(Received for publication, May 13, 1996, and in revised form, February 6, 1997)
From the Divisions of Experimental Medicine and Hematology/Oncology, Beth Israel Deaconess Medical Center (West Campus), Harvard Medical School, Boston, Massachusetts 02215
We have characterized signaling pathways
involving the related adhesion focal tyrosine kinase (RAFTK, also known
as PYK2 or CAK-) in CMK human megakaryocytic cells. Stem cell
factor, which potentiates the growth of megakaryocytes and their
progenitors, and phorbol myristate acetate, which causes
differentiation of megakaryocytic cell lines, induced the tyrosine
phosphorylation of RAFTK but not of focal adhesion kinase. Stimulation
of CMK cells with stem cell factor resulted in an increase in the
autophosphorylation and kinase activity of RAFTK. Phosphorylation of
RAFTK under these conditions was mediated by a protein kinase
C-dependent pathway. Cytochalasin D, which disrupts the
cytoskeleton, abolished the phosphorylation of RAFTK upon phorbol
myristate acetate and stem cell factor stimulation, indicating that
RAFTK association with the actin cytoskeleton appears to be critical
for its phosphorylation. In addition, we observed an association of
RAFTK with paxillin, a 68-kDa cytoskeleton protein. Using in
vitro binding assays, RAFTK and paxillin were shown to bind
directly through the C-terminal proline-rich domain. Transient
overexpression of a dominant-negative mutant of RAFTK inhibited
significantly the tyrosine phosphorylation of paxillin upon phorbol
myristate acetate stimulation. These observations indicate that RAFTK
might play an important role in the phosphorylation of signaling
pathways within the focal adhesions and that RAFTK participates in
signaling events that link signals from the cell surface to the
cytoskeleton. Furthermore, this study suggests that RAFTK might be
involved in megakaryocyte proliferation and differentiation.
Protein tyrosine kinases regulate various signal transduction pathways, including those controlling cell growth, differentiation, and activation (1-5). Integrins, cell surface receptors for proteins of the extracellular matrix, are also transducers of cytoplasmic signals (6-8), and activation of these pathways is linked to one or more protein tyrosine kinases (9, 10).
A cytoplasmic tyrosine kinase, focal adhesion kinase
(FAK)1 (11-13), has been identified as one
of the cellular proteins that becomes phosphorylated in response to
1 or
3 integrin-mediated cell adhesion
(8, 12-17). Supportive in vivo data from FAK-deficient mice
reveal reduced cell motility and enhanced focal adhesion contact
formation in FAK null cells (18).
Recently, we and others have isolated a cDNA encoding a novel human
cytoplasmic tyrosine kinase termed RAFTK (for a related adhesion focal
tyrosine kinase) (19), also known as PYK2 or CAK- (20, 21). The
RAFTK cDNA, encoding a polypeptide of 1009 amino acids, has the
closest homology (48% identity, 65% similarity) to FAK. Analysis of
their deduced amino acid sequences also indicates that RAFTK, like FAK,
lacks a transmembrane region, myristylation sites, and SH2 and SH3
domains. In addition, like FAK, the RAFTK C-terminal domain contains a
predicted proline-rich stretch of residues. RAFTK was reported to be
highly expressed in the central nervous system (19) and is involved in
Ca2+-induced regulation of ion channel and
mitogen-activated protein kinase functions in PC-12 cells (20).
Activation of PYK2 by the inflammatory cytokine tumor necrosis factor
and by stress signals such as UV light and osmotic shock was shown
to couple with the c-Jun N-terminal kinase signaling pathway (22).
Recently, a role for PYK2 and Src in linking G-protein-coupled
receptors with mitogen-activated protein kinase activation was reported (23).
