|
|
|
|
|
|
|
||
| |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
© The Rockefeller University Press,
0021-9525/2001//273 $5.00
The Journal of Cell Biology, Volume 153, Number 2,
, 2001 273-282
Original Article |
Integrin-Mediated Adhesion Regulates ERK Nuclear Translocation and Phosphorylation of Elk-1
aaplin{at}med.unc.edu
Integrin-mediated adhesion to the extracellular matrix permits efficient growth factor-mediated activation of extracellular signal–regulated kinases (ERKs). Points of regulation have been localized to the level of receptor phosphorylation or to activation of the downstream components, Raf and MEK (mitogen-activated protein kinase/ERK kinase). However, it is also well established that ERK translocation from the cytoplasm to the nucleus is required for G1 phase cell cycle progression. Here we show that phosphorylation of the nuclear ERK substrate, Elk-1 at serine 383, is anchorage dependent in response to growth factor treatment of NIH 3T3 fibroblasts. Furthermore, when we activated ERK in nonadherent cells by expression of active components of the ERK cascade, subsequent phosphorylation of Elk-1 at serine 383 and Elk-1–mediated transactivation were still impaired compared with adherent cells. Elk-1 phosphorylation was dependent on an intact actin cytoskeleton, as discerned by treatment with cytochalasin D (CCD). Finally, expression of active MEK failed to predominantly localize ERK to the nucleus in suspended cells or adherent cells treated with CCD. These data show that integrin-mediated organization of the actin cytoskeleton regulates localization of activated ERK, and in turn the ability of ERK to efficiently phosphorylate nuclear substrates.
Key Words: integrins • extracellular signal–regulated kinase • Elk-1 • actin cytoskeleton • translocation
© 2001 The Rockefeller University Press
 |
Introduction |
|---|
 TopAbstract Introduction Materials and MethodsResultsDiscussionReferences |
|---|
Upon mitogenic stimulation, ERK translocates from the cytoplasm to the nucleus, where it phosphorylates the ternary complex factors Elk-1 and Sap-1a (Chen et al. 1992; Gille et al. 1992; Lenormand et al. 1993). Phosphorylation of Elk-1 increases its affinity for the serum response factor and in concert enhances transcription of growth-related proteins, such as c-Fos (Marais et al. 1993; Whitmarsh et al. 1995). Several sites in the COOH terminus of Elk-1 are phosphorylated by ERK, the most critical of which appears to be serine 383 (Marais et al. 1993). ERK-mediated transcriptional events ultimately impinge on cell cycle elements, such as the induction of cyclin D1 (Albanese et al. 1995; Lavoie et al. 1996), although it is becoming evident that activation of additional pathways, such as the phosphatidyl-inositol-3-kinase pathway, are often required for cell cycle progression (Marshall 1999).
Progression through the G1 phase of the cell cycle is jointly regulated by adhesion to the extracellular matrix and circulating growth factors, and is manifested in alterations in the levels of cyclin D1 and the cyclin-dependent kinase inhibitors, p21cip1 and p27kip1 (Assoian 1997; Bottazzi et al. 1999). Integrin–growth factor collaboration leading to efficient activation of ERK correlates with anchorage-dependent effects on cyclin D1 levels (Roovers et al. 1999). Nonetheless, recent reports provide evidence that simply activating ERK in the absence of integrin engagement is not always sufficient for cyclin D1 expression. Thus, Roovers et al. reported that forced activation of ERK in suspended NIH 3T3 cells substantially overrides the adhesion requirement for expression of cyclin D1 (Roovers et al. 1999). In contrast, Le Gall et al. 1998 found that forced ERK activation is not sufficient to induce cyclin D1 and downstream events, such as hyperphosphorylation of the retinoblastoma protein and S phase entry, in suspended CCL 39 fibroblasts. Together, these data raise the possibility that the regulatory effect of integrins on the ERK pathway may extend beyond the level of ERK activation.
