p38 and Extracellular Signal-Regulated Kinases Regulate the Myogenic Program at Multiple Steps

doi:10.1128/MCB.20.11.3951-3964.2000

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Molecular and Cellular Biology, June 2000, p. 3951-3964, Vol. 20, No. 11
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

p38 and Extracellular Signal-Regulated Kinases Regulate the Myogenic Program at Multiple Steps

Zhenguo Wu,¹^,²^, Pamela J. Woodring,³^,⁴ Kunjan S. Bhakta,³ Kumiko Tamura,¹^,² Fang Wen,² James R. Feramisco,²^,⁴ Michael Karin,¹^,²^,⁴ Jean Y. J. Wang,³^,⁴ and Pier Lorenzo Puri³^,⁵^,^*

Laboratory of Gene Regulation and Signal Transduction,¹ Department of Pharmacology,² Department of Biology,³ and Cancer Center,⁴ University of California, San Diego, La Jolla, California 92093-0322, and Laboratory of Gene Expression, Fondazione A. Cesalpino, Istituto I Clinica Medica, Policlinico Umberto I, University of Rome, Rome, Italy⁵

Received 2 December 1999/Returned for modification 10 January 2000/Accepted 10 March 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The extracellular signals which regulate the myogenic program are transduced to the nucleus by mitogen-activated protein kinases(MAPKs). We have investigated the role of two MAPKs, p38 and extracellularsignal-regulated kinase (ERK), whose activities undergo significantchanges during muscle differentiation. p38 is rapidly activatedin myocytes induced to differentiate. This activation differsfrom those triggered by stress and cytokines, because it is notlinked to Jun-N-terminal kinase stimulation and is maintainedduring the whole process of myotube formation. Moreover, p38 activationis independent of a parallel promyogenic pathway stimulated byinsulin-like growth factor 1. Inhibition of p38 prevents the differentiationprogram in myogenic cell lines and human primary myocytes. Conversely,deliberate activation of endogenous p38 stimulates muscle differentiationeven in the presence of antimyogenic cues. Much evidence indicatesthat p38 is an activator of MyoD: (i) p38 kinase activity is requiredfor the expression of MyoD-responsive genes, (ii) enforced inductionof p38 stimulates the transcriptional activity of a Gal4-MyoDfusion protein and allows efficient activation of chromatin-integratedreporters by MyoD, and (iii) MyoD-dependent myogenic conversionis reduced in mouse embryonic fibroblasts derived from p38 $alpha$ ^/ embryos. Activation of p38 also enhances the transcriptionalactivities of myocyte enhancer binding factor 2A (MEF2A) and MEF2Cby direct phosphorylation. With MEF2C, selective phosphorylationof one residue (Thr293) is a tissue-specific activating signalin differentiating myocytes. Finally, ERK shows a biphasic activationprofile, with peaks of activity in undifferentiated myoblastsand postmitotic myotubes. Importantly, activation of ERK is inhibitorytoward myogenic transcription in myoblasts but contributes tothe activation of myogenic transcription and regulates postmitoticresponses (i.e., hypertrophic growth) inmyotubes.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

In the past decade, much has been learned about the molecular mechanisms that govern myogenesis owing mainly to the discoveryof two groups of myogenic transcription factors (4, 45, 62).The first group includes the myogenic regulatory factors (MRFs),which belong to the basic helix-loop-helix (bHLH) protein family.This MRF group consists of four members: Myf5, MyoD, myogenin,and MRF4, all of which are specifically expressed in skeletalmuscles. One of the unique features of these MRFs is that whenthey are ectopically expressed in fibroblasts or certain othernonmuscle cells, each has the ability to initiate the myogenicprogram and convert nonmuscle cells to myogenic derivatives (9,59). Myogenic bHLH proteins heterodimerize with other ubiquitousbHLH proteins (like the E2A gene products, E12, and E47) to efficientlybind a consensus DNA site: CANNTG (also called the E box) (4,33). The second group of transcription factors important inmuscle differentiation consists of four different myocyte enhancerbinding factor 2 (MEF2) proteins, which belong to the MADS boxfamily (7). The MEF2 proteins (MEF2A, MEF2B, MEF2C, and MEF2D)form homo- or heterodimers which bind to a consensus AT-rich sequence(MEF2 site), found in the promoters of many muscle-specific genes.Myogenic bHLH and MEF2 cooperate to synergistically activate muscle-specifictranscription through interactions mediated by the basic regionand the MADS domain, respectively (44, 45).

The study of muscle differentiation has benefited from the availability of several myogenic cell lines which allow biochemicaldissection of the myogenic pathway. These myogenic cell lines(e.g., mouse C2C12 and rat L6) can be induced to differentiateby withdrawal of mitogens, such as serum. Many negative regulatorsof myogenesis (e.g., Id, Twist, oncogenic Ras, and the viral proteinsE1A and simian virus 40 T antigen) have been identified (1,34). However, little is known about the intracellular componentsthat positively regulate the activities of myogenic transcriptionfactors, especially those that are involved in receiving and transducingextracellular cues. One extracellular signal that positively regulatesmyogenesis is insulin-like growth factor (IGF). IGF activatesthe phosphatidylinositol-3 kinase (PI3K) signaling pathway, whichis required for myogenesis (11, 29, 30). However, how thissignaling pathway influences myogenic transcription remains tobedefined.

In eukaryotic cells, mitogen-activated protein kinases (MAPKs) are components of several important signaling pathways thatrelay extracellular cues to transcription factors in the nucleus(24, 25, 32, 41, 51). For mammals, three MAPK pathways,including the extracellular signal-regulated kinases (ERK1 and-2), the Jun-N-terminal kinases (JNK1, -2, and -3), and the p38isoforms ( $alpha$ , $beta$ , $gamma$ , and $delta$ ) have been characterized (references51 and 43 and references therein). In general, each groupof MAPKs is activated by two homologous MAPK kinases (MKKs [alsocalled MAPKKs]), including MEK1 and -2 for the ERKs, JNK kinase1 and 2 (JNKK1 and -2) (or MKK4 and -7) for the JNKs, and MKK3and -6 for the p38s (26, 51). Except for JNKK1, which canalso activate p38 in vitro (14, 38), all other MKKs specificallyactivate their MAPK targets and have little activity on membersof other groups. The ERK pathway has been implicated in the controlof muscle differentiation, although its role remains controversial,with some reports suggesting a positive function (5, 11)and others suggesting a negative function (18). p38 has alsobeen reported to activate certain MEF2 family members (21, 40,48, 61, 67) and to stimulate muscle differentiation (12,64). However, the upstream signals which regulate p38 activationat the onset of muscle differentiation and the mechanism(s) bywhich p38 activates myogenic transcription remainelusive.

Using a combination of different approaches, we found that the p38 kinase is rapidly activated in muscle cells induced todifferentiate by serum withdrawal, through a pathway distinctfrom that activated in response to stress and cytokines. Specificinhibition of p38 prevents differentiation of both establishedmuscle cell lines and human primary myoblasts, while deliberatep38 activation stimulates muscle-specific reporters, acceleratesmyotube formation, and induces the expression of myogenic markersdespite the presence of serum, which otherwise inhibits muscledifferentiation. p38 exerts its stimulatory effect on myogenesisby enhancing the transcriptional activities of both MyoD and MEF2Aand -C through distinct mechanisms. While MEF2 proteins are activatedby direct phosphorylation of residues located within the activationdomain, p38-mediated activation of MyoD is likely to occur byan indirect mechanism. The p38 pathway is activated independentlyof the IGF-PI3K pathway, although the integrity of both thesepathways is required to stimulate muscle differentiation. Conversely,the ERK pathway plays a dual role during myogenic differentiation,being inhibitory at early stages and stimulatory at latestages.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Reagents. Basic fibroblast growth factor (bFGF) was obtained from Sigma. The kinase inhibitors SB202190, SB203580, PD98059, LY294002,and rapamycin were purchased fromCalbiochem.