RAFTK expression is abundant in primary bone marrow megakaryocytes and their progeny, blood platelets (19). To address the role of RAFTK in signal transduction pathways in megakaryocytes, experiments were performed using the model CMK megakaryocytic cell line (24). The c-KIT receptor and its cognate ligand stem cell factor (SCF) were investigated since they play a critical role in the adhesion, migration, motility, proliferation, and maturation of a number of hematopoietic cells, including megakaryocytes and platelets (25-29). Since SCF effects appear to be modulated by protein kinase C (PKC) (30), we focused on determining whether PKC might mediate the effects of SCF and Ca2+ on RAFTK phosphorylation. In this study, we report that SCF and phorbol myristate acetate (PMA) induced the tyrosine phosphorylation of RAFTK in a PKC-dependent pathway. The integrity of the actin cytoskeleton appears to be essential for RAFTK phosphorylation. Association of RAFTK with the cytoskeletal protein paxillin was observed through its proline rich-domain, and a dominant-negative mutant of RAFTK interfered with the PMA-induced phosphorylation of paxillin.
Recombinant SCF/KIT ligand and polyclonal
anti-c-KIT antibodies were generously provided by Keith E. Langley and
L. Bennett (Amgen Inc., Thousand Oaks, CA). Monoclonal
anti-phosphotyrosine antibody (PY-20) and monoclonal anti-paxillin were
obtained from ICN (Costa Mesa, CA); monoclonal antibodies anti-p85,
anti-Shc, anti-Grb2, anti-FAK, anti-PKC-, anti-PKC-
, and
anti-PKC-
were obtained from Transduction Laboratories (Lexington,
KY). Calphostin C, staurosporine, BAPTA-AM, calcium ionophore A23187,
EGTA, and phorbol 12-myristate 13-acetate were obtained from
Calbiochem. Electrophoresis reagents were obtained from Bio-Rad. All
other reagents were purchased from Sigma.
The CMK cell line, provided by T. Sato (Chiba
University, Japan), was maintained in RPMI 1640 medium with 10% fetal
calf serum as described previously (31). The CMK cell line has
properties of cells of the megakaryocytic lineage because it can
proliferate in response to cytokines and differentiate upon induction
with PMA (24, 32). PMA was dissolved in dimethyl sulfoxide and stored
at 20 °C until use, when it was diluted in RPMI 1640 medium.
Anti-RAFTK antiserum was obtained from New Zealand White rabbits immunized with a bacterially expressed fusion protein consisting of glutathione S-transferase (GST) and the C terminus (amino acids 681-1009) of human RAFTK cDNA subcloned into the pGEX-2T expression vector as described (19). The serum (R-4250) exhibiting high titer (1:256,000) was used in subsequent experiments. Preimmune normal rabbit serum was used as a control antibody. No signal was observed when normal rabbit serum was used to immunoprecipitate lysates from unstimulated or SCF- or PMA-stimulated CMK cells (data not shown), indicating that the R-4250 antibody reacted specifically with RAFTK.
Cell Stimulation, Immunoprecipitation, and ImmunoblottingThe CMK cells were starved overnight in RPMI 1640 medium with 0.5% fetal calf serum. Cells (106/ml) were stimulated for 0 to 30 min at room temperature with either SCF (100-500 ng/ml) or PMA (10-100 nM). For BAPTA treatment, CMK cells were pretreated for 30 min at room temperature with BAPTA-AM (20 µM) before stimulation with other reagents. The stimulation was terminated by adding ice-cold RPMI 1640 medium containing sodium vanadate followed by centrifugation. The cells were lysed in modified RIPA buffer (50 mM Tris-HCl, pH 7.4, 1% Nonidet P-40, 0.25% sodium deoxycholate, 150 mM NaCl, 1 mM phenylmethylsulfonyl fluoride, 2 µg/ml aprotinin, leupeptin, and pepstatin, and 1 mM Na3VO4). Total cell lysates were clarified by centrifugation at 10,000 × g for 10 min. Protein concentrations were determined using a protein assay (Bio-Rad). Identical amounts of protein from each sample were precleared by incubation with protein G-Sepharose CL-4B (Sigma) for 1 h at 4 °C. After the removal of protein G-Sepharose by brief centrifugation, the solution was incubated with different primary antibodies as described below for each experiment for 4 h or overnight at 4 °C. Immunoprecipitation of the antigen-antibody complex was accomplished by incubation for 1 h at 4 °C with 40 µl of protein G-Sepharose. Bound proteins were solubilized in 20 µl of 2 × Laemmli buffer. Samples were separated and analyzed by 7.5 or 10% SDS-PAGE and then transferred to nitrocellulose membranes. The membranes were blocked with 5% bovine serum albumin (Boehringer Mannheim) and probed with primary antibody for 1 h at room temperature. Immunoreactive bands were visualized using horseradish peroxidase-conjugated secondary antibody and the ECL reagents (Amersham Corp.).
