Targeting of p38 Mitogen-Activated Protein Kinases to MEF2 Transcription Factors

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Molecular and Cellular Biology, June 1999, p. 4028-4038, Vol. 19, No. 6
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Targeting of p38 Mitogen-Activated Protein Kinases to MEF2 Transcription Factors

Shen-Hsi Yang, Alex Galanis, and Andrew D. Sharrocks^*

Department of Biochemistry and Genetics, The Medical School, University of Newcastle upon Tyne, Newcastle upon Tyne NE2 4HH, United Kingdom

Received 28 December 1998/Returned for modification 8 February 1999/Accepted 12 March 1999

	ABSTRACT

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Mitogen-activated protein (MAP) kinase-mediated signalling to the nucleus is an important event in the conversion of extracellularsignals into a cellular response. However, the existence of multipleMAP kinases which phosphorylate similar phosphoacceptor motifsposes a problem in maintaining substrate specificity and hencethe correct biological response. Both the extracellular signal-regulatedkinase (ERK) and c-Jun NH₂-terminal kinase (JNK) subfamilies ofMAP kinases use a second specificity determinant and require dockingto their transcription factor substrates to achieve maximal substrateactivation. In this study, we demonstrate that among the differentMAP kinases, the MADS-box transcription factors MEF2A and MEF2Care preferentially phosphorylated and activated by the p38 subfamilymembers p38 $alpha$ and p38 $beta$ ₂. The efficiency of phosphorylation in vitroand transcriptional activation in vivo of MEF2A and MEF2C by thesep38 subtypes requires the presence of a kinase docking domain(D-domain). Furthermore, the D-domain from MEF2A is sufficientto confer p38 responsiveness on different transcription factors,and reciprocal effects are observed upon the introduction of alternativeD-domains into MEF2A. These results therefore contribute to ourunderstanding of signalling to MEF2 transcription factors anddemonstrate that the requirement for substrate binding by MAPkinases is an important facet of three different subclasses ofMAP kinases (ERK, JNK, andp38).

	INTRODUCTION

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The mitogen-activated protein (MAP) kinase pathways transduce extracellular signals into distinct nuclear responses (reviewedin references 29 and 33). These pathways are conserved ina diverse set of organisms, ranging from Saccharomyces cerevisiaeto humans, and have been implicated in regulating multiple cellularprocesses (reviewed in reference 29). In humans, there are atleast four separate subclasses of MAP kinases (extracellular signal-regulatedkinase [ERK], c-Jun NH₂-terminal kinase [JNK], p38, and ERK5/BMK),with members of each subclass having significant sequence similarityand apparently, in most cases, sharing several upstream components.Furthermore, the same signals often activate overlapping subsetsof MAP kinases, although the speed and efficiency of activationoften differ (reviewed in reference 1).

An increasing number of nuclear targets for the different MAP kinase cascades are being identified, and in most cases, itappears that each transcription factor acts as a target for oneor a limited subset of MAP kinases (reviewed in reference 29).Several recent advances have contributed to our understandingof how these kinases achieve their substrate specificity and elicitdistinct biological responses (reviewed in references 17 and27). For example, in yeast, the binding of the inactive Kss1pMAP kinase to its nuclear targets (Ste12p-Tec1p) inhibits theactivation of this transcription factor complex by the parallelMAP kinase cascade containing Fus3p. Similarly, Fus3p appearsto have a reciprocal inhibitory action, in this case by blockingthe upstream pheromone-responsive module from spuriously activatingKss1p (2, 16; reviewed in references 17 and 27). In mammals,MAP kinases have also been shown to bind to their nuclear targets,and it has been proposed that this might contribute to their substratespecificity (reviewed in reference 29). In the case of c-Jun,the binding of MAP kinases to a domain which is distinct fromthe phosphoacceptor motifs, the $delta$ -domain, has been shown to bean important part of the kinase specificity-determining mechanismand is required for its efficient phosphorylation by the JNK MAPkinases (3, 4, 7, 12, 13). Similar docking domainshave been identified in activating transcription factor 2 (ATF-2)(for JNK MAP kinases) (6, 7, 15) and in Elk-1 (for JNKand ERK MAP kinases) (37, 38). In Elk-1, the docking domainappears to act to allow the convergence of two diverse MAP kinasepathways on a single transcription factor, whereas the $delta$ -domainin c-Jun permits phosphorylation by a single type of cascade.It is currently unclear how p38 MAP kinases are targeted to transcriptionfactors, although the docking domain in ATF-2 is thought to permittargeting by p38 $alpha$ in addition to the JNK MAP kinases (11a).

It has recently been demonstrated that p38 $alpha$ associates with the MADS-box family transcription factor MEF2C. Subsequent phosphorylationof MEF2C stimulates its ability to activate transcription (8).In mammals, there are four MEF2C-related genes, MEF2A, MEF2B,MEF2C, and MEF2D, that encode proteins which exhibit significantamino acid sequence similarity within their DNA binding domainsand to a lesser extent throughout the rest of the proteins. Oneof the major roles of these proteins is to regulate muscle-specificgene expression (reviewed in references 19 and 24), althoughthey have recently been shown to also contribute to the activationof c-jun transcription (8, 9, 14). Until recently, littlewas known about MAP kinase signalling to MEF2 family proteinsother than MEF2C, which, in addition to being a p38 $alpha$ target, canalso be regulated by ERK5/BMK (14, 36). In this study, wehave investigated the phosphorylation of MEF2C and the relatedfamily member MEF2A by the p38 subclass of MAP kinases. We demonstratep38 $alpha$ - and p38 $beta$ ₂-specific activation of MEF2A and MEF2C and demonstratethe existence of a MAP kinase docking domain which is specificfor these two MAP kinase subtypes. Furthermore, we demonstratethe interchangeability of MAP kinase docking domains and thatthese domains play a major role in determining the specificityof MAP kinase signalling to nuclear transcriptionfactors.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Plasmid constructs. The following plasmids were used for expressing glutathione S-transferase (GST) fusion proteins in Escherichia coli. pAS860(encoding GST-MEF2A; MEF2A amino acids 266 to 413), pAS861 (encodingGST-MEF2A $Delta$ D; MEF2A amino acids 283 to 413), pAS865 (encoding GST-MEF2C;MEF2C amino acids 249 to 378), pAS866 (encoding GST-MEF2C $Delta$ D; MEF2Camino acids 265 to 378), and pAS869 (encoding GST-MEF2B; MEF2Bamino acids 201 to 300) were constructed by inserting BamHI/EcoRI-cleavedPCR-derived fragments into the same sites of pGEX-3X (Pharmacia).pAS406 (encoding GST-Elk-1 $Delta$ D; Elk-1 amino acids 330 to 428), pAS545(encoding GST-Elk-1; Elk-1 amino acids 310 to 428) (37), anda plasmid encoding GST-Jun (c-Jun amino acids 1 to 79) (4)have been described previously. pAS862, pAS863, and pAS864 (encodingGST-MEF2A mutants) are derivatives of pAS860 with the site-directedmutations R269A and K270A (GST-MEF2A[M1]), L273A and V275A (GST-MEF2A[M2]),and I277A and P278A (GST-MEF2A[M3]), respectively. pAS865 (encodingGST-MEF2A-Elk-1; MEF2A amino acids 266 to 292; Elk-1 amino acids330 to 428), pAS866 (encoding GST-MEF2A-c-Jun; MEF2A amino acids266 to 292; c-Jun amino acids 55 to 79), pAS870 (encoding GST-MEF2B-MEF2A;MEF2B amino acids 201 to 224; MEF2A amino acids 292 to 413), pAS871(encoding GST-cJun $delta$ -MEF2A; c-Jun amino acids 1 to 55; MEF2A aminoacids 283 to 413), pAS872 (encoding GST-SAPD-MEF2A; SRF accessoryprotein 1 [SAP-1] amino acids 290 to 334; MEF2A amino acids 283to 413), and pAS873 (encoding GST-ElkD-MEF2A; Elk-1 amino acids310 to 327; MEF2A amino acids 283 to 413) were constructed byinserting a BamHI/EcoRI-cleaved PCR-derived fragment into thesame sites of pGEX-3X. PCR fragments were generated by a two-stepPCR protocol (31) with a mutagenic primer consisting of nucleotideshomologous to each half of the chimeric product, two flankingprimers, and the following pairs of templates in each step: pAS860and pAS407, pAS860 and GST-Jun, pAS860 and pAS869, GST-Jun andpAS860, GST-SAPC (32) and pAS860, and pAS407 and pAS860,respectively.

