Synergistic Interaction of MEK Kinase 2, c-Jun N-Terminal Kinase (JNK) Kinase 2, and JNK1 Results in Efficient and Specific JNK1 Activation

doi:10.1128/MCB.20.7.2334-2342.2000

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Molecular and Cellular Biology, April 2000, p. 2334-2342, Vol. 20, No. 7
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Synergistic Interaction of MEK Kinase 2, c-Jun N-Terminal Kinase (JNK) Kinase 2, and JNK1 Results in Efficient and Specific JNK1 Activation

Jinke Cheng,¹ Jianhua Yang,¹ Ying Xia,² Michael Karin,² and Bing Su¹^,^*

Department of Immunology, The University of Texas, M. D. Anderson Cancer Center, Houston, Texas 77030,¹ and Department of Pharmacology, University of California at San Diego, La Jolla, California 92093²

Received 21 September 1999/Returned for modification 2 November 1999/Accepted 29 January 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Mitogen-activated protein kinases (MAPKs) are activated through cascades or modules consisting of a MAPK, a MAPK kinase (MAPKK),and a MAPKK kinase (MAPKKK). Investigating the molecular basisof activation of the c-Jun N-terminal kinase (JNK) subgroup ofMAPK by the MAPKKK MEKK2, we found that strong and specific JNK1activation by MEKK2 was mediated by the MAPKK JNK kinase 2 (JNKK2)rather than by JNKK1 through formation of a tripartite complexconsisting of MEKK2, JNKK2, and JNK1. No scaffold protein wasrequired for the MEKK2-JNKK2-JNK1 tripartite-complex formation.Expression of JNK1, JNKK2, and MEKK2 significantly augmented thecoprecipitation of, respectively, MEKK2-JNKK2, MEKK2-JNK1, andJNKK2-JNK1, indicating that the interaction of MEKK2, JNKK2, andJNK1 is synergistic. Finally, the JNK1 was activated more efficientlyin the MEKK2-JNKK2-JNK1 complex than was the JNK1 excluded fromthe complex. Thus, formation of a signaling complex through synergisticinteraction of a MAPKKK, a MAPKK, and a MAPK molecule like MEKK2-JNKK2-JNK1is likely to be responsible for the efficient, specific flow ofinformation via MAPKcascades.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Mitogen-activated protein kinase (MAPK) cascades are central components of the intracellular signaling networks involved intransducing a wide spectrum of extracellular signals to nuclearand cytoplasmic effectors that control cell growth, differentiation,and apoptosis (for reviews, see references 6, 20, 25, and26). Multiple MAPK cascades that lead to the activation of extracellularsignal-related kinases 1 and 2 (ERK1 and ERK2), c-Jun N-terminalkinases 1 through 3 (JNK1 through JNK3), p38 $alpha$ through p38 $gamma$ , orERK5 were identified in eukaryotic cells, and each is believedto respond to a distinct set of extracellular stimuli (3, 11,18, 29, 44, 61). Each of these MAPKs is activated by aMAPK kinase (MAPKK), usually with rather narrow specificity (6,19, 33, 43, 46), although individual MAPKKs are believedto respond to several or many MAPKK kinases (MAPKKKs). The MAPKKKsare responsible for responding to a variety of upstream activatorsthat connect them to various cell surface receptors. In additionto amplifying weak receptor-generated signals, MAPK cascades arebelieved to participate in the generation of signaling specificity(5, 16, 20, 26, 33, 46).

A given MAPK cascade can respond to several extracellular stimuli, and a given stimulus can activate several MAPK cascades,but the response and fidelity of MAPK activation are specific(for reviews, see references 8, 25, 26, and 46). AlthoughMAPK cascades may have ample opportunities in vivo for cross talkat different levels, an individual MAPK cascade is generally insulatedfrom other closely related cascades, and each MAPK cascade isbelieved to preferentially respond to a distinct set of stimuli(4, 13, 16, 42, 55).

The molecular mechanism of MAPK cascade specificity is best studied in yeast. Specific MAPK activation in response to matingpheromones is conferred by STE5, a protein that acts as a molecularscaffold tethering the MAPKKK STE11, MAPKK STE7, and MAPK FUS3proteins to form a pheromone-responsive module (4, 32, 39).Direct interaction of the components of a MAPK module has alsobeen observed and suggested to play a role in determining MAPKspecificity. The MAPKK STE7 in yeast was shown, for example, tointeract with its target FUS3 in the absence of STE5 (1), andthe yeast MAPKK PBS2 was shown to assemble a module with the MAPKHOG1 and the MAPKKK STE11 in response to osmotic stress (38).

Although a mammalian homologue of STE5 has not yet been identified, two proteins, MP1 and JIP-1, have been suggested to functionas a scaffold for MAPK modules that leads to specific activationof ERK and JNK (41, 52). MP1 binds both MEK1 and ERK1 in activatingthe ERK pathway (41), whereas JIP-1, a protein originally identifiedas a JNK1-interacting protein, binds to JNK1, JNKK2/MKK7, andMAPKKK MLK3/DLK, thereby facilitating JNK1 activation by MLK3/DLK(52). A different scheme has been suggested for JNK (or p38)activation in response to the MAPKKK MEKK1, in which the MAPKKJNKK1/MKK4 was shown to be involved in specific and sequentialinteractions with MEKK1 and JNK1 (55). These interactions werebipartite and sequential, so that formation of a MEKK1-JNKK1 complexresulted in activation of JNKK1 followed by disassembly and formationof a specific JNKK1-JNK1 complex and then by activation of JNK1(55). No ternary MEKK1-JNKK1-JNK1 complex could be detected,probably because the same interaction surface on JNKK1, its N-terminalregion, was used to contact either MEKK1 or JNK1 (55). The N-terminalregion of MEKK1 was shown in other studies to be directly associatedwith the downstream kinase JNK1, suggesting that this region mayfunction as a scaffold in certain situations (56).

The JNK subgroup of MAPKs is activated by a particularly large number of stimuli, including physical stresses, cytokines,T-cell costimulation, and growth factors (24, 25, 35, 46).Two specific JNK-activating MAPKKs, JNKK1/MKK4 and JNKK2/MKK7,were identified (12, 15, 22, 30, 31, 37, 40, 49,54, 59). Although JNKK1/MKK4 and JNKK2/MKK7 are believed tobe able to activate JNK, a recent study suggested that JNKK1 andJNKK2 may differentially phosphorylate their substrate JNK atthe conserved Thr and Tyr residues, thus synergizing their effecton JNK activation (28). JNKK1/MKK4 and JNKK2/MKK7 are also differentiallyactivated by tumor necrosis factor alpha and cellular stresses,and distinct upstream activators were proposed for their activationin those responses (21, 37). JNKK1/MKK4 was found to be thepreferential substrate of the MAPKKK MEKK1 (55), while JNKK2/MKK7was shown to be activated by several MAPKKKs, including MEKK1,MEKK2, MEKK3, and MLK3/DLK, in JNK activation ((9, 34, 52,55; J. Yang and B. Su, unpublisheddata).

A growing number of MAPKKKs are being identified as capable of JNK activation; they include MEKK1, MEKK2, MEKK3, MEKK4, MEKK5,ASK, TAK, and Tpl (2, 14, 16, 17, 23, 27, 47, 48,51, 58). These kinases have in common a conserved kinase domainwith substantial homology to that of the yeast MAPKKK STE11. TheseMAPKKKs are believed to be major players involved in sorting distinctcell surface signals to the downstream cytoplasmic and nucleareffectors. While MEKK1 clearly prefers JNKK1/MKK4 to JNKK2/MKK7,it is not known whether other MAPKKKs operate preferentially viaJNKK1, JNKK2 or an as yet unidentified JNKK in JNKactivation.