Cell culture. The myogenic cell line C2C12 derived from mouse muscle satellite cells and human primary myoblasts was cultured in growthmedium (GM; Dulbecco modified Eagle medium [DMEM] with 20% fetalbovine serum [FBS]). Differentiation of these muscle cells wasinduced by replacing GM with differentiation medium (DM; DMEMwith 2% horse serum) when cells were 90% confluent. 10T1/2 cellswere maintained in DMEM supplemented with 10% FBS. Reporter cells(3T3 stable cell clones with an integrated MyoD-dependent reporter,3T3 4RE-Luc) were generated by transfecting the 4RE-Luc templatetogether with pcDNA3neo. G418-resistant colonies were grown andconstituted a polyclonal population of reporter cells. Primaryhuman myoblasts and p38^/ and wild-type mouse embryonic fibroblasts (mEFs) were isolatedaccording to standardprocedures.

Immunostaining. Cells were washed twice with phosphate-buffered saline, fixed with 3.6% formaldehyde for 10 min, and permeabilized with 0.25%Triton X-100 for 10 min. After being blocked in 1% bovine serumalbumin, the cells were incubated with diluted primary antibodiesfor 1 h. For immunohistochemical analysis, a Histomouse-SP kit(Zymed Laboratories Inc., South San Francisco, Calif.) was usedaccording to the manufacturer's instructions. Indirect immunofluorescencewas done as described previously (63) with a Nikon fluorescencemicroscope. Either fluorescein isothiocyanate- or rhodamine-conjugatedsecondary antibodies wereused.

Transfection. Transfections were carried out using Lipofectamine Plus as recommended by the manufacturer (Life Technologies, Inc.). WhenGal4-Luc was used, the cells were first cultured in medium containing10% FBS for 24 h immediately after transfection and then shiftedto medium containing 0.1% FBS for another 24 h. Cells were thenharvested to measure luciferase activity. Expression of Gal4 fusionproteins was quantitated by immunoblotting and phosphorimaging,and luciferase activity was normalized according to the immunoblotresults. When transfected with muscle-specific reporters (4RE-Luc,MCK-Luc, or p21-Luc), cells were cultured in GM for 24 h aftertransfection and then shifted to DM for 36 to 48 h. When used,SB202190 was added to the medium immediately after transfectionand the medium was changed every 12 to 24 h with fresh drug. Thedifferent reporters and activators were previously described (21,53, 65).

Metabolic labeling and phosphopeptide mapping. For transient transfections, the cells were labeled at 18 h posttransfection with 0.5 mCi of [³²P]orthophosphate per ml for 5 h in the absence or presence ofSB202190 as indicated in the figures. Alternatively, C2C12 cellstransiently transfected with M2-tagged MEF2C were labeled 48 hafter being cultured in DM for 36 h. The Gal4-MEF2C or M2-MEF2Cproteins were immunoprecipitated with either anti-Gal4 (SantaCruz) or M2 (Sigma) antibody, and after separation by sodium dodecylsulfate-polyacrylamide gel electrophoresis (SDS-PAGE) were transferredto a polyvinylidene difluoride membrane for autoradiography andimmunoblot analysis. Nontransfected C2C12 cells were kept in eitherGM or DM for 2 days and then labeled with 1 mCi of [³²P]orthophosphate per ml for 5 h. Endogenous MEF2C was immunoprecipitatedwith anti-MEF antibody (kindly provided by J. Han). After beingextensively washed in radioimmunoprecipitation assay buffer, theimmune complexes were separated by SDS-PAGE and the MEF2C bandwas excised and analyzed by two-dimensional tryptic phosphopeptidemapping as described previously (21).

Immunoblot analysis. Endogenous myogenin, myosin heavy chain (MHC), MyoD, p21, and actin in C2C12 cells were detected by immunoblotting using themonoclonal anti-myogenin (F5D), anti-MyoD (5.8), anti-MHC (MF20),anti-p21 (Ab-5; Oncogene), and anti-actin (Ab-1; Oncogene) antibodies.Antibodies against normal and phospho-p38, normal and phospho-ERK,and phospho-Akt were all from New England Biolabs. TransfectedGal-MyoD was detected by using anti-Gal4 antibody from SantaCruz.

Kinase assays. Fifty to 100 µg of cell extracts was incubated with antibodies against either p38 $alpha$ or JNK (recognizing all forms) in the presenceof a 30-µl protein A-Sepharose bead suspension for 2 h at 4°C.The immune complexes were washed three times with lysis buffer(20 mM Tris [pH 7.6], 10% glycerol, 1% Triton X-100, 150 mM NaCl,20 mM $beta$ -glycerolphosphate, 1 mM phenylmethylsulfonyl fluoride,1× protease inhibitor cocktail) and once with kinase buffer (20mM HEPES [pH 7.6], 10 mM MgCl₂, 20 mM $beta$ -glycerolphosphate, 20µM ATP), with ATP omitted. Reactions were initiated by adding1 µg of glutathione S-transferase (GST)-ATF2(1-92) (for p38) orGST-c-Jun(1-79) (for JNK) and 10 µCi of [ $gamma$ -³²P]ATP in 25 µl of kinase buffer. Reactions were carried out for20 min at 30°C, and mixtures were analyzed by SDS-PAGE andautoradiography.

Generation of tetracycline-inducible stably transfected C2C12 cell lines. cDNA fragments encoding either MKK6EE, JNKK2CA, or MEK1DD/ $Delta$ N4 were subcloned into pBPSTR1. A 1:1 ratio of the pBSPTR1-basedexpression vector and the pCL_ECO packaging vector (47) werecotransfected into 293T cells to generate retroviruses. Virus-containingsupernatants were added to C2C12 cells for 6 h in the presenceof 4 µg of Polybrene per ml. Cells were selected in a solutioncontaining 1.5 µg of puromycin per ml and 2 µg of tetracyclineper ml 24 h postinfection for 7 days. Mixtures of all puromycin-resistantclones were used for subsequentanalysis.

	RESULTS

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Activation of p38 during muscle differentiation. Given the importance of MAPKs in transmitting extracellular cues to the transcriptional machinery (25, 32), we examinedthe activities of the ERK, JNK, and p38 subgroups in C2C12 myoblastsundergoing differentiation. While serum removal, which inducesC2C12 myoblasts to form multinucleated myotubes, does not alterJNK activity (Fig. 1c), it stimulates p38 kinase activity (Fig.1a) and induces a biphasic change in ERK activity (Fig. 1d), whichdecreases at the onset of differentiation and increases at laterstages, when myotubes are already formed. Activation of p38 isalso detected by immunoblotting with antibodies specific for itsactivated form (Fig. 1b). p38 activity was rapidly elevated within1 day of placing myoblasts in DM and continued to increase forat least 3 days (Fig. 1a and b), a point at which most myoblastsformed well-differentiated myotubes. Thus, sustained p38 activation,unlinked to JNK stimulation, is part of a differentiation-specificpathway which is distinct from that triggered by stress and cytokines.A rapid activation of p38 upon serum starvation is appreciablealso in fibroblasts; however, unlike in muscle cells, this activitydeclines within the first 24 h (data not shown). Ectopic expressionof MyoD is sufficient to sustain a persistent p38 activation inserum-starved fibroblasts (data not shown). This result suggeststhat the acquisition of the myogenic identity confers to the cellsthe ability to trigger a prolonged activation of p38 in responseto serum withdrawal. Immunohistochemical analysis of a mixtureof undifferentiated myoblasts and differentiated myotubes revealedhigh levels of active p38 only in myotubes (Fig. 1e). When examinedin more detail, p38 activation was found to precede the accumulationof the myogenic transcription factor myogenin (Fig. 1f), an earlydifferentiation marker in this cell system (3). Thus, p38 activationmight be functionally linked to myogenic differentiation.