The following plasmids were constructed for use in mammalian cell transfections. pG5E1b contains five GAL4 DNA binding sitescloned upstream of a minimal promoter element and the fireflyluciferase gene (23). pSG424 encodes the GAL4 DNA binding domain(22), and the vectors pCMV5-HA-ERK2 (18), pcDNA3-F-JNK2 (26),pCMV5-F-p38 $alpha$ (21), pcDNA3-F-p38 $beta$ ₂ (5), pcDNA3-F-p38 $gamma$ (5),and pcDNA3-F-p38 $delta$ (30) encoding hemagglutinin (HA)- or Flag(F)-tagged MAP kinases, pCMV5-HA-MEK1 ( $Delta$ NS218E-S222D), pcDNA3-F-MKK6(E),and pcDNA3-F-MKK7 $beta$ , encoding HA- or Flag-tagged wild-type (MKK7 $beta$ )or constitutively active (MEK1 and MKK6) MAP kinase kinases (MKKs)have been described previously (35). pAS874 (GAL4-MEF2A), pAS875(GAL4-MEF2A $Delta$ D), pAS876 (GAL4-MEF2A[M1]), pAS877 (GAL4-MEF2A[M2]),pAS878 (GAL4-MEF2A[M3]), pAS879 (GAL4-MEF2A-Elk-1), pAS880 (GAL4-MEF2A-cJun),pAS881 (GAL4-MEF2C), and pAS882 (GAL4-MEF2C $Delta$ D) were constructedby ligating BamHI/XbaI fragments from pAS860 to pAS868, respectively,into the same sites of pSG424. pAS897 (GAL4-Elk330 [GAL4-Elk-1 $Delta$ D])and pAS898 (GAL4-Elk310 [GAL4-Elk-1]) were constructed by ligatingBamHI/XbaI fragments from pAS406 and pAS545 (37), respectively,into the same sites of pSG424. GAL-c-Jun has previously been described(10). pAS883 and pAS891 encode the same series of GAL4 fusionproteins under the control of the cytomegalovirus (CMV) promoterand were constructed by ligating the HindIII/XbaI fragments frompAS874 to pAS882 into the same sites of pCMV5. pAS900 and pAS1351encode the GAL4 fusion proteins GAL4-Elk-1 and GAL4-Elk-1 $Delta$ D, respectively,under the control of the CMV promoter and were constructed byligating the HindIII/XbaI fragments from pAS897 and pAS898 intothe same sites of pCMV5. pAS572 (encoding CMV promoter-regulatedGAL4-Elk-205) has been described previously (37). Details ofPCR primers can be supplied on request. All plasmid constructsmade by PCR were verified by automated dideoxysequencing.

The following plasmids were constructed for the production of proteins by in vitro transcription and translation. pAS522 (encodingfull-length MEF2A; amino acids 1 to 486) was constructed by insertingan NcoI fragment from pT7C4 (20) into the NcoI site in pAS37.pAS1201 is identical to pAS522 except that an XhoI site was introducedinto the 3' end of the coding region (by using the primer ADS575)and the 3' untranslated region was also lost from the clone. pAS1203(encoding C-terminally Flag- or His-tagged full-length MEF2A underthe control of a T7 promoter) was constructed by inserting anNcoI/XhoI fragment from pAS1201 into the same sites in pETnefPFH.pAS1209 (encoding C-terminally Flag- and His-tagged full-lengthMEF2A under the control of a T3 promoter) was constructed by insertingan NcoI/EcoRI fragment from pAS1203 into the same sites in pAS798(31). pAS1397 (encoding full-length MEF2A with the point mutationsI277A and P278A) was constructed by replacing the BglII/XhoI fragmentin pAS1209 with a PCR-derived fragment incorporating the two pointmutations.

Protein expression and purification. GST fusion proteins were expressed in E. coli JM101 and purified as described previously (25, 37). In vitro-translatedproteins were produced by sequential transcription and translationwith rabbit reticulocyte lysate (Promega). Tagged proteins wereimmunoprecipitated prior to use in protein kinase assays, by using10 µl of anti-Flag antibody conjugated to agarose beads (50% slurry;Sigma). Proteins were bound to the beads for 1 h at room temperature,washed five times with Triton lysis buffer (TLB) (37), and resuspendedin an equal volume ofTLB.

Tissue culture, cell transfection, and reporter gene assays. COS-7 cells were maintained in Dulbecco's modified Eagle's medium (DMEM) supplemented with 10% fetal bovine serum (FBS) (GibcoBRL). CHO cells were maintained in F12 medium supplemented with5% FBS. 293 cells were maintained in DMEM supplemented with 10%FBS. HeLa cells were maintained in DMEM supplemented with 10%FBS. Transfection experiments were carried out with Superfecttransfection reagent (Qiagen) as described previously (37, 38).

For reporter gene assays, a luciferase reporter construct controlled by a GAL4-driven promoter was cotransfected with CMVpromoter-driven vectors encoding various GAL4 fusion proteins.The activities of the GAL4 fusion proteins (usually 50 ng of plasmidDNA but 5 ng with GAL4-MEF2C derivatives) were measured in cotransfectionassays in all cell lines by using 1 µg of the reporter plasmidpG5E1bLuc and, where indicated, 250 ng of vectors encoding a MAPkinase and constitutively activated MKK. Transfection efficiencieswere normalized by measuring the activity from a cotransfectedplasmid (1 µg) which expresses $beta$ -galactosidase (pCH110; PharmaciaKB Biotechnology Inc.). To stimulate the endogenous MAP kinasepathways, COS-7 cells were treated with 50 nM epidermal growthfactor (EGF) (Sigma), and CHO and HeLa cells were treated with10 ng of mouse interleukin 1 $alpha$ (IL-1 $alpha$ ) (Genzyme Corp.) and leftfor 12 h. Cell extracts were prepared and luciferase and $beta$ -galactosidaseassays were carried out as described previously (37, 38).

Protein kinase assays. In order to prepare recombinant JNK2 and p38 MAP kinases ( $alpha$ , $beta$ ₂, $gamma$ , and $delta$ ), COS-7 cells were transfected with constructs encodingFlag epitope-tagged MAP kinases. Kinases were activated by stimulationwith UV light for 30 min (for JNK2) or were cotransfected witha constitutively activated form of MKK6 [MKK6(E)] (for p38 $alpha$ , $beta$ ₂, $gamma$ , and $delta$ ), and the active kinases were purified by immunoprecipitationas described previously (37). Purified kinases were eluted frombeads by competing with 0.1 mg of Flag peptide per ml. Recombinantactive ERK2 was obtained from New England Biolabs. The kinaseassays were carried out in 20-µl reaction volumes containing invitro-translated proteins bound to anti-Flag antibody conjugatedto agarose beads or with 5 pmol of GST fusion proteins as a substrateas described previously (37, 38). The phosphorylation of substrateproteins was examined by autoradiography following sodium dodecylphosphate-polyacrylamide gel electrophoresis and quantified byphosphorimaging (Fuji BAS1500; TINA 2.08e software), and the datawere presented graphically after curve fitting with the appropriateequation by using BIOSOFT Fig.P or Microsoft Excel software. Peptidecompetition experiments were carried out essentially as describedabove, except for the preincubation of the p38 MAP kinases with50 to 5,000 pmol of the peptide competitors before the kinasereactions. Final peptide concentrations were 2.5 to 25 µM (a 10-to 1,000-fold excess over GST fusion proteinsubstrates).

Western blot analysis. GAL4 fusion proteins were detected in total 293 cell extracts by using the anti-GAL4 antibody directed against the amino-terminalDNA-binding domain (Santa Cruz). Elk-1 phosphorylated on Ser383was detected with an anti-phospho-Elk-1(Ser383) antibody (NewEngland Biolabs). Immunocomplexes were detected by using horseradishperoxidase-conjugated secondary antibody followed by enhancedchemiluminescence(Amersham).

Figure generation and data quantification. All figures were generated electronically from scans of autoradiographic images by using Picture Publisher (Micrografix) andPowerpoint version 7.0 (Microsoft) software. Final images arerepresentative of the original autoradiographic images. Phosphorimagerdata were quantified by using Tina software (version 2.08e).

