuouslydeclined thereafter to reach very low values at 60 min (Fig. 6A).At this time point very few P-Elk-1 cells were detectable in thelateral striatum (Fig. 6E). These latter cells were large neuronswith a strong immunoreactive nucleus (Fig. 6E, arrowhead) andlong immunostained proximal dendrites (Fig. 6E, thin arrow). Similarly,P-CREB immunocytochemistry was decreased markedly in the lateralstriatum at 60 min of stimulation (Fig. 6G). Some scarce neuronsalso showed strong nuclear immunolabeling (Fig. 6G, arrowhead).Noteworthy, even the constitutive immunostaining of P-Elk-1 andP-CREB observed in the medial striatum (Fig. 6D,F) was no longerdetectable in the lateral striatum after 60 min of stimulation.

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Figure 6. Inactivation of ERK, Elk-1, and CREB after 60 min of corticostriatal stimulation. A, Quantification of P-ERK, P-Elk-1, and P-CREB immunoreactive striatal cells at 15, 30, 45, and 60 min of corticostriatal stimulation (n = 3 rats for each stimulation period). Cells counts were performed with an image analyzer (Biocom) in the lateral striatum ipsilaterally to the stimulation (total surface area examined, 2.7 mm²). Statistical comparisons were performed with a one-way ANOVA. **p < 0.01 when comparing P-ERK immunostaining between 45 and 30 min; °p < 0.05 when comparing P-Elk-1 and P-CREB immunostaining between 15 and 30 min; p < 0.05 when comparing P-CREB with P-ERK at 45 and 60 min; #p < 0.05 when comparing P-Elk-1 with P-ERK at 60 min. Adjacent brain sections of 60-min-stimulated rats were processed in parallel for P-ERK (B, C), P-Elk-1 (D, E), and P-CREB (F, G) immunohistochemistry. In the lateral striatum (lSt) few P-ERK immunoreactivecells were found (C) when compared with those in Figure 4D. These cells presented both nuclear (arrowhead) and cytoplasmic (thin arrow) staining. E, Very few large neurons remained immunolabeled for P-Elk-1 in the lSt when compared with those in Figure 4H. Here again, the labeling was detectable in the nucleus (arrowhead) as well as in the cytoplasmic compartments (thin arrow). Similarly, CREB hyperphosphorylation (G) occurred in the nucleus of very few cells (arrowhead). Note that the constitutive immunolabeling observed in the medial striatum (mSt) for P-Elk-1 (D) and P-CREB (F) is no longer detectable in the lSt (E and G, respectively). Data are representative of three independent 60-min-stimulated rats. Scale bar, 1 cm = 15 µm.

Thus, after long-term stimulation the drastic decrease of P-Elk-1 and P-CREB immunoreactivity contrasted with a slighter decreaseof P-ERK. These data suggest that the dephosphorylation of thesetranscription factors was not fully coupled with ERK inactivation.

Parke Davis 98059, an inhibitor of ERK activation, abolishes cortically driven IEG induction in the striatum

At 15 min, P-ERK was correlated spatially with the onset of IEG induction, a result strongly suggesting a relationship betweenthese events. To go further in the role of the ERK pathway inIEG induction, we analyzed the role of PD 98059, a specific MEK-1and MEK-2 inhibitor with IC₅₀ values of 10 and 50 µM, respectively(Pang et al., 1995). The specificity of PD 98059 for MEK-1 andMEK-2 has been demonstrated in experiments in which PD 98059 failedto inhibit the activity of 18 other Ser/Thr kinases (Alessi etal., 1995; Dudley et al., 1995). We injected PD 98059 at 100 µMstereotaxically in the lateral striatum. This injection was performedunilaterally (ipsilaterally to the stimulation) 45 min beforeand during the 15 min stimulation. We chose this stimulation periodbecause ERK activation was maximal at this time point (Fig. 6A).

Although the unilateral injection of vehicle did not affect striatal ERK activation (Fig. 7B), cortically driven P-ERK inductionwas abolished completely after PD 98059 injection in the injectedstriatum (Fig. 7D, asterisk), and not contralaterally (Fig. 7C).Total ERK proteins remained unchanged after PD 98059 injection(Fig. 7H), thus demonstrating that PD 98059 affects ERK activation,and not ERK protein levels. Counterstaining by cresyl violet revealedthe integrity of neuronal cells in both striata (data not shown).