We investigated the molecular mechanisms that underlie the strong and specific JNK1 activation by human MEKK2, a moleculewe cloned from human T cells. We identified a tripartite molecularcomplex consisting of MEKK2, JNKK2, and JNK1 that was responsiblefor strong, specific JNK1 activation byMEKK2.

	MATERIALS AND METHODS

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Cell culture and transient transfection. COS-1 cells were cultured in Dulbecco's modified Eagle's medium supplemented with 5% fetal bovine serum, 100 U of penicillinper ml, and 100 mg of streptomycin per ml. Plasmid DNA was transfectedinto COS-1 cells with Lipofectamine (Life Technologies, Gaithersburg,Md.).

Plasmids, proteins, and antibodies. Hemagglutinin (HA)-tagged JNK1, JNKK1, JNKK1(AL), JNKK2, JNKK2(AL), MEK1, MEK2, MKK6, p38, and MEKK1(CT) were cloned intopSR $alpha$ 3 vector as previously described (30, 36, 45, 59).JNKK1(AL) and JNKK2(AL) are the kinase domain mutants in whichSer-257 and Thr-261 (JNKK1) and Ser-271 and Thr-275 (JNKK2) werereplaced with Ala and Lys, respectively, using a PCR-directedmutagenesis method. The HA-tagged MEKK1(CT) expression vectorhas been described by Minden et al. (36). The HA-tagged MEKK2(CT)expression vector was constructed by introducing an NcoI siteat codon 343 by the PCR-based method, followed by subcloning intothe expression vector pSR $alpha$ 3HA at the NcoI site, in which MEKK2(CT)fused in frame with the HA tag. The pCMV-Flag-JNK1 expressionvector has been described previously (11). Glutathione S-transferase(GST)-tagged MEKK2(FL), MEKK2(CT), MEKK1(CT), and JNKK2 mammalianexpression vectors were cloned into the pEGB vector (30) bystandard molecular biology techniques. Briefly, MEKK2(FL) andJNKK2 were introduced into an NcoI site at the first Met codon,MEKK2(CT) at codon 343, and MEKK1(CT) at codon 1199 by the PCR-basedmethod, followed by subcloning into the NcoI site in mammalianexpression vector pEGB and fused in frame with a GST tag. Bacterialrecombinant protein expression vectors for GST-c-Jun, GST-JNK1,and His-p38 have been described previously, as have expressionand purification of the recombinant proteins (30, 36, 45).Anti-HA antibody 12CA5 was prepared from the 12CA5 hybridoma (53)and further purified using a protein A-Sepharose column. Anti-Flagantibody M2 was purchased from IBI-Kodak. Anti-MEKK1 antibody(C22) was purchased from Santa Cruz (Santa Cruz, Calif.). MEKK2-specificantibody 1128 was prepared by immunizing rabbits with a GST fusionprotein fused in frame with a fragment of human MEKK2 peptide(amino acids 343 to 428) (B. Su and J. Cheng, unpublished data).Anti-JNK1 antibody was fromPharmingen.

Immunoprecipitation and in vitro kinase assay. Cell lysates were prepared 40 h after transfection, as described previously (45, 55), and incubated with appropriate antibodiesfor 4 h at 4°C in a rotator; protein A-Sepharose beads were addedfor another 45 min. The beads were washed four times with lysisbuffer (20 mM Tris [pH 7.5], 0.5% Nonidet P-40, 250 mM NaCl, 3mM EDTA, 3 mM EGTA, 100 mM Na₃VO₄) and twice with kinase reactionbuffer (20 mM HEPES [pH 7.6], 1 mM MgCl₂, 10% glycerol). The immunoprecipitateswere then subjected to kinase assays in 30 µl of kinase bufferwith appropriate substrates in the presence of 0.5 µl of [ $gamma$ -³²P]ATP and 20 µM cold ATP. After 20 min at 30°C, the reactionswere terminated by addition of sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) loading buffer and boiling for5 min. The proteins were separated by SDS-PAGE, and ³²P incorporation was determined with an FX Phosphorimager (Bio-RadLaboratories, Richarmond, Calif.).

Coupled-kinase assay. Cell lysates and immunoprecipitates were prepared as described previously (45). The immunoprecipitates were subjected toa coupled-kinase assay as described by Lin et al. (30). Briefly,the immunoprecipitates were incubated in 30 µl of kinase bufferwith two substrates, GST-JNK1 and GST-c-Jun, in the presence of1 µl of [ $gamma$ -³²P]ATP and 30 µM cold ATP. After 40 min at 30°C, the reactionswere terminated by adding SDS-PAGE loading buffer and boilingfor 5 min. The proteins were separated by SDS-PAGE, and ³²P incorporation into GST-JNK1 and GST-c-Jun wasdetermined.

Coprecipitation assay. COS-1 cells transfected with HA-, Flag-, or GST-tagged expression vectors were lysed 40 h after transfection by using low-saltlysis buffer (50 mM HEPES [pH 7.6], 150 mM NaCl, 1.5 mM MgCl₂,1 mM EDTA, 1% Triton X-100, 10% glycerol). The nuclei and celldebris were removed from the lysates by centrifugation in a microcentrifugefor 20 min at 4°C. Expressed proteins were precipitated from theclarified lysates with glutathione (GSH)-Sepharose beads at 4°Cfor a 4-h incubation in a rotator. The beads were washed fourtimes with low-salt lysis buffer, and the precipitates were elutedwith sample buffer and resolved by SDS-PAGE. After electrophoresisand transfer, the proteins were analyzed by Western blotting withappropriate antibodies. Western blotting was quantitated witha Bio-Rad G360 Imagesystem.

Gel filtration. Cell lysates containing 200 µg of proteins were prepared from COS-1 cells expressing GST-MEKK2(CT), HA-JNKK2, or HA-JNK1 andloaded onto a fast protein liquid chromatography (FPLC) Superdex-200column (Pharmacia). The column was washed with buffer containing20 mM Tris-HCl and 150 mM NaCl. Then 0.2-ml fractions were collectedand subjected to Western blotting and coprecipitation assays asdescribedabove.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Strong and specific JNK1 activation by MEKK2 is not mediated by JNKK1. During our investigation of upstream activators of the JNK MAPK cascade expressed in Jurkat T cells, we isolated a cDNA thatencodes human MEKK2 (GenBank accession no. AF111105) and demonstratedits involvement in transducing T-cell-activating signals to JNK(B. Su et al., unpublished data). Human MEKK2 is highly homologousto murine MEKK2, and its expression leads to strong activationof JNKs in many cell lines similar to the murine MEKK2 (2,9; Su et al., unpublished). Like all other MAPKKKs, MEKK2 doesnot activate JNK1 directly; such activation requires the involvementof an intermediary MAPKK, although the specific MAPKK throughwhich MEKK2 operates is notknown.