	RESULTS

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Phosphorylation and activation of MEF2 transcription factors by p38 MAP kinases. The transcription factor MEF2C is phosphorylated and activated by the p38 $alpha$ MAP kinase in response to inflammation (8),thereby providing a link between the p38 pathway and a memberof the MEF2 group of transcription factors. However, several distinctmembers of the p38 MAP kinases have been identified, includingp38 $alpha$ , - $beta$ , - $gamma$ , and - $delta$ (reviewed in references 1 and 30). Theabilities of these different p38 MAP kinases to phosphorylateMEF2 proteins in vitro and stimulate their transcriptional activationproperties in vivo were tested (Fig. 1). Firstly, the phosphorylationof a GST fusion protein containing the transcriptional activationdomain (TAD) of MEF2A and MEF2C by the different p38 MAP kinaseswas tested (Fig. 1B). These fusion proteins contain the minimalTAD, which in the case of MEF2C, has been shown to be sufficientfor maximal phosphorylation-inducible transcriptional activation(8). This region contains the major p38 $alpha$ phosphorylation sitesT²⁹³ and T³⁰⁰ in MEF2C (8) and the corresponding amino acid residues T³⁰⁴ and T³¹¹ in MEF2A (Fig. 1A). An independent study has confirmed that thesetwo residues in MEF2A are the major p38 $alpha$ phosphorylation sites(39; T³¹² and T³¹⁹ in the MEF2A isoform were used in that study). GST-MEF2A andGST-MEF2C are both phosphorylated by p38 $alpha$ and p38 $beta$ ₂ (Fig. 1B,lanes 1 and 2). However, in comparison, neither p38 $gamma$ nor p38 $delta$ can efficiently phosphorylate GST-MEF2A and GST-MEF2C (Fig. 1B,lanes 3 and 4). Moreover, GST-MEF2A and GST-MEF2C appear to bephosphorylated selectively by a subgroup of p38 MAP kinases butnot by other classes of MAP kinases, as ERK and JNK family membersonly poorly phosphorylate these substrates in vitro (data notshown).

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FIG. 1. Phosphorylation and activation of MEF2A or MEF2C by different p38 MAP kinases. (A) Diagram illustrating the domain structure of full-length MEF2C and truncated MEF2A and MEF2C proteins fused to either GST or the GAL4 DNA binding domain (open boxes). The location of the DNA binding domain (DBD), minimal TAD, and p38 $alpha$ (T293 and T300) and ERK5 (S387) phosphorylation sites in MEF2C are indicated. The black box represents the putative kinase docking domain (D-domain) of MEF2A/C, and the numbers of the N- and C-terminal amino acids in the MEF2A or MEF2C moiety are indicated. The sequences of MEF2A and MEF2C around the major phosphoacceptor motifs for p38 $alpha$ MAP kinase are shown. (B) The phosphorylation of GST-MEF2A, GST-MEF2C, and GST-Elk-310 by the p38 MAP kinase subtypes p38 $alpha$ (lane 1), p38 $beta$ ₂ (lane 2), p38 $gamma$ (lane 3), and p38 $delta$ (lane 4) was examined by a protein kinase assay. The activity of each protein kinase was standardized towards the substrate GST-Elk-310 (bottom panel). Kinase assays were performed for 15 min at 30°C with 5 pmol of GST-MEF2A and GST-MEF2C as substrates. (C) COS-7 cells were cotransfected with either GAL4-MEF2A or GAL4-MEF2C expression vectors, a constitutively activated form of MKK6 (MKK6[E]), the indicated p38 MAP kinases, and a GAL4-driven luciferase reporter plasmid. (D) COS-7 cells were cotransfected with expression vectors encoding GAL4-MEF2A, an overexpressed (MKK7 $beta$ ) or constitutively activated form of MKK (MEK and MKK6), a MAP kinase (ERK2, JNK2, and p38 $beta$ ₂), and a GAL4-driven luciferase reporter plasmid. (E) HeLa cells were cotransfected with vectors encoding GAL4-MEF2A and a GAL4-driven luciferase reporter plasmid. Cells either were left unstimulated or were stimulated with IL-1 for 18 h in the absence or presence of the indicated JNK pathway (cotransfected dominant negative form of MKK4 [DN-MKK4]) or p38 pathway (SB202190) inhibitors. (F) COS-7 (for EGF stimulation of ERKs), CHO (for IL-1 stimulation of JNKs), and HeLa (for IL-1 stimulation of p38s) cells were cotransfected with vectors encoding GAL4-MEF2A or GAL4-Elk-1 and a GAL4-driven luciferase reporter plasmid. The cells either were left unstimulated (white bars) or were stimulated (black bars for Elk-1 and grey bars for MEF2A) with EGF or IL-1 as in panel E. Transfection efficiencies were monitored by using the $beta$ -galactosidase expression vector pCH110. The normalized luciferase activities (means ± standard errors; n, 2 or 3) are presented.

In order to determine whether this differential phosphorylation by p38 MAP kinases reflects a difference in their responseto these pathways in vivo, GAL4 fusion proteins containing theTADs of MEF2A and MEF2C were constructed (Fig. 1A) and were testedfor their ability to activate a GAL4-driven luciferase reportergene. The activation of distinct MAP kinase cascades was achievedby cotransfecting a constitutively activated form of MKK6, togetherwith either p38 $alpha$ , p38 $beta$ ₂, p38 $gamma$ , or p38 $delta$ . In the cell line usedin this study (COS-7), the expression of MKK6 alone had littleeffect on the activity of the GAL4 fusion proteins (Fig. 1C),although the activation of MEF2A can be detected by using MKK6alone in other cell lines (e.g., 293 cells [39]). MEF2A andMEF2C were efficiently activated by p38 $alpha$ and p38 $beta$ ₂ but not byp38 $gamma$ and p38 $delta$ (Fig. 1C). To test the ability of the ERK2 and JNK2pathways to activate MEF2A, similar experiments were performedwith the cotransfection of their respective upstream kinases (MAPkinase [or Erk] kinase [MEK] and MKK7 $beta$ , respectively). However,in comparison to p38 $beta$ ₂ (~50-fold induction), both ERK2 and JNK2had little effect on the activity of MEF2A (Fig. 1D). Treatmentwith MEK/ERK2 and MKK7 $beta$ /JNK2 is sufficient to activate other nuclearsubstrates (see Fig. 6) (37, 39).

The response of MEF2A to the activation of endogenous MAP kinase pathways following stimulation by mitogens and cytokinesin the absence of overexpressed pathway components was subsequentlyinvestigated. Initially, HeLa cells were stimulated with IL-1.This treatment results in the stimulation of GAL4-MEF2A via thep38 pathway, as the JNK pathway inhibitor (DN-MKK4) has littleeffect, while the p38 pathway inhibitor (SB202190) almost completelyblocks this stimulation (Fig. 1E). To directly compare the effectof stimulating individual MAP kinase pathways on MEF2A activation,COS-7, CHO, and HeLa cells were transfected with GAL4-MEF2A andtreated with either EGF (to activate the ERK pathway in COS-7cells [37]) or IL-1 (to activate the JNK pathway in CHO cells[34] or the p38 pathway in HeLa cells [Fig. 1E]). While thetreatment of COS-7 cells with EGF and that of CHO cells with IL-1lead to the activation of GAL4-Elk-1 via the ERK and JNK pathways,neither of these treatments activates GAL4-MEF2A (Fig. 1F). However,in comparison, the stimulation of the endogenous p38 pathway byIL-1 treatment of HeLa cells results in a comparable activationof GAL4-Elk-1 and GAL4-MEF2A (Fig. 1F).

Taken together, these results demonstrate that like MEF2C, MEF2A is phosphorylated and activated by p38 $alpha$ . This is in agreementwith the findings of two independent studies (18a, 39). Moreover,while both MEF2A and MEF2C are also targeted by p38 $beta$ ₂, neitherappears to be a target of p38 $gamma$ and p38 $delta$ . Thus, these MEF2 familyproteins appear to be substrates of a subset of p38 MAP kinasesin vitro and invivo.