GST Fusion Protein Production and Binding StudiesThe RAFTK C-terminal proline-rich domain (amino acids 681-1009), the RAFTK N-terminal domain (amino acids 26-286), and the shorter RAFTK C-terminal proline-rich region (amino acids 700-972) GST fusion proteins were amplified by the polymerase chain reaction technique and cloned into the pGEX-2T expression vector (Pharmacia Biotech Inc.) and produced as described previously (19, 33). The GST fusion proteins were purified on a glutathione-Sepharose column by affinity chromatography according to the manufacturer's recommendations (Pharmacia). For the binding experiments, 1 mg of cell lysate was mixed with 15 µg of GST fusion protein and incubated for 1 h at 4 °C on a rotatory shaker. Fifty µl of glutathione-Sepharose 4B beads (Pharmacia) were added to preabsorb the complex. Following incubation for 3 h at 4 °C on a rotatory shaker, the beads were centrifuged and washed three times with modified RIPA buffer. The bound proteins were eluted by boiling in Laemmli sample buffer and subjected to 7.5% SDS-PAGE and Western blot analysis.
Western Blot Binding Assay (Far-Western)Immunoprecipitations were performed using anti-paxillin mouse monoclonal antibody and separated on 7.5% SDS-PAGE gels. The gels were then transferred, and the blots were incubated at 4 °C overnight in 5% dry milk and phosphate-buffered saline plus 0.1% Tween 20. The blots were incubated in GST fusion proteins for 2 h and then washed. Anti-GST mouse monoclonal antibody was added (Santa Cruz Biotechnology, Santa Cruz, CA) for 1 h. After washing, anti-mouse Ig and horseradish peroxidase (Amersham Corp.) were added for 1 h. The membranes were processed using the ECL technique.
In Vitro Kinase and Autophosphorylation AssaysThe immunoprecipitated complexes obtained by immunoprecipitating cell lysates with RAFTK antiserum were washed twice with RIPA buffer and once in kinase buffer. The immune complex was then incubated in kinase buffer containing 25 µg of poly(Glu:Tyr) (4:1, 20-50 kDa, Sigma) and 5 µCi of [32P]ATP at room temperature for 30 min as described (33). For the autophosphorylation assay, the immune complexes were incubated in a kinase buffer containing 5 µCi of [32P]ATP at room temperature for 30 min as described (33). The reaction was stopped by adding 4 × SDS sample buffer and boiling the sample for 5 min. Proteins were then separated on SDS-PAGE and detected by autoradiography.
Transient Transfection of Cos Cells with a Dominant-negative Mutant of RAFTKA kinase-negative mutant of RAFTK (KM) was constructed by replacing Lys-475 with an Ala residue using a site-directed mutagenesis kit (Clontech, Palo Alto, CA) as described (20). The RAFTK cDNA in the pCDNA3-neo vector was constructed as described in our previous studies (19, 33), and the paxillin cDNA in the pRcCMV vector was kindly provided by R. Salgia and J. D. Griffin (Dana Farber Cancer Institute, Harvard Medical School, Boston, MA). Cos cells were transiently transfected with either the wild-type RAFTK construct, RAFTK-KM construct, or paxillin construct or were co-transfected with RAFTK and paxillin constructs or RAFTK-KM and paxillin constructs as described (33). After 72 h of transfection, the cells were starved for 4 h in serum-free medium and then either stimulated with PMA (50 nM, 5 min at 37 °C) or left unstimulated. Cell lysates were prepared and immunoprecipitated with anti-RAFTK antibodies, anti-paxillin antibodies, or preimmune antibodies. The immune precipitates were washed and analyzed for tyrosine phosphorylation as described above.