We used cotransfection experiments to compare the abilities of MEKK1 and MEKK2 to activate JNK1 and found that MEKK2 was aneven more potent JNK1 activator than was MEKK1, one of the mostpotent JNK activators reported to date (J. Cheng and B. Su, unpublishedresults). MEKK1 has a much larger N-terminal domain than MEKK2,and this domain was shown to affect the MEKK1 expression level(55, 57), suggesting that the difference in the abilitiesof full-length MEKK1 and MEKK2 to activate JNK1 may be due totheir different expression levels. Since the expression levelsof the kinase domains of MEKK1 (residues 1199 to 1495) and MEKK2(residues 343 to 618) are compatible and both are potent activatorsof JNK1 (Fig. 1), we compared the activities of the MEKK1 andMEKK2 kinase domains, which have 49% homology. CotransfectingJNK1 and JNKK1 expression vectors with different amounts of expressionvectors for the kinase domains of MEKK1 [MEKK1(CT)] and MEKK2[MEKK2(CT)], we determined the enzymatic activities of JNK1 andJNKK1 by an in vitro kinase assay. At low levels of MEKK1(CT)and MEKK2(CT) expression plasmids, we found MEKK2(CT) to be amore effective JNK activator than MEKK1(CT), but the differencewas diminished when higher levels of MEKK1(CT) and MEKK2(CT) vectorswere used (Fig. 1A). Under the same conditions, however, the patternsof JNKK1 activation by MEKK1(CT) and MEKK2(CT) were reversed:MEKK2(CT) was a less effective activator of JNKK1 than was MEKK1(CT)(Fig. 1B). These results suggested that in activating JNK1, JNKK1may not be the preferred substrate for MEKK2.

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FIG. 1. MEKK2 is a stronger JNK1 activator but weaker JNKK1 activator than is MEKK1. (A) HA-JNK1 expression vector (0.5 µg/plate) was cotransfected into COS-1 cells with increasing amounts of either MEKK2(CT) or MEKK1(CT) expression vectors. HA-JNK1 activity was measured by an immunocomplex kinase assay (KA) as described in Materials and Methods. Expression of HA-JNK1, MEKK1(CT), and MEKK2(CT) was determined by Western blotting (WB). The relative fold increase in JNK1 activity is shown in the upper panel. (B) HA-JNKK1 expression vector (0.5 µg/plate) was cotransfected into COS-1 cells with increasing amounts of either MEKK2(CT) or MEKK1(CT) expression vectors. HA-JNKK1 activity was measured as described in Materials and Methods. Expression levels of HA-JNKK1, MEKK1(CT), and MEKK2(CT) were determined by Western blotting (WB). The relative JNKK1 activity is shown in the upper panel. (C) Either GST-MEKK1(CT) or GST-MEKK2(CT) (each at 10 ng/plate) and Flag-JNK1 (0.5 µg/plate) expression vectors were cotransfected into COS-1 cells with expression vectors for HA-JNKK1(WT) or HA-JNKK1(AL) as indicated. Flag-JNK1 was immunoprecipitated, and its activity was determined by the immunocomplex kinase assay and quantitated by the Bio-Rad FX Imager system. Relative JNK1 activity is shown after being normalized to its expression level. Expression levels of Flag-JNK1, HA-JNKK1(WT), HA-JNKK1(AL), GST-MEKK1(CT), and GST-MEKK2(CT) were determined by Western blotting (WB).

To further address this possibility, we examined the effect of JNKK1 expression on MEKK1(CT)- and MEKK2(CT)-mediated JNK1activation. Coexpression of JNKK1 with MEKK1 had been shown tostrongly potentiate MEKK1-mediated JNK1 activation (30, 55).We found, similarly, that coexpression of JNKK1 clearly augmentedJNK1 activation by MEKK1(CT) (Fig. 1C), although the JNKK1 coexpressionhad only a marginal effect on JNK1 activation by MEKK2 (CT) (Fig.1C). Furthermore, overexpression of a kinase-defective JNKK1 mutant,JNKK1(AL), which has mutations of the conserved Ser-257 and Thr-261to Ala and Leu, respectively, inhibited MEKK1(CT)- but not MEKK2(CT)-mediatedJNK1 activation (Fig. 1C). While confirming the previous resultsthat JNK1 activation by MEKK1 is mediated by JNKK1 (30, 55),these data also indicated that activation of JNK1 by MEKK2 isunlikely to be mediated by JNKK1 but may occur through a JNKK1-relatedMAPKK.

JNKK2 is a major effector MAPKK for MEKK2 in JNK1 activation. A second JNK-activating MAPKK, JNKK2/MKK7, was recently identified (15, 22, 31, 37, 49, 54, 59). JNKK2 was foundnot to activate ERK1 and ERK2 and, unlike JNKK1, not to activatep38. To investigate whether JNKK2 serves as the major intermediaryMAPKK between MEKK2 and JNK1, we performed a coupled-kinase assay.Cotransfection of JNKK2 with MEKK2(CT) resulted in strong JNKK2activation even at very low MEKK2(CT) expression levels (Fig.2A). Although JNKK1 could also be activated by MEKK2(CT) in thisassay, we found that almost 10 times more MEKK2(CT) expressionvectors were needed (100 ng for JNKK1 activation versus 10 ngfor JNKK2 activation) to obtain JNKK1 activation levels similarto those of JNKK2. These results suggested that in activatingJNK1, JNKK2 may be a preferred MAPKK for MEKK2. To study thispossibility more thoroughly, we examined whether coexpressionof wild-type JNKK2 or the JNKK2 kinase-defective mutant JNKK2(AL)could affect MEKK2-mediated JNK1 activation. Coexpression withwild-type JNKK2 augmented JNK1 activation by MEKK2(CT), whereascoexpression with JNKK2(AL) inhibited JNK1 activation by MEKK2(CT)(Fig. 2B). Furthermore, JNKK2 was directly phosphorylated by MEKK2at Ser-271 and Thr-275 in the SXXXT motif, a highly conservedmotif in all members of the MAPKK supergene family. Mutation ofthese residues abolished JNKK2 phosphorylation by MEKK2 (Fig.2C). Although JNKK2 was also phosphorylated by MEKK1(CT), thiswas much less efficient than the phosphorylation mediated by MEKK2(CT).In contrast, JNKK1 was more efficiently phosphorylated by MEKK1(CT)than by MEKK2(CT) on its conserved SXXXT motif (Fig. 2C). Togetherwith the recent finding that JNKK1 but not JNKK2 is the majoreffector MAPKK for MEKK1 (7, 55), these results suggestedthat MEKK1 and MEKK2 use different effector MAPKKs in activatingJNK1.

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FIG. 2. JNKK2 is a major effector of MEKK2 in JNK1 activation. (A) An increasing amount of GST-MEKK2(CT) expression vectors was cotransfected into COS-1 cells with HA-JNKK2 or HA-JNKK1 expression vectors (0.5 µg/plate each) as indicated. HA-JNKK2 and HA-JNKK1 were immunoprecipitated, and their activities were determined by a coupled-kinase assay. The relative fold increases of JNKK1, JNKK2, and JNK1 activities are indicated. Expression of HA-JNKK2 and HA-JNKK1 was determined by western blotting (WB). (B) GST-MEKK2(CT) (10 ng/plate) and Flag-JNK1 (0.5 µg/plate) expression vectors were cotransfected into COS-1 cells alone or with HA-JNKK2 or HA-JNKK2(AL) expression vectors (0.5 µg/plate) as indicated. Flag-JNK1 activity was measured as described for Fig. 1C, and the expression levels of Flag-JNK1, HA-JNKK2(WT), and HA-JNKK2(AL) were determined by western blotting (WB). Relative JNK1 activity is shown in the top panel. (C) Empty vectors or HA-MEKK1(CT) or HA-MEKK2(CT) expression vectors (0.5 µg/plate) were transfected into COS-1 cells. HA-MEKK1(CT) and HA-MEKK2(CT) were immunoprecipitated, and their activities were measured by an in vitro kinase assay with JNKK1, JNKK1(AL), JNKK2 or JNKK2(AL) as substrates as described in Materials and Methods. The amounts of JNKK1, JNKK1(AL), JNKK2, and JNKK2(AL) used in the in vitro kinase assay were shown by Coomassie blue staining (CB). Expression of HA-MEKK1(CT) and HA-MEKK2(CT) was determined by Western blotting (WB).

