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Vol. 11, Issue 5, 1709-1725, May 2000
¶**
*Molecular Oncology Group, McGill University Hospital Center, and
Departments of Anatomy and Cell Biology,
Biochemistry, Medicine, and
¶Oncology, McGill University, Montreal, Quebec, Canada,
H3A 1A1; and §Division of Signal Transduction, Nara
Institute of Science and Technology, Ikoma 630-0101, Japan
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Hepatocyte growth factor (HGF), the ligand for the Met receptor tyrosine kinase, is a potent modulator of epithelial-mesenchymal transition and dispersal of epithelial cells, processes that play crucial roles in tumor development, invasion, and metastasis. Little is known about the Met-dependent proximal signals that regulate these events. We show that HGF stimulation of epithelial cells leads to activation of the Rho GTPases, Cdc42 and Rac, concomitant with the formation of filopodia and lamellipodia. Notably, HGF-dependent activation of Rac but not Cdc42 is dependent on phosphatidylinositol 3-kinase. Moreover, HGF-induced lamellipodia formation and cell spreading require phosphatidylinositol 3-kinase and are inhibited by dominant negative Cdc42 or Rac. HGF induces activation of the Cdc42/Rac-regulated p21-activated kinase (PAK) and c-Jun N-terminal kinase, and translocation of Rac, PAK, and Rho-dependent Rho-kinase to membrane ruffles. Use of dominant negative and activated mutants reveals an essential role for PAK but not Rho-kinase in HGF-induced epithelial cell spreading, whereas Rho-kinase activity is required for the formation of focal adhesions and stress fibers in response to HGF. We conclude that PAK and Rho-kinase play opposing roles in epithelial-mesenchymal transition induced by HGF, and provide new insight regarding the role of Cdc42 in these events.
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Epithelial-mesenchymal transition and cell migration are required
during normal embryonic development and during pathological situations
such as the dispersal of tumor cells. Hepatocyte growth factor (HGF) is
a multifunctional factor that, in addition to promoting epithelial cell
growth and survival, has the ability in vitro to stimulate epithelial
cell dissociation, motility, invasion, and the endogenous morphogenic
program of epithelial cells in three-dimensional matrix or organ
culture (Matsumoto and Nakamura, 1996
, 1997; Montesano et
al., 1997). Genetic studies have shown that HGF/Met signaling is
essential for normal murine embryological development (Birchmeier and
Gherardi, 1998). In addition, HGF/Met signaling was also shown to be
involved in angiogenesis (Bussolino et al., 1992; Grant
et al., 1993) and has been implicated in the dissociation
and migration of muscle precursor cells of the dermomyotome, in the
guidance and survival of motor neurons, and in the development and
survival of sensory neurons (Birchmeier and Gherardi, 1998). HGF and
Met were also shown to play a role in pathological conditions,
including tissue regeneration (Matsumoto and Nakamura, 1997),
tumorigenesis, and metastasis (Jeffers et al., 1996;
Bardelli et al., 1997).
The conversion from a sessile to a migratory phenotype requires an
extensive remodeling of the actin cytoskeleton (Mitchison and Cramer,
1996). Members of the Rho family of small GTP-binding proteins,
including Cdc42, Rac, and Rho, are involved in regulating the
organization of the actin cytoskeleton and the assembly of associated
integrin complexes (Hall, 1998). These proteins cycle between
an inactive (GDP-bound) and an active (GTP-bound) conformation in which
they interact with specific effector proteins. The conversion from the
inactive to the active state is regulated by members of the Dbl family
of guanine nucleotide exchange factors (Cerione and Zheng, 1996),
whereas inactivation is stimulated by the RhoGAP family of
GTPase-activating proteins (Lamarche and Hall, 1994). Initial studies
in Swiss 3T3 fibroblasts have demonstrated that activation of Rho
promotes the formation of stress fibers and focal adhesion complexes
(Ridley and Hall, 1992), that Rac promotes the polymerization of actin
at the cell membrane, producing lamellipodia and membrane ruffles
(Ridley et al., 1992), and that Cdc42 promotes the formation
of filopodia and microspikes at the cell periphery (Kozma et
al., 1995; Nobes and Hall, 1995). Rac and Cdc42 also induce the
assembly of integrin complexes associated with polymerized actin (Nobes and Hall, 1995). Moreover, in Swiss 3T3 fibroblasts, activation of Cdc42 can lead to activation of Rac, which in turn can
lead to activation of Rho, implicating signal cross-talk between these
proteins (Ridley and Hall, 1992; Ridley et al., 1992; Nobes and Hall, 1995).
Several extracellular factors have been shown to activate Rho
family members and induce the corresponding changes on the actin cytoskeleton. In fibroblasts, lysophosphatidic acid or bombesin stimulate Rho activation (Ridley and Hall, 1992); PDGF, EGF, bombesin, and insulin promote Rac activation (Ridley et al., 1992;
Nobes et al., 1995); and bradykinin leads to activation of
Cdc42 (Kozma et al., 1995). Thus, the Rho family proteins
represent key signal transducers that link membrane receptors to the
organization of the actin cytoskeleton. Several downstream target
molecules of the Rho family proteins have now been identified
(Aspenström, 1999), and among them, the p21-activated kinase
(PAK) family and Rho-kinase isoforms have been implicated as mediators
of actin and focal adhesion reorganization (Leung et al.,
1996; Amano et al., 1997; Ishizaki et al., 1997;
Manser et al., 1997; Sells et al., 1997; Frost
et al., 1998). PAK kinases bind to and are strongly activated by both GTP-bound Cdc42 and Rac (Manser et al.,
1994; Bagrodia et al., 1995b; Martin et al.,
1995), whereas Rho-kinase/Rok
and p160ROCK isoforms bind to
activated Rho (Leung et al., 1995; Ishizaki et
al., 1996; Matsui et al., 1996), although they have also been reported to interact with GTP-bound Rac (Joneson et al., 1996; Lamarche et al., 1996).
To understand the HGF-dependent signaling pathways involved in actin
reorganization required for epithelial-mesenchymal transition and cell
dispersal, we have used Madin-Darby canine kidney (MDCK) epithelial
cells that grow as colonies of tightly associated cells. However,
unlike serum-starved quiescent Swiss 3T3 cells that do not contain
highly polymerized actin, MDCK cells grown as colonies contain abundant
circumferential or peripheral bundles of polymerized actin in lateral
membranes in association with junctional complexes involved in
cell-cell adhesion. Therefore, the dispersal of epithelial sheets
requires the dissolution of these peripheral actin bundles in
conjunction with the dissociation of the junctional complexes. We have
shown previously that HGF-induced dissociation of MDCK epithelial cells
is preceded by the centrifugal spreading of cells within colonies. This
is dependent on phosphatidylinositol 3-kinase (PI3K) activity
and is concomitant with the loss of insoluble E-cadherin and
desmoplakins from sites of cell-cell adhesion (Royal and Park, 1995;
Potempa and Ridley, 1998). Moreover, studies by others have revealed
that Ras and Rac were also required for HGF-induced MDCK cell spreading
and dissociation (Hartmann et al., 1994; Ridley et
al., 1995). Epithelial cell spreading is completed 3-5 h after stimulation with HGF; however, nothing was known about the HGF-induced proximal cellular and biochemical events required for these later morphological changes. In this paper, we have characterized the signaling pathways required for the immediate effects of HGF on the
actin cytoskeleton and the subsequent consequences of these signals on
the initial steps of epithelial-mesenchymal transition, cell
spreading, and dissociation.