Requirement of the MEF2 D-domain for phosphorylation by p38 $alpha$ and p38 $beta$ ₂ MAP kinases in vitro and in vivo. We have previously identified within the transcription factor Elk-1 a kinase docking domain, the D-domain, that contains specificitydeterminants and therefore enhances the phosphorylation of Elk-1by ERK and JNK MAP kinases. However, this domain does not appearto affect the phosphorylation of Elk-1 by the p38 MAP kinases(37, 38). Inspection of the sequence of MEF2A and MEF2C indicatedthe presence of a motif which exhibits limited similarity withthe Elk-1 D-domain (see Fig. 5A). To investigate whether the efficiencyof MEF2A and MEF2C phosphorylation by p38 $alpha$ and p38 $beta$ ₂ is enhancedby the presence of a kinase docking domain, the GST fusion proteinsGST-MEF2A $Delta$ D and GST-MEF2C $Delta$ D, which contain the TAD and associatedphosphoacceptor motifs but lack the region which resembles theElk-1 D-domain (Fig. 2A and B), were created. These GST fusionproteins were tested as in vitro MAP kinase substrates, in comparisonto analogous proteins which contain the putative MAP kinase dockingsite (Fig. 2A and B). The activity of the kinases towards GST-Elk-1was initially standardized, and equivalent activities were usedin the kinase assays. The kinetics of phosphorylation of GST-MEF2A(Fig. 2A, lanes 1 to 4) and GST-MEF2C (Fig. 2B, lanes 1 to 4)by p38 $alpha$ , p38 $beta$ ₂, and p38 $gamma$ were virtually indistinguishable. Incontrast, the phosphorylation of GST-MEF2A $Delta$ D (Fig. 2A, lanes 5to 8) and GST-MEF2C $Delta$ D (Fig. 2B, lanes 5 to 8) by p38 $alpha$ and p38 $beta$ ₂was greatly reduced over the same time period. However, the phosphorylationof these two substrates by p38 $gamma$ was virtually indistinguishablefrom that when the putative docking site was present (comparethe graphs and lanes 1 to 4 and 5 to 8 in the bottom panels ofFig. 2A and B).

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FIG. 2. Identification of a domain required for efficient p38-mediated activation of MEF2A and MEF2C. (A and B) Requirement of the D-domain for phosphorylation of MEF2A and MEF2C in vitro. Diagrammatic illustrations of truncated MEF2A or MEF2C and MEF2A $Delta$ D or MEF2C $Delta$ D proteins fused to either GST or the GAL4 DNA binding domain (open boxes) are shown above each gel. The black box represents the putative kinase docking domain (D-domain) of MEF2A, and the numbers of the N- and C-terminal amino acids in MEF2A moiety are shown. (A) Kinetic analysis of GST-MEF2A phosphorylation by p38 $alpha$ , p38 $beta$ ₂, and p38 $gamma$ in vitro. GST-MEF2A (lanes 1 to 4) and GST-MEF2A $Delta$ D (lanes 5 to 8) were phosphorylated by p38 $alpha$ , p38 $beta$ ₂, and p38 $gamma$ MAP kinases for the times indicated above each lane. Due to the lower levels of phosphorylation by p38 $gamma$ , the bottom panels were exposed for longer times than the other panels. The results are presented graphically below these panels with data obtained with GST-MEF2A (squares) and GST-MEF2A $Delta$ D (circles) as p38 substrates. Data are presented relative to the phosphorylation of GST-MEF2A after 120 min (taken as 100). (B) As described for panel A, except that the GST-MEF2C derivatives were used as substrates. (C and D) The D-domain is essential for efficient p38 $beta$ ₂-inducible transcriptional activation by MEF2A and MEF2C in vivo. (C) COS-7 cells were cotransfected with expression vectors encoding GAL4-MEF2A derivatives, a constitutively activated form of MKK6 (MKK6[E]), p38 $beta$ ₂ MAP kinase, and a GAL4-driven luciferase reporter plasmid. The expression levels of the GAL4 fusion proteins in the unstimulated cells were examined by Western blot analysis with an anti-GAL4 antibody (bottom panel). (D) Assays were carried out as described for panel C, except that GAL4-MEF2C was examined. Transfection efficiencies were monitored by using the $beta$ -galactosidase expression vector pCH110. The normalized luciferase activities (means ± standard errors; n = 3) are presented.

To examine the requirement of the D-domain for the activation of MEF2 transcription factors by MAP kinases in vivo, GAL4 fusionproteins to MEF2A and MEF2C which either contain or lack thisdomain were constructed and tested for their ability to activatea GAL4-driven luciferase reporter gene in response to MAP kinaseactivation (Fig. 2C and D). In the absence of cotransfected MKK6(E)and p38 $beta$ ₂ (Fig. 2C and D), all the fusion proteins activated thereporter gene to low levels. However, upon cotransfection of MKK6(E)together with p38 $beta$ ₂ and either GAL4-MEF2A (Fig. 2C) or GAL4-MEF2C(Fig. 2D), greatly enhanced transcriptional activation was observed.In contrast, the deletion of the D-domain in both MEF2A and MEF2Ccaused a large reduction in the GAL4-MEF2A- and GAL4-MEF2C-mediatedtranscriptional activation (Fig. 2C and D). Western blotting indicatesthat the deletion of the D-domain had little effect on the levelsof the GAL4 fusion proteins (Fig. 2C and D, bottom panels). Virtuallyidentical results were observed for the activation of these chimericproteins by p38 $alpha$ (data notshown).

These data therefore indicate that both MEF2A and MEF2C contain a domain, the D-domain, which is distinct from their phosphoacceptormotifs and is required for efficient phosphorylation in vitroand stimulation of their transcriptional activation potentialin vivo by the p38 $alpha$ and p38 $beta$ ₂ MAPkinases.

Identification of important residues in the D-domain required for efficient phosphorylation by p38 MAP kinases. The D-domain plays an important role in enhancing phosphorylation and stimulation of MEF2A- and MEF2C-mediated transcriptionalactivation by the p38 $alpha$ and p38 $beta$ ₂ MAP kinases. In order to investigatethe contribution of residues within this domain of MEF2A towardsthis function, pairs of amino acids conserved between MEF2A andMEF2C (see Fig. 8A) were mutated to alanine residues (Fig. 3A).Such mutations should preserve any structural motifs which arepresent but remove side chains which are available for intermolecularinteractions. The mutant proteins were examined as substratesfor p38 MAP kinases (Fig. 3B). All three of the mutants tested(M1, M2, and M3) exhibited a reduction in the efficiency of theirphosphorylation by p38 $alpha$ and p38 $beta$ ₂ (Fig. 3B). In contrast, noneof the mutations within the D-domain resulted in a decrease inthe efficiency of MEF2A phosphorylation by p38 $gamma$ (Fig. 3B). GAL4fusion proteins were also constructed with each of the mutantMEF2A derivatives to investigate their activation by p38 $alpha$ andp38 $beta$ ₂ in vivo. In comparison to the wild-type (WT) protein, theM1, M2, and M3 mutant GAL4-MEF2A fusion proteins exhibit reducedactivation of transcription in response to MKK6(E) and p38 $alpha$ (Fig.3C) or MKK6(E) and p38 $beta$ ₂ (Fig. 3D) in vivo. Western blotting indicatesthat all the mutant proteins were expressed to equivalent levelsin the presence and absence of activated upstream cascades (Fig.3E). Collectively, these data demonstrate that the conserved residueswithin the MEF2A D-domain play key roles in determining its efficientphosphorylation and transcriptional activation by p38 $alpha$ and p38 $beta$ ₂.Furthermore, the critical residues for activation by p38 $alpha$ andp38 $beta$ ₂ appear to be indistinguishable.

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FIG. 3. Mapping the residues in the D-domain of MEF2A required for targeting by p38 $alpha$ and p38 $beta$ ₂. (A) Amino acid sequences of the WT and D-domain mutants R269A/K270A (M1), L273A/V275A (M2), and I277A/P278A (M3) are shown. Numbers above the sequences represent the N- and C-terminal residues in the D-domain. (B) Kinase assays of WT and mutant GST-MEF2A fusion proteins by p38 MAP kinases were carried out as described in the legend to Fig. 1. The activity of each kinase was standardized relative to the phosphorylation of GST-MEF2A(WT). (C) p38 $alpha$ -inducible transcriptional activation by WT and mutant GAL4-MEF2A fusion proteins. COS-7 cells were cotransfected with expression vectors encoding GAL4 fusions to either WT or D-domain mutant (M1 to M3) MEF2A derivatives, vectors encoding MKK6(E) and p38 $alpha$ , and a GAL4-driven luciferase reporter plasmid. The luciferase activities relative to GAL4-MEF2A-mediated reporter activation in the absence of cotransfected kinases are presented (means ± standard errors; n = 3). (D) Assays were carried out as in panel C, except that vectors encoding p38 $beta$ ₂ were cotransfected where indicated. (E) Expression levels of the GAL4 fusion proteins, in the absence (lanes 1, 3, 5, and 7) and presence (lanes 2, 4, 6, and 8) of cotransfected MKK6(E) and p38 $alpha$ , were examined by Western blotting with an anti-GAL4 antibody.