JNKK2 interacts with MEKK2 and JNK1. Protein-protein interactions have been suggested to play a critical role in determining the specificity of signal transductionpathways. To investigate whether such a mechanism can explainthe selectivity of MEKK2 in JNK1 activation, we performed coprecipitationassays. As shown in Fig. 3A, JNKK2 coprecipitated with MEKK2(CT)about six times more efficiently than JNKK1 did, consistent withthe finding that JNKK1 was activated less efficiently than JNKK2by MEKK2. We also examined the interaction of MEKK2 with MEK1,MEK2, and MKK6 and did not observe any significant complex formation(Fig. 3A). Consistent with a report by Xia et al. (55), MEKK1preferentially interacted with JNKK1 over other MAPKKs, includingJNKK2 (data not shown). In addition to the preformed complex insidecells, JNKK2 and MEKK2 could form a complex in vitro when celllysates prepared from COS-1 cells transfected separately withJNKK2 and MEKK2 expression vectors were mixed (data not shown).We also found, in a similar coprecipitation assay, that JNKK2,like JNKK1, could interact directly with JNK1 (Fig. 3B), confirmingthe finding by Holland et al. (22) and Tournier et al. (50).These results suggested that specific JNK1 activation by MEKK2may be mediated by JNKK2-MEKK2 and JNKK2-JNK1 protein-proteininteractions.

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FIG. 3. JNKK2 binds to MEKK2 and JNK1. (A) GST-MEKK2(CT) expression vectors (0.5 µg/plate) were cotransfected into COS-1 cells with 0.5 µg of HA-JNKK1, HA-JNKK2, HA-MEK1, HA-MEK2, or HA-MKK6 expression vector per plate. GST-MEKK2(CT) was precipitated with GSH-Sepharose beads, and its associated proteins were analyzed as described in Materials and Methods. Expression of HA-JNKK1, HA-JNKK1, HA-MEK1, HA-MEK2, HA-MKK6, and GST-MEKK2(CT) was measured by Western blotting (WB) as indicated. The percentages of HA-JNKK1, HA-JNKK2, HA-MEK1, HA-MEK2, and HA-MKK6 bound to GST-MEKK2(CT) were determined with a Bio-Rad G360 Imager system. (B) Equal amounts of cell lysates prepared from COS-1 cells transfected with GST, GST-JNKK1, or GST-JNKK2 vector (0.5 µg/plate) were mixed with lysates prepared from COS-1 cells transfected with the HA-JNK1 expression vector (0.5 µg/plate). The mixtures were incubated for 4 h at 4°C in a rotator, and GST, GST-JNKK1 or GST-JNKK2 was precipitated with GSH-Sepharose beads as described above. The bound and input HA-JNK1 was analyzed by Western blotting (WB).

MEKK2, JNKK2, and JNK1 form a multimolecular complex through synergistic interaction. The above results provided strong evidence that JNKK2 is a major effector MAPKK for MEKK2 in JNK activation. It is not clear,however, whether MEKK2-JNKK2 and JNKK2-JNK1 interactions occursequentially or simultaneously. Recently, sequential protein-proteininteractions between MEKK1-JNKK1 and JNKK1-JNK1 were shown tounderlie specific JNK activation by MEKK1 (55). MEKK1 was alsoshown to interact directly with JNK1 (56) and JNKK1 (T. Hunter,personal communication), independent of scaffolding molecules.No tripartite complex of MEKK1, JNKK1, and JNK1 has been demonstratedso far, however. To determine whether MEKK2, JNKK2, and JNK1 interactsequentially or simultaneously, we carried out coprecipitationassays using COS-1 cell lysates expressing variously tagged MEKK2,JNKK2, and JNK1. As shown in Fig. 4A, both full-length MEKK2 andits COOH-terminal kinase domain coprecipitated JNK1 (lanes 3 and7). Similarly, both full-length MEKK2 and its COOH-terminal kinasedomain coprecipitated JNKK2 (Fig. 3A and 4A, lanes 2 and 6). Mostimportantly, by using a JNK1-specific monoclonal antibody, wefound that MEKK2 could coprecipitate not only the transfectedHA-JNK1 but also the endogenous JNK1 (Fig. 4B). Since both full-lengthMEKK2 and the COOH-terminal kinase domain of MEKK2 coprecipitatedJNKK2 and JNK1 equally well, the kinase domain of MEKK2 was apparentlysufficient for mounting a specific interaction with its downstreamcomponents. Consistent with this, we could not detect stable interactionsbetween the truncated N-terminal portion of MEKK2 (without theentire COOH-terminal kinase domain) and either JNKK2 or JNK1 (datanot shown).

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FIG. 4. MEKK2, JNKK2, and JNK1 form a tripartite complex through synergistic interaction. (A) COS-1 cells were transfected with various combinations of expression vectors for GST-MEKK2(FL) (1 µg/plate) (lanes 1 to 4), GST-MEKK2(CT) (0.5 µg/plate) (lanes 5 to 8), HA-JNKK2 (0.5 µg/plate) (lanes 2, 4, 6, and 8), and HA-JNK1 (0.5 µg/plate) (lanes 3, 4, 7, and 8) as indicated in the figure. GST-MEKK2(FL) and GST-MEKK2(CT) were precipitated with GSH-Sepharose beads, and their associated proteins were analyzed by Western blotting (WB) as described in the legend to Fig. 3. The percentages of HA-JNK1 bound to the GST-MEKK2(CT)-containing complex were measured. Expression of HA-JNKK2 and HA-JNK1 (middle panel) and of GST-MEKK2(FL) and GST-MEKK2(CT) (bottom panel) was determined by Western blotting. (B) COS-1 cells were transfected with GST-MEKK2(CT). After 40 h, GST-MEKK2(CT) was precipitated with GSH-Sepharose beads and its associated proteins were analyzed by Western blotting (WB) using anti-JNK1 antibody. Expression of GST-MEKK2(CT) was determined by Western blotting. (C) Equal amounts of cell lysates prepared from COS-1 cells transfected with GST-JNKK2 vector were mixed with equal amounts of COS-1 cell lysates expressing HA-JNK1 and increasing amounts of HA-MEKK2(CT). The mixtures were incubated for 4 h at 4°C in a rotator, and GST-JNKK2 was precipitated with GSH-Sepharose beads as described above. JNKK2-bound and input HA-JNK1 and HA-MEKK2(CT) were analyzed by Western blotting. The relative fold increase of JNK1 coprecipitated with JNKK2 is indicated. (D) In gel filtration analysis of the MEKK2-JNKK2-JNK1 complex, cell lysates prepared from COS-1 cells transfected with GST-MEKK2(CT), HA-JNKK2, and HA-JNK1 were loaded on a Superdex-200 column and run on a Pharmacia FPLC system. Then 20 µl of each fraction was analyzed by western blotting (WB) with anti-HA antibody and anti-MEKK2 antibody for HA-JNK1, HA-JNKK2, and MEKK2 respectively (top two panels). The remains of each fractions were subjected to a coprecipitation assay with GSH-Sepharose beads as described in the legend to Fig. 3. The precipitated GST-MEKK2(CT) and GST-MEKK2(CT)-bound HA-JNKK2 and HA-JNK1 were analyzed by western blotting (bottom two panels).