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MATERIALS AND METHODS |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Cell Culture and Microinjection
MDCK epithelial cells were cultured in DMEM supplemented
with 10% FBS and 50 µg/ml gentamicin (Life Technologies, Burlington, Ontario, Canada). For microinjection, MDCK cells (5 × 103) were seeded on glass coverslips (Bellco
Glass, Vineland, NJ) in 24-well dishes (Nunc) and grown for 2-3
d. Cells were injected in serum because prolonged serum starvation
promotes a decrease in E-cadherin at cell-cell junctions. Small
colonies of 10-50 cells were partially microinjected (Eppendorf
Scientific, Westbury, NY). For all experiments, 100-200 cells were
microinjected during a 15-min period, and data shown are representative
of the results obtained in a minimum of four experiments. When assaying
for HGF-induced lamellipodia formation, MDCK cells (5 × 104) were seeded 1 d before injection. In
each experiment, ~100 cells microinjected with the corresponding
constructs were evaluated for biological response. Expression vectors
(50, 100, and 200 µg/ml) were diluted in PBS and occasionally
coinjected with rabbit immunoglobulin G (2 mg/ml; Pierce, Rockford, IL)
to mark injected cells. The cells were incubated for 2-5 h to allow
for protein expression and were further incubated, as indicated, in the
presence of HGF (5 U/ml) before fixation. Human HGF was purified from
conditioned medium of COS cells after their transient transfection with
a human HGF expression construct (Zhu et al., 1994) or was
obtained from Dr. George Vande Woude (National Cancer
Institute-Frederick Cancer Research and Development Center, Frederick,
MD). One unit is defined as the minimal amount of HGF per milliliter of
medium required to induce scatter of MDCK cells and is generally
equivalent to 1-2 ng/ml.
Immunofluorescence Microscopy
Injected cells were fixed in 3.7% formaldehyde for 10 min and permeabilized in 0.2% Triton X-100 in PBS for 5 min. Cells were incubated for 30 min with a FITC-labeled rabbit antibody (Jackson ImmunoResearch Laboratories, West Grove, PA) to detect injected cells. Actin filaments were visualized by incubating cells for 45 min with 0.05 µg/ml TRITC-labeled phalloidin (Sigma, Oakville, Ontario, Canada) diluted in 0.2% Triton X-100 (in PBS). Where indicated, cells were incubated for 30 min with the 9E10 Myc antibody to detect the expressed Myc-tagged proteins, followed by a 30-min incubation with a FITC-labeled mouse antibody (Sigma). For vinculin staining, cells were incubated for 10 min with CSK lysis buffer (10 mM piperazine-N,N'-bis[2-ethanesulfonic acid], pH 7.0, 300 mM sucrose, 50 mM NaCl, 3 mM MgCl2, 0.5% Triton X-100), fixed in 3.7% formaldehyde for 5 min, and then incubated with a mouse vinculin antibody (Sigma) for 30 min, followed by a 30-min incubation with the Cy3-conjugated mouse antibody (Jackson ImmunoResearch Laboratories). The coverslips were mounted on slides in Immuno-Fluore medium (ICN, Costa Mesa, CA), and cells were viewed on a Nikon (Garden City, NY) Labophot-2 epifluorescence microscope. Images were photographed with the use of Kodak (Rochester, NY) TMZ-3200 film and digitalized with an Agfa Canada (Montreal, Quebec, Canada) T-1200 color scanner.
For immunolocalization of endogenous Rac, MDCK cells were fixed and permeabilized as described above and then incubated for 30 min with a Rac mAb (Transduction Laboratories, San Diego, CA), followed by a 30-min incubation with an anti-mouse mAb coupled to Alexa 488 (Molecular Probes, Eugene, OR) and TRITC-phalloidin to stain for actin. In this case, however, cell washes were performed with PBS containing 5% FBS and 0.1% Triton X-100, which was also used to dilute the antibodies. Immunolocalization of Myc-PAK and Myc-Rho-kinase was performed with the 9E10 antibody as described above. Immunostained cells were examined with a Zeiss (Montreal, Quebec, Canada) laser confocal microscope, and sectioning along the z-axis was performed at intervals of 0.35 µm with a pinhole number of 20 and scanning times of 16 s.
Cell Transfection
Cells were transfected by the standard calcium phosphate technique. MDCK cells (6 × 105/100 mm) were transfected with 5 µg of pEF-BOSMyc-Rho-kinase or pRK5Myc-PAK1 in the presence of 25 µg of carrier DNA (pBluescript, Stratagene, La Jolla, CA) and 250 ng of the neomycin-encoding vector pcDNA3.1 (Invitrogen, Carlsbad, CA). The precipitate was removed the next day, and the selection drug G-418 (400 µg/ml) was added to the medium 24 h later. Clones were obtained after 10-14 d, and the levels of expression were determined by Western blotting. Clones were used for Rho-kinase and PAK localization and for PAK kinase assays in response to HGF. For Cdc42 and Rac activation assays, MDCK cells (1 × 106/100 mm) were transiently transfected with 10 µg of pRK5Myc-Cdc42 or pRK5Myc-Rac cDNAs and 50 µl of Geneporter transfection reagent (Gene Therapy System, San Diego, CA) in 5 ml of DMEM without serum. The next day, cells were stimulated with HGF.
Purification of GST-WASP and GST-PAK
GST-WASP (aa 201-321) (Aspenström et
al., 1996) and GST-PAK (aa 56-272 of PAK1; Sander et
al., 1998) (a kind gift of Dr. John Collard, The Netherlands
Cancer Institute, Division of Cell Biology, Amsterdam) were used to
isolate activated Cdc42 and Rac, respectively, from stimulated MDCK
cell lysates. Escherichia coli transformed with the GST-WASP
and GST-PAK constructs were grown at 37°C to an absorbance of 0.5. Expression of the fusion proteins was induced with
isopropyl-
-D-thiogalactopyranoside (0.1 mM) for 3 h at 37°C. Cells were washed once in STE buffer (100 mM Tris-Cl, pH 8.0, 100 mM NaCl, 1 mM EDTA) before sonication in 20 mM
HEPES, pH 7.5, 120 mM NaCl, 2 mM EDTA, 10% glycerol, 10 µg/ml
aprotinin, 10 µg/ml leupeptin, 1 mM PMSF. The lysates were cleared by
centrifugation, and NP-40 was added to a final concentration of 0.5%.
The proteins were stored at 
80°C until use. Per sample, 10-15 µg
of GST-WASP or GST-PAK (as estimated by Coomassie blue staining) was
purified on glutathione-Sepharose beads (Amersham Pharmacia Biotech,
Baie d'Urfe, Quebec, Canada) for 30 min at room temperature with
gentle rocking. The Sepharose beads were washed twice with lysis
buffer, and the protein lysates were added as described below.
Cdc42/Rac Activation Assays
MDCK cells transiently expressing Myc-tagged G12Cdc42 or
G12Rac were stimulated 16-20 h after transfection with 100 or 200 U/ml
HGF for different times. Cells were lysed in 25 mM HEPES, pH 7.5, 1%
NP-40, 10 mM MgCl2, 100 mM NaCl, 5% glycerol, 5 mM sodium fluoride, 1 mM sodium vanadate, 1 mM PMSF, 10 µg/ml
aprotinin, 10 µg/ml leupeptin. Equal protein levels (700 µg) were
incubated for 1 h at 4°C with purified GST-PAK or GST-WASP
(10-15 µg) purified in a twofold volume of binding buffer (25 mM
HEPES, pH 7.5, 30 mM MgCl2, 40 mM NaCl, 0.5%
NP-40, 1 mM DTT) as described (Benard et al., 1999). Beads
were washed four times in binding buffer containing 1% NP-40 and
boiled in Laemmli sample buffer, and the proteins were separated on a
15% SDS-polyacrylamide gel. The levels of Myc-tagged Cdc42 and
Myc-tagged Rac bound to the fusion proteins, as well as the levels
present in whole cell lysates (10 µg), were evaluated by Western
blotting with the 9E10 Myc mAb followed by the ECL detection
according to the manufacturer's protocol (Amersham Pharmacia Biotech).