ERK translocation to the nucleus is essential for G1 phase progression (Brunet et al. 1999). In resting conditions, ERK is anchored in the cytoplasm by its association with MEK (Fukuda et al. 1997), the microtubule network (Reszka et al. 1995), and phosphatases, for example MAP kinase phosphatase-3 (MKP-3), and the protein tyrosine phosphatase SL (Camps et al. 1998; Blanco-Aparicio et al. 1999). MEK–ERK association is disrupted upon mitogenic stimulation and a proportion of ERK translocates to the nucleus. The requirement for MAP kinases to move between the cytoplasmic and nuclear compartments to fulfill many of their actions highlights the importance of regulated movement through nuclear pore complexes. Active transport between the cytoplasmic and nuclear compartments is a bidirectional process: specific cytoplasmic proteins are imported into the nucleus, and proteins, tRNA, and mRNAs are exported from the nucleus (Gorlich 1998; Kaffman and O'Shea 1999). Identification of a consensus nuclear localization signal (NLS) characterized by one or more clusters of basic amino acids in numerous proteins has spurred on the study of the mechanism underlying nucleocytoplasmic trafficking. In general, nuclear import of proteins requires the concerted action of importins 
and β (also known as karyopherins) acting as carrier molecules, the small GTPase Ran, and pp15 (also known as p10 or NTF2). However, ERKs do not contain a consensus nuclear localization sequence. Rather, translocation is dependent on phosphorylation of ERK at the regulatory threonine and tyrosine residues and also on homodimerization (Fukuda et al. 1997; Khokhlatchev et al. 1998). ERK translocation is likely to be an active mechanism possibly through interactions with the importin proteins that play a key role in protein passage across the nuclear membrane (Gorlich 1998). Once dephosphorylated in the nucleus, ERK is rapidly exported via an active mechanism that is mediated, at least in part, by MEK that has entered the nucleus independently from ERK (Adachi et al. 2000).
As ERK translocation is a critical determinant in the transcriptional and biological responses to activation of this pathway, we addressed whether ERK activity, in the absence of integrin engagement, was able to impinge on nuclear events. We demonstrate that under conditions of equivalent ERK activity, ERK-mediated phosphorylation of the transcription factor Elk-1 is diminished in the absence of integrin engagement or upon disruption of the actin cytoskeleton. Additionally, Elk-1–driven gene transcription is low in nonadherent cells despite ERK being activated. Both during nonadherent conditions and in the absence of an intact cytoskeleton in adherent cells, ERK predominantly accumulated in the cytoplasm rather than translocating to the nucleus. Thus, integrin-mediated adhesion permits ERK to efficiently localize in the nucleus and phosphorylate a key downstream nuclear substrate.
|
Materials and Methods |
|---|
|
TopAbstractIntroductionMaterials and MethodsResultsDiscussionReferences |
|---|
ED, encoding an active version of MEK1 with an NH2-terminal deletion of residues 32–51 and serine residues within its activation loop replaced with acidic amino acids, was from Dr. N. Ahn (University of Colorado, Boulder, CO) (Mansour et al. 1994).
Cell Culture and Transfection
NIH 3T3 and Tet-off NIH 3T3 cells were maintained in DMEM containing 10% bovine calf serum. Additionally, 2 µg/ml tetracycline was included in the medium for the Tet-off cell lines as described previously (Roovers et al. 1999; Zhu et al. 2000). Tet-off NIH 3T3 cells harboring either a construct encoding a constitutively active form of MEK1, MEK1-S218D/S222D, [tet-MEK*-3T3], or cyclin D1 [tet-cyclin D1-3T3] were used. To retain high percentages of cells expressing active MEK, clones were used at low (<20) passage numbers. The tet-MEK*-3T3 cell clone 7B was used in these experiments. Transient transfections were performed with SuperFect (QIAGEN) according to the manufacturer's instructions.
Cell Adhesion and Preparation of Cell Lysate
Confluent cells were serum starved and processed as described previously (Aplin and Juliano 1999). In brief, cells were detached with trypsin, which was subsequently quenched with soybean trypsin inhibitor (GIBCO BRL). Cells were resuspended in DMEM with 1% BSA and incubated nonadherently at 37°C for 45 min in a rotator. Cells were then plated onto dishes coated with 10 µg/ml human fibronectin (Collaborative Biomedical Product) for a further 3 h. As indicated, some cells were treated stimulated with 10–20 ng/ml EGF; no significant differences were seen between concentrations within this range. Cells were lysed in a modified RIPA buffer and cell lysates were cleared by centrifugation at 16,000 g.