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FIG. 1. p38 activity increases upon muscle differentiation prior to induction of myogenin. (a) C2C12 myoblasts were cultured in GM until they were 90 to 95% confluent and then shifted to DM. Lysates were prepared from subconfluent cells in GM or cells kept for 1 to 3 days in DM as indicated. p38 was immunoprecipitated and its activity was measured by an immune complex kinase assay (KA) using AFT2 as a substrate. The amount of p38 was assessed by immunoblotting (IB). $alpha$ -p38, anti-p38 antibody. (b) Equal amounts of whole-cell lysates were separated by SDS-PAGE in duplicate. Activation of p38 in C2C12 cell lysates was determined by immunoblotting with antibodies specific to phosphorylated and activated p38 ( $alpha$ -pP38) or total p38. (c) JNK activity and expression in C2C12 cell lysates were determined by an immune complex kinase assay using c-Jun as a substrate and by immunoblotting, respectively. $alpha$ -JNK, anti-JNK antibody. (d) Samples (30 µg) of C2C12 extracts were analyzed by immunoblotting with anti-phospho-ERK antibody ( $alpha$ -pERK). The same membrane was stripped and reprobed with antibody against total ERK ( $alpha$ -ERK) to monitor the amounts of loaded proteins. (e) A coculture of undifferentiated C2C12 myoblasts and differentiated myotubes was prepared by mixing a population of myoblasts growing in GM and myoblasts previously cultured in DM for 24 h. This mixed population was cultured in GM for 1 day. Thereafter, cells were fixed and analyzed by immunohistochemistry with antibody specific to pP38. (f) Subconfluent C2C12 cells in GM were switched to DM and were collected at the indicated times (in hours). p38 activity was examined by an immune complex kinase assay, and expression of myogenin was determined by immunoblotting. $alpha$ -Myog, anti-myogenin antibody.

Inhibition of p38 activity prevents myotube formation. To establish a causal relationship between p38 and muscle differentiation, we employed the specific inhibitor SB202190, whichfully inhibits p38 kinase activity at 5 to 10 µM without affectingJNK or ERK activities (reference 37 and our unpublished data).Instead, at concentrations higher than 20 µM, SB202190 may partiallyinhibit the activity of JNK and other protein kinases (8, 16,27). We first examined the effect of this inhibition on expressionof a luciferase reporter gene controlled by a synthetic promotercontaining four E boxes (4RE-Luc). This reporter gene is activatedonly by myogenic bHLH proteins during muscle differentiation.The ability of SB202190 to inhibit p38 activity correlated withinhibition of 4RE-Luc activity in both C2C12 myoblasts and MyoD-expressing10T1/2 fibroblasts (Fig. 2a). In both cases, reporter gene expressionwas induced by culturing cells in DM. Inhibition of p38 also preventedinduction of both early (myogenin and p21) and late (MHC) myogenicmarkers but had no significant effect on MyoD or p38 expression(Fig. 2b). Most importantly, SB202190 at 5 µM blocked formationof MHC-positive myotubes by C2C12 myoblasts placed in DM (Fig.2c, upper panels). To determine the physiological relevance ofthis effect, we examined the ability of SB202190 to inhibit myogenicdifferentiation of primary human myoblasts (satellite cells).A similar sensitivity to SB202190 was observed in these cells(Fig. 2c, lower panels) as well as in rat L6 myoblasts and MyoD-expressing10T1/2 fibroblasts (data not shown). Collectively, these dataindicate that p38 activity is necessary for activation of themyogenic differentiation program and place its site of actionat a very early step in this process, preceding the inductionof myogenin and the cell cycle inhibitor p21 (3).

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FIG. 2. p38 activity is required for myogenic differentiation. (a) The indicated cell lines were transfected with the myogenic reporter 4RE-Luc (together with MyoD in the case of 10T1/2 cells). The indicated concentrations of SB202190 (SB) were added immediately after transfection, and the cells were switched to DM for 36 h, after which they were collected to measure luciferase (Luc.) activity. (b) C2C12 cells in GM were switched to DM for 2 days with (5 µM) or without SB202190. Cell extracts were analyzed by immunoblotting for the presence of myogenic markers. $alpha$ -Myog, $alpha$ -p21, $alpha$ -MHC, $alpha$ -MyoD, and $alpha$ -p38, anti-myogenin, anti-p21, anti-MHC, anti-MyoD, and anti-p38 antibodies, respectively. (c) Subconfluent C2C12 cells or primary human myoblasts were placed in DM with (5 µM) or without SB202190. At the indicated times, cells were fixed and immunostained with anti-MHC antibody to visualize differentiated cells. C2C12 cells were examined by immunohistochemistry and bright-field microscopy, and primary human myoblasts were examined by indirect immunofluorescence.

Deliberate activation of p38 accelerates muscle differentiation. If p38 is causally involved in myogenic differentiation, then its deliberate activation should be sufficient for inductionor at least acceleration of myoblast differentiation. Therefore,we examined the effect of a constitutively active mutant of MKK6(MKK6EE), a p38-activating kinase (22, 50a ), on myogenic transcription.C2C12 or MyoD-expressing 10T1/2 cells were transfected with either4RE-Luc or a luciferase gene under the control of the muscle creatinekinase (MCK) promoter (MCK-Luc) along with expression vectorsencoding various constitutively active MKKs: MKK6EE (for p38),JNKK2CA (for JNK) (8), and MEK1DD $Delta$ N4 (for ERK) (39). Theconstitutive activities of these mutant MKKs were confirmed byboth kinase and reporter gene assays using luciferase constructsdriven by TRE- or SRE-containing promoters (data not shown). Amongthese vectors, only MKK6EE increased the activity of either the4RE-Luc or the MCK-Luc reporter in C2C12 or 10T1/2 cells in ap38-dependent manner (Fig. 3a). The response of the 4RE-Luc reporterto MKK6EE in 10T1/2 fibroblasts required the expression of MyoD,demonstrating that activation of p38 enhances myogenic transcriptionby a mechanism dependent on the presence of myogenic activators.

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FIG. 3. Deliberate p38 activation induces myotube formation and expression of muscle differentiation markers. (a) Different muscle-specific reporters (4RE-Luc or MCK-Luc) were cotransfected with expression vectors encoding activated MKKs into either C2C12 or MyoD-expressing 10T1/2 cells. After growing in GM for 1 day, cells were shifted to DM for another 36 h and then harvested to measure luciferase activity. All determinations were done in duplicate, and the data shown are representative of three independent experiments. Fold activation is the ratio of luciferase activity in MKK-transfected cells to cells transfected with the empty vector. SB, SB202190. (b) C2C12 cells in GM were cotransfected with a construct encoding a $beta$ -galactosidase protein fused to a nuclear localization signal controlled by the MLC promoter. (see the text) and either an empty vector or a JNKK2CA or MKK6EE expression vector. After 1 day in DM without or with SB202190, the cells were fixed and stained with X-Gal (5-bromo-4-chloro-3-indolyl- $beta$ -D-galactopyranoside). In MKK6EE-transfected cells cultured without SB202190, a blue color appeared 12 h earlier than in the other samples. (c) Conditions were the same as those described above except that the cells were cultured in GM after transfection. (d) Subconfluent (sub) C2C12 clones stably transfected with either an empty vector or an MKK6EE expression vector were cultured in GM. The cells were lysed at the times indicated after reaching confluence and analyzed by immunoblotting for expression of MyoD, MHC, and myogenin. $alpha$ MyoD, $alpha$ MHC, and $alpha$ -myog, anti-MyoD, anti-MHC, and anti-myogenin antibodies, respectively. (e) C2C12 cells stably expressing MKK6EE under the control of a tetracycline (Tet)-regulated promoter were cultured in GM until confluent. Tetracycline was either left in the culture medium or removed. After 48 h the cells were fixed, stained with anti-MHC antibody, and visualized by indirect immunofluorescence.

To couple activation of muscle transcription with induction of morphologic differentiation by deliberate p38 activation inmyoblasts, C2C12 cells were transfected with a constitutivelyactive MKK6EE or JNKK2CA vector together with a construct encodinga $beta$ -galactosidase protein fused to a nuclear localization signalcontrolled by the myosin light chain (MLC) promoter. Coexpressionof MKK6EE, but not JNKK2CA, enhanced the expression of $beta$ -galactosidasein the nuclei of transfected cells and accelerated the formationof multinucleated myotubes upon induction of differentiation (DM)(Fig. 3b). Both the increases in reporter gene expression andmyotube formation were prevented by SB202190. Strikingly, ectopicMKK6EE expression stimulated formation of $beta$ -galactosidase-positivemyotubes even in cells cultured in 20% FBS (Fig. 3c), which normallyinhibits in vitro myogenesis (10, 33). We further analyzedthe effect of deliberate p38 activation on muscle differentiationby establishing stable C2C12 clones that constitutively expressMKK6EE (MKK6EE/C2). These cells expressed higher basal levelsof MyoD than those of vector-transfected cells during logarithmicgrowth (Fig. 3d) and exhibited faster and more pronounced inductionof myogenin and MHC expression after reaching confluence (Fig.3d). Formation of MHC-positive myotubes by postconfluent MKK6EE/C2cells was inhibited by SB202190 (data not shown), supporting thenotion that p38 activation accelerates myogenic differentiation.We also generated stably transfected C2C12 derivatives in whichMKK6EE expression was controlled by a tetracycline-regulated system(47). Removal of the antibiotic resulted in MKK6EE inductionand p38 activation (data not shown) and caused the appearanceof multinucleated MHC-positive myotubes even in cells culturedin the presence of 20% FBS (Fig. 3e). These MKK6EE-induced C2C12myotubes formed in the presence of serum were functionally indistinguishablefrom those formed by normal C2C12 in DM, as determined by theenzymatic activity of MCK (data not shown). Therefore, deliberatep38 activation is sufficient for triggering myogenic differentiationin serum-fed proliferatingmyoblasts.

