The Dual Specificity JKAP Specifically Activates the c-Jun N-terminal Kinase Pathway

doi:10.1074/jbc.M200453200

Ideal method for primary cell transfection

The Dual Specificity JKAP Specifically Activates the c-Jun N-terminal Kinase Pathway^*

Alice J. Chen^§^¶, Guisheng Zhou^¶, Todd Juan^**, Suzanne M. Colicos, John P. Cannon, Maria Cabriera-Hansen, Christian F. Meyer, Roland Jurecic, Neal G. Copeland^§§, Debra J. Gilbert^§§, Nancy A. Jenkins^§§, Fred Fletcher^**, Tse-Hua Tan^¶¶, and John W. Belmont

From the Department of Molecular and Human Genetics and the Department of Immunology, Baylor College of Medicine, Houston, Texas 77030, the ^** Department of Experimental Hematology, Amgen, Inc., Thousand Oaks, California 91320, and the ^§§ Mammalian Genetics Laboratory, ABL-Basic Research Program, NCI-Frederick Cancer Research and Development Center, Frederick, Maryland 21702

Received for publication, January 15, 2002, and in revised form, July 17, 2002

ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The involvement of dual specificity phosphatases (DSPs) in the mitogen-activated protein kinase (MAPK) signaling has beenmostly limited to the inactivation of MAPKs by the direct dephosphorylationof the TXY motif within their activation loop. We report the cloningand characterization of a murine DSP, called JNK pathway-associatedphosphatase (JKAP), which lacks the regulatory region presentin most other MAP kinase phosphatases (MKPs) and is preferentiallyexpressed in murine LinSca-1⁺ stem cells. Overexpression of JKAP in human embryonic kidney293T cells specifically activated c-Jun N-terminal kinase (JNK)but not p38 and extracellular signal-regulated kinase 2. Overexpressionof a mutant JKAP, JKAP-C88S, blocked tumor necrosis factor- $alpha$ -inducedJNK activation. Targeted gene disruption in murine embryonic stemcells abolished JNK activation by tumor necrosis factor- $alpha$ andtransforming growth factor- $beta$ , but not by ultraviolet-C irradiation,indicating that JKAP is necessary for optimal JNK activation.JKAP associated with JNK and MKK7, but not SEK1, in vivo. However,JKAP did not interact with JNK in vitro, suggesting that JKAPexerts its effect on JNK in an indirect manner. Taken together,these studies identify a positive regulator for the JNK pathwayand suggest a novel role for DSP in mitogen-activated proteinkinaseregulation.

INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The evolutionarily conserved mitogen-activated protein kinase (MAPK)¹ family consists of extracellular signal-regulated kinase (ERK),c-Jun N-terminal kinase (JNK), and p38 kinase. MAPKs are activatedby a wide range of diverse stimuli and are essential for variouscellular processes, such as stress responses, apoptosis, proliferation,differentiation, and early embryonic development (1-3). The prototypicalMAPK signaling cascade is a three-kinase module, consisting ofMAP kinase kinase kinase (MAP3K), MAP kinase kinase (MAP2K), andMAPK (1, 2, 4). The upstream molecules that link theMAPK module to extracellular stimuli include small G proteinsand a group of mammalian Ste20-like kinases, including hematopoieticprogenitor kinase 1 (HPK1), germinal center kinase (GCK), HKP1/germinalcenter kinase-like kinase, germinal center kinase-like kinase(GLK), and kinase homologous to Ste20 (KHS), which have been characterizedas potential MAP kinase kinase kinase kinases (MAP4Ks) for theJNK pathway (1, 2, 4, 5). Within the three-kinasemodule, MAPKs are phosphorylated on both threonine and tyrosineresidues within their signature sequence TXY motif by a dual specificityprotein kinase MAP2K. These motifs include TEY in ERK, TPY inJNK, and TGY in p38. MAP2K are activated by phosphorylation ofserine/threonine residues by MAP3Ks (1, 2, 4). In thecase of ERK1/2, phosphorylation of the TEY motif also contributesto the dimerization and nuclear translocation of ERK1/2 in additionto mediating its activation (6).

The extracellular stimuli-induced activation of MAPKs is transient under many conditions, and it has been well establishedthat protein phosphatases play an essential role in the down-regulationof MAP kinases. A variety of classes of protein phosphatases,including tyrosine-specific protein phosphatases, serine/threonineprotein phosphatases, and a family of dual specificity proteinphosphatases (DSPs), have been implicated in the negative regulationof MAPKs (7-9). Among them, DSPs are the major group of phosphatasesthat contribute to the regulated inactivation of MAP kinases bydephosphorylating both phosphotyrosine and phosphothreonine residueswithin the TXY motif, thus also called MAP kinase phosphatases(MKPs) (7-9). Most MKPs identified so far consist of a conservedcatalytic region and an extended regulatory region. However, someMKPs lack this regulatory region, such as VH1 (10) and VH1-related(VHR) phosphatase (11). The regulatory region of MKPs is responsiblefor substrate binding and thus makes MKPs display varying degreesof specificity for inactivating different MAP kinases. For example,MKP-3/PYST1 completely inactivates ERK1 and ERK2 but not JNK andp38 MAP kinases (12, 13), whereas M3/6 (13) and MKP-7 (14,15) appear to be highly specific for inactivating JNK and p38MAPkinases.

In addition to the phosphorylation that is necessary for kinase activation, the kinases within the MAPK cascade are also subjectto negative regulation by phosphorylation. It has been well documentedthat phosphorylation of Ser-259 and Ser-261 on Raf, a MAP3K kinasefor the ERK pathway, prevents the activation of Raf-1 (16-18).Apoptosis signal-regulated kinase 1 (ASK1), a MAP3K that stimulatesJNK and p38 signaling pathways, is subject to negative regulationby AKT-mediated phosphorylation (19). AKT-mediated phosphorylationof stress-activated protein kinase/ERK kinase 1 (SEK1) on Ser-78inhibits its activation and prevents its interaction with JNK,thereby suppressing the SEK1-mediated JNK signaling pathway (20).It has been recently shown that cyclin-dependent kinase 5 (cdk5)directly phosphorylates JNK3 on Thr-131 and inhibits its kinaseactivity and leads to reduced c-Jun phosphorylation (21). Thus,it is likely that some protein phosphatases are involved in positiveregulation of MAPKs by dephosphorylating those inhibitory phosphorylatedresidues. It has been shown that the Shp-2 tyrosine phosphataseis necessary for ERK activation by a number of growth factorsincluding insulin growth factor-1, platelet-derived growth factor,and epidermal growth factor (22). The protein serine/threoninephosphatase PP2A acts as a positive regulator for Raf-1 (17).We have recently shown that protein phosphatase 4 (PP4), anotherserine/threonine phosphatase, is positively involved in tumornecrosis factor (TNF)- $alpha$ -induced activation of the JNK pathway(23). Taken together, the MAPK activity is determined by thecombined influences of kinases and phosphatases, and both phosphorylationand dephosphorylation play essential roles in controlling theduration and magnitude of MAPK activity depending on the celltype andstimuli.