Immunofluorescence Microscopy
Cells replated on glass coverslides were prepared for immunofluorescence microscopy as described previously (Aplin and Juliano 1999). Elk-1 was detected with anti–Elk-1 polyclonal antibody (New England Biolabs, Inc.). Slides were viewed on a ZEISS Axioskop microscope equipped for epifluorescence and images were captured using MetaMorph imaging software. For confocal microscopy experiments, tet-MEK*-3T3 and tet-cyclin D1-3T3 cells were incubated in serum-free DMEM for 24 h and subsequently reseeded onto coverslips for the control monolayer and cytochalasin D (CCD; 2 µg/ml final concentration)-treated cultures, or into petri dishes coated with 1% agarose for the suspension cultures. The cells were maintained in 10% FCS in the absence of tetracycline for either 6 or 9 h to allow for efficient expression of ectopic active MEK and cyclin D1. At selected times spanning G1 phase, control monolayer, CCD, and suspension cultures were fixed and stained as described previously (Zhu et al. 1999). MEK1 was detected with an anti-MEK1 monoclonal antibody (Transduction Laboratories), and ERK was detected with an anti-ERK1 polyclonal antibody (clone K-23; Santa Cruz Biotechnology, Inc.). The immunofluorescence analysis for cyclin D1 was performed using the ammonium sulfate fraction of a polyclonal cyclin D1 antibody prepared against recombinant murine cyclin D1. Slides were visualized using a Leica TCS 4D confocal immunofluorescence microscope and 1-µm sections were captured at 40x magnification using an Image Graphics image recorder.
Immunoprecipitation, Western Blotting, and Kinase Reactions
Immunoprecipitations were performed either overnight or for 2 h at 4°C from precleared lysates followed by a further incubation with protein G-Sepharose for 2 h at 4°C. FLAG–Elk-1, endogenous focal adhesion kinase (FAK), and hemagglutinin (HA)-ERK1 were immunoprecipitated with anti-FLAG antibody (Sigma-Aldrich), clone 2A7 (Upstate Biotechnology), and anti-HA antibody, 12CA5 (Babco), respectively. Precipitates were washed three times with cold RIPA buffer, and boiled with SDS-PAGE sample buffer to dissociate the proteins. For analysis by Western blotting, samples were separated by SDS-PAGE under reducing conditions. Phosphoserine 383 and total levels of Elk-1 were detected using antibodies from New England Biolabs, Inc. and Santa Cruz Biotechnology, Inc. Antibodies to the Raf COOH terminus (clone C-12; Santa Cruz Biotechnology, Inc.), FAK (clone 77, Transduction Laboratories), MEK (Transduction Laboratories), dually phosphorylated ERK (New England Biolabs, Inc.), total ERK (Santa Cruz Biotechnology, Inc.), and phosphotyrosine (clone 4G10; Upstate Biotechnology) were also used. Immunoreactivity was detected using horseradish peroxidase–conjugated secondary antibodies and enhanced chemiluminescence. HA-ERK1 in vitro kinase assays using myelin basic protein as substrate have also been described previously (Aplin and Juliano 1999).
Luciferase Reporter Assays
Elk-1 transcriptional activity was determined using a construct encoding a fusion between the GAL4 DNA binding domain and the transactivation domain of Elk-1 (GAL4–Elk-1). NIH 3T3 cells were transfected with 500 ng GAL4–Elk-1, 500 ng of a reporter plasmid controlling the transcription of firefly luciferase (pFR-luc), 10 ng of pRL-CMV-luc (Renilla luciferase under the control of the CMV promoter), and 1 µg of either pcDNA3-22W Raf or empty vector. Cells were transfected for 4 h, serum starved for 8 h, and then detached from the dish and rolled for 45 min in DMEM/BSA. The subsequent increase in luciferase activity was determined in cells either maintained in suspension or replated on fibronectin for a further 4 h.