PAK Kinase Assay
MDCK cells expressing Myc-tagged PAK1 (8 × 105) were seeded in 100-mm dishes and serum
starved the next day for 24 h in 0.1% FBS. Cells were stimulated
with HGF (100 U/ml) at 37°C for the indicated times. Cells were lysed
in 10 mM HEPES, pH 7.5, 150 mM NaCl, 1 mM EDTA, 0.6% Triton X-100, 20 mM -glycerophosphate, 10% glycerol, 5 mM sodium fluoride, 1 mM
sodium vanadate, 1 mM PMSF, 10 µg/ml aprotinin, 10 µg/ml leupeptin.
Proteins (200 µg of cell lysates) were incubated at 4°C with the
monoclonal 9E10 Myc antibody for 1 h followed by incubation with
30 µl of protein G-Sepharose (40% suspension; Amersham Pharmacia
Biotech) for an additional 1 h. The immune complexes were then
washed three times with the lysis buffer and once with the kinase
buffer (20 mM HEPES, pH 7.5, 20 mM MgCl2, 10 mM
MnCl2, 20 mM -glycerophosphate, 1 mM DTT, 0.1 mM sodium vanadate, 5 mM sodium fluoride, 1 mM PMSF, 10 µg/ml
aprotinin, 10 µg/ml leupeptin). The kinase reaction was performed for
10 min at 37°C in 25 µl of kinase buffer containing 10 µM ATP, 5 µg of myelin basic protein (MBP), and 20 µCi of
[
-32P]ATP. The reaction was stopped by
adding 4× Laemmli sample buffer, and proteins were separated by
electrophoresis on a 15% SDS-polyacrylamide gel. Myc-tagged PAK1
expression levels were evaluated by Western blotting with the 9E10 Myc antibody.
c-Jun N-terminal Kinase Assay
MDCK cells (8 × 105/100 mm) were prepared and
stimulated as described above for the PAK kinase assay. After
stimulation, cells were lysed as described (Adler et al.,
1992). Bacteria expressing GST-c-Jun (aa 5-89) were kindly provided
by Dr. James Woodgett (Ontario Cancer Institute, Toronto, Canada).
Fusion proteins were produced by
isopropyl--D-thiogalactopyranoside induction,
lysed, and purified on glutathione-Sepharose beads. Kinase reactions were performed in the presence of 10 µg of cell lysate from each time
point, 3 µg of GST-c-Jun, 10 µM ATP, and 20 µCi of
[-32P]ATP, as described (Adler et
al., 1992).
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Microspikes and Lamellipodia Are the Earliest Morphological Changes Induced by HGF in MDCK Cells
In response to HGF, colonies of MDCK epithelial cells
undergo multiple morphological changes leading to
epithelial-mesenchymal transition and cell dispersal. This occurs as a
series of sequential events in which the centrifugal spreading of all
cells within the colony is concomitant with a decrease in cell-cell
adhesion molecules by 3-4 h of HGF stimulation and the subsequent loss of cell-cell contacts and the acquisition of a motile mesenchymal cell
phenotype by 8-16 h (Royal and Park, 1995). To characterize the
earliest morphological and biochemical changes induced by HGF and to
evaluate their contribution to the spreading and dissociation of
colonies of MDCK cells, the reorganization of the actin cytoskeleton in
response to HGF was first investigated. Visualization of F-actin with
TRITC-phalloidin revealed that few actin stress fibers were present in
small colonies of unstimulated MDCK cells and that actin was mostly
concentrated at the edge of the colonies (Figure 1, ) and at cell-cell borders in
peripheral bundles associated with the lateral membranes of the cells
(Figure 1). The earliest change observed after stimulation was the
appearance of actin-containing hair-like structures resembling
filopodia or microspikes 5 min after HGF stimulation (Figure 1, 5 min).
By 15 min, lamellipodia harboring small membrane ruffles developed on
the outer membranes of cells at the edge of the colony (Figure 1, 15 min), and by 30 min, actin stress fibers appeared within these
lamellipodia (Figure 1, 30 min). Moreover, by 18 h after HGF
stimulation, MDCK cells had adopted a fibroblastic phenotype and
exhibited lamellipodia and membrane ruffles typical of motile cells
(Figure 1, 18 h, inset). These observations indicate that in the
course of events ultimately leading to epithelial-mesenchymal
transition and cell dispersal, the formation of filopodia and
lamellipodia are the earliest morphological changes observed in
response to HGF.
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Cdc42, Rac, PAK and c-Jun N-terminal Kinase Are Activated by HGF in MDCK Cells
Two members of the Rho family of small GTP-binding proteins, Cdc42
and Rac, control actin polymerization into filopodial and lamellipodial
membrane protrusions in Swiss 3T3 cells (Hall, 1998). To determine if
Cdc42 and Rac were activated by HGF, an assay based on the ability of
activated Cdc42 and activated Rac to bind effector proteins was used
(Sander et al., 1998; Benard et al., 1999).
Lysates of HGF-stimulated MDCK cells, transiently expressing Myc-tagged
Cdc42 or Myc-tagged Rac, were incubated with GST-WASP or GST-PAK fusion
proteins coupled to glutathione-Sepharose beads. GST-WASP (aa
201-321) encodes the Cdc42-binding site of the WASP effector protein
and was used to isolate activated Cdc42, whereas GST-PAK (aa 56-272)
encodes the Cdc42- and Rac-binding domain of the PAK1 effector protein
and was used to isolate activated Rac (Figure
2). Upon stimulation of MDCK cells with
HGF, activated Cdc42 was detected 5 min after stimulation, reached a
maximum at 15 min, and decreased thereafter (Figure 2A). In contrast, after correcting for protein levels, Rac activation was highest at 15 min, decreased at 30 min, and decreased below the basal level at 60 min
(Figure 2B). Significantly, the pretreatment of MDCK cells with the
PI3K inhibitor LY294002 led to the inhibition of Rac but not Cdc42
activity (Figure 2, A and B). Activation of endogenous Rac occurred
with similar kinetics in response to HGF (Figure 2C). Moreover, Rac was
relocalized to membrane ruffles after stimulation with HGF for 15 min
(Figure 2C). Together, these results confirm the data derived from the
actin staining and show for the first time that Cdc42 is activated by
HGF in MDCK cells, with distinct kinetics from Rac activation.
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Constitutively activated Cdc42 or Rac mutants lead to stimulation of
PAK and c-Jun N-terminal kinase (JNK) activity in transiently transfected COS-1, COS-7, and HeLa cells (Bagrodia et al.,
1995a; Coso et al., 1995; Minden et al., 1995;
Olson et al., 1995; Brown et al., 1996). As
further support for Cdc42 and Rac activation by HGF, we investigated if
PAK and JNK were activated after stimulation of MDCK cells (Figure
3). Serum-starved MDCK cells stably
expressing Myc-tagged PAK1 were treated with 100 U/ml HGF for various
times. Myc-PAK1 was immunoprecipitated with the 9E10 Myc mAb, and its kinase activity was assessed using MBP as a substrate. PAK1
autophosphorylation and MBP phosphorylation were increased at 5 min
after HGF stimulation (1.5-fold), were maximal at 15 min (2.1-fold),
and remained high up to 1 h after stimulation (Figure 3A). An
increase in the phosphorylation of GST-c-Jun, indicative of endogenous
JNK activation, was detected 5 min after HGF stimulation (1.4-fold),
was maximal at 15 min (2.2-fold), and decreased below basal levels by
1 h (Figure 3B). Thus, HGF induces activation of PAK and JNK in
MDCK cells, consistent with the observed Cdc42 and Rac activation
(Figure 2).