In order to demonstrate the importance of the D-domain in targeting p38 MAP kinases to MEF2A in the context of a full-lengthprotein rather than truncated fusion proteins, we created a mutantversion of MEF2A with two point mutations in the D-domain (MEF2A[M3];Fig. 4A), which reduce the phosphorylation and activation of truncatedMEF2A derivatives by p38 $alpha$ and p38 $beta$ ₂ (Fig. 3). Full-length MEF2Awas initially tested as a substrate for the different p38 isoforms(data not shown) with results virtually identical to those obtainedwith truncated GST fusion proteins (Fig. 1B). We then comparedthe ability of p38 $beta$ ₂ to phosphorylate MEF2A(WT) and the mutantMEF2A(M3) in vitro. Phosphorylation of MEF2A(WT) was observedby the presence of a slower migrating band (Fig. 4B, lanes 4 and5) and the incorporation of ³²P-labelled ATP (Fig. 4C, lanes 2 to 4). In contrast, over thesame time period, much-reduced MEF2A(M3) phosphorylation was detectedby these assays (Fig. 4B, lanes 6 to 10, and C, lanes 5 to 8).Thus, the D-domain plays an important role in directing the efficiencyof MEF2A phosphorylation by p38 $beta$ ₂ in the context of the full-lengthprotein.

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FIG. 4. The D-domain is required for the efficient phosphorylation of full-length MEF2A by p38 $beta$ ₂. (A) Diagrammatic representation of the domain structure of full-length MEF2A. The locations of the MADS-MEF DNA-binding domain (DBD), the MAP kinase docking domain (black box), and the key phosphoacceptor motifs (T304 and T311) in the TAD are shown. The locations of the mutations in MEF2A(M3) are indicated in italics. (B and C) Phosphorylation of MEF2A(WT) and MEF2A(M3) was carried out in vitro with p38 $beta$ ₂. Equal amounts of in vitro-translated WT and mutant MEF2A proteins were phosphorylated by p38 $beta$ ₂ for the indicated times in the absence (B) or presence (C) of ³²P-labelled ATP. Phosphorylated MEF2A was detected by the reduced mobility of the proteins (arrows in panel B) or by the incorporation of ³²P-labelled ATP (C).

The MEF2A D-domain acts as a binding motif for the p38 MAP kinases. The ability of ERK2 to phosphorylate Elk-1 and that of JNK to phosphorylate c-Jun correlate with their ability to bind tothese substrates via a docking domain (13, 37). However, whilestable interactions are readily detectable in these cases, suchstable interactions are not observed between MAP kinases and othersubstrates (e.g., JNK and Elk-1; 38). Similarly, we were unableto demonstrate a physical interaction between MEF2A and p38 MAPkinases under a variety of experimental conditions (data not shown),although others have previously demonstrated such an interaction(8). We therefore adopted a peptide competition assay to investigatethe binding of the kinases to MEF2A. This approach has previouslybeen used to allow the comparison of ERK and JNK binding to Elk-1under identical experimental conditions and relies on the factthat peptides which bind to the kinase will act as competitorsfor the binding of the kinase to docking sites in the transcriptionfactor targets (38). Peptides were synthesized which correspondto MEF2A amino acids 266 to 283 (encompassing the D-domain) (MEFD[WT])and the same region with two amino acid substitutions (MEFD[M2])(Fig. 5A). Increasing amounts of these peptides were includedin kinase assays to compete for binding of the p38 MAP kinasesto MEF2A via the D-domain (Fig. 5B). The MEFD(WT) peptide actedas an inhibitor of p38 $alpha$ - and p38 $beta$ ₂-mediated phosphorylation ofMEF2A in a concentration-dependent manner (Fig. 5B, lanes 1 to4). However, little effect was seen on the efficiency of phosphorylationby p38 $gamma$ except at the highest concentrations of the wild-typeand mutant peptides used (Fig. 5B, lanes 1 to 4, bottom panel).In contrast, the mutant MEFD(M2) peptide did not act as a competitor(Fig. 5B, lanes 5 to 7). This is consistent with the observationthat the M2 mutant GST- and GAL-MEF2A fusion proteins are poortargets for p38 $alpha$ and p38 $beta$ ₂ (Fig. 3). Peptides corresponding tothe kinase docking domains from Elk-1 (ElkD) and SAP-1 (SAPD)(Fig. 5A) were also tested (Fig. 5B). The SAPD peptide also actedas an efficient inhibitor (Fig. 5B, lane 9), whereas the ElkDpeptide did not act as an inhibitor of the phosphorylation ofMEF2A by p38 $alpha$ and p38 $beta$ ₂ (Fig. 5B, lane 10). These results areconsistent with the observation that the SAP-1 D-domain acts asa docking site for both the p38 $alpha$ and p38 $beta$ ₂ MAP kinases (5a),whereas the Elk-1 D-domain does not act as a p38 MAP kinase dockingsite (38).

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FIG. 5. The MEF2A D-domain acts as a binding site for the p38 $alpha$ and p38 $beta$ ₂ MAP kinases. (A) The sequences of the competitor peptides corresponding to the MAP kinase docking domains from Elk-1, SAP-1, and MEF2A. Sequences are aligned to give maximal similarities, with identical and highly conserved residues highlighted. Residues altered in the mutant MEF2A peptide (MEFD[M2]) are shown in bold. (B) Phosphorylation of GST-MEF2A (5 pmol) by p38 MAP kinases in the presence of indicated competitor peptides. The peptide competition assay was based on the kinase assays described in the legend to Fig. 1, except that the p38 MAP kinases were preincubated in the absence (lanes 1 and 8) or presence of competitor peptides (a 10- to 1,000-fold excess over MEF2A substrate) at 50 pmol (lanes 2 and 5), 500 pmol (lanes 3 and 6), and 5 nmol (lanes 4, 7, 9, and 10), respectively. Increases in the concentration of added competitor peptides are indicated schematically above each set of lanes. The activity of each kinase was standardized relative to the phosphorylation of GST-MEF2A(WT). (C) Specificity of action of inhibitory peptides and phosphorylation of transcription factor substrates (5 pmol) by MAP kinases (combinations indicated above each panel) in the presence of the MEFD(WT) peptide. Assays were carried out as in panel B in the presence of 0 pmol (lanes 1, 5, and 9), 5 pmol (lanes 2, 6, and 10), 50 pmol (lanes 3, 7, and 11), and 500 pmol (lanes 4, 8, and 12) of the competitor peptide. The quantification of the data is shown graphically below each panel, relative to the phosphorylation of each substrate in the absence of added competitor peptide.

In order to investigate the specificity of action of the MEF2A D-domain peptide as a p38 $alpha$ and p38 $beta$ ₂ MAP kinase inhibitor,the ability of the D-domain peptide to inhibit MEF2A phosphorylationby p38 $beta$ ₂ was compared to its inhibitory properties on other MAPkinase-substrate combinations (Fig. 5C). Of the three kinasestested, the D-domain peptide acted as a more efficient competitorof p38 $beta$ ₂ than ERK and JNK. This is most apparent at the highestconcentrations of peptide used (Fig. 5C, lanes 4, 8, and 12),although the inhibition of all three MAP kinases can be observedto some degree. This might reflect some conservation of the peptidebinding site on the MAP kinases, as these proteins are all relatedand the relative order of peptide inhibition efficiency is consistentwith the observation that the highest similarity is between thep38 and ERK MAPkinases.

These data therefore demonstrate that the D-domain of MEF2A preferentially acts as a binding site for p38 $alpha$ and p38 $beta$ ₂ MAP kinasesinvitro.

