Differential Regulation of Mitogen-Activated Protein Kinases ERK1/2 and ERK5 by Neurotrophins, Neuronal Activity, and cAMP in Neurons

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The Journal of Neuroscience, January 15, 2001, 21(2):434-443

Differential Regulation of Mitogen-Activated Protein Kinases ERK1/2 and ERK5 by Neurotrophins, Neuronal Activity, and cAMP in Neurons
Jane E. Cavanaugh¹^,², James Ham¹, Michal Hetman¹^,², Steve Poser², Chen Yan³, and Zhengui Xia¹^,²
Departments of ¹ Environmental Health and ² Pharmacology, University of Washington, Seattle, Washington 98195-7234, and ³ Cardiology Unit, University of Rochester, Rochester, New York 14642

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Activation of the extracellular signal-regulated kinase 1 (ERK1) and ERK2 by neurotrophins, neuronal activity, or cAMP hasbeen strongly implicated in differentiation, survival, and adaptiveresponses of neurons during development and in the adult brain.Recently, a new member of the mitogen-activated protein (MAP)kinase family, ERK5, was discovered. Like ERK1 and ERK2, ERK5is expressed in neurons, and ERK5 stimulation by epidermal growthfactor is blocked by the MAP kinase/ERK kinase 1 (MEK1) inhibitorsPD98059 and U0126. This suggests the interesting possibility thatsome of the functions attributed to ERK1/2 may be mediated byERK5. However, the regulatory properties of ERK5 in primary culturedneurons have not been reported. Here we examined the regulationof ERK5 signaling in primary cultured cortical neurons. Our datademonstrate that, similar to ERK1/2, ERK5 is activated by neurotrophinsincluding brain-derived neurotrophic factor (BDNF), neurotrophin-3(NT-3), and NT-4. BDNF stimulation of ERK5 required the activityof MEK5. Surprisingly, ERK5 was not stimulated by cAMP or neuronalactivity induced by glutamate or membrane depolarization. In contrastto ERK1/2, ERK5 strongly activated the transcriptional activityof myocyte enhancer factor 2C (MEF2C) in pheochromocytoma 12 (PC12)cells and was required for neurotrophin stimulation of MEF2C transcriptionin both PC12 cells and cortical neurons. Furthermore, ERK1/2,but not ERK5, induced transcription from Elk1 and the cAMP/ Ca²⁺ response element in PC12 cells. Our data suggest that mechanismsfor regulation of ERK5 and downstream transcriptional pathwaysregulated by ERK5 are distinct from those of ERK1/2 in neurons.Furthermore, ERK5 is the first MAP kinase identified whose activityis stimulated by neurotrophins but not by neuronalactivity.

Key words: signal transduction; CNS; cortical neurons; neurons; MAP kinase; ERK1/2; ERK5; BMK1; CREB; CRE; MEF2C; BDNF; glutamate; membrane depolarization; neuronal activity; neurotrophin; cAMP

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Activation of extracellular signal-regulated kinase 1 (ERK1) and ERK2 is important for several neuronal functions that areregulated by neurotrophins and neuronal activity. This includesneuronal differentiation and survival during development, as wellas survival and adaptive responses of mature neurons includinglong-term potentiation (LTP) and memory formation. For example,stimulation of the ERK1/2-signaling pathway promotes neuronalsurvival (Xia et al., 1995; Bonni et al., 1999; Hetman et al.,1999) and is important for LTP as well as memory formation invertebrates (English and Sweatt, 1997; Atkins et al., 1998; Impeyet al., 1998a, 1999). The Ca²⁺ response element-binding protein (CREB)/CRE transcriptional pathwayis a major regulatory target of ERK1/2 signaling and may be pivotalfor plasticity and neuronal survival mediated by ERK1/2 (Montminyand Bilezikjian, 1987; Impey et al., 1998a,b; Bonni et al., 1999;Riccio et al., 1999). The transcription factor Elk1 may be anothernuclear target of ERK1/2 important for neuronal plasticity (Bermanet al., 1998). Elk1 is directly phosphorylated and activated byERK1/2 and plays an important role in glutamate-induced gene expressionin neurons (Gille et al., 1992; Xia et al., 1996; Sgambato etal., 1998).

ERK1/2 activity is regulated by the cAMP-signaling pathway. Although cAMP inhibits ERK1/2 in non-neuronal cells (Burgeringet al., 1993; Graves et al., 1993), it activates ERK1/2 in pheochromocytoma12 (PC12) cells and neurons (Erhardt et al., 1995; Martin et al.,1997; Vossler et al., 1997; Wei et al., 1998). cAMP is requiredfor ERK1/2 activation of gene expression (Wei et al., 1998; Yaoet al., 1998), and stimulation of ERK1/2 by cAMP and Ca²⁺ is critical for long-lasting LTP (English and Sweatt, 1996; Impeyet al., 1998b).

ERK5 or big mitogen-activated protein (MAP) kinase 1 is the newest member of the MAP kinase family (Lee et al., 1995; Zhouet al., 1995). Upstream-signaling proteins of the ERK5 pathwayinclude MEK5, MEKK3, and Cot (English et al., 1995; Zhou et al.,1995; Chao et al., 1999; Chiariello et al., 2000). Although ERK5contains a TEY dual phosphorylation motif similar to that of ERK1/2,a large C terminal and a unique loop-12 sequence distinguish itfrom ERK1/2 and other MAP kinase family members. ERK5 is activatedby serum, epidermal growth factor (EGF), nerve growth factor (NGF),and G-protein-coupled receptors and weakly by phorbol esters (Katoet al., 1997, 1998; English et al., 1998; Chao et al., 1999; Kamakuraet al., 1999; Marinissen et al., 1999). ERK5 contributes to EGF-inducedcell proliferation and cell cycle progression (Kato et al., 1998)as well as Ras-dependent cellular transformation (English et al.,1999).

