(Received for publication, October 16, 1996, and in revised form, March 24, 1997)
From the Department of Pharmacology and Medicine and the Lineberger Comprehensive Cancer Center, University of North Carolina, Chapel Hill, North Carolina 27599-7295
We and others have recently cloned a
non-receptor, calcium-dependent tyrosine kinase (CADTK;
also known as PYK2, CAK, and RAFTK) that shares both overall domain
structure and 45% amino acid identity with p125FAK.
We have studied the signaling, activation, and potential function of
these related enzymes in GN4 rat liver epithelial cells that express
CADTK and p125FAK at roughly similar levels.
p125FAK is nearly fully tyrosine-phosphorylated in resting
GN4 cells. In contrast, while CADTK is not tyrosine-autophosphorylated
in untreated cells, angiotensin II increases CADTK Tyr(P) by
5-10-fold. With regard to signaling, CADTK activation is correlated
with stimulation of c-Jun N-terminal kinase and p70S6K
pathways but not with the stimulation of mitogen-activated protein kinase or p90RSK. In this report we assessed the
contribution of CADTK and p125FAK to tyrosine
phosphorylation of focal contact proteins. In adherent GN4 cells, the
constitutive activity of p125FAK was correlated with basal
paxillin, tensin, and p130CAS tyrosine phosphorylation. A
rapid increase in the tyrosine phosphorylation of each protein was
detected after treatment with angiotensin II or other agonists that
stimulate CADTK; the prolonged 3-4-fold increase in paxillin tyrosine
phosphorylation was the most substantial change. In the WB cell line
that expresses 3-fold less CADTK than GN4 cell line
agonist-dependent paxillin tyrosine phosphorylation is
similarly reduced. Immunoprecipitation of CADTK from GN4 cells revealed
CADTK·paxillin complexes that persisted in 500 mM NaCl but not in 0.1% SDS cell lysis buffer. The complexes were largely independent of the tyrosine phosphorylation state of either protein. Surprisingly, we did not detect p125FAK·paxillin
complexes in immunoprecipitates using either of two p125FAK
antibodies. When CADTK and p125FAK were transiently
overexpressed in 293(T) cells, both enzymes associated with paxillin,
but the avidity of CADTK appeared to be greater. In addition, in
transfected 293(T) cells, complexes between CADTK and another potential
substrate, p130CAS, were detected. In summary, in GN4 rat
liver epithelial cells stimulation of CADTK was highly correlated with
paxillin tyrosine phosphorylation; in addition, CADTK but not
p125FAK was complexed to paxillin at detectable levels.
This suggests that agonist-dependent cytoskeletal changes
in epithelial cells might proceed, in part, by
CADTK-dependent mechanisms.
The once separate fields of cell structure and signal transduction have converged due to a number of recent observations. Growth factors and hormones are now known to regulate cell shape and mobility; conversely, proteins involved in cell attachment and cytoskeleton formation can clearly be induced to generate intracellular signals (1-6). For example, integrins engagement stimulates tyrosine phosphorylation (7-10) and alters gene expression (6, 11).
Several years ago our laboratory noted that EGF1 treatment of rat liver epithelial cells produced several waves of protein tyrosine phosphorylation, the second occurring ~30 s after the initial accumulation of EGF-dependent Tyr(P) substrates (12). At least some of the secondary substrates, those in the p115-130-kDa region, corresponded in molecular size to Tyr(P) substrates observed following integrin cross-linking. The delayed EGF-dependent activity was, in part, due to stimulation of a soluble protein tyrosine kinase that appeared to be activated by the small EGF-dependent calcium signal (13). Kinase activation was even greater with the higher intracellular calcium levels produced by angiotensin II (Ang II), [Arg8]vasopressin, or epinephrine (13, 14). Thapsigargin which increases intracellular calcium without stimulating protein kinase C also stimulated tyrosine phosphorylation, an effect greatly diminished by pretreatment of cells with BAPTA-AM, an intracellular calcium chelator (13, 14).