The MAP kinase targeting domain of MEF2A is sufficient to confer p38 responsiveness to Elk-1 and c-Jun. In order to investigate whether the MEF2A D-domain can act in a heterologous context to allow p38 targeting and hence transducesignals via the p38 pathway to different substrates, chimericproteins were created. In these proteins, the p38 targeting domainof MEF2A was fused to the minimal TAD of Elk-1 (which respondsto both the ERK and JNK pathways) and c-Jun (which responds tothe JNK pathway) and either GST or the GAL4-DNA-binding domain(Fig. 6A and E). These minimal TADs lack their natural kinasebinding domains. Firstly, the efficiencies of phosphorylationof the GST fusion proteins by different MAP kinases were compared(Fig. 6B and F). GST-Elk-1 $Delta$ D, which lacks its own kinase targetingdomain, represents a relatively poor MAP kinase substrate (Fig.6B, lane 1). However in comparison, GST-MEF2A-Elk-1 was efficientlyphosphorylated by p38 $alpha$ and p38 $beta$ ₂ (Fig. 6B, lane 2). In contrast,little enhancement of Elk-1 phosphorylation by ERK2, JNK2, andp38 $gamma$ was observed by the inclusion of the MAP kinase docking sitefrom MEF2A (Fig. 6B, lane 2). Moreover, the fusion of the MEF2AD-domain to c-Jun in the GST-MEF2A-cJun chimera converts c-Juninto a better substrate for p38 $alpha$ and p38 $beta$ ₂ but not for p38 $gamma$ (Fig.6F, lane 2). c-Jun can usually be efficiently phosphorylated onlyby JNK and not p38 MAP kinases (Fig. 6F, lane 1), and the propensityof c-Jun as a JNK substrate is severely reduced in the presenceof the MEF2A MAP kinase docking site (Fig. 6F, lane 2, bottompanel).

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FIG. 6. The p38-binding domain of MEF2A (D-domain) functions in a heterologous context. The phosphorylation and activation of GST and GAL4 fusions to MEF2A-Elk-1 (A to D) and MEF2A-cJun (E to H) chimeras by MAP kinases were analyzed. (A and E) Diagrams illustrating fusions of GST to Elk-1 $Delta$ D, MEF2A-Elk-1, cJun, and MEF2A-cJun. The numbers of the N- and C-terminal Elk-1/cJun (roman type) and MEF2A (italics) amino acids included in these constructs are indicated above and below each construct, respectively. The MEF2A D-domain and cJun $delta$ -domain are indicated by solid and open boxes, respectively. The Elk-1 and cJun transcriptional activation domains are shown by open and black boxes, respectively. (B and F) Kinase assays of GST fusion proteins (5 pmol of each substrate) for the indicated MAP kinases were carried out for 15 min as described in the legend to Fig. 1. (C and G) Phosphorylation of the GST-MEF2A-Elk-1 and GST-MEF2A-cJun chimeras by MAP kinases was analyzed in the presence of competitor peptides as described in the legend to Fig. 4. Five picomoles of each chimeric protein was used in the reactions. The indicated p38 MAP kinases were preincubated in the absence (lane 1) or presence of 500 pmol of the following peptides: MEF2A WT D-domain (lane 2; MEFD[WT]), MEF2A mutant D-domain peptide (lane 3; MEFD[M2]), SAP-1 D-domain peptide (lane 4; SAPD), and Elk-1 D-domain peptide (lane 5; ElkD). (D and H) COS-7 cells were cotransfected with vectors encoding GAL4-Elk-1 $Delta$ D, GAL4-MEF2A-Elk-1, GAL4-cJun, and GAL4-MEF2A-cJun fusions, a GAL4-driven luciferase reporter plasmid, and vectors encoding MAP kinases (ERK2, JNK2, and p38 $beta$ ₂) and an overexpressed (MKK7 $beta$ ) or constitutively activated form (MEK $Delta$ N and MKK6[E]) of the upstream MAP kinase kinases. The expression levels of the GAL4 fusion proteins in unstimulated cells were examined by Western blotting with an anti-GAL4 antibody (bottom panel).

In order to demonstrate that these changes in substrate specificity towards MAP kinases, which are dictated by the MEF2A D-domain,reflect a difference in the ability of these domains to bind tothe MAP kinases, peptide competition experiments were performedwith the chimeric proteins MEF2A-Elk-1 (Fig. 6C) and MEF2A-cJun(Fig. 6G). The MEFD(WT) and, to a lesser extent, SAPD peptidesacted as competitors of phosphorylation of these chimeras by p38 $alpha$ and p38 $beta$ ₂ (Fig. 6C and G, lanes 2 and 4), whereas the MEFD(M2)and ElkD peptides were ineffectual competitors (Fig. 6C and G,lanes 3 and 5). These results are essentially the same as thoseobserved with wild-type GST-MEF2A (Fig. 6B), thereby demonstratingthat the MEF2A D-domain acts in a similar manner to permit p38 $alpha$ and p38 $beta$ ₂ binding in a heterologouscontext.

The analogous GAL4 fusion proteins were subsequently analyzed for their activation by p38 $alpha$ (data not shown) and p38 $beta$ ₂ (Fig.6D and H) in vivo. All these GAL4 derivatives are expressed tosimilar levels (Fig. 6D and H, bottom panels). GAL4-Elk-1 $Delta$ D, whichlacks the kinase docking domain, is moderately activated by theERK and p38 pathways (Fig. 6D) (37, 38). In comparison, GAL4-MEF2A-Elk-1exhibits greatly enhanced transcriptional activation in responseto MKK6/p38 $beta$ ₂-mediated stimulation in vivo (Fig. 6D), whereasthe response to MEK/ERK-mediated stimulation barely changes (Fig.6D). Similarly, c-Jun is usually activated by the JNK pathwaybut only poorly by the p38 $beta$ ₂ pathway in vivo. However, reciprocaleffects are seen with the MEF2A-cJun chimera, which is efficientlyactivated by the p38 $beta$ ₂ pathway but in comparison is poorly activatedby the JNK pathway (Fig. 6H).

Taken together, the results clearly demonstrate that the D-domain of MEF2A is sufficient to confer responsiveness to the p38 $alpha$ and p38 $beta$ ₂ signalling pathways in heterologous contexts both invitro and invivo.

The p38-binding domain of MEF2A directs phosphorylation of key phosphoacceptor motifs. The D-domain of MEF2A is sufficient to permit the targeting of p38 $alpha$ and p38 $beta$ ₂ MAP kinases to heterologous substrates. In orderto demonstrate that physiologically relevant residues are targetedfor phosphorylation by the D-domain, we investigated the phosphorylationof Ser383 in MEF2A-Elk-1 chimeras, which has been shown to beone of the key residues which must be phosphorylated to triggerthe DNA binding and transcriptional activation properties of Elk-1(reviewed in reference 33). The phosphorylation of Ser383 wasassessed by Western blotting with a phospho-Elk-1(Ser383)antibody.

Firstly, GST-MEF2A-Elk-1 was phosphorylated by p38 $beta$ ₂ in vitro. In comparison to GST-Elk-1 $Delta$ D, which lacks a p38 docking site,GST-MEF2A-Elk-1 was efficiently phosphorylated on Ser383 (Fig.7A). In order to analyze whether the same effect could be observedin vivo, the phosphorylation of GAL4-MEF2A-Elk-1 was comparedto the phosphorylation of GAL4-Elk-1 in the presence of cotransfectedMKK6/p38 $beta$ ₂ (Fig. 7B). The overall phosphorylation of Elk-1 wasgreater in the presence of the D-domain from MEF2A (Fig. 7B; comparelanes 2 and 4, bottom panel). Moreover, the phosphorylation ofSer383 was greatly enhanced in the GAL4-MEF2A-Elk-1 chimera (Fig.7B; compare lanes 2 and 4, top panel).

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FIG. 7. The p38-binding domain of MEF2A directs the phosphorylation of the key phosphoacceptor motifs in MEF2A-Elk-1 chimeras. (A) In vitro kinase assays of GST fusion proteins (5 pmol of each substrate) by p38 $beta$ ₂ MAP kinase were carried out for 15 min. Phosphorylation of Ser383 was detected by Western blotting with an anti-phospho-Elk-1(Ser383) antibody. (B) In vivo phosphorylation of MEF2A-Elk-1 chimeras. 293 cells were transfected with vectors encoding GAL-Elk-1 or GAL-MEF2A-Elk-1 and a GAL4-driven luciferase reporter plasmid and, where indicated, p38 $beta$ ₂ and MKK6(E). The phosphorylation of the Elk-1 moiety at Ser383 in cell extracts was detected by Western blotting as in panel A (top panel), and the total levels of each GAL4 fusion protein were detected with an anti-GAL4 antibody (bottom panel). The locations of the bands corresponding to nonphosphorylated and phosphorylated GAL4 fusion proteins are indicated.