Activation of MEF2A and MEF2C transcriptional activity by p38 through direct phosphorylation. The results presented above suggest that p38 may directly or indirectly potentiate the activities of myogenic transcriptionfactors. It has previously been shown that p38 phosphorylatesMEF2C in lymphocytes, leading to its activation in response toendotoxin (21). Furthermore, p38 has been reported to phosphorylateother MEF2 family members (40, 61, 67). Despite their ubiquitousexpression (except for MEF2C, which is expressed only in brain,skeletal muscle, and spleen) (42), MEF2 proteins play criticalroles in myogenesis in both invertebrates and vertebrates (7).We examined the effect of p38 activation on the transcriptionalactivities of fusion proteins that contain the Gal4 DNA bindingdomain and MEF2-derived activation domains. MKK6EE enhanced thetranscriptional activities of Gal4-MEF2A and Gal4-MEF2C, and thateffect was blocked by SB202190 (Fig. 4a). Previous studies haveidentified threonines 312 and 319 in MEF2A and threonines 293,300, and serine 387 in MEF2C as targets for p38-mediated phosphorylationin certain cellular systems (21, 48, 67). The replacementof threonines 312 and 319 with alanines in MEF2A abrogated theactivation by MKK6EE. With MEF2C, we found that a single aminoacid substitution (Thr293 to Ala) was sufficient to abolish thestimulatory effect of MKK6EE on Gal4-MEF2C (Fig. 4a). Other mutationsof potential p38 phosphorylation sites that did not involve Thr293failed to abrogate the positive effect of MKK6EE (data not shown).Metabolic labeling with ³²P in C2C12 cells indicated that coexpression of MKK6EE stimulatedthe in vivo phosphorylation of wild-type Gal4-MEF2C and that thisenhancement in phosphorylation was blocked by SB202190 (Fig. 4b).In contrast, MKK6EE had no effect on phosphorylation of a Gal4-MEF2Cmutant (T293A) (Fig. 4b). These results suggest that the phosphorylationpattern of MEF2C by p38 during muscle differentiation differsfrom that found in other cellular systems (i.e., lymphoid cells)in which three residues are simultaneously phosphorylated (21).To further clarify the issue, we carried out a ³²P metabolic labeling experiment with C2C12 cells and isolatedendogenous MEF2C from either myoblasts or myotubes that were incubatedwith or without SB202190. When subjected to two-dimensional phosphopeptidemapping, only one tryptic phosphopeptide that is specific to myotubesand that contains Thr293 and -300 was detectable and its appearancewas reduced by SB202190 (Fig. 4c, upper panels). In contrast,two p38-inducible tryptic phosphopeptides (one containing bothThr293 and Thr300 and the other containing Ser387) have been detectedin lymphoid cells treated with lipopolysaccharide (21). To confirmthat the inducible phosphorylation site on MEF2C during muscledifferentiation is T293, Flag-tagged wild-type, and mutant MEF2C(T293A) were immunoprecipitated from ³²P-labeled myotubes and subjected to tryptic phosphopeptide mapping.As shown in Fig. 4c (lower panels), the myotube-specific phosphopeptideseen in wild-type MEF2C was completely absent in MEF2C (T293A).It should be noted that in both the experiments with exogenousand endogenous MEF2C, other constitutive phosphopeptides detectedby the mapping were not modified by changing the culture conditions,by SB treatment, or by threonine-to-alanine mutation. Collectively,these results support the concept that p38 kinase targets MEF2Cat a unique site (Thr293), whose phosphorylation is required tostimulate MEF2-dependent transcription during muscle differentiation.

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FIG. 4. p38 phosphorylates MEF2C and increases its transcriptional activity during muscle differentiation. (a) 10T1/2 cells were cotransfected with a Gal4-Luc reporter and expression vectors for wild type (wt) and mutant (mt) Gal4-MEF2 fusion proteins [MEF2A(A312/A319) and MEF2C(A293)] along with either an empty vector or an MKK6EE expression vector. Fold activation is the ratio of the luciferase activity in cells transfected with the activator (Gal4-MEF2) to that of cells transfected with the reporter but no activators. The data are representative of three independent experiments. SB, SB202190. (b) C2C12 cells were transfected with either wild-type or mutant Gal4-MEF2C vectors along with either an empty vector or an MKK6EE expression vector. After in vivo labeling with ³²P, Gal4-MEF2C was immunoprecipitated, separated by SDS-PAGE, and visualized by autoradiography. The level of Gal4-MEF2C expression was determined by immunoblotting (IB) with anti-Gal4 antibody ( $alpha$ -gal4). (c, upper panels) C2C12 cells kept in either GM or DM (2 days) were metabolically labeled with ³²P in the absence or presence of SB202190 as indicated. Endogenous MEF2C was immunoprecipitated, the immune complexes were separated by SDS-PAGE, and the MEF2C band was excised and analyzed by two-dimensional tryptic phosphopeptide mapping. (lower panels), M2-tagged wild-type MEF2C or mutant MEF2C(A293) were transfected into C2C12 cells and were kept in DM for 2 days before being subjected to metabolic labeling as described for panel a. Tagged MEF2C proteins were immunoprecipitated and subjected to two-dimensional mapping. o, the origin of the chromatogram. The phosphopeptide containing T293 is indicated by an arrow.

p38 is an essential activator of MyoD-dependent gene transcription. Since p38 activation can stimulate the activity of a promoter containing only E boxes (Fig. 2a and 3a) and lead to the inductionof p21 (Fig. 2c), whose transcription is regulated by MyoD inmuscle cells (19, 20, 49, 66), we conceived that myogenicbHLH factors may also be potential targets for p38. Consistentwith this hypothesis, expression of MKK6EE enhanced MyoD-dependenttransactivation of a luciferase reporter driven by either fourE boxes (4RE-Luc) in 10T1/2 fibroblasts (data not shown) or avariant p21 promoter (p21-Luc) that lacks its p53 binding sitesin C2C12 cells (Fig. 5a). Under these conditions, the p21 promoteris mostly responsive to MyoD (19, 20). The ectopic expressionof MKK6EE did not change the protein levels of MyoD (Fig. 5a,bottom panel) and its effect on the activation of p21-Luc wasinhibited by SB202190 (Fig. 5a). To more directly assess the effectof p38 activation on MyoD transcriptional activity, we examinedits effect on Gal4-MyoD fusion proteins. MKK6EE enhanced the transcriptionalactivity of Gal4-MyoD in a p38-dependent manner (Fig. 5b), withoutchanging the Gal4-MyoD levels (Fig. 5b, bottom panel). As a control,the low basal activity of a mutant containing only the bHLH regionof MyoD was not stimulated by MKK6EE (data not shown). A MyoDmutant whose basic region was replaced by that of the DrosophilabHLH protein Achaete-scute (58) could still be stimulated byMKK6EE, an effect abrogated by SB202190 treatment (Fig. 5b). Thisfinding ruled out the possibility that the activation of MyoDby MKK6EE was mediated through interactions with p38-phosphorylatedMEF2 proteins, as it was demonstrated that MyoD without its ownbasic region does not associate with MEF2 proteins (6). Consistently,physical interactions between MyoD and MEF2C, as detected by amammalian two-hybrid system, were not influenced by either MKK6EEcotransfection, SB202190 treatment, or mutation of threonine 293in MEF2C (P. L. Puri and Z. Wu, unpublished results). These dataalso indicate that p38 regulates MyoD function through eitherthe N-terminal or the C-terminal domain of MyoD, or both. Thesetwo domains have been previously shown to be capable of activatinggene transcription in repressive chromatin by stimulating chromatinremodeling at binding sites in muscle gene enhancers (17a). Thisactivity is blocked by antimyogenic factors, such as bFGF (17b,23). To test whether p38 could stimulate MyoD-mediated chromatinremodeling, we carried out a set of experiments with 3T3 fibroblastscontaining a chromosome-integrated MyoD-dependent reporter (4RE-Lucintegrated). MyoD activates this integrated reporter (chromosomaltemplate) with a lower efficiency than that of the same reportertransiently transfected (extrachromosomal template) (data notshown). Exposure to bFGF, which blocks MyoD-mediated chromatinremodeling (17a) abrogated the activation of the chromosomaltemplate by MyoD (Fig. 5c). Inhibition of p38 by SB202190 resultedin a similar repression of this reporter (Fig. 5c). Importantly,activation of p38 by MKK6EE enhanced MyoD-dependent activationof chromosomal 4RE-Luc and partially counteracted the repressiveeffect exerted by bFGF on the same template (Fig. 5c). These resultsled to the speculations that p38 may stimulate myogenic transcriptionby enhancing the chromatin remodeling activity of MyoD and thatit might bypass inhibitory signals (i.e., bFGF), which block thisactivity.