To investigate whether RAFTK participated in
growth-related signal transduction pathways in megakaryocytes, we
studied model CMK megakaryocytic cells and focused on the c-KIT/SCF
pathway, which is known to be important in the proliferation of this
line (28, 29). The CMK cells were starved in RPMI 1640 medium followed by stimulation with SCF and then harvested at different time intervals as indicated. Cells were lysed and immunoprecipitated with polyclonal RAFTK R-4250 antibodies or FAK antibody. The precipitates were then
immunoblotted with monoclonal anti-phosphotyrosine (PY-20) antibodies,
FAK monoclonal antibodies, or RAFTK-specific antibodies as indicated.
The tyrosine phosphorylation of RAFTK peaked at 5 min at an SCF
concentration of 500 ng/ml (Figs. 1A and 2).
Interestingly, no phosphorylation of FAK was observed under these
conditions (Figs. 1B and 2). The maximum stimulation of
RAFTK in CMK cells was observed within 1 min and peaked at 5 min (Fig.
2).
SCF treatment is known to increase cytoplasmic calcium levels (34) and to stimulate the phosphorylation of the components of c-KIT-associated signaling pathways (35, 36). Since SCF effects are modulated by PKC (30, 37), the role of PKC in RAFTK stimulation was investigated. SCF treatment of CMK cells induced (within 1 min) the rapid phosphorylation of RAFTK, which was inhibited by the PKC inhibitors calphostin C (Fig. 1C) or staurosporine (data not shown).
The autophosphorylation and kinase activity of RAFTK upon SCF stimulation in CMK cells were analyzed. SCF stimulation resulted in an increase in the autophosphorylation as well as the kinase activity of RAFTK (data not shown), which is essential for its phosphorylating role in CMK cell signaling.
PMA Induces the Tyrosine Phosphorylation of RAFTK in CMK Megakaryocytic CellsTo study whether RAFTK might participate in the pathways of megakaryocyte differentiation, we examined whether PMA, which induces differentiation and maturation of these cells (24, 32, 37), was able to stimulate RAFTK phosphorylation (Figs. 1A and 2). Under these conditions, the phosphorylation of RAFTK peaked at 5 min at a PMA concentration of 50 nM.
Since PMA activates PKC, we sought to further characterize the relationship between the PMA-induced tyrosine phosphorylation of RAFTK in CMK cells and PKC activation. The addition of the PKC inhibitors calphostin C (1 µM) (Fig. 1D) or staurosporine (75 nM) (data not shown) inhibited RAFTK phosphorylation following the PMA treatment of CMK cells. In additional correlative experiments, PMA-sensitive isozymes were first down-regulated in CMK cells by prolonged treatment with PMA (1 h at 37 °C at 200 nM), after which these CMK cells were treated with SCF or PMA. This prolonged treatment with PMA completely abolished the subsequent effects of both the PMA and SCF treatments (data not shown), suggesting that the tyrosine phosphorylation of RAFTK by either SCF or PMA is mediated by a PKC-dependent mechanism. Interestingly, PMA stimulation did not result in an increase in the tyrosine phosphorylation of FAK (Fig. 1B), suggesting that these related molecules may have distinct roles in the different signaling pathways in megakaryocytes.
RAFTK Phosphorylation Is Inhibited by BAPTA, Calphostin C, and Cytochalasin DCalcium ionophore (A23187) treatment of cells
elevates intracellular calcium levels and initiates a cascade of
signaling events including PKC activation. CMK cells treated with
calcium ionophore A23187 showed the tyrosine phosphorylation of RAFTK,
which was inhibited by the intracellular calcium chelator, BAPTA (Fig.