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Figure 7. Parke Davis 98059 abolishes IEG induction after 15 min of corticostriatal stimulation. The MEK inhibitor PD 98059 (right columns) or the vehicle (left columns) was injected in the lateral striatum (lSt) unilaterally and ipsilaterally to the electrode implantation. After 15 min of stimulation, brains were processed for P-ERK (A-D) and ERK (E-H) immunoreactivity and in situ hybridization of c-fos (I, J), zif 268 (K, L), and MKP-1 (M, N) mRNAs. In vehicle-injected rats the stimulation induced a strong bilateral activation of ERK in the lSt (A, B). By contrast, in PD 98059-injected rats this stimulation produced ERK activation contralaterally (C), but not ipsilaterally (D; asterisk), to the inhibitor injection site. ERK immunostaining remained unchanged in vehicle-injected (E, F) and PD 98059-injected (G, H) rats. In vehicle-injected rats the cortical stimulation led to a bilateral induction of c-fos (I), zif 268 (K), and MKP-1 (M) mRNAs. In PD 98059-injected rats, although IEG mRNAs were still induced contralaterally to the inhibitor injection site, an impairment of induction for c-fos (J) zif 268 (L), and MKP-1 (N) was observed ipsilaterally (asterisk) to the PD 98059 injection. These data are representative of three independent rats for each group. Scale bar, 1 cm = 50 µm.

We then analyzed, on sections adjacent to those used above, IEG mRNA induction. In vehicle-injected rats the stimulation induceda striatal bilateral induction of c-fos (Fig. 7I), zif 268 (Fig.7K), and MKP-1 (Fig. 7M) mRNAs. By contrast, in PD 98059-injectedrats a complete inhibition of c-fos (Fig. 7J), zif 268 (Fig. 7L),and MKP-1 (Fig. 7N) mRNA induction was observed in the injectedstriatum (Fig. 7, asterisk), in register with the prevention ofERK activation. Cortically driven ERK activation and IEG inductionwere still detected in the contralateral striatum to PD 98059injection, thus demonstrating the efficacy of the cortical stimulation.In some experiments in which a smaller PD 98059 volume was tested,we obtained a limited inhibition of c-fos and zif 268 mRNAs ina spatial register with the blockade of ERK activation (data notshown). Together, these results indicate that IEG induction strictlydepends on the ERK cascade activation.

ERK proteins dually control Elk-1 and CREB hyperphosphorylation

The hyperphosphorylation of Elk-1 and CREB appeared in the lateral striatum at 15 min of stimulation, i.e., concomitantlyto ERK activation and in a strict spatial correspondence withIEG induction. We thus addressed a possible role of the ERK cascadeactivation in the regulation of these transcription factors. Forthis purpose, anti-active Elk-1 (Fig. 8E-H) and CREB (Fig. 8I-L)immunostaining were performed, after PD 98059 injection, on sectionsadjacent to those processed for P-ERK labeling (Fig. 8A-D). Inthe PD 98059-injected striatum, P-Elk-1 immunoreactivity was nolonger increased (compare Fig. 8, H with G), thus indicating itsdownregulation after the ERK blockade. On the contralateral sideto PD 98059 injection, P-Elk-1 immunoreactivity remained increasedin the lateral striatum (compare Fig. 8, E with F). These resultsindicate that Elk-1 hyperphosphorylation depends strictly on theERK cascade activation.

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Figure 8. ERK proteins dually control Elk-1 and CREB hyperphosphorylation. Brains of PD 98059-injected rats, stimulated for 15 min, were processed for P-ERK (A-D), P-Elk-1 (E-H), and P-CREB (I-L) immunoreactivity. The injection of PD 98059 completely prevented ERK activation in the lateral striatum (lSt) ipsilaterally (D), but not contralaterally (A), to the inhibitor injection site. In the medial striatum (mSt) P-ERK immunoreactivity remained low in both sites (B, C). On sections adjacent to those used below, Elk-1 and CREB hyperphosphorylation were impaired in the lSt ipsilaterally (H and L, respectively), but not contralaterally (E and I, respectively), to the PD 98059 injection. The constitutive P-Elk-1 (F, G) and P-CREB (J, K) immunostaining remained low in both medial striata and was comparable to the immunolabeling observed in lSt ipsilaterally to the PD 98059 injection (H, L). Scale bar, 1 cm = 25 µm.