In addition to coprecipitating JNKK2 and JNK1 individually, MEKK2 was found to simultaneously coprecipitate JNKK2 and JNK1(Fig. 4A, lanes 4 and 8). Most interestingly, MEKK2 (either thefull-length or the COOH-terminal kinase domain) coprecipitatedboth JNKK2 and JNK1 more efficiently than when they were coexpressedwith either protein alone (compare lanes 2 and 3 with lane 4,and compare lanes 6 and 7 with lane 8). We consistently observedtwofold increases in JNKK2 coprecipitation with MEKK2 upon JNK1coexpression and two- to threefold increases in JNK1 coprecipitationwith MEKK2 upon JNKK2 coexpression. JNK1 was coprecipitated withMEKK2 without JNKK2 cotransfection (lanes 3 and 7), but this coprecipitationmay be mediated by the endogenous JNKK2. Thus, these data suggestedthat coexpression of JNK1 or JNKK2 could significantly affectthe interaction between MEKK2 and JNKK2 or between MEKK2 and JNK1,indicating a synergistic interaction among the three kinases MEKK2,JNKK2, andJNK1.

To further investigate whether the interaction of MEKK2, JNKK2, and JNK1 was synergistic, we coprecipitated JNK1 with JNKK2in the presence of increasing amounts of MEKK2. If a synergisticinteraction occurred among MEKK2, JNKK2, and JNK1, we would expectJNK1 coprecipitation with JNKK2 to increase significantly whenincreasing amounts of MEKK2 were added. In contrast, if the interactionswere independent, we would expect JNK1 coprecipitation with JNKK2to decrease because of the competition of MEKK with JNKK2. Asshown in Fig. 4C, while JNKK2 and JNK1 expression levels wereconstant in all transfections, JNK1 coprecipitation with JNKK2increased dramatically (up to sevenfold) with the increasing amountsof MEKK2. As expected, MEKK2 also coprecipitated with the JNKK2-JNK1complex (Fig. 4C). Together with the results described above,these data confirmed that the interaction of MEKK2, JNKK2, andJNK1 issynergistic.

To investigate whether the formation of the MEKK2-JNKK2-JNK1 complex required additional scaffolding or anchoring molecules,we carried out gel filtration experiments to determine the molecularweight of the MEKK2-JNKK2-JNK1 multimolecular complex. Cytosolicextracts were prepared from COS-1 cells transfected with GST-MEKK2(CT),HA-JNKK2, and HA-JNK1 expression vectors and subjected to gelfiltration analysis using a Pharmacia FPLC system with a Superdex-200column. Elution of MEKK2, JNKK2, and JNK1 in each fraction wasmonitored by Western blotting with the MEKK2-specific antibody1128 and anti-HA tag antibody 12CA5. The MEKK2-JNKK2-JNK1 complexin each fraction was determined by the coprecipitation assay describedfor the experiment in Fig. 4A. As shown in Fig. 4D, while MEKK2,JNKK2, and JNK1 were coeluted in fractions with a molecular massup to 200 kDa, the MEKK2-JNKK2-JNK1 tripartite complex was detectedonly in fractions corresponding to a molecular mass about 158kDa, approximately the combined molecular masses of GST-MEKK2(CT),HA-JNKK2, and HA-JNK1. Thus, these data strongly indicated thatMEKK2, JNKK2, and JNK1 can form a tripartite complex inside cellsindependent of scaffolding proteins. The MEKK2, JNKK2, and JNK1that were eluted at a molecular mass larger than 158 kDa couldbe from different multimolecular complexes, since no MEKK2-JNKK2-JNK1tripartite complex was detected in these fractions. Such a high-molecular-masscomplex was reported previously by Moriguchi et al. (37); forexample, in L5178Y cells, nearly all JNKK2/MKK7 molecules werefound by a similar gel filtration assay in fractions peaking at180kDa.

To examine whether formation of this tripartite complex is specific, we used p38, a JNK1-related MAPK, and JNKK1 as controls.Although both JNK1 and p38 were expressed at similar levels (Fig.5, lanes 3 through 6), only JNK1 (lanes 3, 5, and 7) and not p38(lanes 4, 6, and 8) was readily coprecipitated by MEKK2. Evenwhen JNKK1 and JNKK2 were coexpressed, p38 could not be coprecipitatedby MEKK2. This result suggested that p38 could not form a specificmolecular complex with MEKK2 and JNKK2. Importantly, althoughJNKK1 is able to interact with and activate p38 (30, 55, 60;Cheng and Su, unpublished), its coexpression with p38 did notresult in coprecipitation of p38 with MEKK2, even though MEKK2could coprecipitate JNKK1 (lane 6). Consistent with the resultsshown in Fig. 3A, MEKK2 also coprecipitated JNKK1 but with a loweraffinity than it coprecipitated JNKK2 (lanes 1 and 2). Importantly,this coprecipitation was not affected by the coexpression of JNK1,nor was MEKK2 coprecipitation with JNK1 affected by the expressionof JNKK1 (lane 5). These results suggested that coprecipitationof JNK1 and JNKK1 by MEKK2 (lane 5) may be due to differentialprecipitations of JNK1 and JNKK1 by MEKK2 rather than by a MEKK2-JNKK1-JNK1tripartite complex.

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FIG. 5. JNK1 but not p38 synergizes with JNKK2 to form a stable multimolecular complex with MEKK2. Equal amounts of COS-1 cell lysates expressing GST-MEKK2(CT) were mixed with lysates of COS-1 cells expressing HA-JNKK1 (lanes 1, 5, and 6), HA-JNKK2 (lanes 2, 7, and 8), HA-JNK1 (lanes 3, 5, and 7), and HA-p38 (lanes 4, 6 and 8) as indicated. The mixtures were incubated in a rotator at 4°C for 4 h. GST-MEKK2(CT) was precipitated by adding GSH-Sepharose beads and analyzed as described in Materials and Methods. The bound (top panel) and input (middle panel) amounts of HA-tagged proteins were determined by Western blotting (WB). The input amount of MEKK2(CT) was determined by Western blotting using an anti-MEKK2 antibody (bottom panel).

Formation of an MEKK2-JNKK2-JNK1 complex leads to efficient JNK activation. To determine the functional significance of the MEKK2-JNKK2-JNK1 complex, we examined whether JNK1 associated with the complexwas activated more strongly and efficiently than were nonassociatedforms. Since only a small portion of JNK1 was found in a complexcontaining MEKK2 (Fig. 4), we used an anti-HA antibody to immunoprecipitatethe entire pool of transiently expressed HA-JNK1 from lysatesof cells in which HA-JNK1 was coexpressed with MEKK2 and comparedits activity to that of JNK1 isolated by coprecipitation withMEKK2 (presumably from the complex). As shown in Fig. 6A, theJNK1 presented in the MEKK2-containing complex was much more activethan that of the total-cell lysate, indicating that the JNK1 inthe complex was activated more efficiently. Furthermore, we foundthat cotransfection of a wild-type JNKK2 caused an even greaterincrease of JNK1 enzymatic activity in the complex (Fig. 6B),probably because more JNK1 was recruited into the complex, asshown in Fig. 4. In contrast, when we cotransfected a JNKK2 mutant,JNKK2(AL), the JNK1 activity decreased (Fig. 6B), suggesting thatthe mutant could block MEKK2-activating signals in the complexand providing further evidence that JNKK2 is a major intermediateMAPKK for MEKK2 in JNK1 activation. Although wild-type JNKK2 andthe mutant JNKK2(AL) were expressed equally in these transfections,a coprecipitation assay showed that more JNKK2(AL) than wild-typeJNKK2 was coprecipitated by MEKK2 (Fig. 6C). This could be causedby the inability of JNKK2(AL) to dissociate from MEKK2. On theother hand, wild-type JNKK2 and JNK1 may quickly dissociate fromMEKK2 when activated. By competing with wild-type JNKK2 for interactionwith MEKK2 and JNK1, the JNKK2(AL) mutant blocks JNK1 activationby MEKK2 (Fig. 2 and 6B). Taken together, these results suggestedthat the MEKK2-JNKK2-JNK1 complex is an efficient MAPK modulethat is capable of strong and specific JNK1 activation.