3A). In the presence of calphostin C, a
specific PKC inhibitor, induction of RAFTK phosphorylation by the
calcium ionophore A23187 was inhibited, indicating that calcium
regulation of this PKC isoform was involved in RAFTK phosphorylation
(Fig. 3A). We have observed previously that RAFTK was
tyrosine phosphorylated upon fibronectin stimulation and was
co-localized with vinculin at focal adhesion sites in CMK cells (33).
Interestingly, upon calcium ionophore A23187 treatment, RAFTK tyrosine
phosphorylation was inhibited in the presence of cytochalasin D,
indicating that the integrity of the cytoskeleton is required for RAFTK
phosphorylation following changes in intracellular calcium.
Similarly, SCF treatment of CMK cells induced rapid and transient tyrosine phosphorylation of RAFTK, which was inhibited in the presence of BAPTA (Fig. 3B), suggesting that SCF may induce RAFTK phosphorylation by elevating intracellular calcium levels. However, in the presence of cytochalasin D, SCF induction of RAFTK phosphorylation was completely inhibited (Fig. 3B), indicating again that the integrity of the cytoskeleton is required for RAFTK phosphorylation. Since SCF stimulation of RAFTK in the presence of calphostin C was also completely inhibited, this mechanism of RAFTK tyrosine phosphorylation appears to be mediated by a PKC-dependent pathway.
PMA phosphorylation of RAFTK was also blocked by calphostin C (Fig. 3C) or by BAPTA, further indicating that calcium regulation of PKC isoforms is involved in RAFTK stimulation. Cytochalasin D treatment inhibited the PMA stimulation of RAFTK, suggesting that the integrity of the megakaryocytic cytoskeleton is critical for RAFTK phosphorylation.
RAFTK Forms a Complex with PaxillinTo address the role of
RAFTK in the formation of focal adhesions, we characterized its
association with the known focal adhesion protein paxillin. Cell
lysates of CMK cells treated with PMA were immunoprecipitated with
either RAFTK-specific antibodies or anti-paxillin antibodies. The
immunoprecipitates were resolved and immunoblotted with PY-20
antibodies. RAFTK was found to co-immunoprecipitate with paxillin in
both unstimulated CMK cells and CMK cells stimulated by PMA and SCF
(Fig. 4). Similar results were obtained when CMK cell
lysates were immunoprecipitated with anti-RAFTK antibodies and
immunoblotted with paxillin (data not shown). These results indicate
constitutive association of RAFTK and paxillin. Using the GST
C-terminal proline-rich domain of the RAFTK protein (amino acids
681-1009), we observed binding of the C terminus of RAFTK to paxillin
(Fig. 4C).
To further analyze whether RAFTK binds directly to paxillin, lysates of
CMK cells were immunoprecipitated with paxillin antibodies. The samples
were separated on a 7.5% SDS-PAGE gel and subjected to Far-Western
blotting. Although the GST-RAFTK N terminus (data not shown) or GST
alone did not bind to paxillin, the GST-RAFTK C-terminal (Fig.
5) proline-rich domain and the shorter GST-RAFTK C-terminal proline-rich domain (data not shown) were found to bind
directly to paxillin. These results demonstrate that RAFTK binds
directly to paxillin through its proline-rich domain.
An increase in the phosphorylation of paxillin was observed upon PMA stimulation, and peaked by 5 min (Fig. 4A). Treatment with the PKC inhibitor calphostin C inhibited the phosphorylation of RAFTK (Fig. 1) and paxillin (Fig. 4A). Similar observations of paxillin phosphorylation and its association with RAFTK were observed in CMK cells stimulated with SCF (data not shown). Taken together, these results suggest that RAFTK forms a complex with paxillin in unstimulated and stimulated CMK cells and that the phosphorylation of RAFTK and paxillin is mediated by a PKC-dependent pathway.