As the relationship between DSPs and MAPK is studied, the complexity of kinase regulation increases. For example, overexpressionof MKP1, which inactivates ERK, activates the ERK-upstream kinasesMKK1, MKK2, and Raf-1 (24). MKP-1 itself is controlled by ERK,which induces both MKP-1 stability and activity (25, 26).In an effort to isolate transcripts differentially up-regulatedin murine hematopoietic stem cells, we identified a dual specificityphosphatase, called the JNK pathway-associated phosphatase (JKAP),that specifically activates the JNK pathway and is required forthe cytokine-induced JNK activation. Moreover, Jkap deficiencyin murine bone marrow progenitor cells resulted in loss of sensitivityof the cells to inhibition of transforming growth factor (TGF)- $beta$ -inducedcolony-forming cells (CFCs). Taken together, our studies haveidentified a new DSP as a positive regulator for the JNK signalingpathway.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Reagents-- [ $gamma$ -³²P]ATP was purchased from ICN Biomedicals (Irvine, CA). An enhanced chemiluminescence system was purchased from AmershamBiosciences. TNF- $alpha$ and TGF- $beta$ were purchased from R & D Systems(Minneapolis, MN). Anti-HA antibody (12CA5) was purchased fromRoche Molecular Biochemicals. Anti-FLAG (M2) antibody was purchasedfrom Sigma. Monoclonal anti-c-Myc (9E10) was purchased from SantaCruz Biotechnology, Inc. (Santa Cruz, CA). Anti-GST antibody waspurchased from abcam Ltd. (Cambridge, UK). Anti-JNK1 antibody(Ab101) was described previously (27, 28). All other chemicalreagents were purchased from Sigma unless otherwisenoted.

Plasmids-- The GST-Jun-(1-79) was a gift from Dr. M. Karin (University of California San Diego), and GST-SEK1 was a gift from Dr. L.I. Zon (Children's Hospital, Boston, MA). GST-ATF2-(1-96) andpHA-ERK2 were provided by Dr. J. S. Gutkind (National Institutesof Health, Bethesda, MD). GST-JNK (also called GST-stress-activatedprotein kinase (GST-SAKP)) was a gift from Dr. D. J. Templeton(University of Virginia Medical School, Charlottesville, VA).pHA-MKK6 was provided by Dr. Z. Yao (Amgen, Boulder, CO). pHA-proteinkinase C- $iota$ was a gift from Dr. Marie W. Wooten (Auburn University);cRaf-BXB was kindly provided by Dr. J. Bruder (GenVec, Rockville,MD). pHA-JNK1 and HA-p38 were gifts from Dr. J. Woodgett (OntarioCancer Institute, Toronto, Canada). pMTSM-Myc-M3/6 was a giftfrom Dr. K. E. Davis (University of Oxford, Oxford, UK) (27).

Cells and Transfection-- Human embryonic kidney 293T (HEK293T) cells were obtained from the American Type Culture Collection (Manassas, VA) and grownin Dulbecco's modified Eagle's medium supplemented with 10% fetalcalf serum and 100 units/ml streptomycin/penicillin at 37 °C ina humidified atmosphere of 5% CO₂. HEK293T cells were plated ata density of either 1.5 × 10⁵ cells/35-mm plate well or 1.5 × 10⁶ cells/100-mm dish and transfected the next day using the modifiedcalcium phosphate precipitation protocol (Specialty Media, Inc.,Lavallette, NJ). Cells were transfected with plasmids encoding $beta$ -galactosidase (0.15 µg) in combination with an empty vectoror various amounts of plasmids encoding phosphatases, phosphatasemutants, kinases, or kinase mutants as indicated in the figurelegends.

Coimmunoprecipitation, Immunocomplex Kinase Assays, Western Blot Analysis, and Phosphatase Assays-- Coimmunoprecipitation and immunocomplex kinase assays were performed as described previously (29, 30). Western blot analysiswas performed using an enhanced chemiluminescence detection kitaccording to the manufacturer's protocols (Amersham Biosciences).The phosphatase activities of Myc-JKAP and Myc-JKAP-C88S wereassayed at 30 °C using p-nitrophenyl phosphate (pNPP) as a substrate.HEK293T cells (1.5 × 10⁶ in 100-mm dishes) were transfected with a vector control, Myc-JKAP,or Myc-JKAP-C88S. Myc-JKAP and Myc-JKAP-C88S were immunoprecipitatedwith an anti-Myc antibody. The immunoprecipitants were then incubatedwith 1 ml of 50 mM imidazole (pH 7.5) with 10 mM dithiothreitol,20 mM pNPP for 1 h at 30 °C. The reactions were terminated bythe addition of 0.1 N NaOH, and the hydrolyzed pNPP was quantifiedby measurement of spectrophotometric absorbance at 410nm.

Interspecific Mouse Backcross Analysis-- Interspecific mouse backcross mapping was performed as described (31, 32) using progeny derived from matings of (C57BL/6J× Mus spretus)F₁ × C57BL/6J mice. The presence or absence of aM. spretus-specific 12.5-kb BglII fragment, detected by a probecorresponding to nucleotide positions 2251-2566 of the Jkap cDNA,was followed in backcross progeny. A total of 205 N₂ mice wereused to map the Jkap locus. Recombination distances were calculatedusing Map Manager, version 2.6.5.

Construction of Mammalian Expression Clone-- An 851-bp EaeI fragment from the Jkap cDNA, consisting of the coding region and 200 bp of 3'-untranslated region, was clonedinto the mammalian expression vector pCI-neo (Promega), linearizedat the NotI site, generating pCI-JKAP. The mutant pCI-JKAP-C88Swas generated by PCR mutagenesis with pCI-JKAP, using mutagenicprimers covering the site (cysteine 88) of the amino acid change,a 5' amplification primer in the vector backbone, and a 3' amplificationprimer in the 3'-untranslatedregion.