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Cdc42, Rac, and PI3K Are Required for HGF-induced Lamellipodia Formation, Cell Spreading, and Dissociation
To assess the requirement for Cdc42 and Rac in the actin
reorganization observed in MDCK cells at early times after HGF
stimulation, expression vectors encoding dominant negative mutants of
Cdc42 (N17Cdc42) and Rac (N17Rac) were injected into the nuclei of MDCK cells. The expression of N17Cdc42 (Figure
4A, a and d) or N17Rac (Figure 4A, b, c,
e, and f) reduced the number of cells that formed HGF-induced
lamellipodia to 55 ± 6% and 34 ± 15%, respectively, that
of control cells injected with vector alone (normalized to 100%; Table
1), and instead, an increase in the
amount of actin stress fibers was observed. In addition, expression of
N17Rac enhanced the presence of microspikes at 15 min after HGF
stimulation in 77 ± 8% of the injected cells (Figure 4A, e and
f). Microinjection of wild-type Cdc42 into MDCK cells promotes the
formation of filopodia and subsequent lamellipodia (I. Royal and M. Park, unpublished observations), whereas microinjection or transfection
of activated Rac promotes lamellipodia formation (Jou and Nelson, 1998;
I. Royal and M. Park, unpublished observation). Hence, the data showing that dominant negative N17Rac expression increases HGF-induced filopodia formation suggest that in colonies of MDCK epithelial cells,
as observed in serum-starved quiescent Swiss 3T3 fibroblasts, Rac acts
downstream from Cdc42 in a signaling cascade required for the formation
of lamellipodia. Moreover, consistent with a requirement for PI3K
activity in lamellipodia formation downstream of PDGF and insulin
(Wennstrom et al., 1994; Nobes et al., 1995) and
in HGF-dependent Rac activation (Figure 2, B and C), MDCK cells
pretreated with the PI3K inhibitor LY294002 were unable to form
lamellipodia in response to HGF for 15 min (our unpublished result).
However, in agreement with the observation that HGF-induced Cdc42
activation is independent of PI3K activation (Figure 2A), pretreatment
of MDCK cells with LY294002 did not inhibit the formation of
microspikes in response to HGF (our unpublished result).
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In addition to inhibiting the formation of lamellipodia in response to
HGF, the expression of N17Cdc42 also blocked HGF-induced MDCK cell
spreading and dissociation that occur as late events at 3-4 h after
stimulation (Figure 4B, a and b). In a similar manner, MDCK cells
injected with N17Rac cDNA (Figure 4B, c and d) (Ridley et
al., 1995) or treated with LY294002 (our unpublished result) or
wortmannin (Royal and Park, 1995) also failed to spread. Together,
these data demonstrate that PI3K, Cdc42, and Rac are essential for the
initial formation of lamellipodia and the subsequent spreading and
dissociation of MDCK colonies in response to HGF.
Rho Family Effector Proteins PAK and Rho-Kinase Translocate to Membrane Ruffles in Response to HGF
Several proteins binding to Rho family GTPases are involved in
actin and focal adhesion reorganization (Aspenström, 1999). Among
these, PAK family members and Rho-kinase isoforms exert opposite
effects, where PAK leads to the disruption and Rho-kinase leads to the
formation of stress fibers and focal adhesions via regulation of the
myosin light chain kinase (Amano et al., 1996, 1997; Kimura
et al., 1996; Manser et al., 1997; Frost et
al., 1998; Sanders et al., 1999). PAK family members,
as mentioned above, interact with and are activated by Cdc42 and Rac,
whereas Rho-kinase isoforms (Rho-kinase/ROK, p160ROCK) bind to
activated Rho, although they have also been reported to bind to
activated Rac (Leung et al., 1995; Ishizaki et
al., 1996; Joneson et al., 1996; Lamarche et
al., 1996; Matsui et al., 1996). Activation of PAK and
Rho-kinase by PDGF and V14Rho, respectively, leads to their
translocation from the cytosol to the cell membrane (Leung et
al., 1995; Matsui et al., 1996; Dharmawardhane et
al., 1997). Consistent with activation of PAK by HGF (Figure 3),
translocation of PAK to membrane ruffles was observed 15 min after HGF
stimulation of MDCK cells stably expressing myc-tagged PAK1 (Figure
5A). Similarly, Rho-kinase translocated
from the cytosol to membrane ruffles 15 min after stimulation of MDCK
cells stably expressing myc-tagged Rho-kinase (Figure 5A). Confocal
sectioning of the cells in the z-axis in successive sections
through the lamellipodia and membrane ruffles demonstrated enrichment
of PAK and Rho-kinase at those sites (Figure 5, B and C). Therefore,
based on the reported activities of these two proteins on the actin
cytoskeleton and on their localization in membrane ruffles at the edge
of lamellipodia in response to HGF, PAK and Rho-kinase represent likely
modulators of MDCK cell morphology.
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HGF-induced Lamellipodia in MDCK Cell Colonies Involves Rho-Kinase and PAK
To examine the role of Rho-kinase in the early HGF-induced
morphological changes, MDCK cells were injected with a dominant interfering mutant of Rho-kinase, RB/PH(TT) (aa 941-1388). This mutant
encompasses the C-terminal pleckstrin homology (PH) domain of
Rho-kinase in addition to the Rho-binding domain (RB) that is rendered
nonfunctional by the substitution of Asn-1027 and Lys-1028 with
threonine (Amano et al., 1998). Consistent with a role for
Rho-kinase in stress fiber formation (Leung et al., 1996;
Amano et al., 1997), the expression of RB/PH(TT) in
unstimulated MDCK cells resulted in the loss of endogenous stress
fibers and, in addition, of peripheral actin (our unpublished results).
After HGF stimulation for 15 min, RB/PH(TT)-expressing cells failed to
develop lamellipodia harboring an organized network of actin, and
lamellipodia were present in only 36 ± 6% of the injected cells
compared with MDCK cells injected with a control vector (normalized to
100%) (Table 1; Figure 6A, a-d).
Similarly, MDCK cells pretreated with HA1077 (20 µM), an inhibitor of
Rho-kinase and other kinases (Uehata et al., 1997), lost
actin fibers and were unable to induce lamellipodia formation after HGF
stimulation (our unpublished results). Thus, Rho-kinase activity and/or
a preassembled actin network was required for the ability of HGF to
induce lamellipodia in MDCK cells. Consistent with this, the injection
of MDCK cells with a construct expressing a constitutively activated
Rho-kinase (Rho-kinase catalytic domain [CAT]) induced an increase in
actin stress fibers, which, in cells at the edge of the colony,
frequently emanated from discrete areas and terminated in membrane
extensions (in 34 ± 3% of the injected cells; Figure 7, a and b), suggesting that Rho-kinase
activity and/or the resulting actin network may act to potentiate
HGF-dependent lamellipodia formation.
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In contrast to CAT, the injection of a cDNA vector encoding a
constitutively activated PAK (PAK1L107F) induced the loss of actin
stress fibers and peripheral actin in 100% of the injected cells
1 h after injection (Figure 7, c and d) and cell rounding by
2 h (our unpublished result). Even at low concentrations of DNA (1 µg/ml), loss of stress fibers could be observed 3.5 h after injection. To establish if PAK activity was required for HGF-induced actin remodeling, MDCK cells were injected with an expression vector
encoding the N-terminal regulatory domain of PAK2 (PAKR; aa 1-225)
(Martin et al., 1995; Minden et al., 1995). In
addition to the Cdc42/Rac interaction domain, PAKR encodes an
autoinhibitory domain that inhibits PAK kinase activity in vitro and in
vivo and contains proline-rich domains with potential to compete for PAK-binding proteins (Frost et al., 1998; Zhao et
al., 1998; Tu and Wigler, 1999). Notably, the ability of MDCK
cells expressing PAKR for 5 h to remodel peripheral actin and to
extend typical lamellipodia in response to HGF for 15 min was decreased
to 19 ± 1% compared with control pRK5-injected cells (Figure 6A,
e and f; Table 1). Together, our results demonstrate that both PAK and
Rho-kinase are required for the early remodeling of peripheral actin
leading to lamellipodia formation in response to HGF.