The MEK1/2 inhibitors PD98059, SL327, and U0126 have been extensively used to implicate ERK1/2 in neuroplasticity (Impey etal., 1999) and neuronal survival (Villalba and Journot, 1997;MeyerFranke et al., 1998; Skaper et al., 1998; Anderson and Tolkovsky,1999; Singer et al., 1999; Bi et al., 2000). Interestingly, ERK5activation by EGF in COS7 cells is also blocked by these inhibitors(Kamakura et al., 1999), suggesting that the ERK5 pathway mayalso regulate cellular processes credited previously to ERK1/2.However, the regulatory properties of ERK5 and the downstreamtranscriptional events involved in the ERK5 signaling in neuronshave not been reported. Consequently, it is crucial to defineERK5-signaling mechanisms inneurons.

In this study, we examined the regulation of ERK5 signaling in primary cultures of cortical neurons and in PC12 cells. Wemeasured ERK5 activity by two well established methods: ERK5 autophosphorylation(Abe et al., 1997; Yan et al., 1999) and reduced electrophoreticmobility (phosphorylation shift) (Kato et al., 1997, 1998). Wereport that ERK5 is activated by neurotrophins but not by neuronalactivity or cAMP in cortical neurons. Furthermore, ERK1/2 andERK5 activate distinct transcription pathways in PC12 cells andcortical neurons. These data suggest that ERK5 and ERK1/2 aredifferentially regulated in corticalneurons.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Materials. The following plasmids have been described: pON260 (Cherrington and Mocarski, 1989), the dominant-negative andconstitutively active MEK1 (Mansour et al., 1994), the pGEX-GST-ERK5[C-terminal 100 amino acids (aa)] (Yan et al., 1999), and CRE( $alpha$ 168)-luciferase(Matthews et al., 1994). The following materials were obtainedfrom Dr. J. D. Lee at Scripps Institute, La Jolla, CA (Kato etal., 1997): the Flag-tagged wild-type ERK5 expression vector,the hemagglutinin (HA)-tagged dominant-negative and constitutivelyactive MEK5 expression vectors, the pGEX-GST-ERK5 (M; short form),and the polyclonal anti-peptide body against the C-terminal sequenceof ERK5 (EGHGMNPADIESLQREIQMDSPML). The polyclonal anti-phospho-ERK1/2antibody (anti-ACTIVE mitogen-activated protein kinase) was purchasedfrom Promega (Madison,WI).

Cell cultures. Primary cortical neurons were prepared from newborn Sprague Dawley rats as described (Hetman et al., 1999,2000). Briefly, dissociated cortical neurons were plated in 60mm culture dishes for biochemistry experiments or in 35 mm dishesfor transfection experiments at a density of 4 × 10⁶ cells/60 mm dish or 2 × 10⁶ cells/35 mm dish, respectively; cultured in basal medium Eagle(BME) supplemented with 10% heat-inactivated bovine calf serum(BCS), 35 mM glucose, 1 mM L-glutamine, 100 U/ml penicillin, and0.1 mg/ml streptomycin; and maintained in a humidified incubatorwith 5% CO₂ at 37°C. Plates and glass coverslips were coated withpoly-D-lysine and laminin. Cytosine- $beta$ -D-arabinofuranoside (Ara-C;2.5 µM; Sigma, St. Louis, MO) was added to cultures on the secondday after seeding (DIV2) to inhibit the proliferation of non-neuronalcells. Previous studies demonstrated that >90% of the cells inthis culture preparation are neurons (Hetman et al., 1999). Corticalneurons were cultured for 6 d (DIV6) before drug treatment. PC12cells were maintained in DMEM (Life Technologies, Gaithersburg,MD) supplemented with 10% BCS, 5% fetal bovine serum (Life Technologies),100 U/ml penicillin, and 0.1 mg/mlstreptomycin.

Transient transfection of primary cortical neurons for kinase assays. Cortical neurons (2 × 10⁶ cells/35 mm dish) were transiently transfected at DIV3 usinga calcium phosphate coprecipitation protocol as described (Xiaet al., 1996; Hetman et al., 1999). Briefly, the DNA-calcium phosphateprecipitates were prepared by mixing 1 vol of DNA in 250 mM CaCl₂with an equal volume of 2× HEPES-buffered saline (HBS; 274 mMNaCl, 10 mM KCl, 1.4 mM Na₂HPO₄, 15 mM D-glucose, and 42 mM HEPES,pH 7.07). The precipitates were allowed to form for 25-30 minat room temperature before addition to the cultures. The conditionedculture media were removed and saved. Cells were washed threetimes with BME, and 1.5 ml of transfection media was added toeach 35 mm dish. The transfection media consist of BME supplementedwith 1 mM sodium kynurenate, 10 mM MgCl₂, and 5 mM HEPES. ThepH of the transfection media was kept high by incubating BME ina dish at 37°C and 0% CO₂ for 30 min to "degas." Sixty microlitersof the DNA-calcium phosphate precipitates were added dropwiseto each 35 mm dish and mixed gently. Plates were incubated atroom temperature and ambient air for 5 min and then in a humidifiedincubator with 5% C0₂ at 37°C for 35-45 min. The incubation wasstopped 20-25 min after the layer of precipitate formed on theplates by "shocking" the cells for 2 min with 1× HBS, 1 mM sodiumkynurenate, and 10 mM MgCl₂ in 5 mM HEPES, pH 7.5, and 5% glycerol.Cells were then washed three times with 2 ml of BME. The savedconditioned media were added back to each plate, and cells werereturned to the 5% CO₂ incubator at 37°C for 48 hr before treatmentorharvesting.

Drug treatment. Drug treatment was performed at DIV6 for cortical neurons. Forskolin was dissolved in ethanol. Ethanol wasused as vehicle control for forskolin treatment. K252a was dissolvedin water and added 30 min before BDNF stimulation. Doses and timesof drug treatment are described in detail in the figurelegends.

Generation of a polyclonal anti-ERK5 antibody. We made a polyclonal antibody against ERK5 by immunizing rabbits (CocalicoBiologicals, Reamstown, PA) with the GST-ERK5 (C-terminal 100aa) fusion protein. This anti-ERK5 antibody was used in the ERK5autophosphorylation kinase assay. The specificity of this antibodywas confirmed by showing that ERK5 autophosphorylation was notseen when the anti-ERK5 antibody was preincubated with the GST-ERK5fusion protein used to generate the antibody or when preimmunesera were used for immune precipitation of ERK5 (data notshown).