Luciferase activities were determined using the dual luciferase assay kit (Promega). Cells were extracted and assayed sequentially for firefly and Renilla luciferase activities. Cell lysate (20 µl) was incubated with 100 µl of luciferin reagent and luminescence recorded for 10 s in an Analytical Luminescence Laboratory Monolight 2010 luminometer. Subsequently, Stop and Glo® reagent (100 µl) was added and the specific luminescence from the Renilla luciferase was recorded for an additional 10 s. Firefly activities were normalized to Renilla luciferase activity.
|
Results |
|---|
|
TopAbstractIntroductionMaterials and MethodsResultsDiscussionReferences |
|---|
|
ED. Akin to 22WRaf, expression of MEK1-ED efficiently activated ERK1 regardless of the cellular state of adhesion (Fig. 2 D). Activation of the c-Jun NH2-terminal kinase (JNK) pathway also results in phosphorylation of Elk-1 (Whitmarsh et al. 1995). As expected, expression of 22W Raf or MEK1-ED did not result in activation of an epitope-tagged version of JNK1 (data not shown). Together, these data show that the adhesion-dependent requirement for the activation of ERK is bypassed by expression of active versions of Raf and MEK.
|
ED resulted in efficient phosphorylation of serine 383 in Elk-1 when cells were adherent to fibronectin but not under suspension conditions (Fig. 3 B). In both the 22W Raf and MEK1-ED experiments, there remained a small but noticeable increase in the phosphorylation of Elk-1 above control conditions in suspended cells. Thus, the adhesion effect on ERK-mediated phosphorylation of Elk-1 is potent but not complete.
|
Disruption of the Actin Cytoskeleton Inhibits ERK Phosphorylation of Elk-1
Integrin signaling events are typically dependent on an intact actin cytoskeleton. We used the actin depolymerizing agent, CCD, that caps the ends of growing actin fibers and inhibits integrin-mediated tyrosine phosphorylation of focal adhesion proteins (Burridge et al. 1992). Treatment of 22W Raf–expressing cells with CCD significantly reduced ERK phosphorylation of Elk-1 in adherent cells (Fig. 4 A, top). Under these conditions, cells remained round but firmly attached when viewed by microscopy, and FAK phosphotyrosine levels were dramatically reduced (Fig. 4 A, bottom). Overall, in these transient transfection experiments, the CCD effect was not quite as dramatic as the inhibition of Elk-1 phosphorylation in suspension. In vitro kinase assays demonstrated that ERK activation by 22W Raf was not inhibited by treatment with CCD (Fig. 4 B). In contrast, treatment of 22W Raf–expressing cells with the microtubule-disrupting agent, colchicine, did not inhibit Elk-1 phosphorylation at serine 383 (Fig. 4 C). Thus, the ability of ERK, once activated, to phosphorylate Elk-1 is dependent on an intact actin cytoskeleton, but not the microtubule network.
|
|
Disruption of the Actin Cytoskeleton Does Not Prevent Nuclear Accumulation of Cyclin D1
Similar to ERK, cyclin D1 does not contain a consensus nuclear localization sequence; rather, it is localized to the nucleus via such sequences in the cyclin-dependent kinase inhibitors, p21cip1 and p27kip1 (LaBaer et al. 1997; Cheng et al. 1999). To examine the possibility that disruption of the actin cytoskeleton has a global effect on nucleocytoplasmic transport, we analyzed nuclear localization of cyclin D1 in CCD-treated cells. Confocal immunolocalization experiments showed that nuclear accumulation of ectopically expressed cyclin D1 in tet-cyclin D1-3T3 cells, was not altered upon disruption of the actin cytoskeleton as indicated by its colocalization with DAPI-stained nuclei (Fig. 6). Thus, nuclear accumulation of cyclin D1 protein via a consensus nuclear signal import mechanism is not dependent on an intact actin cytoskeleton.
|
|
Discussion |
|---|
|
TopAbstractIntroductionMaterials and MethodsResultsDiscussionReferences |
|---|
The observation that integrity of the actin cytoskeleton is necessary for trafficking of ERK to the nucleus is a novel and interesting finding. Although it is well established that activation of the ERK pathway contributes to induction of cyclin D1, previous studies have yielded inconsistent results with regard to the role of ERK signaling in the adhesion-dependent expression of cyclin D1 expression. Roovers et al. 1999 reported that forced activation of the MEK/ERK pathway leads to the expression of cyclin D1 in suspended 3T3 cells, whereas Le Gall et al. 1998, using a similar approach, failed to see cyclin D1 expression when the MEK/ERK pathway was activated in suspended CCL39 cells. As relatively low levels of ERK signaling are sufficient to induce cyclin D1 (for a review see Roovers and Assoian 2000), our results may provide an explanation for these discrepant observations. Perhaps the different results obtained by Roovers et al. 1999 and Le Gall et al. 1998 reflects the fact that ERK translocation to the nucleus is strongly dependent on integrin signaling in some cell lines, whereas it is less strictly dependent on integrin signaling in others. Indeed, we do see low levels of nuclear ERK staining when induced tet-MEK*-3T3 cells used in Roovers et al. 1999 are cultured in suspension or treated with CCD.