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FIG. 6. Effective JNK1 activation in a multimolecular complex. (A) COS-1 cells were transfected with 0.1 µg of control vector or GST-MEKK2(CT) expression vector per plate, together with 0.5 µg of HA-JNK1 per plate. The cells were lysed 40 h later. Half of the lysates was used to precipitate the MEKK2(CT)-containing complex by adding GSH-Sepharose beads as described above; the other half was used to immunoprecipitate (IP) HA-JNK1 by adding the 12CA5 monoclonal antibody. The amount of HA-JNK1 precipitated by IP and GST-Sepharose beads was determined by Western blotting (WB). Equal amounts of HA-JNK1 from each precipitation were assayed for JNK activity using GST-c-Jun as substrate, as described in the legend to Fig. 1A. The relative fold increases of JNK1 activity are shown. (B) GST-MEKK2CT (10 ng/plate) and HA-JNK1 (0.5 µg/plate) expression vectors were cotransfected into COS-1 cells with expression vectors for HA-JNKK2 (0.5 µg/plate) or HA-JNKK2(AL) (0.5 µg/plate) as indicated. Cells were lysed 40 h later, and GSH-Sepharose beads were added to coprecipitate HA-JNK1 from the lysates as described in the legend to Fig. 4. The coprecipitated HA-JNK1 was assayed for kinase activity as described in the legend to Fig. 1A. Expression levels of HA-JNKK2, HA-JNKK2(AL), and HA-JNK1 were determined by Western blotting (WB). The relative fold increases of JNK1 activity are shown. (C) GST-MEKK2(CT) (0.1 µg/plate) and HA-JNK1 (0.5 µg/plate) expression vectors were cotransfected into COS-1 cells with 0.5 µg of expression vectors for HA-JNKK2 or HA-JNKK2(AL) per plate as shown. The cells were lysed 40 h later, and GSH-Sepharose beads were added to precipitate the MEKK2(CT)-containing complex. Coprecipitated HA-JNKK2, HA-JNKK2(AL), and HA-JNK1 (upper panel) and their expression levels in the cell lysates (lower panel) were determined by Western blotting (WB).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

To respond to the vast number of extracellular cues, eukaryotic cells have evolved an efficient "antenna" system with specificcell surface receptors to detect distinct stimuli and a complicatedintracellular network system with many protein kinase cascadesto transduce and integrate the surface signals in order to activateor initiate specific cellular processes that result in cell proliferation,differentiation, or apoptosis. Many of the responses are regulatedby members of the MAPK family of signal-transducing protein kinases.The recent identification of multiple MAPKs, MAPKKs, and MAPKKKsthat can be expressed within a single cell raises the questionof how specific extracellular cues can activate distinct repertoiresof MAPK effectors (13, 24, 25, 42).

We investigated how MEKK2, a member of the MEKK/STE11 subgroup of MAPKKKs, leads to specific JNK activation. Overexpressionof a modest amount of MEKK2 results in strong JNK1 activationbut only marginal activation of ERK1 and ERK2 and of p38 (9;Cheng and Su, unpublished). We found that although both MEKK2and the closely related MAPKKK MEKK1 activated JNK strongly, MEKK2was a weaker activator of JNKK1 but a more efficient activatorof JNKK2 than was MEKK1. Coexpression of JNKK2 augmented MEKK2-mediatedJNK1 activation, whereas coexpression of an inactive JNKK2 mutantinhibited MEKK2-mediated JNK1 activation (Fig. 2B). In contrast,expression of either wild-type or mutant JNKK2 had only a marginaleffect on MEKK1-mediated JNK1 activation (data not shown). Previousstudies have shown that MEKK1 activates JNK and p38 via JNKK1,which is the preferred substrate for this MAPKKK (55). JNKK1/MKK4,but not other MAPKKs such as MEK1 and MEK2, MKK3, MKK6, and JNKK2/MKK7,is the major effector molecule directly downstream of MEKK1 (30,55). Thus, MEKK1-JNKK1 specificity has been attributed to adirect physical interaction between the two molecules. We showed,in contrast, that MEKK2 appears to operate via JNKK2 rather thanvia JNKK1. Since JNKK2 is a more specific JNK kinase than is JNKK1,which is incapable of p38 activation (15, 37, 49, 59),these results also explain why MEKK2 is a less potent activatorof p38 than is MEKK1 (9; Cheng and Su,unpublished).

The strong and specific JNK1 and JNKK2 activation by MEKK2 was found to be caused by a synergistic interaction of MEKK2, JNKK2,and JNK1. In both coprecipitation and gel filtration experiments,MEKK2, JNKK2, and JNK1 were found in the same complex. Most notably,the MEKK2-JNKK2-JNK1 interaction seemed synergistic, since theinteraction between any two of these three kinases was furtherstrengthened by the presence of the third. We observed two- tothreefold augmentation of MEKK2-JNKK2 and MEKK2-JNK1 coprecipitationand up to sevenfold augmentation of JNKK2-JNK1 coprecipitationby expression of JNK1, JNKK2, or MEKK2, respectively (Fig. 4).Although MEKK2 could also interact with JNKK1, expression of JNK1or JNKK1 could not affect the interaction of MEKK2-JNKK1 or MEKK2-JNK1.Furthermore, p38, a MAPK closely related to JNK1, could not forma multimolecular complex with either MEKK2-JNKK2 or MEKK2-JNKK1,even though p38 could interact with JNKK1, suggesting that theMEKK2-JNKK2-JNK1 complex isspecific.

Recently, it was reported that MEKK3, a close homologue of MEKK2 (75% overall homology), also activated JNK1 via JNKK2 (10).Whereas we could not detect a tripartite complex of MEKK3, JNKK2,and JNK1 (data not shown), it remained to be determined whetherthe kinase domain of MEKK3 could form a tripartite complex withJNKK2 and JNK1, since the homology between the kinase domainsof MEKK2 and MEKK3 is much higher than their overall homology(93 and 75%,respectively).

The synergistic interaction of MEKK2-JNKK2-JNK1 is physiologically relevant. Using an in vitro kinase assay, we found thatJNK1 in the MEKK2-containing complex was activated more efficientlythan JNK1 that was not associated with the complex. Its activationof JNK1 in the MEKK2-containing complex depended on the presenceof a functional JNKK2, since such activation could be blockedby expression of a kinase-defective JNKK2 mutant, JNKK2(AL). Inhibitionof JNK1 activation in the complex by such a mutant was not causedby the inability of JNK to bind to the complex. Interestingly,significantly more mutant JNKK2(AL) than wild-type JNKK2 was foundin the MEKK2-containing complex (Fig. 6C). Such an example wasalso observed for STE11 and STE7 in yeast (4). This suggestedthat when JNKK2 and JNK1 in the MEKK2-containing complex are activated,they may quickly disassociate from MEKK2, allowing MEKK2 to phosphorylateand activate more substrates and hence amplify the upstreamsignals.