Construction of Targeting Clone-- To generate the plasmid backbone, pNeoUSEFUL, the 1.35-kb XhoI fragment (neo) of pPol2Sneo (provided by P. Soriano) was blunted,cloned into the EcoRV site of pBluescript-SK( $-$ ), reisolated withBamHI and SalI, and finally cloned into pUSEFUL (provided by A.Bradley) cut with BamHI and SalI (releasing pGK-hprt and leavingthymidine kinase and unique cloning sites intact). The 3' arm,a subcloned 2.8-kb SalI-XbaI fragment consisting of Jkap genomicand cDNA sequence immediately after the second targeted exon,was then blunted and cloned into the BamHI site, also blunted,of pNeoUSEFUL, generating clone B2.8-8-1. The 5' arm, a subcloned5.0-kb XbaI fragment consisting of genomic Jkap sequence immediatelybefore the first targeted exon, was cloned into intermediate plasmidCXS (pSA $beta$ geo, provided by P. Soriano; cut with HindIII and XbaI,blunted, and recircularized), cut with XbaI. The fragment wasreisolated with ClaI and SalI and cloned into B2.8-8-1 cut withClaI and SalI, generating clone B8/4-1, the targetingvector.

Generation of Jkap-targeted Murine Embryonic Stem (ES) Cells and Murine Embryonic Fibroblast (MEF) Cells-- Targeted ES cell clones were generated essentially as described (33). Briefly, a targeting vector was designed that deletesthe two coding exons of JKAP, which encode the catalytic domainof the phosphatase. The vector was constructed using DNA froma murine 129/SV/EV total genomic DNA library. This vector waselectroporated into AB2.2 ES cells derived from 129/SV/EV mice.Resulting clones were screened by Southern blot analysis for evidenceof homologous recombination. Several independent targeted cloneswere obtained. Homozygous JKAP^/ ES clones were obtained by superselection in 1.5 mg/ml G418 andconfirmed by Southern blotting. Jkap^/ animals were derived by breeding Jkap^+/ ES cell chimeras with wild-type 129SvEvBrd female animals. Becausethe AB2.2. ES line was derived from the same strain of the 129SvEvBrdfemale animals, the resulting animals were inbred with respectto all background loci. Jkap^/ animals were born in expected Mendelian ratios (data not shown)and remained overtly healthy through adultlife.

TGF- $beta$ 1 Growth Inhibition Studies-- Early passage (passages 3-6) MEF derived from embryonic day 12.5 Jkap-1^/ embryos were cultured in Dulbecco's modified Eagle's medium with10% fetal bovine serum. 2 × 10⁴ cells were plated, transferred into each well of a 24-well tissueculture dish. After 24 h, triplicate cultures were treated withvariable amounts of TGF- $beta$ 1 (R & D Systems) diluted in 4 mM HClor with diluant only (controls). Cells were then pulsed with 4mCi of [³H]thymidine for 12 h. The percentage decrease in thymidine incorporationin the TGF-treated samples relative to the untreated controlswas scored in six independent experiments. Bone marrow cells werecollected from tibias and femurs of 6-8-week-old Jkap-1^/ and Jkap-1^+/+ littermate controls. Mononucleated cells were isolated by buoyantgradient centrifugation (Histopaque; Sigma). Mononucleated cells(10⁴ cells/ml) were plated in semisolid media (Methocult; StemCellTechnologies) containing 1% methyl-cellose in Iscove's modifiedDulbecco's medium, supplemented with 15% fetal calf serum, 10⁴ M 2-mercaptoethanol, L-glutamine, 1% bovine serum albumin, 10µg/ml bovine pancreatic insulin, 200 µg/ml human transferrin,50 ng/ml stem cell factor, 10 ng/ml interleukin-3, 10 ng/ml interleukin-6,and 3 units/ml erythropoietin. Cultures in duplicate to quadruplicatewere done with or without various concentrations of TGF- $beta$ in a37 °C 5% CO₂ humidified chamber. At day 10, the total number ofcolonies was scored. The TGF- $beta$ activity was measured by the percentageof inhibition observed in treated cultures relative to their respectiveuntreatedcontrols.

In Vitro Binding Assays-- GST and GST-JNK fusion protein were immobilized on glutathione-Sepharose 4B beads equilibrated in incubation buffer containing20 mM Tris-HCl (pH 8.0), 100 mM NaCl, 1 mM EDTA, 0.5% NonidetP-40, 1 mM dithiothreitol, 0.5 mM phenylmethylsulfonyl fluoride,1 µg/ml leupeptin, and 2 µg/ml aprotinin. Cell lysates (600 µg)from HEK293T cells transiently transfected with Myc-JKAP or Myc-M3/6were incubated with GST-JNK fusion protein or GST-4T-Sepharosebeads in incubation buffer containing 3 mg/ml bovine serum albuminat 4 °C for 2 h. The beads were washed five times with the incubationbuffer, boiled in an SDS-PAGE loading buffer for 5 min, resolvedby 10% SDS-PAGE, transferred to polyvinylidene difluoride membranes,and then subjected to Western blotting with an anti-Myc antibody.The membrane was then stripped with stripping buffer (62.5 mMTris-HCl (pH 6.7), 100 mM 2-mercaptoethanol, 2% SDS) and reprobedwith an anti-GSTantibody.

RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Isolation of a Putative MAPK Phosphatase Gene, jkap, Preferentially Expressed in Murine LinSca-1⁺ Stem Cells-- In an effort to isolate transcripts differentially up-regulated in murine hematopoietic stem cells by employing differentialdisplay PCR, we identified the Jkap transcript, among others,as being expressed preferentially in the stem cell-enriched LinSca-1⁺ population of murine bone marrow cells obtained by fluorescence-activatedcell sorting, compared with the LinSca-1 population, which is deficient in pluripotent stem cell activity.Lin (i.e. lineage negative) refers to the absence of cell surfaceexpression of CD4, CD8, B220, Mac-1, GR-1, and Ter115, which areexpressed upon commitment to helper T cell, killer T cell, B cell,macrophage, granulocyte, and erythrocyte lineages, respectively.Sca-1⁺ or Sca-1 refers the presence or absence of cell surface expression ofstem cell antigen 1 encoded by Ly6A2. A full-length murine JkapcDNA consisting of 3012 bp was obtained by screening an adultmuscle cDNA library. This cDNA contained a 700-bp open readingframe with similarity to a subgroup of protein phosphatases, dualspecificity phosphatases, that have activities in the MAPK pathways(Fig. 1A). The human orthologue of Jkap was subsequently identified.The inferred murine and human JKAP amino acid sequences are 89%identical (Fig. 1A). The predicted JKAP protein contains the catalyticC-terminal domain of dual specificity phosphatases but lacks anN-terminal noncatalytic domain and is consequently ~100 aminoacid shorter than most other MAPK phosphatases. All residues ofthe signature motif I/VHCXXGXSRS of dual specificity phosphatases(34, 35) are conserved in the JKAP protein (Fig. 1, A andB). Within the phosphatase catalytic domain, JKAP displayed 31-39%amino acid identity to other MKPs (Fig. 1C). A phylogenetic comparisonof MAPK DUSP was carried out using a recently described methodthat employs Baysian inference to assess the reliability of theresulting tree. This analysis suggests that JKAP is a mouse orthologueof recently described human DSP, JNK-stimulatory phosphatase 1(JSP-1) (36), and that JKAP/JSP-1 is distinctive in its catalyticmotif, with the relationship to human VHR moderately supported(clade credibility 77%) (Fig. 1D). By interspecific mouse backcrossanalysis, Jkap mapped to the proximal region of mouse chromosome13. Jkap is linked to Btn, Fim1, and Edn1, with the followingrecombination frequencies, expressed as genetic distances in centimorgans± S.E.: centromere-Btn-1.3 ± 0.9-Fim1-3.5 ± 1.4-Jkap-8.6 ± 2.1-Edn1.The human orthologue of Jkap was subsequently identified, andthe inferred map position in chromosome 6p (based on the currenthuman genome sequence assembly available in the public data base)is consistent with known mouse and human synteny.