We favor the explanation that integrins support efficient ERK translocation to the nucleus, as we find that in cells expressing active MEK, ERK preferentially colocalizes with MEK in the cytoplasm of nonadherent but not adherent cells. Other recent findings have pointed towards an adhesion dependence of ERK translocation to the nucleus (Danilkovitch et al. 2000). In these studies, macrophage-stimulating protein showed reduced ERK activation and a further lack of detectable ERK translocation to the nucleus in suspended RE7 epithelial cells; however, this study did not examine ERK translocation under conditions where high ERK activity is maintained in suspended cells. ERK is deactivated by the activity of a variety of cellular phosphatases, including MKPs, and dephosphorylation of nuclear ERK leads to its rapid export (Khokhlatchev et al. 1998), thus possibly presenting an alternative explanation of our results. However, in our system it is unlikely that dephosphorylation of ERK is upregulated in suspended cells, as ERK activation mediated by active versions of either Raf or MEK was unaltered in suspension versus adherent conditions. Additionally, under serum-free conditions levels of the nuclear-localized MKP-2 are unaltered in suspended versus adherent cells (data not shown). The activities controlling Elk-1 dephosphorylation are not well characterized, although recent studies in COS cells have implicated a role for the calcium-dependent protein phosphatase 2B (calcineurin) (Sugimoto et al. 1997; Tian and Karin 1999).
Integrin-mediated adhesion has been shown to recruit a variety of structural and signaling molecules into specialized sites and to cause the membrane localization of the GTPase, Rac (Burridge et al. 1992; del Pozo et al. 2000). However, the mechanism underlying effects of adhesion on ERK trafficking to the nucleus is as yet undetermined. ERK is sequestered in the cytoplasm through its interaction with binding partners, such as its upstream activator MEK, and efficient ERK-mediated activation of gene transcription is enhanced through the binding of the scaffolding protein, MEK partner 1 (MP-1) (Schaeffer et al. 1998). Thus, the balance of ERK interactions between its upstream activators and scaffolding proteins may be altered by the state of cellular adhesion. Nuclear translocation of ERK is dependent on its ability to homodimerize; ERK mutants defective in this ability poorly translocate to the nucleus when microinjected into fibroblasts (Khokhlatchev et al. 1998). An intriguing notion is that integrins, via the formation of an actin-based platform, enhance the ability of ERK monomers to homodimerize. Consistent with this idea, recent evidence suggests, at least under in vitro conditions, that ERK can directly bind to actin and actin-binding proteins, such as -actinin (Leinweber et al. 1999). Furthermore, active ERK molecules can be detected at sites of integrin-mediated adhesion (Fincham et al. 2000). Future research will be directed at understanding the mechanism underlying the adhesion regulation of ERK nucleocytoplasmic trafficking.
Our findings add credence to the emerging theme that cell adhesion molecules regulate nuclear signaling events. Ingber and colleagues have shown that integrin "hard-wiring" is able to impact on nuclear structure (Maniotis et al. 1997). Further, certain integrins may provide direct modulation of nuclear events. For example, engagement of the leukocyte integrin LFA-1/Lβ2 has been shown to initially bind and subsequently promote the nuclear localization of the c-Jun coactivator, JAB1, leading to enhanced activating protein 1 (AP-1) transcriptional activity (Bianchi et al. 2000). High expression levels of the cell–cell adhesion molecules, E- and N-cadherin, reduce the nuclear localization and transcription potential of β-catenin, by recruiting it to sites of cell–cell contact (Sadot et al. 1998; Orsulic et al. 1999). In conjunction with our current findings on integrin regulation of ERK localization, these other reports highlight an important role for cell adhesion molecules and the actin cytoskeleton in the nuclear trafficking of signaling molecules.
|
Acknowledgments |
|---|
This work was supported by National Institutes of Health grants GM26165 (R.L. Juliano) and CA72639 (R.K. Assoian). Sheryl Stewart is supported by a predoctoral fellowship from the American Heart Association.