More surprisingly, we also observed an abolition of P-CREB increase after PD 98059 injection (compare Fig. 8, L with K). Thiswas not the case in the contralateral side, where a strong hyperphosphorylationof CREB was still detectable in the lateral striatum (compareFig. 8, I with J). Thus CREB hyperphosphorylation also dependson the ERK cascade activation in our model.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Three central findings emerge from this in vivo study. First, a transient activation of the ERK signaling pathway is crucialfor cortically driven IEG induction. Second, both Elk-1 and CREBtranscription factors are targeted by this signaling pathway.This is, to our knowledge, the first demonstration of a dual roleof ERK proteins in CRE- and SRE-driven transcriptional regulationin the adult CNS. Third, although CREB activation is strictlynuclear, Elk-1 hyperphosphorylation occurs in both cytoplasmicand nuclear compartments of striatal neurons.

Cortically driven IEG induction is controlled by ERK proteins

From in vitro models that use the transiently transfected c-fos reporter gene, we know that ERK-mediated gene regulation dependson cell lines and mode of calcium entry (Miranti et al., 1995;Xia et al., 1996; Johnson et al., 1997). To address the involvementof ERK in gene regulation in vivo, we used electrical stimulationof the glutamatergic corticostriatal pathway that leads to a topographicalinduction of IEGs in the striatum (Sgambato et al., 1997, 1998).The strict spatiotemporal coincidence between ERK activation andthe onset of messenger induction suggested that this signalingpathway is required for cortically driven gene regulation. Thiswas confirmed after intrastriatal injection of the MEK inhibitorPD 98059, which completely abolished c-fos and zif 268 as wellas MKP-1 mRNA upregulation. Analysis of the transcription factorsElk-1 and CREB allowed us to better understand how ERK proteinscontrolled the expression of these genes.

ERK dually controls Elk-1 and CREB hyperphosphorylation

We traced intracellular events linking ERK activation to gene regulation and found a hyperphosphorylation of Elk-1 and CREBin a strict spatial register with P-ERK and IEG mRNA induction.The critical role played by ERK in the activation of these transcriptionfactors was demonstrated after PD 98059 injection. This treatmentimpaired Elk-1 hyperphosphorylation, a result in agreement withits being a target of ERK. Although the activation of the SRFwas not measured in our study, our data suggest that the ERK/Elk-1module played a necessary and sufficient role in the activationof SRE sites located in the promoter of both c-fos and zif 268.

Calcium-induced CREB phosphorylation classically depends on CaMKs (Sheng et al., 1990) or PKA (Impey et al., 1996). In thelatter case a calcium/calmodulin-sensitive adenylyl cyclase couldbe stimulated by calcium influx. However, neither CaMK nor PKAseems to be implicated directly in CREB phosphorylation in ourmodel, because the PD 98059 inhibitor completely abolished CREBhyperphosphorylation. Thus, we hypothesize that ERK activationplays a critical role in CREB regulation (results discussed below).This result highlights the interesting hypothesis that genes containingCRE, and not SRE, DNA regulatory elements, like MKP-1 (Noguchiet al., 1993; Kwak et al., 1994), could be regulated by an ERK-dependentpathway. In neurotrophin-treated PC12 cells and primary corticalneurons, CREB is targeted by RSK (Xing et al., 1996; Finkbeineret al., 1997), a substrate of ERK proteins (Strugill et al., 1988).Thus we might propose that the ERK-dependent CREB activation implicatesRSK as an intermediate in our model. This hypothesis was not testedbecause of the lack of commercially available anti-active RSKantibodies.