We have now purified the calcium-dependent tyrosine kinase
(CADTK) from rat liver epithelial cells (15) and obtained a complete cDNA (16). Rat CADTK encodes the same protein as human PYK2 (17),
RAFTK (18), and rat CAK (19). CADTK and p125FAK are
highly related, and thus comparison is instructive. The 45% overall
amino acid identity is particularly striking within the tyrosine kinase
and C-terminal domains. p125FAK, originally identified as a
v-src substrate is localized to focal adhesions (20) where a
network of proteins connects the extracellular matrix to the actin
cytoskeleton (4) and is activated in response to cellular interaction
with the extracellular matrix (7, 10, 21, 22). This latter effect is
often correlated with but may or may not be causally related to signals
that activate the MAPK pathway (23-27). In summary,
p125FAK sits at a conceptual and physical juncture where it
is capable of integrating cell structure and signaling.
p125FAK does not contain SH2 or SH3 domains but can interact with proteins containing SH2 and SH3 binding domains. When autophosphorylated on tyrosines, p125FAK creates binding sites for other SH2 domain-containing proteins including Src tyrosine kinase family members (28-30). p125FAK also exhibits a proline-rich region that can interact with SH3 domain-containing proteins including p130CAS (31-34). Additionally, the C terminus encompasses the focal adhesion targeting domain that forms direct or indirect complexes with several focal adhesion proteins including paxillin (35). The association with paxillin presumably occurs through two vinculin homology domains within the C-terminal focal adhesion targeting sequence; in turn, paxillin binding has been suggested to localize p125FAK to focal adhesions (36). However, others have reported that paxillin association may not be required for p125FAK focal adhesions' localization (37). As noted, tyrosine-phosphorylated p125FAK binds (and may activate) Src family tyrosine kinases, concentrating these enzymes and other proteins within focal adhesions, in effect assembling a large potential signaling complex (5, 6, 24).
p125FAK has been most extensively studied in fibroblasts, a cell type that does not express CADTK (19) (data not shown). The latter kinase is abundant in neural tissue and is expressed in epithelial cells and hematopoietic cells (16-18). However, CADTK is not excluded from cells of mesenchymal origin as we have found it to be activated by multiple agonists in rat smooth muscle cells.2 While some cells express only one or the other enzyme, at least several cell types including rat liver epithelial cells express CADTK and p125FAK. CADTK is rapidly activated by a Gq protein-coupled signal using either the calcium- or protein kinase C-dependent branches of phospholipase C-activated pathways (15-17). Neither the effect of calcium nor protein kinase C appear to be direct (calcium does not directly activate the purified enzyme and protein kinase C activation is slower). In Swiss 3T3 cells, p125FAK is rapidly stimulated by bombesin and other neuropeptides (38-41). However, in cells in which both enzymes are expressed the stimulation of CADTK activity is more rapid, of greater magnitude, and is far more dependent upon hormonal and growth factor stimulation than changes in p125FAK (16, 17).2 For example, in adherent WB and GN4 cells, p125FAK exhibits a high basal level of tyrosine phosphorylation and is only minimally increased by Ang II treatment, whereas CADTK is stimulated by 5-10-fold (16). In many instances p125FAK activation is correlated with stimulation of the MAPK pathway although a direct causal relationship is not universally agreed upon. The calcium-dependent activation of CADTK in GN4 liver epithelial cells does not activate MAPK (16) but is correlated with substantial increases in c-Jun N-terminal kinase and the p70S6 kinase (p70S6K) activities (16, 42, 43).
But what of CADTK's interaction with and phosphorylation of cytoskeletal proteins, a dominant feature of p125FAK biology? In this article we report that Ang II treatment stimulates the tyrosine phosphorylation of paxillin, tensin, and p130CAS. The effect on paxillin phosphorylation is the most dramatic and prolonged. While p125FAK probably regulates basal paxillin tyrosine phosphorylation in adherent GN4 cells (since CADTK activity is minimal), the rapid and extensive paxillin tyrosine phosphorylation observed after agonist stimulation correlates with both the activation and expression of CADTK. Moreover, even though the levels of tyrosine-phosphorylated p125FAK and CADTK are similar in GN4 cells, paxillin forms a noncovalent complex with CADTK, whereas paxillin·p125FAK complexes could not be detected. Overexpression of CADTK and p125FAK by transient transfection again revealed the increased affinity of paxillin for CADTK and also demonstrated CADTK·p130CAS complexes. Thus, in GN4 cells, hormonal activation of CADTK significantly increases paxillin tyrosine phosphorylation, acute changes that are played out upon a background level of extracellular matrix dictated protein tyrosine phosphorylation mediated, in part, by p125FAK.