PAK Activity Is Required for HGF-induced Cell Spreading and Dissociation
To determine if PAK and Rho-kinase activity were also required for the late HGF-induced cell spreading and dissociation, MDCK cells injected with vectors expressing the PAKR or RB/PH(TT) dominant negative mutant were stimulated with HGF for 3-4 h. Strikingly, MDCK cells expressing PAKR remained small and tightly associated 3 h after HGF stimulation (Figure 6B, a and b). In contrast, MDCK cells expressing RB/PH(TT) (Figure 6B, c and d) spread equally or more than noninjected cells in response to HGF for 4 h. Notably, expression of RB/PH(TT) could induce cell spreading on its own (our unpublished result). In addition, the vast majority of cells expressing RB/PH(TT) had dissociated and changed shape, whereas noninjected cells were still associated (Figure 6B, e and f). Thus, in contrast to PAK, inhibition of Rho-kinase activation by dominant negative Rho-kinase RB/PH(TT) enhanced HGF-induced MDCK cell spreading and dissociation. Moreover, MDCK cells pretreated for 1.5 h with HA1077 (20 µM) showed a similar phenotype to cells expressing RB/PH(TT) in response to HGF for 4 h and were equally or more spread than DMSO-treated control cells (our unpublished result).
Both Rho-kinase and PAK have been implicated in focal complex and focal
adhesion dynamics (Leung et al., 1996; Amano et
al., 1997; Ishizaki et al., 1997; Manser et
al., 1997). To establish if the alterations observed in cell
morphology and the actin cytoskeleton after expression of RB/PH(TT) or
PAKR correlated with alterations in focal complexes/focal adhesions,
injected cells were subjected to indirect immunofluorescence with the
use of vinculin antibodies (Figure 8).
Unstimulated MDCK cells contain predominantly small vinculin-containing
focal complexes throughout the cells and at cell-cell contacts,
whereas larger focal complexes are concentrated at the periphery of the
cell colony (Figure 8a). After HGF stimulation for 3-4 h, there is a
decrease in the density of small focal complexes, concomitant with the
appearance of larger focal complexes throughout the cells (Figure 8, b
and c, noninjected cells). The HGF-dependent formation of the large
focal complexes was blocked in MDCK cells expressing RB/PH(TT) (Figure
8b, arrows), consistent with the observed decrease in actin stress
fibers in these cells (Figure 6). However, few of the smaller
vinculin-containing complexes localized at sites of cell-cell
junctions and at the cell periphery were still observed in cells
expressing RB/PH(TT), indicating that RB/PH(TT) expression at that time
did not lead to a complete loss of focal adhesive contacts (Figure 8b).
In contrast, MDCK cells expressing PAKR showed an increase in the
number of, and larger, vinculin-containing focal complexes after HGF
stimulation for 3 h compared with uninjected cells (Figure 8c).
These results suggest a role for PAK in the turnover or breakdown of
focal complexes critical for cell spreading in response to HGF. In
contrast, Rho-kinase is required for the maintenance and generation of
new focal complexes associated with HGF-induced MDCK cell spreading,
but their presence or formation is not essential for spreading.
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Epithelial-mesenchymal transition, which leads to the dissociation and dispersal of epithelial cells, is a critical event during development, tumor invasion, and metastasis. HGF, the ligand for the Met receptor tyrosine kinase, is a potent inducer of epithelial-mesenchymal transition. Although several signaling pathways have been shown to play a role in epithelial cell dispersal regulated by HGF, little is known about the proximal signals regulating these later events. In this study, we show for the first time that HGF stimulation of epithelial MDCK cells leads within minutes to transient activation of the Rho GTPases, Cdc42 and Rac, which correlates with the induction of filopodia and lamellipodia by HGF. Rac translocates to membrane ruffles, and this is accompanied by activation and translocation of downstream effectors of Rho GTPases, PAK and Rho-kinase. Our results provide evidence that the activation and targeting of Rho GTPases, as well as their effectors PAK and Rho-kinase, are critical for the HGF-induced remodeling of the actin cytoskeleton, cell spreading, and dissociation.
Although Cdc42 has been implicated in cell spreading of fibroblasts and
macrophages (Clark et al., 1998; Price et al.,
1998), its activation downstream from receptor tyrosine kinases has not been demonstrated. Notably, microinjection of dominant negative N17Cdc42 expression constructs inhibits the formation of HGF-dependent lamellipodia (Figure 4). Moreover, as was shown for Rac (Ridley et al., 1995), N17Cdc42 also inhibits the spreading and
dissociation of MDCK cells in response to HGF (Figure 4). These data
place Cdc42 as an important modulator of the HGF-dependent biological responses that lead to epithelial-mesenchymal transition. The observation that N17Rac expression enhances the formation of filopodia in response to HGF (Figure 4), which is indicative of sustained Cdc42
activity, suggests that the HGF-dependent activation of Cdc42 is
independent of Rac and that Rac activity is essential for lamellipodia
formation even in the presence of activated Cdc42. Consistent with
this, the PI3K inhibitor LY294002 does not inhibit HGF-dependent
activation of Cdc42 or the formation of filopodia downstream of HGF
(Figure 2 and our unpublished result), whereas HGF-dependent activation
of Rac and lamellipodia formation is blocked in the presence of
LY294002 (Figure 2 and our unpublished result). This is in agreement
with our previous data that PI3K is required for spreading of MDCK
cells in response to HGF (Royal and Park, 1995). Interestingly,
LY294002 does not inhibit the formation of lamellipodia downstream from
activated L61Rac in MDCK cells (I. Royal and M. Park, unpublished
observation), suggesting that PI3K activity is required upstream of
HGF-dependent Rac activation, possibly as a consequence of the PI3K
product, phosphatidylinositol 3,4,5-trisphosphate, recruiting
and activating exchange factors for Rac in MDCK cells (Cerione and
Zheng, 1996; Han et al., 1998; Sander et al.,
1998) .
MDCK cells expressing N17Cdc42 show a decreased ability to form
lamellipodia in response to HGF, suggesting a requirement for Cdc42
activity in the formation of HGF-dependent lamellipodia (Table 1). This
may suggest that, in a similar manner to Swiss 3T3 cells (reviewed by
Hall, 1998), activation of Cdc42 contributes to activation of Rac.
However, the kinetics of activation of Cdc42 and Rac in response to HGF
are distinct. HGF-dependent activation of Rac is transient (15-30
min), whereas that of Cdc42 is prolonged (>60 min; Figure 2). This
supports the interpretation that Cdc42 and Rac may be activated by HGF
independently of one another, although it does not exclude the
possibility that Cdc42 activates Rac. Hence, from these studies we show
for the first time that activation of Cdc42 is critical for both the
formation of HGF-dependent lamellipodia and the spreading and
dissociation of colonies of MDCK cells.
In MDCK epithelial cells, activated Rac and Cdc42 were shown previously
to promote enhanced E-cadherin-mediated cell-cell adhesion and not
spreading (Hordijk et al., 1997; Kuroda et al., 1997; Takaishi et al., 1997; Jou and Nelson, 1998). However,
in low-density MDCK cells, macrophages, T lymphocytes, and HeLa cells, activated Rac can promote cell spreading and in some instances enhance
cell migration (Allen et al., 1997; Manser et
al., 1997; D'Souza-Schorey et al., 1998; Jou and
Nelson, 1998; Sander et al., 1998). Thus, at high cell
density when cell-cell junctions are favored, other HGF-induced
signals are required to break down cell-cell junctions and promote
cell spreading. For example, HGF-induced cell dispersal is inhibited in
cells expressing dominant negative Ras proteins or after the inhibition
of MEK1, an activator of ERK kinases, implicating the Ras pathway
(Hartmann et al., 1994; Ridley et al., 1995;
Khwaja et al., 1998; Potempa and Ridley, 1998). Moreover, in
the context of HGF-stimulated MDCK cells, both the subcellular
localization and the cycling of Rho GTPases between active and inactive
states may promote a biological response that will be distinct from
that induced by the expression of their constitutively activated forms.
Consistent with activation of Cdc42 and Rac and the translocation of
Rac to membrane ruffles in HGF-stimulated MDCK cells, we have observed
that the PAK1 serine/threonine kinase, an effector protein activated by
Cdc42 and Rac, is activated and translocates to membrane ruffles at the
edge of lamellipodia by 15 min of HGF stimulation (Figures 3 and 5).