Together, these data show that glutamate-induced IEG induction is dependent on ERK activation targeting both SRE and CRE sites.This is consistent with a study showing that these DNA sequencesare essential for the calcium-driven induction of a c-fos reportergene in transgenic mice (Robertson et al., 1995). In vitro, thephosphorylation of CREB or Elk-1 can recruit the CREB bindingprotein (CBP) coactivator (Kwok et al., 1994; Janknecht and Nordheim,1996) to facilitate the assembly of the polymerase II transcriptioncomplex at the TATA box that leads to the initiation of transcription.Whether the concomitant activation of CBP by CREB and Elk-1 occursin vivo remains to be established. However, this could providethe molecular mechanism by which the activation of different DNAregulatory elements can act synergistically to activate IEG transcription.

Persistent IEG induction contrasts with transient activation of both ERK modules

ERK protein activation was transient in our model. This is consistent with data showing that a transient activation of theseproteins is necessary and sufficient to drive LTP in the rat hippocampus(English and Sweatt, 1997). Whether the transient activation ofERK was sufficient to drive long-term gene regulation in our modelremains to be established. In that way, considering that bothElk-1 and CREB also were dephosphorylated at this time point,a CaMK-SRF module (Miranti et al., 1995) could relay glutamate-inducedgene regulation at late time points.

The strong and early induction of mRNA encoding MKP-1 protein, one of the phosphatases involved in ERK inactivation in transfectedcells (Alessi et al., 1993; Sun et al., 1993), was coincidentwith the progressive ERK inactivation. Although MKP-1 preferentiallyattenuates signaling via the JNK/SAPK and p38 MAPK pathways (Franklinand Kraft, 1997), its strong induction likely was related to ERKinactivation, because neither JNK/SAPK nor p38 MAPK was activatedafter short- or long-term corticostriatal stimulation (data notshown). Additional mechanisms may underlie the drastic dephosphorylationof Elk-1 and CREB, which showed lower levels of phosphorylationthan in basal conditions. Calcineurin, a calcium-responsive phosphatasewidely expressed in the striatum (Yakel, 1997), is implicatedin CREB dephosphorylation (Bito et al., 1996) and also representsthe major Elk-1 serine-threonine phosphatase (Sugimoto et al.,1997). Its role in the dephosphorylation of both transcriptionfactors would be consistent with its being critically involvedin LTP (Winder et al., 1998).

Elk-1 and CREB activation occurs in different subcellular compartments

A striking feature of this work was the visualization of activated proteins in various subcellular compartments, i.e., activationof ERK and Elk-1 in cytoplasmic (dendritic and somatic) and nuclearcompartments, and an exclusively nuclear CREB activation. ERKproteins are, in their nonactivated state, enriched in dendriticand somatic compartments (Fiore et al., 1993a; Ortiz et al., 1995).The presence of activated proteins, i.e., phosphorylated, in dendritessuggests a local activation by calcium influx. Corticostriatalafferents impinge precisely on the dendritic spines (Smith andBolam, 1990) of striatal neurons, on which are localized bothAMPA and NMDA glutamatergic receptors (Bernard et al., 1997; V.Bernard and J. P. Bolam, unpublished observations). The NMDA receptors,which may be critically involved in calcium-dependent LTP in thestriatum (Charpier and Deniau, 1997), is implicated in striatalFos induction after cortical stimulation (Abo et al., 1994; Listeet al., 1995). Key intermediate downstream NMDA receptors appearto be the calcium-dependent nonreceptor tyrosine kinases, PYK2or FAK, which in turn can activate the ras-dependent signalingpathway: ras/raf/MEK/ERK (Lev et al., 1995; Siciliano et al.,1996). Interestingly, B-Raf, a member of the raf family, whichis enriched in the striatum (Barnier et al., 1995), also is localizedin dendrites of striatal neurons.

On cell line models Elk-1 is described as a nuclear transcription factor (Janknecht et al., 1994), which can be phosphorylatedlocally after the nuclear translocation of activated ERK proteins(Chen et al., 1992). However, in postmitotic neuronal cells Elk-1is present in its nonactivated state in cytoplasmic and nuclearcompartments (Sgambato et al., 1998). The finding of hyperphosphorylatedElk-1 in nuclear compartments after glutamate activation is inagreement with its being a nuclear transcription factor. The presenceof activated Elk-1 along with P-ERK in non-nuclear compartments(including the dendrites) indicates that it can be phosphorylatedlocally, near the calcium entry, by activated ERK proteins. Insupport of this is the observation that PD 98059 injection abolishedthe dendritic hyperphosphorylation of Elk-1. Whether Elk-1 thencan translocate to the nucleus to trigger gene regulation or playa specific role in the cytoplasm remains to be established; thiswould be a critical issue in understanding intracellular mechanismsthat relay information from the distal dendritic glutamatergicreceptors to the nucleus (Fig. 9).