Kinase assays. Cell lysates were prepared as described previously (Dérijard et al., 1995; Xia et al., 1995), and proteinconcentrations were assayed by the Bradford method. Equal amountsof protein extracts (300 µg) were used for each kinase assay.To measure endogenous ERK5 activity, cell lysates were incubatedat 4°C for 2.5 hr with 6 µl of the antisera against the GST-ERK5C-terminal 100 aa fusion protein that we generated. Protein A-Sepharosebeads (60 µl) were then added, and the mixture was incubated at4°C for an additional hour. The endogenous ERK5 activity in theimmune precipitates was then quantitated by an autophosphorylationassay as described (Abe et al., 1997; Yan et al., 1999).

To measure the activity of transfected ERK5 or ERK2, cell lysates (200-300 µg) were incubated with an anti-Flag antibody preboundto a slurry of 80% protein G-Sepharose and 20% protein A-Sepharose.The activity of transfected ERK5 or ERK2 in the immune precipitateswas quantitated by a kinase assay using recombinant GST-MEF2C(10 µg) or MBP (2.5 µg) as the substrate, respectively (Xia etal., 1995; Kato et al., 1997, 1998; Hetman et al., 1999).

To measure endogenous MEK5 activity, cell lysates (300 µg) were incubated at 4°C for 3 hr with an anti-MEK5 antibody (N-19;Santa Cruz Biotechnology, Santa Cruz, CA) prebound to proteinG-Sepharose beads. The MEK5 activity in the immune precipitateswas quantitated by a kinase assay using a recombinant GST-ERK5(M)as the substrate (Kato et al., 1997, 1998; Kamakura et al., 1999;Marinissen et al., 1999). Quantitation of kinase activity wasachieved by PhosphorImager analysis (Molecular Dynamics, Sunnyvale,CA) or by using the ImageQuant program after scanning the autoradiographicimages.

Western analysis. Western blot analysis of ERK5 and anti-phospho-ERK1/2 was performed as described (Kato et al., 1997; Chaoet al., 1999; Hetman et al., 1999). The polyclonal anti-ERK5 peptideantibody used for Western analysis was kindly provided by Dr.J. D. Lee and was used at a dilution of 1:5000.

Reporter gene assays. PC12 cells were transfected using Transfast (Promega) as described by the manufacturer. Briefly, 1 ×10⁵ cells were plated onto each well of a 24-well plate coated withpoly-D-lysine (Sigma). One day later, cells were transfected witha CRE-luciferase reporter gene (1.2 µg/3 wells) or a Gal4-luciferasereporter gene (0.2 µg/3 wells) together with various expressionvectors for Gal4 fusion proteins (0.4 µg/3 wells). The EF1a.LacZDNA (Invitrogen, San Diego, CA) was added at 0.125 µg/3 wellsfor normalization of transfection efficiency. Cortical neuronswere transfected using LipofectAMINE 2000 (Life Technologies)(Impey et al., 1996; Poser et al., 2000). Briefly, 0.5 × 10⁶ cells were plated onto each well of a 24-well plate coated withpoly-D-lysine (Research Collaborative). At DIV4-DIV5, neuronswere cotransfected with the Gal4-luciferase reporter gene (1.4µg/4 wells), Gal4-MEF2C fusion protein (0.9 µg/well), and EF1a.LacZDNA (0.55 µg/4 wells). Where indicated, PC12 cells and corticalneurons were also cotransfected with various expression vectorsfor the ERK5- and ERK1/2-signaling pathways. For PC12 cells, cellswere serum starved at 1 d after transfection for 24 hr and thentreated with NGF (50 ng/ml) for 6 hr when indicated. For corticalneurons, cells were treated at 2 d after transfection with 10ng/ml BDNF or 55 mM KCl for 6 hr when indicated. Cell lysateswere prepared, and the activities of luciferase or $beta$ -galactosidasewere measured as described (Impey et al., 1996). The reportergene luciferase activity was normalized to $beta$ -galactosidase activityand expressed as the fold induction relative tocontrol.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

ERK5 is activated by neurotrophins in primary cortical neurons

ERK1/2 is activated by growth factors and neurotrophins in several cell types including neurons (Ahn et al., 1992; Castellinoand Chao, 1996; Segal and Greenberg, 1996). Similarly, ERK5 isactivated by EGF and NGF in PC12 and non-neuronal cells (Katoet al., 1998; Kamakura et al., 1999). However, the regulationof ERK5 by neurotrophins in primary cultured neurons derived fromCNS has not been reported. Therefore, we examined whether ERK5is stimulated by various physiological stimuli in cortical neuronsand compared the regulation of ERK5 with that of ERK1/2. Corticalneurons were treated with various concentrations (0-50 ng/ml)of BDNF for 1 hr, and the cell lysates were analyzed by Westernanalysis using antibodies against ERK5 or phospho-ERK1/2 (Fig.1A). BDNF treatment, at concentrations as low as 5 ng/ml, causeda reduced electrophoretic mobility (phosphorylation shift) ofERK5, indicative of ERK5 activation (Kato et al., 1997, 1998).The phosphorylation shift of ERK5 was maximal at 10 ng/ml BDNF,a concentration of BDNF used in subsequent studies. ERK1/2 activationwas measured by Western analysis using the anti-phospho-ERK1/2antibody that recognizes phosphorylated and activated ERK1/2.As reported previously (Marsh et al., 1993; Hetman et al., 1999),BDNF activated ERK1/2 in cortical neurons, and the dose-responsecurves for activation of ERK5 and ERK1/2 were similar.