PAK1 is involved in actin reorganization (Manser et al.,
1997; Sells et al., 1997; Frost et al., 1998) and
localizes to PDGF- or Rac-induced membrane ruffles (Dharmawardhane et al., 1997) and focal complexes (Manser et al.,
1997). Pak1 activation is sustained for >60 min after HGF stimulation
(Figure 3), which correlates with the prolonged activation of Cdc42 and not the transient activation of Rac, suggesting that PAK activation in
response to HGF may be mediated by Cdc42.
A role for Pak in HGF-dependent remodeling of the actin cytoskeleton is
supported by the finding that a dominant negative PAK mutant (PAKR)
inhibits HGF-dependent lamellipodia formation (Figure 6A) and spreading
(Figure 6B) of MDCK cells. In response to HGF, cells expressing PAKR
showed an increase in poorly organized F-actin and both an increased
number of and larger focal complexes (Figure 8). Similarly, expression
of the PAK autoinhibitory domain in single HeLa cells, which leads to
the inhibition of endogenous PAK kinase activity, increased the size of
focal complexes formed downstream of V12Rac or V12Cdc42 (Zhao et
al., 1998). Our results show that the increase in focal adhesions
in the presence of the PAKR dominant negative mutant cannot be rescued
by the activation of Met-dependent signals, indicating that PAKR
inhibits HGF-dependent turnover of focal adhesions required for MDCK
cell spreading. Conversely, as observed in MDCK cells (Figure 7),
activated PAK kinase was shown to inhibit the formation of stress
fibers and focal adhesions, to induce cell retraction of adhering
cells, and to inhibit cell spreading after plating (Manser et
al., 1997; Frost et al., 1998; Zhao et al.,
1998; Sanders et al., 1999). Together, these results are
consistent with the recent demonstration that PAK activity, through
phosphorylation and inhibition of myosin light chain kinase, promotes a
decrease in actin-myosin filament assembly (Sanders et al.,
1999). Thus, the targeting of an activated PAK kinase to membrane
ruffles would be predicted to inhibit actin-myosin assembly and stress
fiber formation, thus allowing remodeling of the actin cytoskeleton to
form a lamellipodium and allow cell spreading.
PAKR, which encodes the Cdc42/Rac-binding site in addition to the
autoinhibitory domain and proline-rich sequences, may compete with
other Cdc42/Rac effectors involved in lamellipodia formation. However,
as observed in HeLa cells, in which the PAK autoinhibitory domain had
no effect on V12Rac-induced lamellipodia (Zhao et al., 1998), PAKR expression failed to inhibit L61Rac-induced lamellipodia in
MDCK cells (I. Royal and M. Park, unpublished observation), demonstrating that PAKR does not block or soak up Rac-dependent signaling per se but instead inhibits HGF-dependent signaling pathways
acting upstream of and leading to lamellipodia formation. A possible
role for PAK upstream of Rac in lamellipodia formation has been
suggested through the interaction of the PAK proline-rich N terminus
with the Rac exchange factor PIX, a complex that has been proposed to
be involved in Cdc42-to-Rac signaling (Manser et al., 1998;
Obermeier et al., 1998). Thus, PAKR may both inhibit endogenous PAK kinase activity, via the autoinhibitory domain, and
block remodeling of peripheral actin through the ability of the
N-terminal proline-rich domain to inhibit Pak localization or
interactions with proteins such as PIX.
In addition to Rac and Pak, Rho-kinase, an effector of Rho, is rapidly
translocated to membrane ruffles after stimulation of MDCK cells with
HGF (Figure 5). Rho-kinase translocation in response to activation of
receptor tyrosine kinases has not been documented, but this is similar
to the recruitment of Rho-kinase to cell membranes downstream from
activated Rho (Leung et al., 1995; Matsui et al.,
1996). Rho-kinase isoforms are implicated as regulators of actin
organization and focal adhesion dynamics downstream from activated Rho
(Leung et al., 1996; Amano et al., 1997; Ishizaki
et al., 1997), possibly through the ability of Rho-kinase to
increase myosin light chain phosphorylation and activation, promoting
bundling of actin stress fibers into filaments (Amano et
al., 1996; Kimura et al., 1996). Hence Rho-kinase would act to antagonize the activity of PAK (Burridge, 1999). Consistent with
this notion, the expression of a constitutively activated Rho-kinase
(CAT) promoted stress fiber bundling (Figure 7), whereas the expression
of the dominant negative Rho-kinase mutant RB/PH(TT) in MDCK cells
induced the loss of stress fibers and peripheral actin (Figure 6 and
our unpublished results). Importantly, in cells expressing RB/PH(TT) or
treated with HA1077, an inhibitor of Rho-kinase as well as other
kinases (Uehata et al., 1997), HGF was unable to stimulate
de novo stress fiber formation, indicating an essential role for
Rho-kinase in HGF-dependent actin bundling. Moreover, these cells were
unable to form typical lamellipodia containing an obvious actin network
emanating from peripheral actin bundles, as was observed in control
cells (Figure 6 and our unpublished result). These data are in
agreement with the recent observation that Rho-kinase is required for
tetradecanoylphorbol-13-acetate (TPA)-induced membrane ruffling in MDCK
cells, possibly through its ability to phosphorylate adducin, a
membrane protein that promotes the formation of a spectrin-actin
meshwork beneath plasma membranes (Fukata et al., 1999). The
targeting of Rho-kinase to membrane ruffles after HGF stimulation
supports a role for Rho-kinase in the rapid reorganization of the actin
cytoskeleton required for lamellipodium formation in MDCK cells,
possibly to antagonize the activity of PAK1 and promote actin bundling
and stabilization of newly formed lamellipodia.
HGF-dependent cell spreading, dissociation, and acquisition of a
spindle cell shape were enhanced after prolonged expression of
RB/PH(TT) (Figure 6B) or of a kinase-dead Rho-kinase mutant (our
unpublished result), and cell spreading could be observed in the
absence of HGF stimulation (our unpublished result). The enhanced cell
spreading and dissociation observed in HGF-stimulated RB/PH(TT)-expressing cells were accompanied by the loss of focal complexes present throughout the ventral surface of the cell, whereas
some focal complexes around the cell perimeter and at areas of
cell-cell contact were retained (Figure 8). Because both Rac and Cdc42
stimulate the assembly of peripheral focal complexes in Swiss 3T3 cells
(Nobes and Hall, 1995), the remaining or de novo HGF-induced focal
complex formation in spread MDCK cells expressing RB/PH(TT) is likely
to be dependent on Cdc42 and possibly Rac (Figure 8). These data are in
agreement with a recent report (Nobes and Hall, 1999) showing that
inhibition of Rho-kinase enhanced the speed of wound closure by a
fibroblast monolayer containing few actin stress fibers, although other
authors have reported that Rho-kinase was required for wound-induced
migration of NRK49F fibroblasts and transcellular migration of mm1
hepatoma cells (Fukata et al., 1999; Itoh et al.,
1999). These opposing observations might be attributed to cell type
differences or to different mechanisms involved in the migration of
single cells versus cell sheets or colonies. Whether Rho-kinase is
required for the migration of single MDCK cells remains to be determined.
In the present study, we show that HGF is a potent activator of Cdc42, Rac, and Pak1 and promotes translocation of these proteins to membrane ruffles. We provide new insight regarding a critical role of Cdc42 in the formation of lamellipodia and in the dispersal of sheets of epithelial cells and show opposing actions of PAK1 and Rho-kinase in HGF-induced cell dispersal. We conclude that the regulation of activation and subcellular localization of different Rho family GTPases and their effectors by HGF is a critical event in the epithelial-mesenchymal transition, a process required for tumor cell dispersal.
Note Added in Proof. In agreement with our
data, Kiosses et al. (1999) demonstrated that the
amino-terminal proline-rich domain of Pak, and not the Rac/Cdc42
interaction domain, was required for the inhibition of cell migration
by a dominant negative Pak protein.