Submitted: 3 November 2000
Revised: 16 January 2001
Accepted: 20 February 2001
Abbreviations used in this paper: CCD, cytochalasin D; ERK, extracellular signal–regulated kinase; FAK, focal adhesion kinase; HA, hemagglutinin; MAP, mitogen-activated protein; MEK, MAP kinase/ERK kinase; MKP, MAP kinase phosphatase.
|
References |
|---|
|
TopAbstractIntroductionMaterials and MethodsResultsDiscussionReferences |
|---|
Adachi M., Fukuda M. & Nishida E.. Nuclear export of MAP kinase (ERK) involves a MAP kinase kinase (MEK)-dependent active transport mechanism, J. Cell Biol, 148, 2000, 849–856.
Albanese C., Johnson J., Watanabe G., Eklund N., Vu D., Arnold A. & Pestell R.G.. Transforming p21ras mutants and c-Ets-2 activate the cyclin D1 promoter through distinguishable regions, J. Biol. Chem., 270, 1995, 23589–23597.
Aplin A.E. & Juliano R.L.. Integrin and cytoskeletal regulation of growth factor signaling to the MAP kinase pathway, J. Cell Sci., 112, 1999, 695–706.[Abstract]
Aplin A.E., Short S.M. & Juliano R.L.. Anchorage-dependent regulation of the mitogen-activated protein kinase cascade by growth factors is supported by a variety of integrin alpha chains, J. Biol. Chem, 274, 1999, 31223–31228.
Assoian R.K.. Anchorage-dependent cell cycle progression, J. Cell Biol., 136, 1997, 1–4.
Bianchi E., Denti S., Granata A., Bossi G., Geginat J., Villa A., Rogge L. & Pardi R.. Integrin LFA-1 interacts with the transcriptional co-activator JAB1 to modulate AP-1 activity, Nature., 404, 2000, 617–621.[Medline]
Blanco-Aparicio C., Torres J. & Pulido R.. A novel regulatory mechanism of MAP kinases activation and nuclear translocation mediated by PKA and the PTP-SL tyrosine phosphatase, J. Cell Biol, 147, 1999, 1129–1136.
Bottazzi M.E., Zhu X., Bohmer R.M. & Assoian R.K.. Regulation of p21cip1 expression by growth factors and the extracellular matrix reveals a role for transient ERK activity in G1 phase, J. Cell Biol, 146, 1999, 1255–1264.
Brunet A., Roux D., Lenormand P., Dowd S., Keyse S. & Pouyssegur J.. Nuclear translocation of p42/p44 mitogen-activated protein kinase is required for growth factor-induced gene expression and cell cycle entry, EMBO (Eur. Mol. Biol. Organ.) J, 18, 1999, 664–674.[Medline]
Burridge K., Turner C.E. & Romer L.H.. Tyrosine phosphorylation of paxillin and pp125FAK accompanies cell adhesion to extracellular matrixa role in cytoskeletal assembly, J. Cell Biol., 119, 1992, 893–903.
Calderwood D.A., Shattil S.J. & Ginsberg M.H.. Integrins and actin filamentsreciprocal regulation of cell adhesion and signaling, J. Biol. Chem, 275, 2000, 22607–22610.
Camps M., Nichols A., Gillieron C., Antonsson B., Muda M., Chabert C., Boschert U. & Arkinstall S.. Catalytic activation of the phosphatase MKP-3 by ERK2 mitogen-activated protein kinase, Science, 280, 1998, 1262–1265.
Chen R.H., Sarnecki C. & Blenis J.. Nuclear localization and regulation of ERK- and RSK-encoded protein kinases, Mol. Cell. Biol., 12, 1992, 915–927.