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Figure 1. Neurotrophins induce ERK5 and ERK1/2 phosphorylation in cortical neurons. A, Dose-response relationship of BDNF stimulation of ERK5 and ERK1/2 phosphorylation is shown. At DIV5, cortical neurons were treated with 0, 2, 5, 10, 25, or 50 ng/ml BDNF for 1 hr. Cell lysates from human embryonic kidney 293 cells transiently transfected with a constitutively active MEK5 and a wild-type ERK5 were used as a positive control (+) for the ERK5 phosphorylation shift. B, Kinetics of BDNF stimulation of ERK5 and ERK1/2 phosphorylation is shown. At DIV5, cortical neurons were treated with 10 ng/ml BDNF for the indicated times. C, NT-3 and NT-4 also induce ERK5 and ERK1/2 phosphorylation. At DIV5, cortical neurons were treated with 10 ng/ml NT-3 or NT-4 for 0.5, 2, or 12 hr. Cell lysates were prepared, and 20 µg of total protein was submitted to Western analysis using antibodies recognizing ERK5 (Abe et al., 1996) or phosphorylated (p) ERK1/2. Phosphorylation of ERK5 was observed as a shift in ERK5 mobility, indicative of ERK5 activation. The anti-phospho-ERK1/2 antibody recognizes the phosphorylated and activated ERK1/2, indicative of ERK1/2 activation. Data are representative of four (A, B) or three (C) independent experiments. The positions of molecular weight markers are indicated on the right of the figures.

To determine the kinetics of ERK5 activation, cortical neurons were treated with 10 ng/ml BDNF for various times. Like ERK1/2activation, ERK5 activation was prolonged and sustained for upto 24 hr after BDNF treatment (Fig. 1B). However, the peak activationof ERK5 was slower than that of ERK1/2. Although ERK5 activationwas detectable at 5 min, it did not reach a maximum until 1-2hr after BDNF treatment. The slow kinetics of ERK5 activationwas also confirmed by the autophosphorylation assay (e.g., seeFig. 3). In contrast, ERK1/2 was maximally activated by BDNF at30 min under the same conditions using the same cultured neuronpreparations. In addition to BDNF, other neurotrophins, includingneurotrophin-3 (NT-3), NT-4, and NGF, also activate ERK1/2 (Castellinoand Chao, 1996; Segal and Greenberg, 1996). Similarly, ERK5 wasactivated by NT-3 or NT-4 treatment of cortical neurons (Fig.1C). In agreement with other reports (Kamakura et al., 1999),NGF treatment of PC12 cells activated ERK5 (data notshown).

To determine whether BDNF activation of ERK5 requires TrkB tyrosine kinase activity, cortical neurons were treated with K252a,an inhibitor of receptor tyrosine kinases. Like ERK1/2, ERK5 activationwas inhibited by K252a (Fig. 2), suggesting that inhibition ofreceptor tyrosine kinase prevents BDNF stimulation of both ERK5and ERK1/2.

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Figure 2. BDNF stimulation of ERK5 phosphorylation requires receptor tyrosine kinase activity. Cortical neurons (DIV5-DIV6) were pretreated with 0, 2, or 5 µM K252a for 30 min and then stimulated with 10 ng/ml BDNF for 0.5, 1, or 2 hr as indicated. Phosphorylation (p) of ERK5 and ERK1/2 was measured by Western analysis as described in Figure 1. Similar results were obtained in two independent experiments.

To confirm ERK5 activation by BDNF, ERK5 activity was quantitated using an ERK5 autophosphorylation assay after immune precipitationof ERK5. This alternative assay was used because activation ofERK5 leads to increased ERK5 autophosphorylation (Abe et al.,1997; Yan et al., 1999). BDNF stimulation of cortical neuronsincreased ERK5 autophosphorylation fourfold, and the kineticsof activation was comparable with that measured using the phosphorylationshift assay (Fig. 3). Together, the phosphorylation shift andautophosphorylation data indicate that neurotrophins activateboth ERK5 and ERK1/2 in cortical neurons.

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Figure 3. BDNF activates ERK5 in cortical neurons. Cortical neurons (DIV5-DIV6) were treated with 10 ng/ml BDNF for various times. Three hundred micrograms of total protein were used to measure ERK5 activity by the autophosphorylation assay. A, A representative autoradiograph of the ERK5 autophosphorylation kinase assay. B, Quantitation of ERK5 autophosphorylation. Inset, A more detailed profile of ERK5 activation at early time points. Data are the average of five to seven experiments. Error bars represent SEM.

MEK5 is activated by BDNF and is required for BDNF stimulation of ERK5

MEK5 is an upstream kinase that phosphorylates and activates ERK5 in several non-neuronal cells (Zhou et al., 1995; Kato etal., 1997, 1998; English et al., 1999; Kamakura et al., 1999).To determine whether MEK5 mediates BDNF stimulation of ERK5 incortical neurons, MEK5 kinase activity was monitored by an immunecomplex kinase assay using GST-ERK5(M) as the substrate (Katoet al., 1997). BDNF activated MEK5 in cortical neurons, and likeERK5, MEK5 activation was maximal at 1 hr and persisted for upto 24 hr after BDNF stimulation (Fig. 4A).

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Figure 4. MEK5 is activated by BDNF and is required for BDNF stimulation of ERK5 in cortical neurons. A, Endogenous MEK5 is activated by BDNF. At DIV5, cortical neurons were treated with 10 ng/ml BDNF for various times. Three hundred micrograms of total protein were used for an MEK5 immune complex kinase assay with truncated GST-ERK5(M) as the substrate. Inset, A more detailed profile of MEK5 activation at early time points is shown. Data shown are averages of two independent experiments. Error bars represent SEM. B, C, Expression of a dominant-negative MEK5 blocks BDNF stimulation of ERK5 (B) but not ERK2 (C). Cortical neurons (DIV3; 2 × 10⁶ cells/35 mm dish) were cotransfected with 2 µg each of plasmid DNA encoding a wild-type Flag-tagged ERK5 (ERK5wt) or ERK2 (ERK2wt), a dominant-negative HA-tagged MEK5 (MEK5DN), or a vector control (pCMV5) as indicated. Two days later, cells were treated with 10 ng/ml BDNF for 1 hr. Three hundred micrograms of total protein were used for immunoprecipitation with anti-Flag antibody. The transfected ERK5 and ERK2 kinase activities in the precipitates were assayed using GST-MEF2C or MBP as the respective substrates. Data shown are averages of three independent experiments. Error bars represent SEM.