Ang II was purchased from Sigma and prepared in 50 mM acetic acid prior to use. Thapsigargin and BAPTA-AM were purchased from Sigma and Biomol, respectively, and prepared in Me2SO. Anti-paxillin monoclonal antibody and anti-Tyr(P) monoclonal antibody (RC20H) were purchased from Transduction Laboratories. Anti-Tyr(P) monoclonal antibody (PT66) was purchased from Sigma. Anti-p125FAK, monoclonal antibody 2A7, and polyclonal antibody BC3 were generously provided by Drs. Tom Parsons (University of Virginia) and Michael Schaller (University of North Carolina). Anti-p125FAK polyclonal antibody, A17, was purchased from Santa Cruz Biotechnology. Anti-p130CAS monoclonal and polyclonal antibodies were purchased from Transduction Laboratories and Santa Cruz Biotechnology, respectively. Anti-tensin monoclonal antibody was generously provided by Dr. Keith Burridge (University of North Carolina). Rabbit anti-rat CADTK polyclonal antisera were raised to two glutathione S-transferase fusion proteins (amino acids 1-80 and 680-860 of rat CADTK, respectively) as described previously (16).
Cell CulturesRat liver epithelial cells (GN4 or WB) were cultured in Richter's minimal essential medium supplemented with 10% fetal bovine serum and 0.1 µM insulin as described earlier (15). Human 293 embryonic kidney cells with SV40 T antigen (human 293(T) cells) were kindly provided by Dr. Brian Varnum (Amgen) and grown in Dulbecco's modified Eagle's medium with 10% fetal bovine serum.
Cell Lysate PreparationCell lysis was performed essentially as described previously (15). Briefly, cells treated with agonists were scraped into ice-cold cell lysis buffer. One of three lysis buffers was used and referred to as follows: (i) low salt lysis buffer (150 mM NaCl, 20 mM Tris (pH 7.5), 1% Triton X-100, 5 mM EDTA, 50 mM NaF, and 10% (v/v) glycerol); (ii) high salt buffer (500 mM NaCl, 20 mM HEPES (pH 7.3), 1% Triton X-100, 5 mM EDTA, 50 mM NaF, and 10% (v/v) glycerol); or (iii) RIPA lysis buffer (150 mM NaCl, 20 mM Tris (pH 7.5), 1% Triton X-100, 2 mM EDTA, 10% (v/v) glycerol, 0.1% SDS, and 0.5% deoxycholate). To all cell lysis buffers the following reagents were added before use: 1 mM Na3VO4, 20 µg/ml phenylmethylsulfonyl fluoride, 10 µg/ml leupeptin, and 100 kallikrein inhibitor units of aprotinin per ml. Cell lysates were clarified by centrifugation at 14,000 × g for 10 min at 4 °C and the protein content determined prior to immunoprecipitation.
Anti-Tyr(P), p125FAK, CADTK, and Paxillin Immunoprecipitation and ImmunoblottingIn a typical experiment,
500 µg of cell lysate was immunoprecipitated by incubation with the
antibody for 2 h at 4 °C, followed by addition of 20 µl of
protein A or protein A/G-agarose beads (Santa Cruz) for 1 h.
Immune complexes were collected by centrifugation (in some cases the
supernatant was used for a second antibody immunoprecipitation). Immune
complexes were then washed three times with the lysis buffer and then
resuspended in SDS-PAGE sample buffer. Samples were subjected to
SDS-PAGE, transferred to Immobilon (Millipore), and detected by
incubating the blots with the specified antibody as described (15).
Immunoblots were incubated with either goat anti-rabbit or anti-mouse
horseradish peroxidase-conjugated antibodies and developed using
enhanced chemiluminescence according to the manufacturer's procedure
(Amersham Corp.). When indicated, immunoblots were stripped in the
buffer (62.5 mM Tris (pH 6.8), 2% SDS, 100 mM
-mercaptoethanol) at 50 °C for 30 min, and reprobed with another
specific antibody.
The full-length CADTK cDNA was isolated as described (16) and was subcloned into a pcDNA3 vector (Invitrogen). Human p125FAK cDNA, subcloned into the pcDNA3 vector, was kindly provided by Dr. William Cance (University of North Carolina). The control vector (pcDNA3), pcDNA3-CADTK, and pcDNA3-p125FAK were transfected into subconfluent human 293(T) cells with LipofectAMINE according to the manufacturer's procedure (Life Technologies, Inc.). After 48 h, transfected cells were harvested and lysed on ice with low salt buffer, and the lysates were analyzed by immunoprecipitation, followed by immunoblotting with anti-Tyr(P), CADTK, p125FAK, paxillin, or p130CAS.
As previously reported, Ang II and thapsigargin
increase the tyrosine phosphorylation of proteins with a molecular
weight of p115-130, p72/75, and p66 (13-15). One of the 115-kDa
tyrosine-phosphorylated proteins was identified as the major
calcium-dependent tyrosine kinase (CADTK). Since integrin
engagement stimulates p125FAK and paxillin Tyr(P) and Ang
II has been shown to increase paxillin tyrosine phosphorylation in
smooth muscle cells (44, 45), we tested whether one of the GN4 cell
p72/75-kDa tyrosine phosphoproteins was paxillin. Immunoprecipitation
and anti-Tyr(P) immunoblot revealed that Ang II treatment of GN4 cells
increased paxillin tyrosine phosphorylation by 90 s, an effect
that persisted for at least 30 min (Fig. 1A).