Direct and specific protein-protein interaction between kinases in the MAPK module has been demonstrated in both yeast andmammalian cells. Such an interaction is crucial in the formationof multimolecular signaling complexes. In mammals, MEKK1 interactsdirectly with its preferred MAPKK, JNKK1 (55), and with JNK1independent of JNKK1 (56). JNKK1 and JNKK2 also interact directlywith their substrates, JNK or p38 (22, 50, 55). Althoughthe subject of speculation, a MEKKK, a MAPKK, and a MAPK havenot been shown to form a tripartite complex without anchoringor scaffolding molecules in yeast and mammalian cells before.Our present study demonstrated that a mammalian MAPKKK, a MAPKK,and a MAPK could interact synergistically to form a specific signalingcomplex.

Two mammalian molecules, MP-1 and JIP-1, were shown recently to function as scaffold proteins, like STE5 in yeast, in organizingthe ERK-MAPK and JNK-MAPK modules (4, 32, 39, 41, 52).MP1 was shown to significantly increase the complex formationbetween MEK1 and ERK1, the two kinases in the ERK MAPK module.JIP-1 was shown to bind simultaneously to MLK3/DLK, JNKK2/MKK7,and JNK1, thus organizing a JNK MAPK module. Whether MLK3/DLK,JNKK2/MKK7, and JNK1 in the JIP-1-organized kinase module couldsynergistically interact with one another was unclear. Studiesfrom several groups including ours have shown that MLK3/DLK andJNKK2/MKK7 could directly interact with one another, as couldJNKK2/MKK7 and JNK1 (22, 34, 50; Cheng and Su, unpublished).Such interactions may be crucial for initiating the stable MAPKmodule formation organized by the scaffolding protein JIP-1 (52).The interactions could also increase the fidelity of individualMAPK pathways. Although our study suggested that coordinated interactionbetween the kinase molecules in certain MAPK pathways could formdistinct signaling modules without an anchoring or scaffoldingprotein, it did not rule out the possibility that additional moleculescould participate in the complex under certain conditions. Theirparticipation could provide additional levels of specificity controlfor each MAPK module. For instance, participation of such moleculescould provide additional surface area for interaction with variousupstream activating molecules or could insulate the MAPK modulefrom cross talk with functionally unrelated kinases in the samecell. Thus, both scaffold proteins and direct kinase-kinase interactionwithin a MAPK module may be required to determine the specificityof the MAPK cascade. Together with the sequential-activation model(55), three distinct JNK1 MAPK modules may be responsible forefficient and specific JNK1 activation in response to distinctupstream stimuli, as illustrated in Fig. 7.

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FIG. 7. Schematic diagram of three postulated mammalian JNK1 MAPK modules.

The functional role of the putative N-terminal regulatory domain of MEKK2 is still not clear. We found that the full-lengthMEKK2 and COOH-terminal kinase domain of MEKK2 interact with andactivate JNKK2 and JNK1 similarly, suggesting that the N-terminalregion of MEKK2 may have a more distinct regulatory function thanthe C-terminal kinase domain. Interestingly, overexpression ofthe N-terminal region of MEKK2 could block MEKK2 activation ofJNK1 (Cheng and Su, unpublished), suggesting that the N-terminalregion of MEKK2 may interact with another, as yet unidentifiedmolecule that regulates the activity of the MEKK2-JNKK2-JNK1 signalingcomplex. By using the yeast two-hybrid system, we recently isolatedseveral candidate genes whose products seem to interact specificallywith the N-terminal region of MEKK2. Studies of such interactingmolecules should provide further clues to understanding the specificityand regulating mechanisms of MEKK2 and other members of the MEKK/STE11gene family ingeneral.

	ACKNOWLEDGMENTS

We thank T. Hunter for helpful discussion and critical comments that improved the manuscript. We thank R. Davis, G. Johnson,J. Han, T. Deng, and A. Minden for expression plasmids; F. Zhangand Z. Dong for gel filtration analysis; and Sue Adams and LoreFeldman for their excellent assistance in preparation of themanuscript.

B.S. was a Special Fellow of the Leukemia Society of America. This work was partially supported by a grant from the AmericanAssociation for Cancer Research (RPG-97-090-01) to B.S.

Jinke Cheng and Jianhua Yang contributed equally to thiswork.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Immunology, The University of Texas, M. D. Anderson Cancer Center, 1515Holcombe Blvd., Houston, TX 77030. Phone: (713) 792-8742. Fax:(713) 745-1633. E-mail: bingsu{at}odin.mdacc.tmc.edu.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
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35. Minden, A., and M. Karin. 1997. Regulation and function of the JNK subgroup of MAP kinases. Biochim. Biophys. Acta 1333:F85-F104[Medline].

36. Minden, A., A. Lin, M. McMahon, C. Lange-Carter, B. Derijard, R. J. Davis, G. L. Johnson, and M. Karin. 1994. Differential activation of ERK and JNK mitogen-activated protein kinases by Raf-1 and MEKK. Science 266:1719-1723[Abstract/Free Full Text].

37. Moriguchi, T., F. Toyoshima, N. Masuyama, H. Hanafusa, Y. Gotoh, and E. Nishida. 1997. A novel SAPK/JNK kinase, MKK7, stimulated by TNFalpha and cellular stresses. EMBO J. 16:7045-7053[CrossRef][Medline].

38. Posas, F., and H. Saito. 1997. Osmotic activation of the HOG MAPK pathway via Ste11p MAPKKK: scaffold role of Pbs2p MAPKK. Science 276:1702-1705[Abstract/Free Full Text].

39. Printen, J. A., and G. F. Sprague, Jr. 1994. Protein-protein interactions in the yeast pheromone response pathway: Ste5p interacts with all members of the MAP kinase cascade. Genetics 138:609-619[Abstract].

40. Sanchez, I., R. T. Hughes, B. J. Mayer, K. Yee, J. R. Woodgett, J. Avruch, J. M. Kyriakis, and L. I. Zon. 1994. Role of SAPK/ERK kinase-1 in the stress-activated pathway regulating transcription factor c-Jun. Nature 372:794-798[Medline].

41. Schaeffer, H. J., A. D. Catling, S. T. Eblen, L. S. Collier, A. Krauss, and M. J. Weber. 1998. MP1: a MEK binding partner that enhances enzymatic activation of the MAP kinase cascade. Science 281:1668-1671[Abstract/Free Full Text].

42. Schlesinger, T. K., G. R. Fanger, T. Yujiri, and G. L. Johnson. 1998. The TAO of MEKK. Front. Biosci. 3:D1181-D1186[Medline].

43. Seger, R., and E. G. Krebs. 1995. The MAPK signaling cascade. FASEB J. 9:726-735[Abstract].

44. Stein, B., M. X. Yang, D. B. Young, R. Janknecht, T. Hunter, B. W. Murray, and M. S. Barbosa. 1997. p38-2, a novel mitogen-activated protein kinase with distinct properties. J. Biol. Chem. 272:19509-19517[Abstract/Free Full Text].

45. Su, B., E. Jacinto, M. Hibi, T. Kallunki, M. Karin, and Y. Ben-Neriah. 1994. JNK is involved in signal integration during costimulation of T lymphocytes. Cell 77:727-736[CrossRef][Medline].

46. Su, B., and M. Karin. 1996. Mitogen-activated protein kinase cascades and regulation of gene expression. Curr. Opin. Immunol. 8:402-411[CrossRef][Medline].