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Fig. 1. JKAP sequence analysis. A, JKAP is a dual specificity phosphatase. Amino acid sequences corresponding to the catalytic domains of JKAP and selected MKPs were aligned in ClustalW version 1.8. The catalytic signature motifs are indicated by a shaded box. GenBank^TM protein sequence accession numbers are as follows: DUSP9 (MKP-4), Q99956; DUSP6 (MKP-3), XP038308; DUSP7 (MKP-X), XP037430; DUSP3 (human VHR), P51452; SKRP1, AB063186; DUSP10 (MKP-5), XP039625; DUSP5 (hVH3), Q16690; DUSP12 (YVH-1), XP001951; DUSP14 (MKP-6), NP008957; DUSP4 (MKP-2), XP027545; DUSP1 (MKP-1), XP001951; DUSP2 (PAC-1), Q05923; DUSP8 (hVH-5, M3/6), DUSP8 (hVH-5, M3/6), Q13202; MKP-7, XP039106. B, JKAP is a mouse orthologue of human JSP-1. Full-length amino acid sequences of mouse JKAP, human JKAP, and human JSP-1 (AAL18850) are aligned. The catalytic signature motifs are indicated by a shaded box. The conserved amino acids are indicated by asterisks on the consensus line. C, schematic representation of JKAP amino acid identity with other MKPs. Cdc25 homology domain 2 (CH2) domains and phosphatase catalytic domains are indicated by black and open boxes, respectively. The numbers represent the percentage of JKAP amino acid identity with other MKPs within the phosphatase catalytic domain. D, phylogenetic comparison of the catalytic domains of MKPs. Aligned sequences encompassing the entire catalytic domain of each MKP were prepared in ClustalW and manually edited. Sequence affinities were then estimated by Bayesian phylogenetic inference using Metropolis-coupled Markov chain Monte Carlo methods implemented in MRBAYES version 2.01. The consensus tree resulted from an estimate of the posterior probabilities after 500,000 replicates with burn in of 50,000 replicates (27).

Tissue Distribution of JKAP mRNA-- The expression pattern of JKAP mRNA in mouse tissues was examined by Northern blot analysis using mouse JKAP cDNA probe. Asshown in Fig. 2, two mRNA species of 3.0 and 1.3 kb were detected.The longer 3.0-kb transcript was abundantly expressed in the heart,brain, liver, and kidney but expressed at low levels in the testisand skeletal muscle. The shorter 1.3-kb transcript was abundantlyexpressed in the testis and liver and, to a lesser extent, inthe kidney and heart. Neither 3.0-kb transcript nor 1.3-kb transcriptwas detected in the spleen. The broad expression of JKAP impliesthat JKAP functions in a wide range of tissues in the adult mouse.The differential expression patterns of the 3.0- and 1.3-kb transcripts(e.g. only the 3.0-kb transcript in the brain and the 1.3-kb transcriptin the testis) indicate a tissue-specific splicing or processingof JKAP mRNA.

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Fig. 2. JKAP expression pattern. Polyadenylated mRNA from adult murine tissues was hybridized with a Jkap cDNA probe. mRNA integrity and quantity were confirmed by hybridization with $beta$ -actin. Molecular sizes in kilobase pairs are indicated on the left.

Jkap Is Expressed in Adult, but Not Embryonic, Murine Hematopoietic Stem Cells-- To further characterize the expression pattern of Jkap in murine tissues, we isolated LinSca-1⁺ and LinSca-1 cells from adult murine bone marrow by fluorescence-activatedcell sorting and performed in situ hybridization analysis witha Jkap antisense riboprobe. As expected, we confirmed that Jkapis preferentially expressed in LinSca-1⁺ cells, as compared with LinSca-1 cells (Fig. 3, A and B), suggesting a role for JKAP in hematopoieticprecursor cells. Whole-mount in situ hybridization of embryonicday 10.5 mouse embryos detected the highest levels of Jkap transcriptsin the somites and branchial arches (Fig. 3, C-E). No expressionwas observed in the embryonic dorsal aorta, a region identifiedas a site of definitive hematopoiesis in chick, Xenopus, mouse,and human embryos at similar developmental stages (37, 38),suggesting that the earliest intraembryonic hematopoietic cellsdo not express Jkap at a high level (Fig. 3F).

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Fig. 3. In situ expression analysis of Jkap. A and B, LinSca-1⁺ cells (A) and LinSca-1 cells (B) obtained from adult murine bone marrow by fluorescence-activated cell sorting were hybridized with a Jkap antisense riboprobe. C and D, embryonic day 10.5 mouse embryos were hybridized with a Jkap antisense riboprobe (C) (×20 magnification) and a Jkap sense riboprobe (D) (×20 magnification). E and F, the caudal region of the embryo in C is shown at ×50 (E) and in a 10-µm transverse section (F) (×200 magnification). The arrows indicate the caudal somites.