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FIG. 5. p38 activation enhances MyoD transcriptional activity. (a) A p21-Luc reporter lacking p53 binding sites was transfected into C2C12 cells along with either an empty vector or an MKK6EE expression vector in the presence or absence of SB202190 (SB) as indicated. After growing in GM for 1 day, cells were shifted to DM for another 36 h and then harvested to measure luciferase activity. Fold activation is the luciferase activity in MKK6EE-transfected cells relative to that in empty-vector-transfected cells. The levels of endogenous MyoD in each sample were monitored by Western blotting using the monoclonal MyoD antibody (MyoD) 5.8 and are presented in the gel below the graph. (b) A Gal4-Luc reporter and various Gal4-MyoD activator constructs (galMyoD) (58) were cotransfected into C2C12 cells along with either an empty vector or an MKK6EE expression vector. After growing in GM for 1 day, cells were shifted to DM for another 36 h and then harvested to measure luciferase activity. galMyoD(AS), Gal4 DNA binding domain fused to a mutant MyoD whose basic region is replaced by that of the Drosophila bHLH protein Achaete-scute. The levels of wild-type galMyoD and galMyoD(AS) proteins were monitored by Western blotting using antibody against Gal4 and are presented in the gel below the graph. The sample order in the Western blot is the same as that in the bar graph. gal4, anti-Gal4 antibody. (c) 3T3 clones with a chromosome-integrated MyoD-responsive reporter (3T3 4RE-Luc) were transfected with the indicated plasmids. After growing in GM for 1 day, cells were shifted to DM, in the presence or absence of bFGF (25 ng/ml) and SB202190, for an additional 36 h and then harvested to measure luciferase activity. All transfections and measurements were done in duplicate, and the results shown are representative of two independent experiments.

The molecular mechanism by which p38 stimulates MyoD transcriptional activity remains unclear. Although MyoD itself is a directtarget for p38-mediated phosphorylation in vitro, mutation ofa proline-directed serine (Ser5), which is in vivo phosphorylatedin MKK6EE-induced myotubes, failed to abolish the stimulatoryeffect of MKK6EE on MyoD activity (P. J. Woodring, Z. Wu, andP. L. Puri, unpublished results). Thus, the regulatory functionof this phosphorylation is not clear and p38 is rather likelyto activate MyoD-dependent transcription by an indirectmechanism(s).

p38 $alpha$ and - $beta$ isoforms are the main activators of the myogenic program. The repression of myogenic differentiation by SB202190, which selectively inhibits the p38 $alpha$ and - $beta$ kinases, suggests a specificrole of these two isoforms in regulating myogenic differentiation.We have observed that transient overexpression of p38 $alpha$ and - $beta$ isoforms can increase the activation of the muscle-specific reportergene by MyoD (data not shown). The availability of embryonic fibroblastsderived from p38 $alpha$ ^/ embryos allowed us to test the importance of p38 $alpha$ in the activationof the myogenic program. We compared the extents of myogenic conversionby ectopic expression of MyoD in mEFs derived from p38 $alpha$ ^/ and p38 $alpha$ wild-type embryos. In the absence of p38 $alpha$ , the efficiencyof MyoD-dependent conversion was reduced by about 45%, as judgedby the formation of MHC-positive myotubes (Table 1). Reintroductionof p38 $alpha$ by transient transfection completely restored the activationof MyoD-dependent transcription in p38 $alpha$ ^/ mEFs (Table 1). These results demonstrate that p38 $alpha$ plays animportant role in the activation of MyoD-dependent transcription.The presence of p38 $beta$ might account for the residual activationof the myogenic program in the absence of p38 $alpha$ . Interestingly,we have observed that p38 $beta$ can functionally replace p38 $alpha$ , sincethe overexpression of the p38 $beta$ isoform, but not of the p38 $gamma$ and- $delta$ isoforms, could restore the MyoD-dependent myogenic conversionin p38 $alpha$ ^/ mEFs (Z. Wu and P. L. Puri, unpublished observations). Althoughthe specific role of p38 $alpha$ and - $beta$ remains to be defined, it istempting for us to speculate that these two isoforms might exerta redundant function in activating the myogenic program.

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TABLE 1. Extents of ectopic expression of MyoD in mEFs derived from p38 $alpha$ ^/ and wild-type p38 $alpha$ embryos^a

p38 acts in parallel with the IGF-PI3K pathway. One exogenous factor that can stimulate muscle differentiation is IGF. The activities of IGF1 and IGF2 are transduced mostlythrough the PI3K-Akt (PKB) signaling pathway (11, 28, 29).We set out to investigate whether p38 MAPKs might function downstreamof the IGF-PI3K-Akt pathway during muscle differentiation. Thisissue is pertinent because PI3K was shown to cause activationof the related JNK MAPK cascade in other cell systems (52) andcan therefore also contribute to the activation of p38 MAPKs inmuscle cells. As shown in Fig. 6a, the fold increases and thekinetics of p38 activation during muscle differentiation werevery similar in the absence and presence of IGF1, although theextent of differentiation was dramatically increased in the presenceof IGF1 (Fig. 6b). Furthermore, the addition of 10 µM SB202190severely blocked both C2C12 and L6 (data not shown) differentiationinduced by IGF, without affecting the integrity of the IGF-PI3K-Aktpathway as measured by Akt phosphorylation (Fig. 6b and c). Asa control, the addition of 25 µM PD98059 or 10 ng of rapamycinper ml did not inhibit the stimulation of Akt phosphorylationby IGF1, while the addition of 25 µM LY294002, a specific inhibitorof PI3K (57), abolished IGF1-induced Akt phosphorylation (Fig.6c). We also examined whether p38 activation has any effect onAkt phosphorylation using the MKK6EE/C2 stable cell line, andno measurable effect was detected (data not shown). Furthermore,the specific PI3K inhibitor LY294002 inhibited MKK6EE-induceddifferentiation without affecting p38 kinase activity in thesecells (Fig. 7). As a control, PD98059 and rapamycin did not inhibitMKK6EE-mediated p38 activation (Fig. 7b). These results stronglysuggest that the p38 MAPKs and the IGF-PI3K-Akt signaling pathwaysare independent but that they operate in parallel to stimulatemyogenic differentiation. Inhibition of either pathway resultsin the abrogation of the myogenic program.

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FIG. 6. Inhibition of p38 blocks IGF-induced myogenic differentiation without affecting the IGF-PI3K-Akt pathway. Nearly confluent C2C12 cells were shifted to serum-free medium in either the absence or presence of IGF1 (50 µg/ml). (a) Cells were harvested at the indicated times, and 100-µg samples of cell lysates were used for a p38 immune complex kinase assay (KA) using AFT2 as a substrate. The level of p38 was determined by immunoblotting (IB) with anti-p38 antibody ( $alpha$ -p38). (b) C2C12 cells were cultured in serum-free medium without or with IGF1 (50 ng/ml). One of the cultures was also treated with SB202190, as indicated. Cells were fixed 24 h after treatment and subjected to immunofluorescence analysis with anti-MHC antibody. (c) Cells were either left untreated or pretreated with different kinase inhibitors for 30 min before IGF1 was added. Whole-cell extracts were analyzed by immunoblotting with antibodies against phospho-Akt (p-Akt) or $alpha$ -actin. NT, nontreated; SF, serum free; SB, SB202190 (10 µM); PD, PD98059 (25 µM); LY, LY294002 (25 µM); Rapa, rapamycin (10 ng/ml).