47. Teramoto, H., O. A. Coso, H. Miyata, T. Igishi, T. Miki, and J. S. Gutkind. 1996. Signaling from the small GTP-binding proteins Rac1 and Cdc42 to the c-Jun N-terminal kinase/stress-activated protein kinase pathway. A role for mixed lineage kinase 3/protein-tyrosine kinase 1, a novel member of the mixed lineage kinase family. J. Biol. Chem. 271:27225-27228[Abstract/Free Full Text].

48. Tibbles, L. A., Y. L. Ing, F. Kiefer, J. Chan, N. Iscove, J. R. Woodgett, and N. J. Lassam. 1996. MLK-3 activates the SAPK/JNK and p38/RK pathways via SEK1 and MKK3/6. EMBO J. 15:7026-7035[Medline].

49. Tournier, C., A. J. Whitmarsh, J. Cavanagh, T. Barrett, and R. J. Davis. 1997. Mitogen-activated protein kinase kinase 7 is an activator of the c-Jun NH2-terminal kinase. Proc. Natl. Acad. Sci. USA 94:7337-7342[Abstract/Free Full Text].

50. Tournier, C., A. J. Whitmarsh, J. Cavanagh, T. Barrett, and R. J. Davis. 1999. The MKK7 gene encodes a group of c-Jun NH2-terminal kinase kinases. Mol. Cell. Biol. 19:1569-1581[Abstract/Free Full Text].

51. Wang, X. S., K. Diener, D. Jannuzzi, D. Trollinger, T. H. Tan, H. Lichenstein, M. Zukowski, and Z. Yao. 1996. Molecular cloning and characterization of a novel protein kinase with a catalytic domain homologous to mitogen-activated protein kinase kinase kinase. J. Biol. Chem. 271:31607-31611[Abstract/Free Full Text].

52. Whitmarsh, A. J., J. Cavanagh, C. Tournier, J. Yasuda, and R. J. Davis. 1998. A mammalian scaffold complex that selectively mediates MAP kinase activation. Science 281:1671-1674[Abstract/Free Full Text].

53. Wilson, I. A., H. L. Niman, R. A. Houghten, A. R. Cherenson, M. L. Connolly, and R. A. Lerner. 1984. The structure of an antigenic determinant in a protein. Cell 37:767-778[CrossRef][Medline].

54. Wu, Z., J. Wu, E. Jacinto, and M. Karin. 1997. Molecular cloning and characterization of human JNKK2, a novel Jun NH2-terminal kinase-specific kinase. Mol. Cell. Biol. 17:7407-7416[Abstract].

55. Xia, Y., Z. Wu, B. Su, B. Murray, and M. Karin. 1998. JNKK1 organizes a MAP kinase module through specific and sequential interactions with upstream and downstream components mediated by its amino-terminal extension. Genes Dev. 12:3369-3381[Abstract/Free Full Text].

56. Xu, S., and M. H. Cobb. 1997. MEKK1 binds directly to the c-Jun N-terminal kinases/stress-activated protein kinases. J. Biol. Chem. 272:32056-32060[Abstract/Free Full Text].

57. Xu, S., D. J. Robbins, L. B. Christerson, J. M. English, C. A. Vanderbilt, and M. H. Cobb. 1996. Cloning of rat MEK kinase 1 cDNA reveals an endogenous membrane-associated 195-kDa protein with a large regulatory domain. Proc. Natl. Acad. Sci. USA 93:5291-5295[Abstract/Free Full Text].

58. Yamaguchi, K., K. Shirakabe, H. Shibuya, K. Irie, I. Oishi, N. Ueno, T. Taniguchi, E. Nishida, and K. Matsumoto. 1995. Identification of a member of the MAPKKK family as a potential mediator of TGF-beta signal transduction. Science 270:2008-2011[Abstract/Free Full Text].

59. Yang, J., L. New, Y. Jiang, J. Han, and B. Su. 1998. Molecular cloning and characterization of a human protein kinase that specifically activates c-Jun N-terminal kinase. Gene 212:95-102[CrossRef][Medline].

60. Zanke, B. W., E. A. Rubie, E. Winnett, J. Chan, S. Randall, M. Parsons, K. Boudreau, M. McInnis, M. Yan, D. J. Templeton, and J. R. Woodgett. 1996. Mammalian mitogen-activated protein kinase pathways are regulated through formation of specific kinase-activator complexes. J. Biol. Chem. 271:29876-29881[Abstract/Free Full Text].

61. Zhou, G., Z. Q. Bao, and J. E. Dixon. 1995. Components of a new human protein kinase signal transduction pathway. J. Biol. Chem. 270:12665-12669[Abstract/Free Full Text].

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52.	Whitmarsh, A. J., J. Cavanagh, C. Tournier, J. Yasuda, and R. J. Davis. 1998. A mammalian scaffold complex that selectively mediates MAP kinase activation. Science 281:1671-1674[Abstract/Free Full Text].
53.	Wilson, I. A., H. L. Niman, R. A. Houghten, A. R. Cherenson, M. L. Connolly, and R. A. Lerner. 1984. The structure of an antigenic determinant in a protein. Cell 37:767-778[CrossRef][Medline].
54.	Wu, Z., J. Wu, E. Jacinto, and M. Karin. 1997. Molecular cloning and characterization of human JNKK2, a novel Jun NH2-terminal kinase-specific kinase. Mol. Cell. Biol. 17:7407-7416[Abstract].
55.	Xia, Y., Z. Wu, B. Su, B. Murray, and M. Karin. 1998. JNKK1 organizes a MAP kinase module through specific and sequential interactions with upstream and downstream components mediated by its amino-terminal extension. Genes Dev. 12:3369-3381[Abstract/Free Full Text].
56.	Xu, S., and M. H. Cobb. 1997. MEKK1 binds directly to the c-Jun N-terminal kinases/stress-activated protein kinases. J. Biol. Chem. 272:32056-32060[Abstract/Free Full Text].
57.	Xu, S., D. J. Robbins, L. B. Christerson, J. M. English, C. A. Vanderbilt, and M. H. Cobb. 1996. Cloning of rat MEK kinase 1 cDNA reveals an endogenous membrane-associated 195-kDa protein with a large regulatory domain. Proc. Natl. Acad. Sci. USA 93:5291-5295[Abstract/Free Full Text].
58.	Yamaguchi, K., K. Shirakabe, H. Shibuya, K. Irie, I. Oishi, N. Ueno, T. Taniguchi, E. Nishida, and K. Matsumoto. 1995. Identification of a member of the MAPKKK family as a potential mediator of TGF-beta signal transduction. Science 270:2008-2011[Abstract/Free Full Text].
59.	Yang, J., L. New, Y. Jiang, J. Han, and B. Su. 1998. Molecular cloning and characterization of a human protein kinase that specifically activates c-Jun N-terminal kinase. Gene 212:95-102[CrossRef][Medline].
60.	Zanke, B. W., E. A. Rubie, E. Winnett, J. Chan, S. Randall, M. Parsons, K. Boudreau, M. McInnis, M. Yan, D. J. Templeton, and J. R. Woodgett. 1996. Mammalian mitogen-activated protein kinase pathways are regulated through formation of specific kinase-activator complexes. J. Biol. Chem. 271:29876-29881[Abstract/Free Full Text].
61.	Zhou, G., Z. Q. Bao, and J. E. Dixon. 1995. Components of a new human protein kinase signal transduction pathway. J. Biol. Chem. 270:12665-12669[Abstract/Free Full Text].