JKAP Selectively Activates the JNK Pathway-- Given the close sequence similarity of JKAP to MKPs, we sought to determine the effects of JKAP on JNK, p38, and ERK2. Toour surprise, overexpressed JKAP had no inhibitory effect on theactivity of either TGF- $beta$ -activated kinase 1-activated JNK1, MKK6-activatedp38, or protein kinase C- $iota$ -activated ERK2 (data not shown). Instead,we found that JKAP had the ability to activate JNK1 (Fig. 4).We cotransfected HA-JNK1 into HEK293T cells with wild-type JKAPor a catalytic site mutant of JKAP, JKAP-C88S. In JKAP-C88S, theCys $right-arrow$ Ser substitution allows the phosphatase to be isolated ina complex with its target substrate due to failure of cleavageof the scissile bond and, therefore, results in the loss of itsphosphatase activity as indicated by hydrolyzing pNPP, a chromogenicsubstrate (Fig. 4A, lower panel). HA-JNK1 was immunoprecipitatedwith an anti-HA antibody, and its activity was determined in vitroby immunocomplex kinase assays using GST-c-Jun-(1-79) as a substrate.We found that cotransfection of JKAP resulted in activation ofJNK1, whereas JKAP-C88S did not (Fig. 4A, upper panel). Thesedata indicate that the stimulatory effect of JKAP on JNK was dependenton the phosphatase activity of JKAP. To determine the specificityof this effect, we examined the effects of JKAP on p38 and ERK2.We cotransfected HA-p38 (Fig. 4B) or HA-ERK2 (Fig. 4C) with JKAPinto HEK293T cells. As a positive control, MKK6 was cotransfectedwith p38, and Raf-BXB was cotransfected with ERK2. HA-p38 andHA-ERK2 were immunoprecipitated with an anti-HA antibody, andtheir activities were determined in vitro by immunocomplex kinaseassays using GST-ATF2 as a substrate for p38 and myelin basicprotein as a substrate for ERK2. As shown in Fig. 4, B and C,neither p38 nor ERK2 was activated by overexpression of JKAP.Therefore, JKAP acts as a specific positive regulator of JNK.

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Fig. 4. JKAP activates JNK but not p38 or ERK in HEK293T cells. A, JKAP, but not JKAP-C88S, activates JNK1. HEK293T cells were transfected with 0.1 µg of HA-JNK1 alone, or HA-JNK1 plus 2 µg of either JKAP or JKAP-C88S. Empty vectors were used to normalize the amount of transfected DNA. At 44 h post-transfection, cells were collected, and cell lysates were prepared. HA-JNK1 was immunoprecipitated with an anti-HA antibody, and immunocomplex kinase assays were performed using GST-c-Jun-(1-79). Equivalent levels of HA-JNK1 expression were verified by immunoblot (IB) analysis using an anti-HA antibody. Lower panel, in vitro phosphatase activity of JKAP. 293T cells were transfected with a vector control, Myc-JKAP, or Myc-JKAP-C88S. Myc-JKAP and Myc-JKAP-C88S were immunoprecipitated with anti-Myc antibody and then incubated with pNPP. Cleavage of pNPP was measured by absorbance at 410 nm. B, JKAP cannot activate p38. HEK293T cells were transfected with 2 µg of HA-p38 alone or plus 2 µg of JKAP. As a control, HA-p38 was cotransfected with 2 µg of MKK6. Empty vectors were used to normalize the amount of transfected DNA. HA-p38 was immunoprecipitated with an anti-HA antibody, and immunocomplex kinase assays were performed using GST-ATF2 as a substrate. C, JKAP cannot activate ERK2. HEK293T cells were transfected with 2 µg of HA-ERK2 either alone or plus 2 µg of JKAP. HA-ERK2 was cotransfected with 0.5 µg of Raf-BXB as a control. Empty vectors were used to normalize the amount of transfected DNA. HA-ERK2 kinase assays were performed as described above except that myelin basic protein (MBP) was used as a substrate. Equivalent levels of HA-p38 and HA-ERK2 expression were verified by immunoblot analysis using an anti-HA antibody. D, JKAP mutant blocks TNF $alpha$ -induced JNK activation. HEK293T cells transfected with 0.1 µg of HA-JNK1 alone or HA-JNK1 plus 2 µg of JKAP-C88S were treated with TNF- $alpha$ (10 ng/ml) for 10 min. The cells were then collected, and cell lysates were prepared. HA-JNK1 was immunoprecipitated with an anti-HA antibody (12CA5), and immunocomplex kinase assays were performed using GST-c-Jun-(1-79) as a substrate. Equivalent levels of HA-JNK1 expression were verified by immunoblot analysis using an anti-HA antibody.

To confirm the functional relevance of JKAP to the JNK signaling pathway, we examined the contribution of JKAP to JNK activationby TNF- $alpha$ , a known JNK stimulus. HEK293T cells were transfectedwith HA-JNK1 alone or HA-JNK1 plus JKAP-C88S. The transfectedcells were treated with TNF- $alpha$ (10 ng/ml) for 10 min. We foundthat TNF- $alpha$ -induced JNK activation was blocked by JKAP-C88S (Fig.4D), suggesting that intact phosphatase activity of JKAP is necessaryfor JNK activation in TNF- $alpha$ signaling.

JKAP Is Necessary for Full Induction of the JNK Pathway-- To further confirm the functional involvement of JKAP in JNK signaling, we investigated the response of cells deficient inJKAP to various known JNK stimuli. We generated murine ES cellsheterozygous for the deletion of Jkap through homologous recombinationand derived homozygous clones by secondary selection (Fig. 5A).The inferred gene structure of Jkap based on the current humangenome assembly indicates that the locus is composed of sevenexons and spans about 60 kb (Fig. 5A). The targeted mutation (Fig.5B) deleted all of exons 5 and 6 (cDNA positions 249-495 and codonpositions 64-145) and resulted in a null for mRNA as assessedby Northern blot (Fig. 5C). Jkap^+/+ and Jkap^/ ES cells were exposed to TNF- $alpha$ , TGF- $beta$ , and ultraviolet-C (UV-C)irradiation, which are known stimuli for the JNK pathway. TNF- $alpha$ -and TGF- $beta$ -induced JNK activation was significantly reduced inJkap^/ cells in comparison with Jkap^+/+ cells (Fig. 6A, top and middle panels, respectively). In contrast,the fold induction of JNK activity by UV-C was comparable in Jkap^+/+ and Jkap^/ cells (Fig. 6A, bottom panel). These data indicate that JKAPis necessary for full activation of JNK in response to cytokinesbut not UV-C irradiation. Comparable JNK1 protein was expressedin Jkap^+/+ and Jkap^/ cells (Fig. 6B), indicating that JKAP deficiency does not causean obvious secondary disturbance in JNK expression or stability.The specific involvement of JKAP in the JNK signaling pathwaywas further confirmed by the comparable responses of p38 to UV-Cirradiation and of ERK2 to phorbol 12-myristate 13-acetate inJkap^+/+ and Jkap^/ MEF cells (data not shown). Taken together, these data furthersuggest that JKAP is a critical signaling component of the JNKpathway in response to TNF- $alpha$ and TGF- $beta$ .