Cheng M., Olivier P., Diehl J.A., Fero M., Roussel M.F., Roberts J.M. & Sherr C.J.. The p21cip1 and p27kip1 CDK ‘inhibitors’ are essential activators of cyclin D-dependent kinases in murine fibroblasts, EMBO (Eur. Mol. Biol. Organ.) J, 18, 1999, 1571–1583.[Medline]
Danilkovitch A., Donley S., Skeel A. & Leonard E.J.. Two independent signaling pathways mediate the antiapoptotic action of macrophage-stimulating protein on epithelial cells, Mol. Cell. Biol, 20, 2000, 2218–2227.
del Pozo M.A., Price L.S., Alderson N.B., Ren X.D. & Schwartz M.A.. Adhesion to the extracellular matrix regulates the coupling of the small GTPase Rac to its effector PAK, EMBO (Eur. Mol. Biol. Organ.) J, 19, 2000, 2008–2014.[Medline]
Fincham V.J., James M., Frame M.C. & Winder S.J.. Active ERK/MAP kinase is targeted to newly forming cell-matrix adhesions by integrin engagement and v-Src, EMBO (Eur. Mol. Biol. Organ.) J, 19, 2000, 2911–2923.[Medline]
Fukuda M., Gotoh Y. & Nishida E.. Interaction of MAP kinase with MAP kinase kinaseits possible role in the control of nucleocytoplasmic transport of MAP kinase, EMBO (Eur. Mol. Biol. Organ.) J., 16, 1997, 1901–1908.[Medline]
Gille H., Sharrocks A.D. & Shaw P.E.. Phosphorylation of transcription factor p62TCF by MAP kinase stimulates ternary complex formation at c-fos promoter, Nature., 358, 1992, 414–417.[Medline]
Gorlich D.. Transport into and out of the cell nucleus, EMBO (Eur. Mol. Biol. Organ.) J, 17, 1998, 2721–2727.[Medline]
Kaffman A. & O'Shea E.K.. Regulation of nuclear localizationa key to a door, Annu. Rev. Cell Dev. Biol, 15, 1999, 291–339.[Medline]
Khokhlatchev A.V., Canagarajah B., Wilsbacher J., Robinson M., Atkinson M., Goldsmith E. & Cobb M.H.. Phosphorylation of the MAP kinase ERK2 promotes its homodimerization and nuclear translocation, Cell, 93, 1998, 605–615.[Medline]
LaBaer J., Garrett M.D., Stevenson L.F., Slingerland J.M., Sandhu C., Chou H.S., Fattaey A. & Harlow E.. New functional activities for the p21 family of CDK inhibitors, Genes Dev, 11, 1997, 847–862.
Lavoie J.N., L'Allemain G., Brunet A., Muller R. & Pouyssegur J.. Cyclin D1 expression is regulated positively by the p42/p44MAPK and negatively by the p38/HOGMAPK pathway, J. Biol. Chem., 271, 1996, 20608–20616.
Le Gall M., Grall D., Chambard J.C., Pouyssegur J. & Van Obberghen-Schilling E.. An anchorage-dependent signal distinct from p42/44 MAP kinase activation is required for cell cycle progression, Oncogene, 17, 1998, 1271–1277.[Medline]
Leinweber B.D., Leavis P.C., Grabarek Z., Wang C.L. & Morgan K.G.. Extracellular regulated kinase (ERK) interaction with actin and the calponin homology (CH) domain of actin-binding proteins, Biochem. J, 344, 1999, 117–123.[Medline]
Lenormand P., Sardet C., Pages G., L'Allemain G., Brunet A. & Pouyssegur J.. Growth factors induce nuclear translocation of MAP kinases (p42mapk and p44mapk) but not of their activator MAP kinase kinase (p45mapkk) in fibroblasts, J. Cell Biol., 122, 1993, 1079–1088.
Lin T.H., Chen Q., Howe A. & Juliano R.L.. Cell anchorage permits efficient signal transduction between Ras and its downstream kinases, J. Biol. Chem., 272, 1997, 8849–8852.
Maniotis A.J., Chen C.S. & Ingber D.E.. Demonstration of mechanical connections between integrins, cytoskeletal filaments, and nucleoplasm that stabilize nuclear structure, Proc. Natl. Acad. Sci. USA, 94, 1997, 849–854.
Mansour S.J., Matten W.T., Hermann A.S., Candia J.M., Rong S., Fukasawa K., Vande Woude G.F. & Ahn N.G.. Transformation of mammalian cells by constitutively active MAP kinase kinase, Science, 265, 1994, 966–970.