Furthermore, in the MEF2A-cJun chimeras analyzed in Fig. 6, there are only two potential phosphoacceptor motifs in the c-Junmoiety which correspond to the physiologically relevant sites.Together these results therefore demonstrate that in additionto enhancing the overall efficiency of substrate phosphorylationby p38 $alpha$ and p38 $beta$ ₂, the MEF2A D-domain also directs the phosphorylationof physiologically relevant sites in vitro and invivo.

The kinase docking domain determines the specificity of MAP kinases towards MEF2A. The kinase docking domain of MEF2A is sufficient to change the specificity of heterologous proteins as substrates for phosphorylationand activation by different MAP kinases. Reciprocal constructswere made in which either known or putative kinase docking domainsfrom other transcription factors were fused to the transcriptionactivation domain of MEF2A (Fig. 8A and C). Firstly, the homologousregion of MEF2B was substituted for the kinase docking domainof MEF2A (Fig. 8A), and the resulting chimeric protein was testedas a substrate for p38 MAP kinases. In contrast to MEF2A, MEF2Bappears not to be phosphorylated by p38 MAP kinases (Fig. 8B;compare lanes 1 and 3). Moreover, the putative kinase dockingdomain in MEF2B is unable to permit the efficient phosphorylationof MEF2A in the GST-MEF2B-MEF2A chimera (Fig. 8B, lane 2). Thus,the amino acid sequence differences in this region of MEF2B inactivateits ability to act as a kinase binding motif.

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FIG. 8. The identity of the kinase docking domain determines the specificity of MAP kinases towards MEF2A. (A) Diagrammatic illustration of GST fusions to MEF2B, the MEF2B-MEF2A chimera, and MEF2A. The numbers of the N- and C-terminal MEF2A (italics) and MEF2B (roman type) amino acids are indicated above and below each construct. The p38-binding motifs in MEF2A and MEF2B are indicated by black and grey boxes, respectively, the amino acid sequences of these regions in MEF2A, MEF2B, MEF2C and MEF2D are shown, and identical residues are highlighted. (B) Kinase assays with the indicated GST fusion proteins and p38 MAP kinases were carried out as described in the legend to Fig. 1. (C) Diagram illustrating fusions of GST to MEF2A and MEF2A $Delta$ D and the chimeric proteins cJun $delta$ -MEF2A, SAPD-MEF2A, and ElkD-MEF2A. These constructs contain the transcriptional activation domain of MEF2A and the kinase docking domain of cJun ( $delta$ ), SAP-1 (D), Elk-1 (white box), MEF2A (black box), or no docking site, respectively. The numbers of the N- and C-terminal c-Jun/SAP-1/Elk-1 (italics) and MEF2A (roman type) amino acids are indicated above and below each construct, respectively. (D) Kinase assays with the indicated chimeric GST fusion proteins as substrates for MAP kinases (as indicated on the right) were carried out with 5 pmol of each protein for 15-min reactions as described in the legend to Fig. 1.

The MAP kinase docking domains from c-Jun (for JNK MAP kinases) (4, 12, 13), SAP-1 (for ERK, p38 $alpha$ , and p38 $beta$ ₂ MAP kinases)(5a), and Elk-1 (for JNK and ERK MAP kinases) (37, 38) werefused with the transcriptional activation domain of MEF2A (Fig.8C) and tested as substrates for different MAP kinases (Fig. 8D).MEF2A is phosphorylated efficiently by p38 $alpha$ and p38 $beta$ ₂ but is apoor substrate for the ERK and JNK MAP kinases (Fig. 8D, lane4, and Fig. 1). However, in the absence of the D-domain, MEF2Ais a poor substrate for all of these MAP kinases (Fig. 8D, lane5, and Fig. 2). Significantly, the introduction of the c-Jun $delta$ -domainconverts MEF2A into a good JNK substrate (Fig. 8D, lane 1). Similarly,the ElkD-MEF2A chimera is a good JNK substrate (Fig. 8D, lane3). In contrast, the fusion of the SAP-1 D-domain to MEF2A restoresits ability to act as a substrate for p38 $alpha$ and p38 $beta$ ₂ (Fig. 8D,lane 2). None of the chimeric proteins are good ERK2 substrates(Fig. 8D, top panel), indicating that the docking site alone isinsufficient to permit the targeting of ERK MAP kinases (seeDiscussion).

Together these results demonstrate that the docking domains from several different transcription factors can direct the targetingof specific subsets of stress-activated MAP kinases to MEF2A.Thus, MAP kinase docking sites appear to be common, conservedelements in transcription factors which can act as independentdomains and contribute significantly to the specificity of actionof the diverse MAP kinasecascades.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The MAP kinase cascades play important roles in regulating multiple diverse cellular processes. However, as different MAPkinases all phosphorylate similar sites containing the minimalconsensus motif (Ser/Thr)-Pro, it is unclear how substrate specificityis achieved. It has recently been shown that one component ofthis specificity-determining mechanism for the JNK and ERK MAPkinases involves binding of the MAP kinases to a docking domainon their nuclear targets (3, 4, 6, 7, 12, 13,26, 37, 38). In this study, we demonstrate that membersof the p38 subclass of MAP kinases are targeted to the transcriptionfactors MEF2A and MEF2C by a docking domain which is distinctfrom the phosphoacceptor motifs. This domain is sufficient toconfer p38 responsiveness on heterologous substrates and can befunctionally replaced by alternative kinase docking motifs fromother transcription factors. Similarly, a docking site in ATF-2is required for efficient activation by p38 $alpha$ (11a). Our resultstherefore demonstrate the generality of the phenomenon of MAPkinase docking with transcription factors as a major part of themechanism of substrate specificitydetermination.

MAP kinase docking domains. The sequence of the MAP kinase docking domain in MEF2A and MEF2C is highly conserved between these two proteins (Fig. 8A)and is also evolutionarily conserved in the Drosophila MEF2 homologue(28). This sequence conservation is reflected by the functionalconservation of these domains as docking sites for both p38 $alpha$ andp38 $beta$ ₂ (Fig. 2). However, neither domain appears to be a dockingsite for p38 $gamma$ (Fig. 2A and B) and p38 $delta$ (data not shown), as theirdeletion does not affect the efficiency of phosphorylation ofMEF2A and MEF2C. It is unclear whether p38 $gamma$ uses a different dockingdomain or alternatively, as suggested by in vivo experiments (Fig.1) (39), MEF2A and MEF2C do not represent true substrates forthis kinase. A similar phenomenon has been noted for Elk-1, forwhich it was proposed that the lack of a targeting domain forthe p38 MAP kinases is reflected in its poor response to the p38pathways in vivo (38).

Residues throughout the docking domain are important in targeting p38 $alpha$ and p38 $beta$ ₂ to MEF2A (Fig. 3 and 4), and in common withother kinase docking domains (37, 38), hydrophobic residuesplay the most important roles. Moreover, an excellent correlationexists between the ability of the docking site to permit efficientphosphorylation in vitro and transcriptional activation in vivo(compare Fig. 2A and B, Fig. 2C and D, and Fig. 3B and C and D),indicating the functional importance of these sites. The specificityof action of the D-domain of MEF2A towards p38 $alpha$ and p38 $beta$ ₂ subtypesin vitro and in vivo was demonstrated by using chimeric transcriptionfactors which contain the MEF2A docking domain and transcriptionalactivation domains of different proteins (Fig. 6 and 7). Neitherthe JNK nor the ERK MAP kinases can be targeted to transcriptionfactors by the MAP kinase docking domain from MEF2A. However,by using reciprocal chimeric proteins with the MEF2A transcriptionalactivation domain and the kinase docking domains of either c-Jun,Elk-1, or SAP-1, the propensity of MEF2A as a substrate for theJNK and p38 MAP kinases can be altered in a manner which is predictablefrom the known characteristics of each domain (Fig. 8). Interestingly,MEF2A could not be converted into an ERK substrate by the inclusionof the ERK binding domain from Elk-1 (Fig. 8D), indicating thatthe docking domain itself is not sufficient to direct efficientphosphorylation. A similar chimeric protein with the c-Jun transcriptionalactivation domain is also not responsive to ERKs (38). Thismight reflect the requirement for additional docking componentssuch as that observed for ERK targeting to the ETS domain transcriptionfactors Elk-1 and LIN-1, which uses both a docking domain locatedN-terminally from the phosphoacceptor residues and an FXFP motiflocated C-terminally from these residues to target ERKs to theseproteins (11). Moreover, in addition to these docking domains,the local context of the phosphoacceptor motifs may also playa major role in determining substrate specificity towards MAPkinases as suggested previously for c-Jun (13). In MEF2A andc-Jun, the phosphoacceptor motifs presumably represent good JNK,p38 $alpha$ , and p38 $beta$ ₂ sites, and it is the presence of the correct dockingsite which ultimately determines which MAP kinase phosphorylatesthese transcription factors (Fig. 6F toH).