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FIG. 7. Inhibition of PI3K blocks MKK6EE-induced myogenic differentiation without affecting p38 activity. Tetracycline (Tet)-inducible MKK6EE/C2 cells were cultured in the presence of tetracycline (2 µg/ml) until they were 70% confluent. Tetracycline was then removed to induce MKK6EE expression. Cells were cultured in tetracycline-free medium for 24 h and then shifted to DM. (a) Cells were treated with either the vehicle (dimethyl sulfoxide) or different kinase inhibitors for 36 h in DM. (b) Whole-cell extracts were analyzed by immunoblotting with antibodies against phospho-p38 (p-p38) and total p38. The final concentrations of inhibitors used were 10 µM for SB202190, 25 µM for PD98059 (PD), 25 µM for LY294002 (LY), and 10 ng/ml for rapamycin (Rapa). NT, nontreated.

Dual role of ERK activity during C2C12 myogenic differentiation. Several investigators have reported that the ERK group of MAPKs also plays a role in muscle differentiation. While some investigatorsindicated that ERK members inhibit differentiation (5, 11),one report indicated that ERKs are positive regulators of myogenesis(18). Our own observations of biphasic regulation of ERK activityduring myogenic differentiation (Fig. 1d) suggest that the ERKpathway may play a dual role in this process. To examine thispossibility, we generated an inducible C2 stable cell line overexpressinga constitutively active mutant of MEK1 (MEK1CA or MEK1DD/ $Delta$ N4)(39), a specific activator of the ERK1 and -2. As in the caseof MKK6EE, we used the tetracycline system to achieve regulatedMEK1CA expression and confirmed that its induction leads to specificactivation of ERKs but not of p38 or JNK (data not shown). Weobserved that, when induced to differentiate by serum withdrawal,this stable cell line initially lagged behind vector-transfectedcells in the formation of MHC-positive myotubes (Fig. 8a, day1, middle panel). Consistently, forced activation of endogenousERKs by transient expression of its activator, MEK1CA, reducedthe activation of myogenic reporters in both C2C12 cells and 10T1/2fibroblasts converted by MyoD (Fig. 3a). However, after a fewdays of lagging behind their wild-type counterparts in MHC expression,MEK1CA/C2 cells started to form multinucleated myotubes largerthan those in vector-transfected cells (Fig. 8a, day 4, middlepanel). In a distinct experiment, continuous treatment of eithervector-transfected C2C12 cells or MEK1CA/C2 cells with PD98059,a specific inhibitor of MEK1 and -2 (15), initially (day 1 ofgrowth in DM) increased the number of MHC-positive myocytes. However,continuous exposure to PD98059 for 3 days resulted in a reducednumber of mature multinucleated myotubes (data not shown), inagreement with a previous report (5). Thus, ectopic activationof ERK, while initially interfering with terminal differentiation,eventually enhances the formation of multinucleated myotubes atlate stages of differentiation. We also tested whether inhibitionof one MAPK pathway could interfere with the differentiation programmediated by another MAPK. As shown in Fig. 8b, we found that treatmentwith SB202190 inhibited late myotube formation in MEK1CA/C2 cells.Treatment with PD98059 also reduced myotube formation in the C2cell line expressing MKK6EE, albeit to a lesser extent (Fig. 8b).Furthermore, we tested the effect of either the p38 or ERK inhibitorin preformed multinucleated myotubes. Figure 8c shows that myotubescontinuously exposed to either SB202190 or PD98059 displayed areduced size, collapsed, and became round. These results collectivelyindicate that activation of both the p38 and ERK pathways is requiredfor optimal differentiation and myotube survival. Also, theseresults suggest that the ERK pathway may play opposite roles inthe regulation of myogenic transcription, depending on the particularstage of the myogenic program. We directly tested this hypothesisby investigating the effect of ERK activation on a myogenic reporterin undifferentiated versus differentiated muscle cells. Towardthis aim, we used the MEK1CA/C2 cell line, in which the ERK pathwaycan be ectopically stimulated by inducing MEK1CA expression throughtetracycline withdrawal. These cells were transfected with thep21 promoter lacking the p53 binding sites, which is regulatedby MyoD in muscle cells and has been reported to be responsiveto ERK in other cell types (4a, 38a). The expression of thisreporter was reduced by MEK1CA activation in myoblasts inducedto differentiate, and the effect was reversed by PD98059 treatment(Fig. 8d). In contrast, deliberate activation of ERK in formedmyotubes, as achieved by tetracycline removal from the medium,increased the expression of the p21 promoter. Again, exposureto PD98059 abrogated this response (Fig. 8d). It is interestingthat the activation of ERK is reminiscent of the effect of serum,which is inhibitory toward myogenic differentiation in myoblastsbut which stimulates myogenic transcription in myotubes (P. L.Puri, unpublished results). This consideration prompted us toinvestigate whether the ERK pathway is also involved in growthfactor-induced hypertrophy of terminally differentiated myotubes(50a). As already reported (52a), ERK activity can be stimulatedabout twofold by growth factors in myotubes contained in serum(data not shown). The stimulation of ERK activity was accompaniedby an evident increase in the sizes of exposed myotubes (Fig.8e, middle panel), which reflects the hypertrophic response ofthese cells. Inhibition of ERK by exposure to PD98059 completelyabrogated serum-induced myotube hypertrophy (Fig. 8e, right panel),indicating an essential role of the ERK pathway in this process.Interestingly, treatment with SB202190 also inhibited both serum-dependentand MEK1-mediated hypertrophy of myotubes (P. L. Puri, unpublishedresults). These results implicate ERK and p38 kinases as componentsof a pathway which regulates postmitotic growth of terminallydifferentiated muscle cells.

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FIG. 8. Dual roles of ERK during myogenesis. (a) Nearly confluent C2C12 cells stably transfected with either an empty vector, an MEK1(CA) expression vector, or an MKK6EE expression vector were first induced by tetracycline removal from the culture medium for 1 day and then shifted to DM for various times as indicated. Cells were fixed and stained for the expression of MHC. (b) Conditions were the same as those described for panel a except that SB202190 (final concentration, 10 µM) was added to MEK1CA/C2 cells and PD98059 (final concentration, 25 µM) was added to MKK6EE/C2 cells at the time when cells were shifted to DM and inhibitors were kept for 4 days. Culture medium was replaced every 24 h with freshly added inhibitors. (c) C2C12 myotubes were exposed to either SB202190 (final concentration, 10 µM) or PD98059 (final concentration, 25 µM) for 36 h and then fixed and stained for the expression of MHC. (d) The MEK1CA/C2 cell line was transfected with the p53-site-deleted p21-Luc reporter. The ERK pathway was either stimulated by tetracycline removal or inhibited by PD98059 treatment of myoblasts (MEK1CA/C2 Mb) induced to differentiate by being cultured in DM and of myotubes (MEK1CA/C2 MT). Cells were harvested to measure luciferase activity. All determinations were done in duplicate, and the data shown are representative of three independent experiments. Fold activation is the ratio of luciferase activity in MKK-transfected cells to cells transfected with an empty vector. (e) C2C12 cells were allowed to differentiate into multinucleated myotubes by culturing them in DM for 3 days (left panel) and then restimulated by 20% FBS in the absence (middle image) or in the presence (right panel) of the ERK inhibitor PD98059. Cells were fixed at the indicated times and examined for MHC expression by indirect immunofluorescence. DM $right-arrow$ GM, serum restimulation.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Selective activation of the p38 pathway during muscle differentiation. The results described above illustrate a pathway by which extracellular factors can modulate myogenesis through activationof distinct MAPKs. p38 activation in muscle cells placed in DMdisplays features (i.e., persistent activation in the absenceof parallel JNK stimulation) which distinguish this pathway fromthose activated in response to stress or cytokines. Since p38is activated in muscle cells upon serum removal, it may be a partof a regulatory circuit by which serum growth factors silencethe myogenic program in proliferating myoblasts. We have observedthat serum starvation of confluent cells results in p38 activationalso in 10T1/2 and NIH 3T3 fibroblasts (Z. Wu and P. L. Puri,unpublished data). However, only transient activation of p38 wasobserved in these cells in response to serum withdrawal. In contrast,fibroblasts stably expressing MyoD display an activation of p38that persists along the whole process of myogenic conversion (Z.Wu and P. L. Puri, unpublished data), implicating a role for MyoD(or MyoD-dependent genes) in maintaining p38 activation in myogeniccells. This observation suggests the possible existence of a positivefeedback between p38 and MyoD during the differentiationprogram.