To determine whether MEK5 is required for BDNF stimulation of ERK5, cortical neurons were transiently cotransfected with plasmidDNA encoding a Flag-tagged, wild-type ERK5 and a dominant-negativeMEK5 or the MEK5 vector control (Fig. 4B). To determine the specificityof MEK5 for the ERK5 pathway, dominant-negative MEK5 was cotransfectedwith a Flag-tagged, wild-type ERK2. Two days after transfection,neurons were stimulated with 10 ng/ml BDNF for 1 hr. The activitiesof transfected ERK5 or ERK2 were determined by anti-Flag immuneprecipitation followed by an immune complex kinase assay usingMEF2C or MBP as the substrate, respectively (Xia et al., 1995;Kato et al., 1997; Hetman et al., 1999). Similar to endogenousERK5 and ERK2, the transfected wild-type ERK5 and ERK2 were activatedby BDNF (Fig. 4B,C). Cotransfection of a dominant-negative MEK5,but not the vector control, inhibited BDNF stimulation of ERK5(Fig. 4B). However, BDNF stimulation of ERK2 was not inhibitedby this dominant-negative MEK5 (Fig. 4C). These data suggest thatMEK5 is an upstream kinase that mediates BDNF activation ofERK5.

Glutamate, membrane depolarization, and cAMP do not activate ERK5

Because ERK1/2 activation by neuronal activity is critical for many aspects of neuronal function including neuronal survival(Curtis and Finkbeiner, 1999; Grewal et al., 1999) and neuronalplasticity (Siegelbaum and Kandel, 1991; Impey et al., 1999; Vanhoutteet al., 1999), it was important to determine whether ERK5 is alsoregulated by neuronal activity. Because ERK5 and ERK1/2 are bothactivated by neurotrophins, one might expect that ERK5, like ERK1/2,would also be activated by neuronal activity. To mimic neuronalactivity in vitro, cultured neurons were treated with membrane-depolarizingconcentrations of KCl (55 mM) or with the excitatory neurotransmitterglutamate. Surprisingly, ERK5 was not stimulated by treatmentwith 55 mM KCl for up to 2 hr (Fig. 5A). Similarly, 30 or 100µM glutamate treatment for various times (5-120 min) did not activateERK5 (Fig. 5B; data not shown). In contrast, both glutamate andmembrane depolarization induced ERK1/2 phosphorylation (Fig. 5A,B),confirming that the cortical neurons used in the experiment showednormal responses to membrane depolarization and activation ofglutamate receptors.

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Figure 5. cAMP, KCl, and glutamate activate ERK1/2 but not ERK5 in cortical neurons. Cortical neurons (DIV5) were treated with vehicle control, 55 mM KCl (A), 100 µM glutamate (B), or 2, 5, 10, or 50 µM forskolin (C) that increases intracellular cAMP for the indicated times. For a positive control, neurons were treated with BDNF (10 ng/ml; 1 hr). Phosphorylation (p) of ERK5 and ERK1/2 was measured by Western analysis as described in Figure 1. Similar results were obtained in three independent experiments. Fsk, Forskolin.

In neurons and PC12 cells, cAMP activates the ERK1/2 regulatory pathway. To determine whether ERK5 is also regulated by cAMP,cortical neurons were treated with forskolin, a general activatorof adenylyl cyclases. Treatment of cortical neurons with 2-50µM forskolin for 0.5, 2, or 12 hr stimulated ERK1/2 (Fig. 5C),consistent with previous reports (Erhardt et al., 1995; Martinet al., 1997; Vossler et al., 1997; de Rooij et al., 1998; Kawasakiet al., 1998; Wei et al., 1998). However, under identical conditions,forskolin did not stimulate ERK5. We also quantitated ERK5 activityafter glutamate, KCl, or forskolin treatment using the ERK5 autophosphorylationassay (Fig. 6). In agreement with the results obtained using thephosphorylation shift assay, ERK5 was not activated after treatmentwith 30 µM glutamate, 55 mM KCl, or 2 µM forskolin (Fig. 6). Thesedata indicate that ERK5 is stimulated by neurotrophins but notneuronal activity or cAMP.

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Figure 6. ERK5 autophosphorylation is not increased by KCl, glutamate, or forskolin treatment of cortical neurons. Cortical neurons (DIV5-DIV6) were treated with 10 ng/ml BDNF, 55 mM KCl, 30 µM glutamate, or 2 µM forskolin for various times. Three hundred micrograms of total protein were used to measure ERK5 activity by the autophosphorylation assay. Similar results were obtained with 50 µM forskolin. Data shown are the averages of four to seven experiments. Error bars represent SEM.

ERK5 and ERK1/2 regulate different downstream transcriptional pathways in PC12 cells and cortical neurons

Although ERK5 and ERK1/2 activate some of the same transcription pathways in non-neuronal cells, there are differences intheir downstream transcriptional targets. For example, they bothphosphorylate transcription factors c-Myc and Sap1a (Kato et al.,1997; English et al., 1998; Yang et al., 1998; Kamakura et al.,1999; Marinissen et al., 1999). However, MEF2A and MEF2C are phosphorylatedand activated by ERK5 but not by ERK1/2, whereas Elk1 is phosphorylatedand activated by ERK1/2 but not by ERK5 (Gille et al., 1992; Janknechtet al., 1993; Marais et al., 1993; Kato et al., 1997; Englishet al., 1998; Yang et al., 1998; Marinissen et al., 1999). Todetermine whether ERK5 and ERK1/2 activate distinct transcriptionalpathways in neurons, we examined the effect of ERK5 and ERK1/2activation on transcription mediated by transcription factorsMEF2C and Elk1 and on transcription initiated from the CRE usingPC12 cells and cortical neurons. These transcription events wereanalyzed because MEF2C and CREB have been implicated in neuronalsurvival (Bonni et al., 1999; Mao et al., 1999; Riccio et al.,1999). Furthermore, the Elk1 and the CREB/CRE transcription pathwaysare thought to contribute to memory formation (Berman et al.,1998; Impey et al., 1998b, 1999; Sgambato et al., 1998).