Paxillin tyrosine phosphorylation could be detected at 15-30 s
coincident with the tyrosine phosphorylation of CADTK (data not shown).
Ang II stimulation also altered paxillin electrophoretic mobility,
suggesting sequential, multi-site phosphorylation on Tyr, Ser, or Thr
residues. The mobility shift, while detected at early time points,
became more pronounced at 5 min.
Ang II treatment also rapidly increased tensin (Fig. 1C) and p130CAS (Fig. 1E) tyrosine phosphorylation. In contrast to paxillin, both tensin and p130CAS reached their maximum level of tyrosine phosphorylation by 90 s and gradually decreased their Tyr(P) content. This more closely parallels the time course of CADTK tyrosine phosphorylation (Fig. 1G) but may also suggest that tensin and p130CAS are more susceptible to tyrosine phosphatases than paxillin. Tensin but not p130CAS also exhibited a significant gel mobility shift with Ang II treatment (Fig. 1C). The gel mobility shift persists even though total Tyr(P) as assessed by immunoblot recedes. It is likely that the gel mobility shift of both paxillin and tensin progress as due to Ser/Thr phosphorylations or by tyrosine phosphorylation at new sites. Tryptic phosphopeptide mapping followed by phosphoamino analysis may resolve this issue.
Agonist-dependent CADTK and Paxillin Tyrosine Phosphorylation Are CorrelatedRat liver epithelial cells express
both p125FAK and CADTK. Stimulation with Ang II leads to a
variable alteration in p125FAK tyrosine phosphorylation and
autokinase activity ranging from barely detectable to 50-100%
increases (15). This is presumably due to the fact that
p125FAK is near maximally phosphorylated in adherent,
confluent GN4 cells. In contrast, CADTK tyrosine phosphorylation is
barely detectable in control cells but is rapidly induced (5-10-fold)
by Ang II or other agonists. To test whether CADTK or
p125FAK stimulation correlated with acute changes in
paxillin tyrosine phosphorylation, GN4 cells were treated with a series
of agonists known to stimulate CADTK followed by comparison of the
Tyr(P) content of paxillin, CADTK, and p125FAK. Agonists
that significantly increased CADTK tyrosine phosphorylation (Fig.
2A) were the most effective at acutely
increasing paxillin tyrosine phosphorylation (Fig. 2C). In
general, the extent of CADTK and paxillin Tyr(P) was correlated. For
example, prolonged EGF treatment (5 min) slightly increased CADTK
tyrosine phosphorylation (Fig. 2A, lane 3) and slightly
stimulated paxillin tyrosine phosphorylation (Fig. 2C, lane
3), whereas Ang II and sorbitol maximally stimulated CADTK and
paxillin Tyr(P) content. In contrast, p125FAK tyrosine
phosphorylation was only minimally altered by agonist treatment (Fig.
2B). Therefore, basal paxillin tyrosine phosphorylation may
be determined by constitutive p125FAK activity. The
correlation between CADTK and paxillin tyrosine phosphorylation
suggests that Gq protein-coupled receptor and other
agonists stimulate additional paxillin tyrosine phosphorylation via
CADTK.
Agonist-stimulated Paxillin Tyrosine Phosphorylation Correlates with CADTK Expression and Extent of Activation
To further examine
the role of the two enzymes, Ang II-dependent paxillin
tyrosine phosphorylation was investigated in cells known to express
similar levels of p125FAK but different levels of CADTK. We
had previously shown that confluent GN4 cells (derived by chemical
transformation of a normal rat liver epithelial cell line, WB) have
~3-4 times more Ang II-dependent tyrosine
phosphorylation than its parent WB cell (13). Immunoprecipitation with
specific CADTK antiserum demonstrated that GN4 cells exhibit ~4-5-fold higher maximal Ang II-dependent CADTK tyrosine
phosphorylation (90 s) than similarly treated WB cells (16). Likewise,
Ang II treatment resulted in significantly more paxillin tyrosine
phosphorylation in GN4 cells than in WB cells (Fig.