At present we do not know the signal that triggers p38 activation in myogenic cells placed in DM. It is possible that p38activity is mostly under a negative control factor in proliferatingmyogenic progenitors. Serum withdrawal and/or cell-to-cell contactmay stimulate the p38 pathway by silencing the activity of a mitogen-dependentfactor (e.g., a phosphatase). However, the findings that deliberatep38 activation overcomes the inhibitory effect of serum on muscledifferentiation and stimulates myotube formation in the presenceof mitogens also raise the possibility that the p38 pathway maybe directly triggered by positive regulators of myogenesis thatremain to be identified. In this regard, we have observed thatIGF, which is known to stimulate muscle differentiation, doesnot activate the p38 cascade in muscle cells (Fig. 6a). Nevertheless,other upstream signaling molecules reported to stimulate myogenesis(e.g., the transmembrane protein CDO) (31a) may be implicatedin the activation of the p38 pathway. With respect to this, ithas been observed that the p38 pathway is more efficiently activatedin confluent muscle cells placed in DM than in subconfluent myocytescultured under the same conditions (P. L. Puri, unpublished results).This observation underscores the importance of cell density inthe activation of p38 during muscledifferentiation.

p38 MAPKs positively regulate myogenesis through MyoD and MEF2 proteins. Once activated, p38 can phosphorylate and stimulate the activities of MEF2C and MEF2A (our data and references 21, 48,61, and 67). Given the essential function of MEF2 proteinsin muscle differentiation (7), the enhancement of their transcriptionalactivities by p38-mediated phosphorylation should result in activationof many myogenesis effector genes. While this work was in preparation,others reported that p38 MAPKs are required for myogenic differentiationof rat L8 and mouse C2C12 cells, respectively (12, 64). However,these conclusions rested mainly on the use of p38 inhibitors anddo not provide insight into the mechanisms that underlie p38-dependentactivation of the myogenic program. Although MEF2C and -A wereshown to be p38 targets in nonmuscle cells as well as in musclecells (21, 48, 61, 64), it was not demonstrated that endogenousMEF2C is actually phosphorylated by p38 in differentiating myoblasts.We therefore carried out a detailed mapping of the phosphorylationsites relevant to MEF2C activation during myogenesis. It has beenpreviously shown that p38 can phosphorylate MEF2C on three residues(T293, T300, and S387) located in the activation domain (21,61, 67). The simultaneous phosphorylation of these residuesis important for MEF2C activation in nonmuscle cells (e.g., lymphoidcells) (21). The results presented in Fig. 4 indicate that thephosphorylation of threonine 293 is critical for the activationof MEF2C transcriptional function in muscle cells, suggestingthat MEF2C regulation by p38 kinases occurs through selectivephosphorylation at distinct residues in a tissue-restricted manner.MEF2 proteins affect muscle differentiation through synergisticinteractions with myogenic bHLH factors (45). This raises thepossibility that p38-mediated phosphorylation of MEF2 membersmay enhance the transcriptional synergy between MyoD and MEF2.Our data argue against this possibility, since we failed to detectany effect of p38 on MEF2C-MyoD interactions using a mammaliantwo-hybrid system (P. L. Puri and Z. Wu, unpublished data). Inaddition, we and others (47a) have observed that mutation ofthreonine 293 to alanine, which prevents in vivo p38-mediatedphosphorylation and activation of MEF2C, does not affect MyoD-MEF2Cfunctional synergism (P. L. Puri and Z. Wu, unpublished results).Finally, a Gal4-MyoD fusion protein without the basic domain andtherefore impaired in associating with MEF2 proteins is stillactivated by MKK6EE. However, it is still formally possible thatp38 stimulates bHLH-MEF2 functional synergism by an alternativemechanism, since a functional collaboration between MyoD and MEF2Chas been reported also in the absence of their physical interaction(47a). In agreement with our results, Novitch et al. reportedthat the mutation of serine 387 to alanine does not affect thetranscriptional activation of MEF2C by p38 kinase (47a). Moreover,they observed that this mutation abrogates the enhancement ofMEF2C activity by MyoD (47a). This finding suggests that stimulationof the intrinsic transcriptional activity of MEF2C and inductionof functional synergism between MEF2C and MyoD may be two separateprocesses controlled by distinct mechanisms. It is possible that,in muscle cells, p38-mediated phosphorylation of threonine 293is important for induction of MEF2C intrinsic transcriptionalactivity but that phosphorylation of serine 387, which might notbe mediated by p38, can be a signal required for functional synergismwith myogenic bHLHfactors.

The observation that the p38 pathway is essential for activation of both the MyoD-dependent promoter and the MyoD-mediatedconversion of fibroblasts into myogenic cells suggests the possibilitythat MyoD might also be a target of p38. Due to the use of a weakp38 activator (the wild-type MKK6 construct), previous works failedto detect a p38-mediated enhancement of MyoD transcriptional activity(64). By using the constitutive activated p38 activator MKK6EE,we could consistently detect a positive effect of p38 on severalMyoD-responsive reporters (Fig. 3a and 5). As discussed above,it is unlikely that the stimulatory effect of MKK6EE on MyoD ismediated through physical interactions with MEF2 proteins. Experimentscarried out with reporter cell lines and chromatin-integratedMyoD-responsive templates suggest that p38 might stimulate MyoD-dependentchromatin remodeling. Although we have observed efficient phosphorylationof MyoD by p38 in vitro and we have detected a p38-dependent phosphorylationof serine 5 at the N terminus of MyoD during myotube formation(P. J. Woodring, Z. Wu, and P. L. Puri, unpublished results),the replacement of this serine with an alanine did not significantlyalter MyoD transcriptional activity. Thus, it is likely that p38stimulates MyoD-dependent transcription by an indirect mechanism.Consistent with this, it has been observed that the activitiesof other myogenic bHLH proteins, which do not share in vitro putativep38 phosphorylation sites (like serine 5 in MyoD), can also bestimulated by MKK6EE (P. L. Puri, unpublished results). This mayalso explain the functional relevance of the p38 pathway in musclecell lines deficient in MyoD expression, like rat L6 myoblasts(64). One possibility is that p38 indirectly stimulates myogenictranscription by targeting bHLH transcriptional coactivators,such as p300 and PCAF (50, 53).

As there are four p38 isoforms encoded by separate genes, another relevant question is which of the four isozymes is involvedin myogenic activation. Since SB202190 inhibits only p38 $alpha$ andp38 $beta$ (37), it is likely that one or both of these isozymes maybe involved in myogenic differentiation. Congruently, transientoverexpression of either isozyme leads to activation of muscle-specificreporter genes (Z. Wu and P. L. Puri, unpublished data). Althoughthe p38 $gamma$ isozyme was reported to be expressed exclusively in skeletalmuscle (36), it is insensitive to SB202190 and therefore isan unlikely major mediator of the stimulatory effect of MKK6 inmuscle cells. Similar arguments can be made against p38 $delta$ . In accordancewith that, overexpression of either the p38 $gamma$ or p38 $delta$ isoform didnot enhance myogenic transcription (Z. Wu and P. L. Puri, unpublisheddata). Genetic evidence provided by experiments performed withp38 $alpha$ ^/ mEFs demonstrates that in the absence of p38 $alpha$ the ability ofMyoD to activate the myogenic program in cultured nonmuscle cellsis reduced and that reexpression of p38 $alpha$ may restore this activity.While these results indicate an essential role for p38 $alpha$ in promotingMyoD-dependent myogenic conversion of fibroblasts, the presenceof p38 $beta$ might account for the residual activation of the myogenicprogram in the absence of p38 $alpha$ and can explain the lack of anapparent muscle phenotype in p38 knockout mice (K. Tamura andM. Karin, unpublished data). In agreement with this, it was recentlyshown that both p38 $alpha$ and p38 $beta$ phosphorylate MEF2C and MEF2A andenhance their transcriptional activities. In contrast, p38 $gamma$ onlyweakly phosphorylates MEF2A and MEF2C in vitro and barely stimulatestheir transcriptional activities in vivo while p38 $delta$ does not phosphorylateMEF2A or MEF2C at all (61, 65). These results suggest thatthe different p38 isoforms may have their own preferred substrates,as previously reported for different isoforms of JNK (31).