PC12 cells were transiently transfected with a constitutively active MEK5 and a wild-type ERK5 or a constitutively activeMEK1 and a wild-type ERK2 to activate ERK5 or ERK1/2 signalingspecifically. Activation of the ERK5- or ERK1/2-signaling pathwaycaused 22-fold and 5-fold increases in Gal4-MEF2C-mediated transcription,respectively, indicating that MEF2C transcription is preferentiallyactivated by ERK5 (Fig. 7A). This is consistent with previousreports (Kato et al., 1997, 2000; English et al., 1998; Yang etal., 1998; Marinissen et al., 1999).

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Figure 7. MEF2C-transactivating activity is stimulated by NGF and ERK5 in PC12 cells. PC12 cells were transfected with a Gal4-luciferase reporter gene (0.2 µg/3 wells) and an expression vector for Gal4-MEF2C fusion protein (0.4 µg/3 wells) to measure MEF2C transcriptional activity. An EF promoter-driven LacZ expression vector was cotransfected in all cases to normalize for transfection efficiency. A, MEF2C-mediated transactivation is preferentially stimulated by constitutive activation of the ERK5 pathway. To activate ERK5 or ERK1/2, cells were cotransfected with expression vectors (0.1 µg each/3 wells) encoding a constitutively active MEK5 (MEK5CA) with a wild-type ERK5 (ERK5wt) or a MEK1CA with an ERK2wt, respectively. Data shown are the averages of 12 independent experiments ± SEM. B, MEF2C-mediated transcription is activated by NGF via an ERK5-dependent mechanism. To block ERK5 signaling, PC12 cells were transiently transfected with a dominant-negative MEK5 (0.9 µg/4 wells; MEK5DN) together with a dominant-negative ERK5 (0.9 µg/4 wells; ERK5DN) or the corresponding vector controls. Cells were treated with 50 ng/ml NGF (+NGF) or vehicle control ( $-$ NGF) for 6 hr. Data shown are the averages of three independent experiments ± SEM. Luc, Luciferase.

It has been reported that MEF2C transcription is stimulated by membrane depolarization in cerebellar neurons (Mao and Wiedmann,1999; Mao et al., 1999). However, it is not known whether neurotrophinsstimulate MEF2C transcription in neurons. To address this issue,PC12 cells and cortical neurons were transiently transfected witha Gal4-MEF2C expression vector and a Gal4-luciferase reportergene and treated with NGF or BDNF, respectively (Figs. 7B, 8A).NGF and BDNF both activated Gal4-MEF2C-induced transcription,suggesting that MEF2C transcription is also regulated by neurotrophinsin neurons. Neurotrophins activate several kinase pathways inaddition to ERK5 including the p38 MAP kinase pathway (Xing etal., 1998) that can also stimulate MEF2C transcription (Han etal., 1997). To determine the contribution of ERK5 signaling inneurotrophin stimulation of MEF2C transcription, we cotransfectedPC12 cells and cortical neurons with a dominant-negative MEK5together with a dominant-negative ERK5 to inhibit neurotrophinactivation of the ERK5 pathway. Expression of the dominant-negativeMEK5 plus dominant-negative ERK5 inhibited MEF2C transcriptioninduced by NGF and BDNF (Figs. 7B, 8A). To determine the specificinvolvement of the ERK5 pathway in neurotrophin stimulation ofMEF2C transcription, we used a dominant-negative MEK1 as a negativecontrol. Expression of this dominant-negative MEK1 construct blockedCRE-mediated transcription in cortical neurons after KCl stimulation(Fig. 8B), consistent with other reports (Impey et al., 1998a).However, it did not affect BDNF stimulation of MEF2C transcription(Fig. 8A). Together, these data suggest that MEF2C transcriptionis activated by neurotrophins via a mechanism involving the ERK5but not the ERK1/2 pathway.

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Figure 8. BDNF activates MEF2C in cortical neurons that require ERK5 signaling. A, MEF2C-mediated transcription is activated by BDNF via an ERK5-dependent mechanism. Cortical neurons (DIV4-DIV5; 0.5 × 10⁶ cells/well) were transiently transfected with a Gal4-luciferase reporter gene (1.4 µg/4 wells) and an expression vector for Gal4-MEF2C fusion protein (0.9 µg/4 wells) to measure MEF2C transcriptional activity. To block ERK5 or ERK1/2 signaling, neurons were cotransfected with a dominant-negative MEK5 (0.9 µg/4 wells; MEK5DN) together with a dominant-negative ERK5 (0.9 µg/4 wells; ERK5DN) or with a dominant-negative MEK1 (1.8 µg/4 wells; MEK1DN), respectively. The corresponding vectors were used as controls. Cells were treated with 10 ng/ml BDNF (+BDNF) or vehicle control ( $-$ BDNF) for 6 hr. Data are representative of quadruplicate determinations from three independent experiments. B, KCl-activated CRE transcription is inhibited by the dominant-negative MEK1 used in A. To confirm that the MEK1DN used in A functioned properly as a dominant negative, cortical neurons were cotransfected with a CRE-luciferase reporter (2.4 µg/4 wells), a MEK1DN, or its vector control (1.8 µg/4 wells). Cells were treated with 55 mM KCl for 6 hr. Data shown are the averages of quadruplicate determinations. For both A and B, an EF promoter-driven LacZ expression vector (0.55 µg/4 wells) was cotransfected to normalize for transfection efficiency, and error bars indicate SEM. Luc, Luciferase.

In contrast to MEF2C, Gal4-Elk1-induced transcription was enhanced by activation of ERK1/2 but not by ERK5 (Fig. 9A). Furthermore,unlike ERK1/2, ERK5 did not stimulate transcription from CRE (Fig.9B). These data suggest that ERK5 and ERK1/2 activate distincttranscription pathways in PC12 cells and cortical neurons.