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Figure 9. Proposed model for ERK-dependent IEG induction on corticostriatal pathway stimulation. Cortical fibers impinge specifically on dendritic spines of striatal neurons (Smith and Bolam, 1990). The electrical stimulation of these afferents leads to glutamate release at corticostriatal synapses (Reubi and Cuenod, 1979), which in turn act via glutamatergic receptors (1). The subsequent and local elevation of intracellular calcium levels, via NMDA receptors, activates ERK machinery (2) located in the dendrites (Fiore et al., 1993a; Ortiz et al., 1995). Elk-1 proteins that are present in dendrites (Sgambato et al., 1998) are phosphorylated locally by ERK proteins (3). Because both ERK and Elk-1 hyperphosphorylated proteins also are found in the nucleus, we suggest that they are translocated into the nucleus on activation (4, 5). In the nucleus Elk-1 can mediate the transcriptional regulation of SRE-containing IEGs like c-fos and zif 268 (6). In parallel, we show that activated ERK proteins lead to a hyperphosphorylation of the nuclear CREB protein. The activation of the CREB kinase RSK, a cytoplasmic substrate of ERK proteins (Strugill et al., 1988) (7), and its subsequent translocation into the nucleus (Chen et al., 1992) could explain the ERK-dependent CREB activation in our model. In the nucleus CREB mediates the transcriptional regulation of CRE-containing IEGs like c-fos, zif 268 (8), and MKP-1 (9). The protein MKP-1 may act in a negative feedback loop (10) to downregulate ERK activation. Thus, two different ERK modules are critically involved in IEG induction: ERK/Elk-1/SRE and ERK/?/CREB/CRE.

Contrasting with the dual localization of P-Elk-1, activated CREB was exclusively nuclear. This is in agreement with previousdata indicating that this transcription factor is a nuclear protein(Yamamoto et al., 1989). Whereas on pituitary cell lines (AtT20)CREB phosphorylation occurs after nuclear translocation of calcium(Hardingham et al., 1997), on hippocampal neurons the increasesin nuclear calcium are not sufficient to drive CREB activation(Deisseroth et al., 1996). The mean difference between these celltypes is the presence of dendritic processes in hippocampal neurons,and not in AtT20 cells. In other words, when calcium entry occursfar from the soma, and this is precisely the case in striatalneurons, CREB activation can depend on a cytoplasmic kinase. Because(1) ERK machinery is enriched in dendrites and (2) CREB activationis abolished after PD 98059, we suggest that ERK activation isthe major event in triggering CREB hyperphosphorylation in ourmodel. The link between ERK and CREB activation could be the cytoplasmicsubstrate of ERK, RSK, which in turn could translocate to thenucleus (Chen et al., 1992) to activate CREB (Fig. 9).

In conclusion, our data provide the first in vivo evidence of a strictly ERK-dependent gene regulation by corticostriatalpathway stimulation and bring new insights in intracellular mechanismsunderlying LTP in the striatum.

  FOOTNOTES

Received June 25, 1998; revised Aug. 10, 1998; accepted Aug. 14, 1998.

This work was supported by the Université Pierre et Marie Curie, the Centre National de la Recherche Scientifique, InstitutLilly, and Biomed Program (PL 962215). V.S. is a doctoral fellowof the Ministere de l'Education Nationale et de l'EnseignementSuperieur. We thank Dr. J. M. Deniau for helpful advice; Dr. R.A. Hipskind for critical discussion and for providing c-fos, zif268, and MKP-1 cDNAs; and Parke Davis for generously providingPD 98059.
Correspondence should be addressed to Dr. Jocelyne Caboche, Laboratoire Neurochimie-Anatomie, Institut des Neurosciences,Unité Mixte de Recherche 7624, Université Pierre et Marie Curie,9 Quai St. Bernard, 75005 Paris, France.

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Results
Discussion
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