The MKK6-p38 pathway and IGF-regulated signaling are two parallel cascades involved in myogenesis. IGFs are the only peptide hormones known to induce myogenic differentiation in mammalian systems (11). We investigated whetherp38 could be an effector of IGF's myogenic activity. Such a relationshipseemed reasonable, because PI3K, whose activity is strongly stimulatedby IGF (60), was previously shown to lead to activation of JNK(52), whose activity is usually regulated similarly to thatof p38 (43). Much to our surprise, activation of p38 duringmuscle differentiation was independent of IGF action (Fig. 6a).Furthermore, p38 activation had no effect on Akt activity, animportant component of the IGF-PI3K signaling pathway. Nevertheless,specific inhibition of p38 with SB202190 blocked the myogeniceffect of IGF1 in both mouse C2C12 cells and rat L6 cells, withoutinterfering with activation of Akt. Recently, ectopic expressionof Akt was found to stimulate myogenic differentiation (17,28). Accordingly, a constitutively activated form of PI3K enhancesboth MyoD- and MEF2-dependent transcription (Z. Wu, unpublishedresults). Specific inhibition of PI3K by LY294002 abrogated myogenicdifferentiation not only in response to IGF1 but also in responseto MKK6EE, without severely affecting p38 activation (Fig. 7).Taken together, these results indicate that these two signalingpathways must act in parallel and that both are absolutely requiredfor myogenic differentiation, at least in culturedcells.

Another target for IGF-PI3K signaling is the p70 S6 kinase (p70S6K) (10, 46a, 56). A specific inhibitor of IGF- and PI3K-mediatedp70S6K activation is rapamycin (13). As rapamycin was foundto inhibit myogenic differentiation, p70S6K is another proteinkinase implicated in the control of myogenesis (11, 12). Therelationship between Akt and p70S6K in PI3K signaling is stillnot clear. Our results suggest that p70S6K acts either downstreamof Akt or in a parallel branch downstream of PI3K, because IGFinduced Akt phosphorylation was not inhibited by rapamycin (Fig.6c). Interestingly, rapamycin also blocked MKK6EE-mediated myogenicdifferentiation (unpublished data) without affecting p38 activity.Thus, IGF may stimulate myogenesis via either one linear PI3K-to-Akt-to-p70S6Kpathway or via a branched pathway in which Akt and p70S6K bothserve essential functions downstream of PI3K. Although these pathwayshave no effect on p38 activity, they are also required for inductionof differentiation in response to MKK6EE expression. One interestingquestion that remains to be answered is whether the signals fromthe two pathways converge on the same or differenttargets.

Dual role of ERK during the myogenic program. The ERK pathway has also been implicated in the control of myogenesis, but its functions seem to be controversial, as somereports have proposed an inhibitory role at the beginning of themyogenic program (5, 11) while another report proposed apositive regulatory function (18). We were able to unify theseseemingly conflicting results by demonstrating that ERK activityis subject to biphasic regulation and has a dual function duringmyogenesis. The concomitant decline in ERK activity and stimulationof p38 kinase during the early phase of terminal differentiationmay facilitate a reduction in cyclin D1 levels (5, 35), therebyleading to activation of MyoD (54, 65), followed by the inductionof myogenic markers, including p21. The combined effects of cyclinD1 downregulation and p21 upregulation contribute to the permanentwithdrawal of myoblasts from the cell cycle. Forced ERK activationat this stage, as achieved by using a constitutively active MEK1mutant, interferes with initiation of the differentiation program.During later stages of myogenic differentiation, ERK activityincreases and seems to cooperate with p38 in promoting differentiationand/or myotube fusion. This explains why prolonged inactivationof ERK either by PD98059 (data not shown and reference 18) orby overexpression of the dual-specificity phosphatase MKP-1 (5)prevents formation of mature myotubes. Furthermore, results presentedin Fig. 8 implicate ERK and p38 in the process of myotube survivaland in the hypertrophic growth of myotubes following growth factorstimulation. These results illustrate a multistep regulation ofthe myogenic program by p38 and ERK, with p38 being an essentialactivator of myogenic transcription and ERK exerting two oppositefunctions depending on the stage of the differentiation program.In proliferating myoblasts, the ERK pathway represses myogenictranscription and contributes to the maintenance of the undifferentiatedphenotype. The reduction of ERK activity upon serum removal cantherefore relieve that repression and allow p38-mediated muscle-specifictranscription. Once the activation of the myogenic program isinitiated, ERK activation is no longer repressive and cooperateswith p38 in promoting postmitotic responses in differentiatedmyotubes. It is therefore likely that the antimyogenic functionof ERK depends on its mitogenic potential in undifferentiatedmyoblasts. After the acquisition of their postmitotic state, myotubesbecome refractory to the mitogenic activity of ERK and the ERKpathway is converted into a promyogenic one. At the stage of multinucleatedmyotubes, ERK activation by serum contributes to p21 activation(Fig. 8d), and this can be important in rendering myotubes refractoryto mitogenic stimuli. Remarkably, a dual function has also beendescribed for IGF1 (15a). Sarbassov et al. have reported theability of IGFs to activate ERKs in muscle cells (52a). SinceIGFs are secreted by muscle cells in culture, the ERK pathwaymust be an important mediator of such an autocrine loop, whichregulates myogenic differentiation and myocyte hypertrophy (46).

The results presented here may have biological implications in therapeutic strategies aimed at stimulating the differentiationof satellite cells after muscle injury (2) or in muscle degenerativediseases. Recruitment of satellite cells followed by fusion intomultinucleated myofibers is regulated by paracrine growth factors,whose effects are transduced by MAPK pathways. Therefore, propermodulation of these pathways can be used to stimulate muscle regeneration.Similarly, modulation of the activities of MAPKs can be usefulin improving the efficiency of muscle-mediated gene therapy. Forinstance, it may be possible to stimulate proliferation of transplantedmuscle satellite cells by first increasing ERK activity in orderto expand the pool of myoblasts further available for p38-induceddifferentiation. Moreover, the described role of the ERK pathwayin mediating the hypertrophic response of postmitotic myocytesmight also have implications in designing strategies aimed atenhancing both the size and activity of muscle fibers in patientswith myopathies. Finally, the ability of p38 to activate MyoDcan be used to stimulate the differentiation of muscle-derivedtumors (rhabdomyosarcomas) in which MyoD is functionally latent(55) and the p38 pathway is not activated (50b).

	ACKNOWLEDGMENTS

Z.W. and P.L.P. contributed equally to thiswork.

We thank J. Han, V. Sartorelli, L. Kedes, F. Tatò, W. Wright, E. Bengal, J. Houghton, and R. Henry for reagents and B. Thompsonfor manuscriptpreparation.

This work was supported by grants from the National Institutes of Health (M.K.) and NCI (J.Y.J.W.) and by grants from theCalifornia Department of Health Services Cancer Research Program(M.K. and J.R.F.) and Telethon (P.L.P.). M.K. is an American CancerSociety research professor. P.L.P. was partially supported bya postdoctoral fellowship from the Human Frontier Science Program.Z.W. was supported by postdoctoral fellowships from the MedicalResearch Council of Canada and the Human Frontier Science Program,and P.J.W. was supported by a postdoctoral fellowship from theNational Institutes ofHealth.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biology, UCSD, 9500 Gilman Dr., La Jolla, CA 92093-0322. Phone: (858)534-2828. Fax: (858) 534-2821. E-mail: plorenzo{at}biomail.ucsd.edu.

Present address: Department of Biochemistry, Hong Kong University of Science and Technology, Clear Water Bay, Kowloon, HongKong,China.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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