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Figure 9. ERK5 does not stimulate Gal4-Elk1 transactivation or CRE-mediated transcription in PC12 cells. A, Transactivation of Elk1 is increased after NGF treatment or stimulation of the ERK1/2 but not the ERK5 pathway. PC12 cells were transfected with a Gal4-luciferase reporter gene (0.2 µg/3 wells) and an expression vector for the Gal4-Elk1 fusion protein (0.4 µg/3 wells). To activate ERK5 or ERK1/2, cells were cotransfected with expression vectors encoding a constitutively active MEK5 (0.2 µg/3 wells; MEK5CA) with a wild-type ERK5 (0.6 µg/3 wells; ERK5wt) or a MEK1CA (0.6 µg/3 wells), respectively. B, NGF treatment or constitutive activation of ERK1/2, but not ERK5, stimulates CRE-mediated transcription. PC12 cells were transfected with a CRE-luciferase reporter (1.2 µg/3 wells) to measure transcription initiated from CRE. To activate ERK5 or ERK1/2, cells were cotransfected with expression vectors encoding MEK5CA (0.1 µg/3 wells) and ERK5wt (0.3 µg/3 wells) or MEK1CA (0.1 µg/3 wells) and ERK2wt (0.3 µg/3 wells), respectively. An EF promoter-driven LacZ expression vector was cotransfected in all cases to normalize for transfection efficiency. When indicated, cells were treated with NGF (50 ng/ml) for 6 hr. Data shown are the averages of triplicate determinations ± SEM. Similar results were obtained in three to four independent experiments. Luc, Luciferase.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The objective of this study was to define the regulatory properties of ERK5 in primary cultures of cortical neurons in responseto neurotrophins, neuronal activity, or cAMP. Neuronal activitywas mimicked in vitro by treating cultured neurons with membrane-depolarizingconcentrations of KCl or glutamate. The activity of endogenousERK5 activity in cortical neurons was measured by two well establishedmethods: the ERK5 autophosphorylation assay (Abe et al., 1997;Yan et al., 1999) and the reduced electrophoretic mobility assay(phosphorylation shift) (Kato et al., 1997, 1998). Neurotrophinsincluding BDNF, NGF, NT-3, and NT-4 caused a sustained activationof MEK5 as well as ERK5 in PC12 cells and cortical neurons. BDNFactivation of ERK5 was blocked by K252a, indicating a requirementfor the receptor tyrosine kinase of TrkB. Furthermore, expressionof a dominant-negative MEK5 blocked BDNF stimulation of ERK5,suggesting that MEK5 mediates neurotrophin stimulation of ERK5inneurons.

Surprisingly, membrane depolarization, glutamate, or cAMP did not activate ERK5 in cortical neurons although they stimulatedERK1/2 activity. Furthermore, MEF2C was activated by neurotrophins,and the ERK5 signaling was required for neurotrophin stimulationof MEF2C transcription. On the other hand, ERK1/2, but not ERK5,activated Elk-1 transcriptional activity and stimulated transcriptioninitiated from CRE. These data suggest that the regulatory propertiesof ERK5 as well as the downstream transcriptional pathways regulatedby ERK5 are distinct from those of ERK1/2 inneurons.

Although neurotrophins activated both ERK5 and ERK1/2 pathways in cortical neurons, the kinetics of ERK5/MEK5 activation wasslower than that of ERK1/2. One possibility for this differenceis that the ERK5 and ERK1/2 pathways are activated by distinctupstream components, such as small G-proteins. For example, NGFactivation of the ERK1/2 pathway in PC12 cells is both rapid andsustained. However, distinct mechanisms account for the two phases;the sustained activation of ERK1/2 by NGF requires the small G-proteinRap1, whereas the initial rapid activation requires Ras (Yorket al., 1998). It is possible that BDNF stimulation of the MEK5/ERK5pathway is mediated by Rap1-like small G-proteins.

Because neuronal activity is critical for neuronal survival and synapse formation (Oppenheim, 1991; Bear and Malenka, 1994;Goldberg and Barres, 2000), it is important to elucidate mechanismsthat translate activity changes to long-lasting modificationsof neurons, particularly transcriptional changes. Activation ofNMDA receptors or voltage-sensitive calcium channels increasesintracellular Ca²⁺ and stimulates ERK1/2 in neuronal cells (Ely et al., 1990; Badingand Greenberg, 1991; Baraban et al., 1993; Fiore et al., 1993;Rosen et al., 1994; Kurino et al., 1995). ERK1/2 is also activatedduring LTP in mice and long-term facilitation in Aplysia (Englishand Sweatt, 1996; Martin et al., 1997; Impey et al., 1998b). Activity-dependentactivation of ERK1/2 has been implicated in several importantaspects of CNS neuron function including LTP (Brambilla et al.,1997; English and Sweatt, 1997; Impey et al., 1998b, 1999) andmemory formation (Atkins et al., 1998; Berman et al., 1998; Impeyet al., 1999). Similar to ERK1/2, several other kinase-signalingpathways are stimulated by both neurotrophins and neuronal activityincluding those of the phosphatidylinositol-3 kinase, Akt, thec-Jun N-terminal protein kinase, and p38 MAP kinases (Farnsworthet al., 1995; Rusanescu et al., 1995; Tan et al., 1996; Kawasakiet al., 1997; Miller et al., 1997; Schwarzschild et al., 1997;Chen et al., 1998; Xing et al., 1998; Yano et al., 1998; Zhanget al., 1998; Grewal et al., 2000). Our data indicate that ERK5is not activated by glutamate or membrane depolarization in corticalneurons, distinguishing this kinase from all of the other MAPkinases. ERK5 is the first MAP kinase identified that is activatedby neurotrophins but not by neuronalactivity.