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Fig. 5. Generation of Jkap^/ ES cells. A, the Jkap genomic locus, targeting vector, and mutated locus are schematically represented. Restriction enzyme sites (BamHI (B), XbaI (X), and SalI (S)) and the probe used to detect targeting events are indicated. B, genomic DNA was isolated from Jkap^+/+, Jkap^+/, and Jkap^/ ES cells, which were derived through selection of Jkap^+/ ES cell lines in 2 mg/ml G418. The DNA was digested with BamHI, transferred for Southern analysis, and hybridized with a probe flanking the 5' insertion site of the targeting vector. Molecular weights in kilobase pairs are indicated on the left. C, total RNA from Jkap^+/+, Jkap^+/, and Jkap^/ ES cells was isolated and hybridized with a Jkap cDNA probe. RNA integrity and quantity were evaluated by methylene blue staining after Northern transfer. Molecular size in kilobase pairs is indicated on the left.

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Fig. 6. JKAP deficiency abolishes JNK activation by TNF- $alpha$ and TGF- $beta$ but not by UV-C. A, Jkap^+/+ and Jkap^/ murine ES cells grown to ~80% confluence in 60-mm dishes were treated with TNF- $alpha$ (10 ng/ml) for 10 min (top panel), TGF- $beta$ (10 ng/ml) for 10 min (middle panel), or UV-C (300 J/m²) for 30 min (bottom panel). Endogenous JNK1 was immunoprecipitated (IP) with an anti-JNK1 antibody (Ab101), and immunocomplex kinase assays were performed using GST-c-Jun-(1-79) as a substrate. B, JNK1 expression in Jkap^+/+ and Jkap^/ ES cells. The expression levels of JNK1 in Jkap^+/+ and Jkap^/ ES cells were monitored by immunoblot analysis using an anti-JNK1 antibody (Ab101). WB, Western blot.

JKAP Plays a Role in TGF- $beta$ 1-induced Inhibition of CFCs-- The original finding that Jkap is differentially expressed in cell populations with the more primitive LinSca-1⁺ cell surface phenotype suggested that a functional role for JKAPmight be discerned in the hematopoietic lineage. Extensive studieshave demonstrated a particular role for TGF- $beta$ 1 in the inhibitionof hematopoietic precursors (39). Primitive hematopoietic precursorsare exquisitely sensitive to inhibition by TGF- $beta$ 1 (40, 41).We were then prompted to investigate the responses of MEF cellsand bone marrow progenitors derived from either wild-type or Jkapmutant embryos to TGF- $beta$ 1 stimulation, which results in promptgrowth arrest in a variety of cell types. MEFs derived from eitherwild-type or Jkap mutant embryos responded equally to TGF- $beta$ 1,with both showing a dose-dependent decrease in proliferation (Fig.7A). Jkap^/ bone marrow progenitors, in contrast, show less inhibition byTGF- $beta$ compared with wild type (Fig. 7B). These progenitors representpredominantly cells committed to the myeloid lineage. The reducedinhibition of Jkap^/ cells was TGF- $beta$ 1 dose-dependent and could be partially overcomeat the highest doses of the cytokine. The results demonstratea functional requirement for JKAP in regulating the quantitativeresponse of hematopoietic precursors to TGF- $beta$ 1. This is the firstevidence of any functional requirement for a DSP in a hematopoieticcell type.

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Fig. 7. Inhibition of TGF- $beta$ -induced CFCs in Jkap-deficient cells. A, comparable responses of Jkap^+/+ and Jkap^/ MEFs to TGF- $beta$ -induced growth arrest. Jkap^+/+ and Jkap^/ MEFs were cultured in various concentrations of TGF- $beta$ as indicated. Growth inhibition was measured by [³H]thymidine incorporation 24 h after induction. B, bone marrow cultures collected from tibias and femurs of 6-8-week-old JKAP^+/+ and JKAP^/ littermates were established in various concentrations of TGF- $beta$ as indicated. CFCs were counted at 10 days after culture initiation.

JKAP Associates with JNK in Cells, but Not in Vitro-- We next investigated whether JKAP interacts with JNK. We cotransfected Myc-JKAP into HEK293T cells with HA-JNK1 and examinedthe JKAP-JNK1 association by immunoprecipitation and Western blottinganalysis. HA-JNK1 was coimmunoprecipitated with Myc-JKAP whenan anti-Myc antibody was used to immunoprecipitate JKAP (Fig.8A, top panel). Conversely, Myc-JKAP was coimmunoprecipitatedwith HA-JNK1 when HA-JNK1 was immunoprecipitated with an anti-HA(12CA5) antibody (Fig. 8A, panel second from top). Therefore,a complex was formed between JKAP and JNK1 in transfected HEK293Tcells. To further determine whether JKAP and JNK1 interact directlywith each other in vitro, we incubated GST-JNK fusion proteinwith cell lysates from HEK293T cells overexpressing Myc-JKAP.The JKAP-JNK interaction was analyzed by SDS-PAGE and Westernblotting using an anti-Myc antibody. Association of JKAP withGST-JNK was not detectable (Fig. 8B, left panel). Under the sameconditions, however, M3/6, a known JNK-inactivating DSP that interactswith JNK and dephosphorylates the TPY motif of JNK (13), interactedwith GST-JNK (Fig. 8B, right panel). These data suggest that JKAPexerts its effect on the JNK pathway in an indirect manner. Thelack of immunoprecipitation does not prove that JKAP exerts itseffect on the JNK pathway indirectly, however. It may not interactwith JNK in vitro because an additional protein is missing orthe correct modification (such as phosphorylation by another kinase)of one or more of the proteins is not present.

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Fig. 8. JKAP associates with JNK in vivo but not in vitro. A, JKAP associates with JNK1 in HEK293T cells. HEK293T cells (1.5 × 10⁶ cells in a 100-mm dish) were transfected with Myc-JKAP (10 µg) alone, HA-JNK1 (10 µg) alone, or Myc-JKAP (10 µg) plus HA-JNK1 (10 µg). Empty vector was used to normalize the amount of transfected DNA. 42 h post-transfection, cell lysates were prepared. JKAP was immunoprecipitated with an anti-Myc antibody. The immunoprecipitants were then immunoblotted with an anti-HA antibody (12CA5). Conversely, JNK1 was immunoprecipitated with an anti-HA antibody (12CA5), and the immunoprecipitants were immunoblotted with an anti-Myc antibody. The expression levels of JKAP and HA-JNK1 were monitored by immunoblotting using anti-Myc and anti-HA (12CA5) antibodies, respectively. B, JKAP does not interact with JNK in vitro. HEK293T cells (1.5 × 10⁶ cells in 100-mm dishes) were transfected with 10 µg of either Myc-JKAP or Myc-M3/6. 42 h post-transfection, the cell lysates were prepared. 600 µg of lysate was incubated with GST or GST-JNK fusion protein immobilized onto glutathione-agarose beads for 2 h at 4 °C. The JKAP-JNK and M3/6-JNK interactions were analyzed by immunoblotting with an anti-Myc antibody to detect Myc-JKAP (upper panel) or Myc-M3/6 (lower panel) bound to GST-JNK after SDS-PAGE. The GST and GST-JNK were monitored by immunoblotting with an anti-GST antibody (middle panel). IP, immunoprecipitation; WB, Western blot.