Recently, the existence of cytoplasmic MAP kinase modules has been proposed in yeast (reviewed in references 17 and 27)and mammals (35), in which the MAP kinases are stably associatedwith the upstream components in the cascade by specific dockingproteins. The identification of MAP kinase docking sites in nucleartranscription factors suggests that nuclear complexes might alsoexist. However, in general, MAP kinases do not appear to stablyassociate with transcription factors in their active state, withthe exception of ERK-2 and Elk-1 (37). Furthermore, the bindingof inactive kinases appears to be weak, as we are unable to detectsignificant stable binding of p38 $alpha$ to MEF2C or that of JNKs toc-Jun under standard binding conditions, although others havedetected these interactions (3, 4, 7, 9, 12, 13).However, binding can be directly inferred from peptide competitionexperiments (Fig. 4A and 5C and G) (38).

To date, MAP kinase targeting domains have been identified in c-Jun (3, 4, 7, 12, 13), Elk-1 (37, 38), SAP-1(5a), MEF2A (this study), and ATF-2 (6, 7, 11a, 15).In all cases, the docking site is located immediately N-terminallyto the phosphoacceptor motifs within the transcriptional activationdomain. It remains unclear whether this positioning is functionallysignificant or reflects the evolutionary conservation of a MAPkinase recognition module. In c-Jun, a spacer can be insertedbetween the docking domain and its transcriptional activationdomain (13), and in Elk-1 deletions can be made between thesemodules (5a) without changing their proficiency as MAP kinasesubstrates. Recently, an additional docking domain has been identifiedin several substrates, which is located C-terminally from thephosphoacceptor motifs (11). Further systematic studies, however,are required to examine the requirement for specific spatial alignmentof the docking domains and phosphoacceptormotifs.

Activation of MEF2 family members by the p38 MAP kinases. The MEF2 subfamily of MADS-box transcription factors is composed of four members: MEF2A, MEF2B, MEF2C, and MEF2D (reviewedin references 19 and 24). Of these, MEF2A and MEF2C exhibitsignificant sequence conservation throughout their lengths ( $approx$ 56%identity), including that within their transcription activationdomains and the MAP kinase phosphorylation sites, which have beenshown to be functionally important in MEF2C. Both p38 $alpha$ (8)and ERK5/BMK (14, 36) have been shown to phosphorylate andenhance the transcriptional activation potential of MEF2C. MEF2Dcontains the sites for p38 $alpha$ but lacks the site for ERK5/BMK, whileMEF2B appears to contain only one of the p38 $alpha$ phosphoacceptormotifs. Here we demonstrate that p38 $alpha$ phosphorylates and activatesthe transcription activation domains of both MEF2A and MEF2C andrequires targeting by a docking domain. Similarly, p38 $beta$ ₂ activatesboth these transcription factors and requires docking via thesame domain. Neither p38 $gamma$ nor p38 $delta$ efficiently phosphorylatesand activates MEF2A and MEF2C. Thus, only a subset of p38 MAPkinase subtypes activate the transcriptional activation domainof MEF2A and MEF2C. Similarly, neither the ERK nor JNK MAP kinasessignificantly activate MEF2A and MEF2C (Fig. 1D andE).

Our data are consistent with the findings of two independent studies, which demonstrate that MEF2A is a p38 $alpha$ substrate (18a,39), although this study is different in that we clearly demonstratethat p38 $beta$ ₂ phosphorylates and activates MEF2A, whereas p38 $beta$ ₁ apparentlydoes not phosphorylate MEF2A (39). This discrepancy might beattributable to the differences observed between p38 $beta$ ₁ and p38 $beta$ ₂(identical apart from an 8-amino-acid deletion in p38 $beta$ ₁), whichconfer on p38 $beta$ ₂ the ability to phosphorylate other substratesmore efficiently than p38 $beta$ ₁ (5). MEF2B lacks one of the p38 $alpha$ phosphorylation sites found in MEF2A and MEF2C but still exhibitssome sequence similarity with the D-domain of MEF2A/C (Fig. 8A).However, MEF2B is a poor substrate for the p38 MAP kinases (Fig.8B). Moreover, the putative MAP kinase docking site is unableto act as a p38 docking motif in a heterologous substrate (Fig.8B). Thus, MEF2B differs from MEF2A and MEF2C, as it is unableto either recruit p38 MAP kinases or act as a p38 substrate. Itis currently unknown whether MEF2D is regulated by p38 MAP kinasesubtypes, although from sequence conservation, it might representa p38 $alpha$ and p38 $beta$ ₂ substrate, as both the phosphoacceptor motifsand the docking domain are conserved. However, in the case ofthe docking domain, sufficient differences exist (especially inthe C-terminal half) to suggest that its MAP kinase targetingproperties might differ from those of MEF2A and MEF2C (Fig. 8A).MEF2D, however, lacks the C-terminal ERK5/BMK phosphoacceptormotif. Interestingly, MEF2A and MEF2C have been shown to physicallyassociate with ERK5/BMK (36) via a motif contained within theminimal DNA-binding domain, which is distinct from the dockingsites described here. However, the functional consequences ofthis interaction have not been investigated. As MEF2 proteinsact as dimers and can associate to form different combinationsof heterodimers, the resulting complexes will respond differentlyto different MAP kinase cascades, depending on the docking domainsand phosphoacceptor motifs present in each subset. Such diversityin response to p38 MAP kinase cascades might contribute to differentresponses by alternative MEF2-containing heterodimers. The activationof MEF2C by p38 $alpha$ , it has been proposed, is important in inflammatoryresponses in the immune system (8). In addition, the activationof MEF2C by ERK5/BMK has been shown to be an important part ofthe mechanism of serum induction of the c-jun promoter. As theMEF2 proteins play a major role in regulating muscle-specificgene expression (19), it will be interesting to discover whetherp38 $alpha$ and/or p38 $beta$ ₂-mediated signalling to MEF2 proteins plays arole in muscle differentiation and/or proliferation during developmentor in response todamage.

Conclusion. It is becoming clear that the binding of MAP kinases to transcription factors is a critical determinant of their specificity.Here we demonstrate the selective targeting of p38 $alpha$ and p38 $beta$ ₂MAP kinases to MEF2A and MEF2C by binding to a distinct dockingdomain and that this binding is an important determinant of theefficiency of p38 $alpha$ - and p38 $beta$ ₂-mediated phosphorylation of MEF2Aand MEF2C in vitro and transcriptional activation in vivo. Membersof three classes of MAP kinases in mammals (ERK, JNK, and p38)have now been shown to require docking sites on transcriptionfactors for their correct function. It is likely that such interactionswill prove to be essential specificity determinants in other MAPkinase-transcription factor signallingmodules.

	ACKNOWLEDGMENTS

We thank Margaret Bell and Katherine Stewart for excellent technical and secretarial assistance and Bob Liddell for DNA sequencing.We are grateful to John McDermott, Alan Whitmarsh, and membersof our laboratories for comments on the manuscript and for stimulatingdiscussions and to Nic Jones and John McDermott for communicatingdata prior to publication. We also thank Adam West for help withthe inception of this project and Fei-Ling Lim for constructingsome of the intermediate plasmids. We are grateful to Stuart Lipton,Richard Treisman, Alan Whitmarsh, and Roger Davis for providingreagents and to Simon Ridley for helpful advice about p38activation.

This work was supported by the North of England Cancer Research Campaign, the Cancer Research Campaign (CRC), the WellcomeTrust, and a Jeffcock Ph.D. studentship from the University ofNewcastle Upon Tyne to A.G. A.D.S. is a Research Fellow of theLister Institute of PreventativeMedicine.

	FOOTNOTES

^* Corresponding author. Present address: School of Biological Sciences, 2.205 Stopford Building, University of Manchester, OxfordRd., Manchester M13 9PT, United Kingdom. Phone: 0044-161 275 5979.Fax: 0044-161 275 5082. E-mail: a.d.sharrocks{at}man.ac.uk.

Present address: School of Biological Sciences, University of Manchester, Manchester M13 9PT, UnitedKingdom.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

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