Effects of the Dominant-negative RAFTK (KM) on Paxillin PhosphorylationTo analyze further the interaction between RAFTK
and paxillin and to test whether RAFTK is required as an upstream
regulatory molecule of the paxillin signaling pathway, we used a
catalytically inactive mutant of RAFTK (KM) that acts as a
dominant-negative of the wild-type RAFTK in Cos cells. Cos cells were
transiently transfected with KM, wild-type RAFTK (19, 33), or paxillin expression vectors. After 72 h, cells were starved for 4 h in serum-free medium and then stimulated with PMA, lysed, and analyzed for
the phosphorylation of RAFTK. As expected, no tyrosine phosphorylation of RAFTK was observed in the presence of KM upon PMA stimulation (data
not shown), whereas RAFTK phosphorylation was observed in PMA-stimulated Cos cells transiently transfected with the wild-type RAFTK (data not shown). Paxillin phosphorylation was observed in the
PMA-stimulated Cos cells transfected with the paxillin construct (Fig.
6). When Cos cells were transiently co-transfected with
RAFTK-KM and paxillin constructs, overexpression of RAFTK-KM inhibited
the tyrosine phosphorylation of paxillin by competition with other
tyrosine kinases (Fig. 6). However, when wild-type RAFTK and paxillin
constructs (33) were co-transfected, there was an increase in paxillin
phosphorylation. Interestingly, in Cos cells transfected with the
paxillin construct alone, the phosphorylation of paxillin was observed.
However, in Cos cells co-transfected with paxillin and RAFTK-KM, the
expression of RAFTK-KM resulted in the inhibition of paxillin
phosphorylation, indicating that intact RAFTK kinase activity is
important for paxillin phosphorylation. These results demonstrate that
RAFTK is required for paxillin phosphorylation and suggest that RAFTK
can act as a mediator of the paxillin signaling pathway.
In this report, we have characterized new signaling pathways involving RAFTK in CMK human megakaryocytic cells. SCF and PMA induced the tyrosine phosphorylation of RAFTK but not of FAK. The effect of SCF, PMA, and Ca2+ on the phosphorylation of RAFTK appeared to be mediated by a PKC-dependent pathway. Association of RAFTK with paxillin was demonstrated, and cytochalasin D abolished the phosphorylation of RAFTK upon SCF and PMA stimulation.
Upon stimulation of CMK cells by SCF, RAFTK was phosphorylated and there was an enhanced autophosphorylation of RAFTK as well as an increase in its in vitro kinase activity as determined using a poly(Glu:Tyr) (1:4) substrate. These results are consistent with our previous work (33), which indicated that RAFTK had intrinsic tyrosine kinase and autokinase activities.
PKC plays an important role in the cellular responses to various hormones, growth factors, neurotransmitters, and cytokines and transduces signals promoting lipid hydrolysis (39, 40). PKC regulates the action of a variety of ion channels, G-protein-coupled receptors, tyrosine kinase receptors, and nonreceptor tyrosine kinases (41, 42). Since the proliferative effects of SCF appeared to be modulated in part by PKC (30-37, 39-43), we sought to identify a role for PKC in RAFTK phosphorylation. Indeed, SCF induced the rapid phosphorylation of RAFTK, which was completely blocked by the PKC inhibitors calphostin C (Fig. 1) or staurosporine (data not shown). Furthermore, PMA, which induces the differentiation of CMK megakaryocytic cells (24, 32, 37), also stimulated the tyrosine phosphorylation of RAFTK, and this phosphorylation was abolished by the PKC inhibitors (Fig. 1) or by prolonged treatment with PMA. Rat brain PKC was able to phosphorylate the GST C-terminal RAFTK in a lipid-activator, Ca2+-dependent manner.2 Taken together, these results indicate that RAFTK phosphorylation is mediated by a PKC-dependent pathway.
