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HEMOSTASIS, THROMBOSIS, AND VASCULAR BIOLOGY
From the Department of Pharmacology, University of
Oxford, United Kingdom; the National Institute for Medical Research,
London, United Kingdom; and the Lymphocyte Signaling and Development
Laboratory, Molecular Immunology Programme, The Babraham Institute,
Cambridge, United Kingdom.
We have investigated the role of the Rho and Rac family
small guanine triphosphate (GTP) exchange factors (RhoGEFs),
Vav1 and Vav2, in the activation of platelets by the immunoreceptor tyrosine-based activation motif (ITAM)-coupled collagen receptor GPVI and by the G protein-coupled receptor agonist thrombin.
The glycoprotein VI (GPVI)-specific agonist collagen-related peptide (CRP) and thrombin stimulated tyrosine phosphorylation of Vav1 but not
Vav2 in human platelets. Surprisingly, however, CRP did not activate
the low-molecular-weight G protein Rac and stimulated only a
small increase in activity of p21-associated kinase 2 (PAK2), despite
the fact that both proteins are regulated downstream of Vav1 in other
cells. Further, activation of Rac and PAK2 by thrombin was maintained
in platelets from mice deficient in Vav1. Activation of phospholipase C
(PLC) by GPVI and thrombin was unaltered in Vav1-, Vav2-, and
Vav1/Vav2-deficient platelets. A weak inhibition of late-stage
aggregation to CRP and thrombin was observed in platelets deficient in
Vav1 but not Vav2, whereas spreading on fibrinogen was not changed. The
present results demonstrate that neither Vav1 nor Vav2 lie upstream of
PLC or Rac in platelets, highlighting an important difference in their
role in signaling by ITAM-coupled receptors in other cell types. The
present study has provided evidence for a possible role of Vav1 but not
Vav2 in the later stages of platelet aggregation.
(Blood. 2002;100:3561-3569) Vav proteins are GTP exchange factors for
members of the Rho family of low-molecular-weight G
proteins. In addition, they are involved in the regulation of
phospholipase C (PLC) by a number of immunoreceptor tyrosine-based
activation motif (ITAM)-coupled receptors. There are 3 members of the
Vav family, all of which share a common structural arrangement. At the
amino termini is a calponin homology domain, followed by an acidic
region, a Dbl homology (DH) domain, a pleckstrin homology (PH) domain,
a zinc finger (ZF) domain, a short proline-rich region, and a
C-terminal SH3-SH2-SH3 region. Vav proteins are also tyrosine
phosphorylated by Src and Syk family kinases and associate with many of
the membrane proximal molecules in ITAM-dependent signaling cascades,
including Syk and Zap70, SLP-76, Grb2, Nck, and the p85 subunit of
phosphatidylinositol 3-kinase (PI 3-K) (reviewed in
Bustelo1). Vav1 is specifically expressed in hematopoietic
cells, whereas Vav22,3 and Vav34 show a broader
profile of expression.
The DH, PH, and ZF domains form the guanine diphosphate
(GDP)-GTP exchange factor region of Vav-family proteins with the DH domain containing the active site enabling activation of the Rho family
of small G proteins. Rho proteins regulate critical changes in the
cytoskeleton and participate in events such as lymphocyte development.5,6 Vav1 has been shown to selectively
activate Rac1, Rac2, RhoG, and to a lesser extent RhoA. A majority of
studies indicate that Cdc42 is not a good substrate for
Vav1.1 3-Phosphoinositides and tyrosine phosphorylation of
Vav1 have been shown to stimulate GTP-GDP exchange activity of
Vav1.1,7 Vav2 and Vav3 also activate RhoA and RhoG but
show less activity towards Rac1.4,8 The activity of these
2 members of the Vav family is also modulated by tyrosine
phosphorylation.4,8
Insights into the role of Vav proteins have come from studying mice
engineered to lack these proteins. T-cell development and proliferation
are retarded in Vav1-deficient mice. Vav1 Vav1 undergoes an increase in tyrosine phosphorylation in platelet
suspensions challenged with thrombin and collagen but not in response
to the thromboxane mimetic U46619 and adenosine diphosphate
(ADP).15 In addition, platelet adhesion via the platelet