JKAP Associates with MKK7-- The absence of a direct interaction between JNK and JKAP could suggest that JKAP exerts its effect on JNK by regulating moleculesthat regulate JNK, in particular the molecule(s) that are subjectto negative regulation by phosphorylation. It has been recentlyshown that SEK1 (also called MKK4), an immediate JNK upstreamactivating kinase, is subject to phosphorylation that interfereswith the SEK1-JNK interaction and prevents JNK from activation(20). It is reasonable to expect that a phosphatase that iscapable of dephosphorylating the inhibitory phosphoresidue shouldfinally exert a positive effect on the JNK pathway. We were thenprompted to examine whether JKAP could interact with SEK1 andMKK7, the other immediate JNK upstream activating kinase. We cotransfectedMyc-JKAP into HEK293T cells with FLAG-MKK7 or GST-SEK1 and examinedthe association of JKAP with MKK7 or SEK1 by immunoprecipitationand Western blotting analysis. Myc-JKAP was immunoprecipitatedwith an anti-Myc antibody. The immunoprecipitants were then subjectedto Western blotting using an anti-FLAG antibody for MKK7 or ananti-GST antibody for SEK1. We found that JKAP associated withMKK7 (Fig. 9A). However, no JKAP-SEK1 association was detected(Fig. 9B). These data suggest that MKK7 may be a specific interactingtarget for JKAP.

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Fig. 9. JKAP associates with MKK7 but not with SEK1. A, JKAP associates with MKK7. HEK293T cells (1.5 × 10⁶ cells in a 100-mm dish) were transfected with Myc-JKAP (10 µg) alone, FLAG-MKK7 (10 µg) alone, or Myc-JKAP (10 µg) plus FLAG-MKK7 (10 µg). Empty vector was used to normalize the amount of transfected DNA. 42 h post-transfection, cell lysates were prepared. JKAP was immunoprecipitated with an anti-Myc antibody. The immunoprecipitants were then immunoblotted with an anti-FLAG antibody (M2). The expression levels of JKAP and FLAG-MKK7 were monitored by immunoblotting using anti-Myc and anti-FLAG (M2) antibodies, respectively. B, JKAP does not associate with SEK1. HEK293T cells (1.5 × 10⁶ cells in a 100-mm dish) were transfected with Myc-JKAP (10 µg) alone, GST-SEK1 (10 µg) alone, or Myc-JKAP (10 µg) plus GST-SEK1 (10 µg). Empty vector was used to normalize the amount of transfected DNA. 42 h post-transfection, cell lysates were prepared. JKAP was immunoprecipitated with an anti-Myc antibody. The immunoprecipitants were then immunoblotted with an anti-GST antibody. The expression levels of JKAP and GST-SEK1 were monitored by immunoblotting using anti-Myc and anti-GST antibodies, respectively. IP, immunoprecipitation; WB, Western blot.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

A well accepted model is that a phosphorylating kinase is coupled with a dephosphorylating phosphatase to balance the responseof a signaling pathway to a stimulus (42). Previous functionalstudies of DSPs with activity in the MAPK pathways have primarilyhighlighted their roles as down-regulators, inactivating the targetMAPK through direct dephosphorylation of the phosphothreonineand phosphotyrosine residues in the TXY motif of the catalyticdomain of the kinase (7, 9). We reported here that a dualspecificity phosphatase is preferentially expressed in the stemcell-enriched LinSca-1⁺ population of murine bone marrow cells, referred to as JKAP.Unlike most other DSPs/MKPs identified so far, JKAP is uniquein two aspects. First, JKAP protein lacks an extended noncatalyticdomain and is consequently ~100 amino acids shorter than mostother MAPK phosphatases. Second, JKAP acted as a specific positiveregulator for the JNK signaling pathway. It appeared that activationof JNK requires phosphatase activity, since the catalyticallyinactive C88S mutant of JKAP could not activate JNK. The requirementof JKAP for the JNK signaling pathway was further demonstratedby the genetic studies. In Jkap-deficient murine ES cells, cytokine-inducedJNK activation was significantly reduced. To our knowledge, thisis the first report that has combined both biochemical and geneticstudies to indicate that a DSP acts as a specific positive regulatorfor the JNK signalingpathway.

During the preparation of this manuscript, we found by sequence analysis that JKAP is a murine orthologue of human JNK-stimulatoryphosphatase (JSP)-1 (36) or VHR-related MKPX (VHX) (43). Allof these phosphatases lack the regulatory region containing theCdc25 homology domain, which is conserved in most known MKPs.However, the effects of these lower molecular weight DSPs on MAPKsare controversial in the literature. Whereas human VHX possessesa higher capacity than VHR phosphatase, which is thought to bespecific for ERK1/2, to dephosphorylate ERK2 in vitro (43),JSP-1 acts as a specific positive regulator for the JNK pathway(36). Moreover, low molecular weight (LMW) DSP2, another identifiedmurine orthologue of human JSP-1/VHX, is able to dephosphorylateand inactivate p38 and JNK both in vitro and in cells (44).Overexpression of JKAP or JSP-1 resulted in activation of JNK,but these results do not demonstrate a direct regulatory rolein the JNK pathway, since JNK responds to a variety of cell stresses,and overexpression may have acted in one of those pathways indirectlyactivating JNK. The targeted mutation of Jkap demonstrated definitivelythat it both acts as a positive regulator for the JNK pathwayand is required for the cytokine-induced activation of the JNKpathway. This result provides the first demonstration of a functionalrequirement for a DSP in MAPK signaling. It is not clear at thispoint what causes the significant difference for these low molecularweight DSPs in both their substrate specificity and the natureof their effect on MAPKs. JKAP is 20 amino acids longer than JSP-1,VHX, and LMW DSP2. We, in fact, detected two transcripts of 3.0and 1.3 kb in mouse tissues (Fig. 2). It is possible that JKAPfunctions differently from LMW DSP2 simply due to the fact thatthey are different isoforms of the same gene through differentialsplicing.