SCF induction of the tyrosine phosphorylation of RAFTK could be
mediated by elevated intracellular calcium levels and/or by the
activation of PKC through phospholipase C- (44). Indeed, RAFTK
phosphorylation was inhibited following treatment by the PKC inhibitors
calphostin C or staurosporine as well as by BAPTA (an intracellular
Ca2+ chelator) (Fig. 3), indicating that PKC is involved in
RAFTK phosphorylation. BAPTA blocked PMA- or SCF-induced RAFTK
phosphorylation, suggesting that calcium was essential for PKC-mediated
RAFTK phosphorylation (Fig. 3). Moreover, the calcium ionophore
(A23187) also stimulated RAFTK phosphorylation and was inhibited by the
PKC inhibitors calphostin C and staurosporine or by BAPTA (Fig. 3),
indicating a role for PKC as a mediator of several signaling pathways
including Ca2+ in RAFTK phosphorylation. The finding that
FAK is not phosphorylated under these conditions is consistent with
prior studies of FAK activation in Mo7e megakaryocytic cells (45) and
suggests important differences in the roles of FAK and RAFTK in cells
of this lineage.
The cytoskeleton is essential for many cellular functions including the
regulation of cell shape, flexibility, and adhesive properties (8, 9).
Part of the cytoskeleton and plasma membrane form a region known as the
focal adhesion (46). Focal adhesions are structures that form adherent
contacts with the extracellular matrix. Proteins contained in the focal
adhesion include talin, -actinin, vinculin, paxillin, and other
proteins (47-52). The signal transduction pathways initiated by the
integrins involve the cytoskeleton-dependent activation of
tyrosine kinases and the phosphorylation of a number of substrates
including the FAK protein (9, 10, 13).
We have observed previously that RAFTK was tyrosine phosphorylated upon fibronectin stimulation and was co-localized with vinculin at "focal adhesion-like structures" in CMK cells (33). The observation that RAFTK phosphorylation upon calcium ionophore (A23187) treatment or SCF or PMA stimulation of CMK cells was completely abolished in the presence of cytochalasin D, which disrupts the cytoskeleton (Fig. 3), suggested that the integrity of the cytoskeleton is required for RAFTK phosphorylation; these results are similar to what was found with FAK phosphorylation by integrins and external stimuli (11).
We observed constitutive association of RAFTK and paxillin, indicating
that RAFTK forms a complex with paxillin (Fig. 4). Moreover, we have
demonstrated that the C-terminal proline-rich region of RAFTK binds
directly to paxillin (Fig. 5) and that overexpression of a
dominant-negative mutant of RAFTK co-transfected with paxillin into Cos
cells abolished the tyrosine phosphorylation of paxillin upon PMA
stimulation (Fig. 6). The observation that in Cos cells transfected
with the paxillin construct alone paxillin was phosphorylated indicates
the involvement of other kinases in the phosphorylation of paxillin
(52, 53). However, overexpression of the dominant-negative mutant of
RAFTK prevented the tyrosine phosphorylation of paxillin upon PMA
stimulation by other kinases. This association suggests a role for
RAFTK in the linking and cross-talk between various signaling proteins
localized in the cytosol and focal adhesion contacts. Interestingly,
the RhoA-dependent assembly of focal adhesions in Swiss 3T3
cells was associated with an increased tyrosine phosphorylation and the
recruitment of both p125FAK and PKC- to focal adhesions
(38).
We have recently shown that the stimulation of megakaryocytes with thrombin leads to the tyrosine phosphorylation of RAFTK (19). In this study, we observed that RAFTK is involved in PKC-mediated c-KIT growth factor and Ca2+ signaling pathways in megakaryocytic cells. Taken together, these studies indicate the potentially important function of RAFTK signaling in these cells.
We thank Drs. Sandhya Raja, Sheila Zrihan-Licht, Bijia Deng, and Daniel Price for their critical help in revising the manuscript. We also thank Dr. Keith E. Langley and Dr. L. Bennett (Amgen Inc.) for providing recombinant SCF/KIT ligand and polyclonal anti-c-KIT antibodies. This paper is dedicated to Ronald Ansin for friendship and support for our research program. We thank Janet Delahanty for editing and preparation of the figures. We also thank Evelyn Gould for assistance with the figures and Tee Trac for secretarial assistance.