3A). p125FAK expression and
tyrosine autophosphorylation in response to Ang II stimulation was
similar in the GN4 and WB cell lines (Fig. 3C). Thus the
similar basal level of paxillin tyrosine phosphorylation in WB and GN4
(Fig. 3A) cells correlated with the equivalent
p125FAK levels (Fig. 3C). The much greater Ang
II-dependent paxillin tyrosine phosphorylation in GN4 cells
was observed consistently. It supports the hypothesis that increased
CADTK activation acutely regulates paxillin Tyr(P) content.
Intracellular Calcium Chelation and Cytochalasin D Block Ang II-dependent Paxillin Tyrosine Phosphorylation
CADTK
activation by Ang II or thapsigargin is, in part, a
calcium-dependent process. To test the calcium dependence
of Ang II and thapsigargin-stimulated paxillin tyrosine
phosphorylation, GN4 cells were preincubated with the cell-permeable,
calcium chelator BAPTA-AM that abolishes the calcium signal in these
cells (13, 14). BAPTA attenuated the acute increase in both CADTK and
paxillin tyrosine phosphorylation in response to Ang II (Fig.
4, A and C). The effect of BAPTA
was not complete since Ang II also regulates CADTK activity via protein
kinase C. However, BAPTA, which completely blocked
thapsigargin-dependent CADTK activation (Fig. 4A,
lane 6), almost totally inhibited
thapsigargin-dependent paxillin tyrosine phosphorylation
(Fig. 4C, lane 6). Preincubation with BAPTA-AM alone
decreased both basal p125FAK and paxillin tyrosine
phosphorylation (Fig. 4B). These results suggest that
calcium-dependent activation of CADTK is in part responsible for initiating paxillin tyrosine phosphorylation in response to Ang II and thapsigargin.
Paxillin, a member of the complex of cytoskeletal proteins, is
concentrated at focal contacts, the cytoplasmic face of regions attaching the cell to the extracellular matrix (46, 47). Cytochalasin D, an agent that disrupts actin microfilaments and cytoskeletal movement, inhibits p125FAK tyrosine autophosphorylation and
prevents paxillin tyrosine phosphorylation in Swiss 3T3 cells (22, 39,
41, 48). To test whether cytochalasin D inhibited CADTK,
p125FAK, or paxillin tyrosine phosphorylation, GN4 cells
were preincubated with cytochalasin D and subsequently treated with Ang
II or NaCl, another agonist that stimulates CADTK activity (see Ref. 16 and Fig. 2). Cytochalasin D pretreatment dramatically changed cell
morphology (data not shown) and partially inhibited Ang II and
NaCl-stimulated CADTK (Fig. 5, A and
C) and basal p125FAK tyrosine phosphorylation
(Fig. 5B). The effect of cytochalasin D on paxillin tyrosine
phosphorylation was even more dramatic; both basal and stimulated
paxillin Tyr(P) were nearly eliminated by cytochalasin D pretreatment.
If our thesis is correct, i.e. that p125FAK is
responsible for basal paxillin tyrosine phosphorylation in adherent
cells and CADTK is responsible for the hormonally induced increment,
this experiment suggests that both processes require an intact
cytoskeleton.
Tyrosine-phosphorylated Paxillin Associates with CADTK in Ang II-treated Cells
The results in Figs. 1, 2, 3 suggested that Ang II
stimulates paxillin tyrosine phosphorylation and that this
agonist-dependent process is best correlated with
activation and expression of CADTK rather than p125FAK.
Since paxillin associates with p125FAK in chicken embryo
fibroblasts (37), we tested whether tyrosine-phosphorylated paxillin
bound to CADTK or p125FAK in control and Ang II-treated GN4
cells. Confluent GN4 cells were treated with vehicle or Ang II for
90 s, lysed, and immunoprecipitated with antiserum to CADTK or
with one of two antibodies to p125FAK, 2A7 or A17. CADTK
tyrosine phosphorylation was stimulated in Ang II-treated cells, and
p125FAK, which runs slightly above the 115-kDa CADTK, was
tyrosine-phosphorylated in both control and Ang II-stimulated GN4 cells
(Fig. 6). Equal amounts of cell lysates were used for
all immunoprecipitations and were immunoblotted with the same
anti-Tyr(P) antibody; thus, the result depicted in Fig. 6 suggests that
maximal level of tyrosine-phosphorylated p125FAK is at
least equivalent and in fact is probably slightly greater than that of
CADTK. Because we do not have an antibody that recognizes both enzymes,
we have compared total Tyr(P) in the immunoprecipitated kinases. The
sequence and autophosphorylation sites in both kinases are highly
conserved. Moreover, we have mutated the predicted major tyrosine
autophosphorylation site of CADTK Tyr402 and demonstrated
that this mutation drastically decreases CADTK autophosphorylation in
the same manner that Tyr397 mutation reduces
p125FAK autophosphorylation.3
Thus, the equivalent level of maximal tyrosine phosphorylation in GN4
cell CADTK and p125FAK provides a reasonable indication
that p125FAK and CADTK expression are similar in these
cells.