Marais R., Wynne J. & Treisman R.. The SRF accessory protein Elk-1 contains a growth factor-regulated transcriptional activation domain, Cell, 73, 1993, 381–393.[Medline]
Marshall C.. How do small GTPase signal transduction pathways regulate cell cycle entry?, Curr. Opin. Cell Biol., 11, 1999, 732–736.[Medline]
Miyamoto S., Teramoto H., Gutkind J.S. & Yamada K.M.. Integrins can collaborate with growth factors for phosphorylation of receptor tyrosine kinases and MAP kinase activationroles of integrin aggregation and occupancy of receptors, J. Cell Biol., 135, 1996, 1633–1642.
Orsulic S., Huber O., Aberle H., Arnold S. & Kemler R.. E-cadherin binding prevents beta-catenin nuclear localization and beta-catenin/LEF-1-mediated transactivation, J. Cell Sci., 112, 1999, 1237–1245.[Abstract]
Renshaw M.W., Ren X.D. & Schwartz M.A.. Growth factor activation of MAP kinase requires cell adhesion, EMBO (Eur. Mol. Biol. Organ.) J., 16, 1997, 5592–5599.[Medline]
Reszka A.A., Seger R., Diltz C.D., Krebs E.G. & Fischer E.H.. Association of mitogen-activated protein kinase with the microtubule cytoskeleton, Proc. Natl. Acad. Sci. USA, 92, 1995, 8881–8885.
Roovers K., Davey G., Zhu X., Bottazzi M.E. & Assoian R.K.. 5β1 integrin controls cyclin D1 expression by sustaining mitogen-activated protein kinase activity in growth factor-treated cells, Mol. Biol. Cell, 10, 1999, 3197–3204.
Roovers K. & Assoian R.K.. Integrating the MAP kinase signal into the G1 phase cell cycle machinery, BioEssays., 22, 2000, 818–826.[Medline]
Sadot E., Simcha I., Shtutman M., Ben-Ze'ev A. & Geiger B.. Inhibition of β-catenin-mediated transactivation by cadherin derivatives, Proc. Natl. Acad. Sci. USA, 95, 1998, 15339–15344.
Schaeffer H.J., Catling A.D., Eblen S.T., Collier L.S., Krauss A. & Weber M.J.. MP1a MEK binding partner that enhances enzymatic activation of the MAP kinase cascade, Science, 281, 1998, 1668–1671.
Short S.M., Boyer J.L. & Juliano R.L.. Integrins regulate the linkage between upstream and downstream events in G-protein-coupled receptor signaling to mitogen-activated protein kinase, J. Biol. Chem., 275, 2000, 12970–12977.
Stanton V.P. Jr. & Cooper G.M.. Activation of human raf transforming genes by deletion of normal amino-terminal coding sequences, Mol. Cell. Biol, 7, 1987, 1171–1179.
Sugimoto T., Stewart S. & Guan K.L.. The calcium/calmodulin-dependent protein phosphatase calcineurin is the major Elk-1 phosphatase, J. Biol. Chem, 272, 1997, 29415–29418.
Tian J. & Karin M.. Stimulation of Elk1 transcriptional activity by mitogen-activated protein kinases is negatively regulated by protein phosphatase 2B (calcineurin), J. Biol. Chem, 274, 1999, 15173–15180.
Whitmarsh A.J., Shore P., Sharrocks A.D. & Davis R.J.. Integration of MAP kinase signal transduction pathways at the serum response element, Science, 269, 1995, 403–407.
Yang S.H., Whitmarsh A.J., Davis R.J. & Sharrocks A.D.. Differential targeting of MAP kinases to the ETS-domain transcription factor Elk-1, EMBO (Eur. Mol. Biol. Organ.) J, 17, 1998, 1740–1749.[Medline]
Zhu X., Roovers K., Davey G. & Assoian R.K.. Methods for analysis of adhesion-dependent cell cycle progression, Guan J.-L.. Signaling Through Cell Adhesion Molecules, 1999, 129–140, CRC Press, Boca Raton, FL.
Zhu X., Scharf E. & Assoian R.K.. Induction of anchorage-independent growth by transforming growth factor-beta linked to anchorage-independent expression of cyclin D1, J. Biol. Chem, 275, 2000, 6703–6706.
CiteULike 
Complore 
Connotea 
Del.icio.us 
Digg 
Facebook 
Reddit 
Technorati 
Twitter What's this?
Related Article
| |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
|
|