Our observation that ERK5 in cortical neurons is not stimulated by Ca²⁺ is in accord with previous studies with non-neuronal cells showingthat the Ca²⁺ ionophore A23187 does not activate ERK5 in COS7 and bovineaortic endothelial cells (BAEC) (Kamakura et al., 1999; Yan etal., 1999). However, the intracellular Ca²⁺ chelator BAPTA AM prevented ERK5 activation by EGF in mouse embryofibroblasts and by shear stress in BAEC (Yan et al., 1999; Jiand Carpenter, 2000). This suggests that Ca²⁺ may be required, but is not sufficient, for ERK5 activation innon-neuronalcells.

cAMP inhibits growth factor stimulation of ERK1/2 in non-neuronal cells (Burgering et al., 1993; Graves et al., 1993) butstimulates ERK1/2 in neurons via Rap1 and B-raf (Erhardt et al.,1995; Vossler et al., 1997; de Rooij et al., 1998; Kawasaki etal., 1998). This emphasizes the importance of defining regulatorymechanisms for the MAP kinases in neurons because they are oftendifferent from those in non-neuronal cells. Activators of adenylylcyclases markedly increase ERK1/2 activity in hippocampal neurons(Martin et al., 1997; Wei et al., 1998). Furthermore, activationof ERK1/2 by cAMP is critical for long-lasting LTP (English andSweatt, 1996; Impey et al., 1998b). In contrast, our results suggestthat ERK5 is not activated by increases in intracellular cAMP,which further distinguishes ERK5 from ERK1/2.

The MEF2 proteins constitute a family of transcription factors: MEF2A, MEF2B, MEF2C, and MEF2D. They cooperate with membersof the MyoD family in muscle differentiation (Kaushal et al.,1994; Molkentin et al., 1995). In addition to muscle, MEF2A andMEF2C are also expressed in developing and adult brain includingcortex and cerebellum (Leifer et al., 1993, 1994; McDermott etal., 1993; Lyons et al., 1995; Lin et al., 1996; Mao et al., 1999;Marinissen et al., 1999). Cortex contains a high level of MEF2Cprotein (Lin et al., 1996). However, the function and regulationof MEF2 in the nervous system have not been extensively studied.Although MEF2 mediates T cell receptor-induced apoptosis in Tcells (Youn et al., 1999), a recent study suggests that MEF2 mediatesactivity-dependent survival of cortical and cerebellar neurons(Mao et al., 1999). Although MEF2C transcription is stimulatedby membrane depolarization in cerebellar neurons (Mao and Wiedmann,1999; Mao et al., 1999), it has not been reported whether neurotrophinsstimulate MEF2C transcription in neurons. Furthermore, the kinase-signalingmechanisms that mediate this transcription are unknown. Our datasuggest that neurotrophins (NGF and BDNF) activate MEF2C transcriptionin both neuron-like PC12 cells and in primary-cultured corticalneurons. Furthermore, ERK5 but not ERK1/2 signaling contributesto neurotrophin stimulation of MEF2Ctranscription.

The CREB/CRE transcriptional pathway is a major downstream target of ERK1/2 signaling that contributes to neuroplasticity(Impey et al., 1998b, 1999; Sgambato et al., 1998) and neuronalsurvival (Bonni et al., 1999; Riccio et al., 1999). Although CREBis not directly phosphorylated by ERK1/2, it is phosphorylatedand transactivated by the ERK1/2-activated Rsk family of proteinkinases p90^rsk (Xing et al., 1996, 1998; Impey et al., 1998a). In addition toCREB, the transcription factor Elk1 may also be a major nucleartarget of ERK1/2 important for synaptic plasticity (Berman etal., 1998; Sgambato et al., 1998). Elk1 is directly phosphorylatedand activated by ERK1/2 (Gille et al., 1992, 1995; Janknecht etal., 1993; Marais et al., 1993) and plays an important role inNMDA-induced gene expression in neurons via serum response element(Xia et al., 1996). Our data suggest that ERK5 does not stimulatethe transcriptional activity of Elk1 or transcription initiatedfrom CRE. Together with the fact that ERK5 is not activated byneuronal activity, these results emphasize the importance of ERK1/2signaling for activity-dependent neural plasticity. Although ERK5may not be directly stimulated by neuronal activity, it may besubsequently activated as a result of neurotrophin synthesis.For example, the promoter for BDNF contains a CRE element, andneuronal activity induces BDNF synthesis via the CREB/CRE transcriptionalpathway (Shieh et al., 1998; Tao et al., 1998). BDNF expressionis increased in brain during training for associative fear learning(Hall et al., 2000), a process that stimulates CRE-mediated transcription(Impey et al., 1998a) and is inhibited by MEK inhibitors (Atkinset al., 1998). Consequently, BDNF stimulation of ERK5 may contributeto synaptic plasticity and memory formation by stimulating othertranscriptional pathways, e.g., MEF2C-mediatedtranscription.

In summary, our data identify several key differences between ERK5 and ERK1/2 in their response to neuronal activity and cAMP,as well as in downstream transcriptional targets. This suggeststhat ERK5 may have unique functions in the nervous system. Forexample, ERK5 may be particularly important for promoting neurotrophin-mediatedneuronal survival during development when activity is not crucialfor neuronal survival (Shatz, 1990; Oppenheim, 1991; Johnson andDeckwerth, 1993; Linden, 1994; Ikonomidou et al., 1999, 2000;Goldberg and Barres, 2000). It may also play a key role in neurotrophin-promotedsurvival when ERK1/2 expression is low during early development(Boulton et al., 1991) or in regions of the brain where ERK1/2activity is low (Thomas and Hunt, 1993). Furthermore, the ERK5survival mechanism may differ from and complement the ERK1/2 survivalmechanism by activating distinct downstream transcriptionalpathways.

  FOOTNOTES

Received June 7, 2000; revised Sept. 26, 2000; accepted Nov. 2, 2000.

This work was supported by the National Institute of Neurological Disorders and Stroke Grant NS37359 and the Burroughs WellcomeFund for New Investigator Award in Toxicology Grant APP#3010 (Z.X.).J.E.C. was supported by the National Institutes of Health PostdoctoralTraining Grant Genetic Approaches to Aging (2 T32 AG00057-21).We thank Dr. J. D. Lee for providing anti-ERK5 antibody and expressionvectors for ERK5, MEK5, and GST-ERK5 (M). We thank Dr. J. SilvioGutkind for GST-MEF2C. We thank Dr. J. Han for providing the Gal4-MEF2Cand Flag-tagged wild-type ERK2plasmids.
Correspondence should be addressed to Dr. Zhengui Xia, Department of Environmental Health, Box 357234, University of Washington,HSB, Room F561C, Seattle, WA 98195. E-mail: zxia{at}u.washington.edu.

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