Surprisingly, 68-75-kDa range Tyr(P) proteins were associated with
CADTK, but there was little or no 68-75-kDa Tyr(P) protein associated
with p125FAK (Fig. 6). Analysis of the CADTK
immunoprecipitation with paxillin antibody showed that at least some of
the 68-75-kDa Tyr(P) protein was paxillin (see below). The result
suggests that while paxillin can associate with p125FAK
(see Refs. 36 and 37 and Fig. 9) in adherent cells, little or no
tyrosine-phosphorylated paxillin can be found in precipitable p125FAK·paxillin complexes.
Paxillin and CADTK Associate in Intact Cells
Having observed
CADTK association with tyrosine-phosphorylated paxillin in GN4 cells,
we further investigated the nature of the CADTK·paxillin complex. GN4
cells were treated with vehicle, Ang II, or thapsigargin and lysed in
three different lysis buffers, low salt, high salt, and 0.1% SDS RIPA
buffer. Cell lysates were first immunoprecipitated using anti-CADTK
antiserum; subsequently the CADTK-cleared lysate was
reimmunoprecipitated with anti-paxillin antibody. Following SDS-PAGE
and transfer, a paxillin immunoblot demonstrated nearly equal amounts
of paxillin present in CADTK immunocomplexes precipitated in low salt
buffer from either control or agonist-treated cells. Thus, Ang II or
thapsigargin treatment did not alter CADTK-paxillin association; the
complex exists prior to agonist treatment (Fig.
7A). The results were the same after lysis in
a high salt buffer (Fig. 7B), a condition that would disrupt
protein-protein association based on Tyr(P)-SH2 domain interaction.
CADTK-paxillin association was eliminated in 0.1% SDS suggesting that
native conformation of one or both proteins was required (Fig.
7C). The above results suggested that CADTK-paxillin association in vivo is an intrinsic property of the proteins
and does not require CADTK or paxillin tyrosine phosphorylation.
CADTK Appears to Bind More Avidly to Paxillin Than p125FAK
We next tested whether disrupting the
cytoskeleton structure with cytochalasin D could disrupt the
CADTK-paxillin or p125FAK association. As shown in Fig.
8A, CADTK associated with paxillin regardless
of whether the GN4 cells were treated with cytochalasin D or not.
Although, cytochalasin D pretreatment inhibited CADTK tyrosine
phosphorylation and prevented paxillin tyrosine phosphorylation in Ang
II-treated cells (Fig. 5), it did not disrupt the CADTK-paxillin association. Paxillin·p125FAK complexes were not detected
under these conditions (with or without cytochalasin D) (Fig.
8B). The antibody, 2A7, used to immunoprecipitate p125FAK is the same antibody that detects the
p125FAK-paxillin association in chicken embryo fibroblasts
(37). Paxillin immunoblotting after immunoprecipitating with
p125FAK antibody, A17, also failed to detect
paxillin·p125FAK complexes in GN4 cells (data not
shown).
To further examine the paxillin complexes, p125FAK and CADTK were overexpressed by transient transfection cDNAs driven by cytomegalovirus promotor in human 293(T) cells. 293(T) cells exhibit minimal p125FAK expression (as seen on an overexposed immunoblot), but we could not detect any endogenous CADTK. As shown in Fig. 9, after transfection, p125FAK tyrosine phosphorylation level was much higher than that of CADTK (Fig. 9A). Immunoprecipitation demonstrated p125FAK·paxillin complex under this condition (Fig. 9C), ruling out an experimental artifact as the reason for our failure to detect p125FAK·paxillin complex in GN4 cells.
To examine another potential CADTK substrate complex, we tested CADTK
immunoprecipitates from CADTK-transfected 293(T) cells for the presence
of p130CAS. CADTK overexpression in human 293(T) cells
allows detection of CADTK-p130CAS association (Fig.
10) as defined by co-immunoprecipitation. In contrast
to paxillin, the CADTK·p130CAS complex was not detected
in GN4 cells (data not shown), but the experiment in Fig. 10 does
demonstrate a direct interaction of this potential substrate
(p130CAS), kinase (CADTK) pair.