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ACKNOWLEDGMENTS |
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We thank members of the Park laboratory for critical reading of the manuscript and Dr. Svetlana Sadekova for helping with confocal microscopy. We also thank those who generously gave us reagents used in this study: Dr. Alan Hall for Rho family constructs, Dr. Arie Abo for the PAKR construct, Dr. John Chant for the PAKWT and PAKL107F constructs, Dr. James Woodgett for the GST-c-Jun construct, Dr. John Collard for the GST-PAK (aa 56-272) construct, Dr. George Vande Woude for HGF, and Asahi Chemical Industry (Shizuoka, Japan) for the HA1077 inhibitor. This research was supported by operating grants to M.P. from the National Cancer Institute of Canada. I.R. was the recipient of fellowships from the Fonds de la Recherche en Santé du Québec and the Medical Research Council of Canada. N.L.-V. is a junior scholar of the Fonds de la Recherche en Santé du Québec. L.L. is the recipient of a Natural Sciences and Engineering Research Council studentship. M.P. is a Scientist of the Medical Research Council of Canada.
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FOOTNOTES |
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** Corresponding author. E-mail address: morag{at}lan1.molonc.mcgill.ca.
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ABBREVIATIONS |
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Abbreviations used: aa, amino acids; CAT, Rho-kinase catalytic domain; HGF, hepatocyte growth factor; JNK, c-Jun N-terminal kinase; MBP, myelin basic protein; MDCK, Madin-Darby canine kidney; PAK, p21-activated kinase; PH, pleckstrin homology; PI3K, phosphatidylinositol 3-kinase; RB, Rho-binding domain.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Proc. Natl. Acad. Sci. USA
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Mol. Cell. Biol.
17, 1129-1143[Abstract].PAK: inhibition of PAK kinases reveals their morphological roles downstream of Cdc42 and Rac1.
Mol. Cell. Biol.
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H. Zhou and R. H. Kramer Integrin Engagement Differentially Modulates Epithelial Cell Motility by RhoA/ROCK and PAK1 J. Biol. Chem., March 18, 2005; 280(11): 10624 - 10635. [Abstract] [Full Text] [PDF]
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 H. Nakata and T. Kozasa Functional Characterization of G{alpha}o Signaling through G Protein-Regulated Inducer of Neurite Outgrowth 1 Mol. Pharmacol., March 1, 2005; 67(3): 695 - 702. [Abstract] [Full Text] [PDF]
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H. Khoury, M. A. Naujokas, D. Zuo, V. Sangwan, M. M. Frigault, S. Petkiewicz, D. L. Dankort, W. J. Muller, and M. Park HGF Converts ErbB2/Neu Epithelial Morphogenesis to Cell Invasion Mol. Biol. Cell, February 1, 2005; 16(2): 550 - 561. [Abstract] [Full Text] [PDF]
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K. Kawamura, K. Takano, S. Suetsugu, S. Kurisu, D. Yamazaki, H. Miki, T. Takenawa, and T. Endo N-WASP and WAVE2 Acting Downstream of Phosphatidylinositol 3-Kinase Are Required for Myogenic Cell Migration Induced by Hepatocyte Growth Factor J. Biol. Chem., December 24, 2004; 279(52): 54862 - 54871. [Abstract] [Full Text] [PDF]
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K. Mori, M. Shibanuma, and K. Nose Invasive Potential Induced under Long-Term Oxidative Stress in Mammary Epithelial Cells Cancer Res., October 15, 2004; 64(20): 7464 - 7472. [Abstract] [Full Text] [PDF]
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 A. Astrinidis and E. Petri Henske Aberrant Cellular Differentiation and Migration in Renal and Pulmonary Tuberous Sclerosis Complex J Child Neurol, September 1, 2004; 19(9): 710 - 715. [Abstract] [PDF]
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 G. Prindull and D. Zipori Environmental guidance of normal and tumor cell plasticity: epithelial mesenchymal transitions as a paradigm Blood, April 15, 2004; 103(8): 2892 - 2899. [Abstract] [Full Text] [PDF]
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E.-Y. Shin, K.-N. Woo, C.-S. Lee, S.-H. Koo, Y. G. Kim, W.-J. Kim, C.-D. Bae, S.-I. Chang, and E.-G. Kim Basic Fibroblast Growth Factor Stimulates Activation of Rac1 through a p85 {beta}PIX Phosphorylation-dependent Pathway J. Biol. Chem., January 16, 2004; 279(3): 1994 - 2004. [Abstract] [Full Text] [PDF]
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M. C. Wilkes, S. J. Murphy, N. Garamszegi, and E. B. Leof Cell-Type-Specific Activation of PAK2 by Transforming Growth Factor {beta} Independent of Smad2 and Smad3 Mol. Cell. Biol., December 1, 2003; 23(23): 8878 - 8889. [Abstract] [Full Text] [PDF]
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R. Athman, D. Louvard, and S. Robine Villin Enhances Hepatocyte Growth Factor-induced Actin Cytoskeleton Remodeling in Epithelial Cells Mol. Biol. Cell, November 1, 2003; 14(11): 4641 - 4653. [Abstract] [Full Text] [PDF]
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B. Fournes, J. Farrah, M. Olson, N. Lamarche-Vane, and N. Beauchemin Distinct Rho GTPase Activities Regulate Epithelial Cell Localization of the Adhesion Molecule CEACAM1: Involvement of the CEACAM1 Transmembrane Domain Mol. Cell. Biol., October 15, 2003; 23(20): 7291 - 7304. [Abstract] [Full Text] [PDF]
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P. B. van Hennik, J. P. t. Klooster, J. R. Halstead, C. Voermans, E. C. Anthony, N. Divecha, and P. L. Hordijk The C-terminal Domain of Rac1 Contains Two Motifs That Control Targeting and Signaling Specificity J. Biol. Chem., October 3, 2003; 278(40): 39166 - 39175. [Abstract] [Full Text] [PDF]
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C. Zhao, H. Ma, E. Bossy-Wetzel, S. A. Lipton, Z. Zhang, and G.-S. Feng GC-GAP, a Rho Family GTPase-activating Protein That Interacts with Signaling Adapters Gab1 and Gab2 J. Biol. Chem., September 5, 2003; 278(36): 34641 - 34653. [Abstract] [Full Text] [PDF]
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D. GRATZINGER, S. CANOSA, B. ENGELHARDT, and J. A. MADRI Platelet endothelial cell adhesion molecule-1 modulates endothelial cell motility through the small G-protein Rho FASEB J, August 1, 2003; 17(11): 1458 - 1469. [Abstract] [Full Text] [PDF]
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L. Lamorte, S. Rodrigues, V. Sangwan, C. E. Turner, and M. Park Crk Associates with a Multimolecular Paxillin/GIT2/{beta}-PIX Complex and Promotes Rac-dependent Relocalization of Paxillin to Focal Contacts Mol. Biol. Cell, July 1, 2003; 14(7): 2818 - 2831. [Abstract] [Full Text] [PDF]
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F. Palacios and C. D'Souza-Schorey Modulation of Rac1 and ARF6 Activation during Epithelial Cell Scattering J. Biol. Chem., May 2, 2003; 278(19): 17395 - 17400. [Abstract] [Full Text] [PDF]
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M. Cozzolino, V. Stagni, L. Spinardi, N. Campioni, C. Fiorentini, E. Salvati, S. Alema, and A. M. Salvatore p120 Catenin Is Required for Growth Factor-dependent Cell Motility and Scattering in Epithelial Cells Mol. Biol. Cell, May 1, 2003; 14(5): 1964 - 1977. [Abstract] [Full Text] [PDF]