It is unique for JKAP and JSP-1 isoforms to be able to activate JNK. It is not clear how these low molecular weight DSPs controltheir substrate specificity without the regulatory region, whichis conserved in most other MKPs containing an essential domainfor its substrate binding and substrate specificity. It was reportedthat the conserved docking motifs of p38 and JNK are not essentialfor their interaction with LMW DSP2 (44). Since the physiologicalsubstrate for JKAP remains to be determined, the pathway specificitymight be achieved in one of the following ways. First, if JKAP,like other MKPs, acts directly on JNK, a distinct mechanism mustexist to determine its substrate specificity. The apparent specificityof JKAP for JNK could be inherent in the catalytic pocket or couldbe mediated through an interacting protein complex. Second, ifJKAP loses its ability to bind MAPK/JNK due to its lack of thenoncatalytic domain, it could exert its positive effect on theJNK pathway through interacting with and activating other signalingcomponents of the JNKpathway.

The absence of a direct interaction between JNK and JKAP could suggest that JKAP exerts its effect on JNK by regulating molecules(e.g. kinases or phosphatases) that regulate JNK. This is consistentwith the notion that JSP-1 may act upstream of SEK1 (36). SinceJKAP acts as a specific activator for the JNK pathway, it is reasonableto expect that the potential target for JKAP should be JNK pathway-specific.We found that JKAP interacts with MKK7, but not SEK1. It is interestingto note that MKK7 is the only MAP2K identified so far that specificallyactivates JNK (45), although both MKK7 and SEK1 are immediateupstream activating kinases for JNK. SEK1 can activate p38 aswell as JNK. It was recently shown that AKT-mediated phosphorylationof SEK1 on Ser-78 results in dissociation of SEK1 and JNK and,thus, inactivation of JNK (20). It would not be surprising ifMKK7 is also subject to similar negative regulation by phosphorylation.Thus, the MKK7-JKAP interaction suggests a potential physiologicalrelevance and mechanism by which the JNK pathway is positivelyregulated by JKAP. However, it is still unclear which componentis the target of JKAP in the JNK cascade. It remains to be clarifiedwhat the JKAP-JNK and JKAP-MKK7 associations in cells mean tothe output of stimulus-specific JNK signaling. JKAP may only targetand activate one signaling component of the JNK cascade, whichis negatively regulated by phosphorylation. In this case, theassociation of JKAP with other signaling components of the JNKpathway may only reflect the fact that JKAP is a component ofthe JNK signaling complex. Alternatively, JKAP may target andact on multiple components of the JNK pathway, depending on thecell type and the stimulus the cellreceives.

The physiological roles of individual MAPK phosphatases have been difficult to assess due to cross-pathway specificity andsome functional redundancy. VHR/DUSP3 (46) and hVH-3/DUSP5 (47)exhibit pathway specificity for ERKs. PYST2/DUSP7 is selectivefor the ERK and p38 pathways but does not seem to act on JNK (48).M3/6 (13), MKP-5/DUSP10 (49), and MKP-7 (14, 15) are selectivefor the p38 and JNK pathways. None of the previously known mammaliandual specificity phosphatases have been found to be specific forJNK, although Drosophila puckered may be selective for the JNKhomologue basket (50). Investigation of the functional activityof MAPK phosphatases has largely relied on in vitro models. Targeteddisruption of Mkp-1, for example, does not seem to affect MAPkinase activity (51), indicating that its functional requirementsare either subtle or redundant. Besides MKP-1, no other in vivomutation study has been reported with a mammalian MAPK phosphatase.Thus far, the requirement for JKAP in optimal JNK activation distinguishesJKAP among the DSPs. Specific regulators of JNK activation, likeJKAP, could be reasonable targets for therapeutic drug development,given the broad roles of the JNK pathway in response to stress,growth, and apoptosis. The effects of this unique phosphatasein the JNK pathway support a more complex role for phosphatasesin MAP kinasesignaling.

ACKNOWLEDGEMENTS

We thank our colleagues for providing valuable reagents, members of the Tan and the Belmont laboratories for helpful discussionsand critical reading of the manuscript, and S. Robertson for secretarialassistance.

	FOOTNOTES

^* This work was supported in part by National Institutes of Health (NIH) Grants RO1 DK48647 and HD36280 (to J. W. B.) and RO1AI42532 and RO1 CA87076 (to T.-H. T.).The costs of publicationof this article were defrayed in part by the payment of page charges.The article must therefore be hereby marked "advertisement" inaccordance with 18 U.S.C. Section 1734 solely to indicate thisfact.

^§ Supported by NIH Grants T32 HG00003 and T32GM08307.

^¶ These authors contributed equally to thiswork.

Present address: Dept. of Microbiology and Immunology and Sylvester Comprehensive Cancer Center, University of Miami Schoolof Medicine, Miami, FL33136.

^¶¶ A Scholar of the Leukemia and Lymphoma Society. To whom correspondence may be addressed: Dept. of Immunology, Baylor Collegeof Medicine, Houston, TX77030.

To whom correspondence may be addressed: Dept. of Molecular and Human Genetics, Baylor College of Medicine, Houston, TX77030.

Published, JBC Papers in Press, July 23, 2002, DOI 10.1074/jbc.M200453200

ABBREVIATIONS

The abbreviations used are: MAPK, mitogen-activated protein kinase; ERK, extracellular signal-regulated kinase; JNK, c-Jun N-terminal kinase; MAP, mitogen-activated protein; MAP4K, MAP kinase kinase kinase kinase; MAP3K, MAP kinase kinase kinase; MAP2K/MKK, MAP kinase kinase; DSP, dual specificity phosphatase; MKP, MAP kinase phosphatase; SEK1, stress-activated protein kinase/ERK kinase 1; JKAP, JNK pathway-associated phosphatase; TNF- $alpha$ , tumor necrosis factor- $alpha$ ; TGF- $beta$ , transforming growth factor- $beta$ ; HEK293T, human embryonic kidney 293T cells; pNPP, p-nitrophenyl phosphate; GST, glutathione S-transferase; ATF2, activating transcription factor 2; ES, embryonic stem; MEF, mouse embryonic fibroblast; UV-C, ultraviolet-C; CFC, colony-forming cell; MKK7, MAP kinase kinase 7; JSP-1, JNK-stimulatory phosphatase-1; VHX, VHR-related MKPX; LMW, low molecular weight.

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The Dual Specificity JKAP Specifically Activates the c-Jun N-terminal Kinase Pathway*

The Dual Specificity JKAP Specifically Activates the c-Jun N-terminal Kinase Pathway^*