Ang II initiates its signal via Gq protein-coupled receptor-activating phospholipase C, serine/threonine kinases, and at least one tyrosine kinase that we have recently purified and cloned and referred to as CADTK (16). Although CADTK is stimulated by a calcium signal, the calcium effect is indirect as neither calcium nor calcium/calmodulin directly activate the enzyme. Treatment of GN4 cells with phorbol esters also activates CADTK, but the activation is slower than that of Ang II or thapsigargin and is therefore also probably indirect. Thus, the mechanism by which calcium and other signals regulate CADTK is currently unknown. In GN4 cells, thapsigargin, which produces a calcium signal and activates CADTK, also stimulates both c-Jun N-terminal kinase and p70S6K but not MAPK or p90RSK (16, 42, 43). However, in PC12 cells, agonist-dependent CADTK/PYK2 stimulation increased Shc tyrosine phosphorylation and MAPK activity. We are currently trying to understand the basis of this cell type difference in CADTK signaling and must, in addition, determine whether CADTK and p125FAK have distinct effects on the MAPK pathway.
To broaden the comparison between CADTK and p125FAK, we
investigated the Ang II-dependent tyrosine phosphorylation
of paxillin, a protein tyrosine phosphorylated upon engagement of cell
surface integrins (37). In Swiss 3T3 cells (which do not express
CADTK), paxillin and p125FAK become coordinately and
substantially tyrosine-phosphorylated in response to a variety of
stimulators, including bombesin, lysophosphatidic acid,
platelet-derived growth factor, and GTPS (38-41, 48). Paxillin can
also be phosphorylated in vitro by p60src and Csk,
both of which are potentially regulated and/or localized through
p125FAK (30). In this report, we show that Ang II rapidly
increased tyrosine phosphorylation of paxillin, tensin, and
p130CAS in adherent GN4 rat liver epithelial cells. The
effect on paxillin is the greatest. The increment in paxillin tyrosine
phosphorylation produced by CADTK agonists (i) is rapid (Fig. 1), (ii)
correlates with CADTK activation for a range of agonists (Figs. 2 and
5), (iii) correlates with the CADTK expression and activation in GN4 and WB cells (Fig. 3), and (iv) is largely
calcium-dependent (Fig. 4). A key element of this argument
is depicted in Fig. 6. Tyrosine-phosphorylated p125FAK is
expressed at levels that are similar or slightly greater than the
maximal level of tyrosine-phosphorylated CADTK. Since it is known that
the major autophosphorylation site in p125FAK is
Tyr397 (30, 49) and we have demonstrated the equivalent
site Tyr402 is the major autophosphorylation site in
CADTK,3 the comparison of maximal tyrosine phosphorylation
of these two enzymes provides a reasonable estimate of their relative
expression. p125FAK is near maximally
tyrosine-phosphorylated in confluent, untreated cells. Since
p125FAK activity is thought to be primarily controlled by
extracellular factors, the near maximal level of p125FAK
activation may well dictate the basal level of paxillin tyrosine phosphorylation. This is concordant with the fact that basal level of
paxillin Tyr(P) is equivalent in WB and GN4 cell lines expressing similar amounts of p125FAK (Fig. 3). Ang II treatment only
minimally altered p125FAK tyrosine phosphorylation (Fig. 6)
and autokinase activity (15), but Ang II increases CADTK tyrosine
phosphorylation (Fig. 2) and activity (16). This activation correlates
with a substantial increase in paxillin and smaller but definable
increases in tensin and p130CAS tyrosine
phosphorylation.
The intracellular calcium chelator, BAPTA, significantly inhibits thapsigargin-dependent CADTK and paxillin tyrosine phosphorylation. In agonist-treated cells, BAPTA inhibition has less effect on p125FAK tyrosine phosphorylation than on CADTK (Fig. 4), suggesting that CADTK is the tyrosine kinase responsible for the Gq protein-coupled receptor-mediated increase in paxillin tyrosine phosphorylation. However, we cannot rule out other possibilities. First, CADTK tyrosine autophosphorylation like that of p125FAK may provide SH2 domain binding sites to recruit tyrosine kinases, such as Src family tyrosine kinases (2, 28, 29, 49, 50). These enzymes in turn may phosphorylate paxillin. We have shown a major autophosphorylation site (Tyr402 AEI) on CADTK is identical to Tyr397 AEI in p125FAK (49, 50), and both are close to the consensus sequence (YEEI) recognized by the SH2 domain of p60src and its family members (51). Our preliminary data show that CADTK immune complexes can directly phosphorylate the N-terminal portion of paxillin in vitro,4 but this does not preclude the action of a CADTK-associated tyrosine kinase. Fig. 6 demonstrates a high level of p125FAK Tyr(P) in resting cells, presumably phosphorylated at Tyr397. The rapid, agonist-induced increases in both CADTK and paxillin tyrosine phosphorylation suggest direct CADTK phosphorylation of paxillin but again do not rule out CADTK autophosphorylation followed by recruitment of another tyrosine kinase. In this latter scenario, activated CADTK could recruit and activate a tyrosine kinase with an affinity for CADTK Tyr402 greater than its affinity for p125FAK Tyr397. Alternatively, other secondary mechanisms of activation might occur via SH3-proline-rich region interactions. It seems more likely that agonist-activated CADTK directly phosphorylates paxillin.