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C. R. Maroun, M. A. Naujokas, and M. Park Membrane Targeting of Grb2-associated Binder-1 (Gab1) Scaffolding Protein through Src Myristoylation Sequence Substitutes for Gab1 Pleckstrin Homology Domain and Switches an Epidermal Growth Factor Response to an Invasive Morphogenic Program Mol. Biol. Cell, April 1, 2003; 14(4): 1691 - 1708. [Abstract] [Full Text] [PDF]
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S. Pelletier, F. Duhamel, P. Coulombe, M. R. Popoff, and S. Meloche Rho Family GTPases Are Required for Activation of Jak/STAT Signaling by G Protein-Coupled Receptors Mol. Cell. Biol., February 15, 2003; 23(4): 1316 - 1333. [Abstract] [Full Text] [PDF]
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 P. J. M. Noble, G. Wilde, M. R. H. White, S. R. Pennington, G. J. Dockray, and A. Varro Stimulation of gastrin-CCKB receptor promotes migration of gastric AGS cells via multiple paracrine pathways Am J Physiol Gastrointest Liver Physiol, January 1, 2003; 284(1): G75 - G84. [Abstract] [Full Text] [PDF]
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C. M. Wells, A. Abo, and A. J. Ridley PAK4 is activated via PI3K in HGF-stimulated epithelial cells J. Cell Sci., October 15, 2002; 115(20): 3947 - 3956. [Abstract] [Full Text] [PDF]
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F. Berditchevski, E. Odintsova, S. Sawada, and E. Gilbert Expression of the Palmitoylation-deficient CD151 Weakens the Association of alpha 3beta 1 Integrin with the Tetraspanin-enriched Microdomains and Affects Integrin-dependent Signaling J. Biol. Chem., September 27, 2002; 277(40): 36991 - 37000. [Abstract] [Full Text] [PDF]
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L. Lamorte, S. Rodrigues, M. Naujokas, and M. Park Crk Synergizes with Epidermal Growth Factor for Epithelial Invasion and Morphogenesis and Is Required for the Met Morphogenic Program J. Biol. Chem., September 27, 2002; 277(40): 37904 - 37911. [Abstract] [Full Text] [PDF]
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A. Pagliocca, L. E. Wroblewski, F. J. Ashcroft, P. J. Noble, G. J. Dockray, and A. Varro Stimulation of the gastrin-cholecystokininB receptor promotes branching morphogenesis in gastric AGS cells Am J Physiol Gastrointest Liver Physiol, August 1, 2002; 283(2): G292 - G299. [Abstract] [Full Text] [PDF]
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S. Tanimura, K. Nomura, K.-i. Ozaki, M. Tsujimoto, T. Kondo, and M. Kohno Prolonged Nuclear Retention of Activated Extracellular Signal-regulated Kinase 1/2 Is Required for Hepatocyte Growth Factor-induced Cell Motility J. Biol. Chem., July 26, 2002; 277(31): 28256 - 28264. [Abstract] [Full Text] [PDF]
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F. LIU, K. L. SCHAPHORST, A. D. VERIN, K. JACOBS, A. BIRUKOVA, R. M. DAY, N. BOGATCHEVA, D. P. BOTTARO, and J. G. N. GARCIA Hepatocyte growth factor enhances endothelial cell barrier function and cortical cytoskeletal rearrangement: potential role of glycogen synthase kinase-3{beta} FASEB J, July 1, 2002; 16(9): 950 - 962. [Abstract] [Full Text] [PDF]
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H. Yamaguchi, H. Miki, and T. Takenawa Neural Wiskott-Aldrich Syndrome Protein Is Involved in Hepatocyte Growth Factor-induced Migration, Invasion, and Tubulogenesis of Epithelial Cells Cancer Res., May 1, 2002; 62(9): 2503 - 2509. [Abstract] [Full Text] [PDF]
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 L. Van Aelst and M. Symons Role of Rho family GTPases in epithelial morphogenesis Genes & Dev., May 1, 2002; 16(9): 1032 - 1054. [Full Text] [PDF]
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L. Lamorte, I. Royal, M. Naujokas, and M. Park Crk Adapter Proteins Promote an Epithelial-Mesenchymal-like Transition and Are Required for HGF-mediated Cell Spreading and Breakdown of Epithelial Adherens Junctions Mol. Biol. Cell, May 1, 2002; 13(5): 1449 - 1461. [Abstract] [Full Text] [PDF]
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X. Li, E. Saint-Cyr-Proulx, K. Aktories, and N. Lamarche-Vane Rac1 and Cdc42 but Not RhoA or Rho Kinase Activities Are Required for Neurite Outgrowth Induced by the Netrin-1 Receptor DCC (Deleted in Colorectal Cancer) in N1E-115 Neuroblastoma Cells J. Biol. Chem., April 19, 2002; 277(17): 15207 - 15214. [Abstract] [Full Text] [PDF]
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H. Bierne and P. Cossart InlB, a surface protein of Listeria monocytogenes that behaves as an invasin and a growth factor J. Cell Sci., January 9, 2002; 115(17): 3357 - 3367. [Abstract] [Full Text] [PDF]
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A. V. Bakin, C. Rinehart, A. K. Tomlinson, and C. L. Arteaga p38 mitogen-activated protein kinase is required for TGF{beta}-mediated fibroblastic transdifferentiation and cell migration J. Cell Sci., January 8, 2002; 115(15): 3193 - 3206. [Abstract] [Full Text] [PDF]
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C. Shelly and R. Herrera Activation of SGK1 by HGF, Rac1 and integrin-mediated cell adhesion in MDCK cells: PI-3K-dependent and -independent pathways J. Cell Sci., January 5, 2002; 115(9): 1985 - 1993. [Abstract] [Full Text] [PDF]
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O'N. Wiggan, M. P. Fadel, and P. A. Hamel Pax3 induces cell aggregation and regulates phenotypic mesenchymal-epithelial interconversion J. Cell Sci., January 2, 2002; 115(3): 517 - 529. [Abstract] [Full Text] [PDF]
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 J. YU, A. ASTRINIDIS, and E. P. HENSKE Chromosome 16 Loss of Heterozygosity in Tuberous Sclerosis and Sporadic Lymphangiomyomatosis Am. J. Respir. Crit. Care Med., October 15, 2001; 164(8): 1537 - 1540. [Abstract] [Full Text] [PDF]
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S. Fan, Y. X. Ma, M. Gao, R.-Q. Yuan, Q. Meng, I. D. Goldberg, and E. M. Rosen The Multisubstrate Adapter Gab1 Regulates Hepatocyte Growth Factor (Scatter Factor)-c-Met Signaling for Cell Survival and DNA Repair Mol. Cell. Biol., August 1, 2001; 21(15): 4968 - 4984. [Abstract] [Full Text] [PDF]
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A. J. Ridley Rho GTPases and cell migration J. Cell Sci., January 8, 2001; 114(15): 2713 - 2722. [Abstract] [Full Text] [PDF]
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T. M. Fournier, L. Lamorte, C. R. Maroun, M. Lupher, H. Band, W. Langdon, and M. Park Cbl-transforming Variants Trigger a Cascade of Molecular Alterations That Lead to Epithelial Mesenchymal Conversion Mol. Biol. Cell, October 1, 2000; 11(10): 3397 - 3410. [Abstract] [Full Text]
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R. J. Solaro Myosin Light Chain Phosphatase : A Cinderella of Cellular Signaling Circ. Res., August 4, 2000; 87(3): 173 - 175. [Full Text] [PDF]
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T. Umata, M. Hirata, T. Takahashi, F. Ryu, S. Shida, Y. Takahashi, M. Tsuneoka, Y. Miura, M. Masuda, Y. Horiguchi, et al. A Dual Signaling Cascade That Regulates the Ectodomain Shedding of Heparin-binding Epidermal Growth Factor-like Growth Factor J. Biol. Chem., August 3, 2001; 276(32): 30475 - 30482. [Abstract] [Full Text] [PDF]
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H. Bierne, E. Gouin, P. Roux, P. Caroni, H. L. Yin, and P. Cossart A role for cofilin and LIM kinase in Listeria-induced phagocytosis J. Cell Biol., October 1, 2001; 155(1): 101 - 112. [Abstract] [Full Text] [PDF]
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