The CADTK and p125FAK similarity is higher within the focal adhesion targeting domain that has two vinculin homologous domains (36). These two domains, which are essential for paxillin binding, have been named paxillin binding sequence 1 and 2 (PBS1 and PBS2). Both PBS1 (919RSNDKVYENVTGLVKAVIEM938) and PBS2 (1029VDAKNLLDVIDQARL1043) homologous domains are present in CADTK: (875RTDDLVYHNVMTLVEAVLEL894) and (986VDAKNLLDAVDQAKV999) with 55 and 73% identity, respectively. Treatment with cytochalasin D shows that CADTK·paxillin complexes do not require either tyrosine phosphorylation or an intact cytoskeleton (Figs. 7 and 8) suggesting that CADTK may directly associate with paxillin through primary protein structures, e.g. the two PBS1- and PBS2-like domains. In fact, we have demonstrated that a glutathione S-transferase N terminus of paxillin binds to CADTK synthesized by in vitro translation of the rat CADTK cDNA using rabbit reticulocytes.3 Surprisingly, p125FAK-paxillin association was not detected in GN4 cells even though protein expression levels of p125FAK and CADTK appear to be similar. Further experiments will be necessary to determine the mechanism (direct or indirect) and domains involved in CADTK and p125FAK interactions with cytoskeletal proteins. This information could then be used to determine, in epithelial cells, whether the affinity of CADTK for paxillin is higher than that of p125FAK.
Since they are expressed in the same cells, p125FAK and CADTK are not likely to be cell type-specific functional equivalents. For example, CADTK cannot fully replace p125FAK as p125FAK-deficient mice, produced by gene targeting, result in mutant embryos (52). However, the two enzymes have similarities; for example, cell adherence to extracellular matrix leads to CADTK/RAFTK activation (53). The fact that CADTK and p125FAK appear to have different abilities to complex with paxillin suggests subtle differences in function, even with respect to the cytoskeleton. Further experiments will help us define the relationship between these two protein tyrosine kinases.
Ang II treatment also increases p130CAS and tensin tyrosine phosphorylation, and overexpression of CADTK in 293(T) cells demonstrated CADTK·p130CAS complexes (Fig. 10). Transfecting cells with Rous sarcoma virus or spreading of cells on extracellular matrix induces both p130CAS and tensin tyrosine phosphorylation (24, 54-57). Indeed, both p125FAK and Src can phosphorylate these two cytoskeletal proteins in vitro (58, 59). p130CAS can associate with p125FAK in vivo through its SH3 domain (32, 34). Interestingly, the proline-rich region of p125FAK (711APPKPSR717), which interacts with the p130CAS SH3 domain, is almost identical to (703PPPKPSR709) in CADTK, and this may be the basis of CADTK-p130CAS association detected in transfected 293(T) cells (Fig. 10). Whether CADTK directly phosphorylates p130CAS and tensin remains to be determined.
The role of tyrosine phosphorylation of paxillin, p130CAS, and tensin in G protein-coupled receptor-directed signaling is currently unknown. Although no enzymatic activity has been described, paxillin and tensin do form complexes with other cytoskeletal proteins such as vinculin and talin (47, 58). Tyrosine-phosphorylated paxillin, p130CAS, and tensin may also provide binding sites for the SH2 containing proteins such as Crk family members (30, 34, 60, 61). In turn, Crk can associate with a number of proteins through its SH3 domains, such as two guanine nucleotide exchange proteins, C3G and SOS, and a non-receptor tyrosine kinase, Abl (62-64). It will be interesting to see whether CADTK induces paxillin, p130CAS, and tensin tyrosine phosphorylation at sites different than those phosphorylated by p125FAK; if so, CADTK may bring in different SH2 containing proteins and initiate unique signaling pathways.
We thank Ruth Dy, Debra Hunter, and Tim Harding for excellent technical assistance. We particularly thank Dr. Ben Calvo and Evelyn Falls for developing the anti-CADTK antisera. We also thank Drs. Leslie Petch and Michael Schaller for critical reading and helpful discussion. We thank Darla Nichols for manuscript preparation.