integrin GPIIb-IIIa ( Collagen activates platelets through a tyrosine kinase-dependent
pathway via the receptor complex GPVI and Fc receptor (FcR) In view of the similarities between the signaling events downstream of
the T-cell and B-cell antigen receptors and those downstream of GPVI,
we have analyzed the roles of Vav1 and Vav2 in GPVI signaling in
platelets. Experiments were performed alongside the G protein-coupled receptor agonist thrombin in order to examine whether defects were
specific to GPVI. Activation of PLC Reagents
The generation of mice disrupted in the Vav1 gene
(Vav1 Platelet preparation, stimulation, and aggregation
Immunoblotting and immunoprecipitation Platelets were lysed with an equal volume of lysis buffer (2% NP-40, 300 mM NaCl, 20 mM Tris, 10 mM ethylenediaminetetraacetic acid [EDTA], 2 mM Na3VO4, 1 mM phenylmethylsulfonyl fluoride, 10 µg/mL leupeptin, 10 µg/mL aprotinin, and 1 µg/mL pepstatin A, pH 7.4). Insoluble cell debris were removed by centrifugation for 5 minutes at 13000 rpm, 4°C, and cell lysates were precleared using protein A-Sepharose. Platelet lysates were incubated with the following antibodies: Vav1, Vav2, PLC 2, and PAK2. Resulting protein complexes and immunoprecipitates
were resolved by sodium dodecyl sulfate-polyacrylamide gel
electrophoresis (SDS-PAGE) and transferred to polyvinylidene difluoride
(PVDF) membranes. Immunoblotting was performed as described
previously25 with detection by enhanced chemiluminescence
(ECL; Amersham Biosciences, Bucks, United Kingdom).
Measurement of phosphatidic acid levels and pleckstrin phosphorylation Platelets were resuspended in modified Tyrodes without phosphate and incubated with [32P]orthophosphate (0.5 mCi/mL [18.5 MBq/mL]) for 1 hour at 37°C, washed, and activated as described above. An aliquot of each reaction was suspended in Laemmli buffer for measurement of pleckstrin phosphorylation by SDS-PAGE and subsequent autoradiography of the dried gel. The remaining reaction was stopped by the addition of one volume chloroform-methanol-HCl (100/200/1 vol/vol/vol), phospholipids extracted, and [32P]phosphatidic acid separated by thin layer chromatography and analyzed by subsequent autoradiography.39Analysis of platelets by scanning electron microscopy The analysis of platelets by scanning electron microscopy was carried out as described previously.40 Briefly, platelets were resuspended in modified Tyrodes, stimulated as described above for 60 seconds, and then mixed with an equal volume of 4% gluteraldehyde/phosphate-buffered saline (PBS), pH 7.4. Platelets were collected with gentle suction onto 0.6-µm polycarbonate filters (Whatman, Maidstone, United Kingdom). Filters were then washed, sequentially dehydrated with ethanol, subjected to critical point drying and gold coating, and then analyzed on a Philips 515 scanner (FEI UK, Cambridge, United Kingdom).Platelet adhesion studies The ability of mouse platelets to spread on fibrinogen was assessed as follows. Glass coverslips were coated with fibrinogen (400 µL of 100 µg/mL solution) for 1 hour at 37°C, followed by washing with PBS. Mouse platelets in modified Tyrodes (400 µL of 1 × 108 platelets/mL) were transferred to the coverslips. The coverslips were incubated at 37°C for 1 hour in a humid atmosphere, then washed gently with PBS and the attached platelets fixed with 3.7% formaldehyde (10 minutes, RT). After washing with PBS, the cells were permeabilized with 0.2% Triton X-100 (10 minutes, RT), washed, and F-actin-labeled with rhodamine phalloidin for 1 hour at room temperature. The coverslips were washed in PBS, mounted using Immuno Fluore Mounting Medium (ICN Biomedicals, Aurora, CA), and viewed in an inverted microscope (Axiovert S100; Carl Zeiss, Herts, United Kingdom) under a 100 × oil immersion lens using Openlab software (Improvision, Warwick, United Kingdom).Measurement of Rac and PAK2 activity Rac activity was measured essentially as described in Benard et al34 using the CRIB domain of PAK1 (amino acids 67-150), which binds the GTP-bound form of Rac. Reactions were stopped with an equal volume of 2 × lysis buffer (2% [vol/vol] NP-40, 2% [wt/vol] N-octyl glucoside, 300 mM NaCl, 20 mM Tris/HCl, 2 mM EGTA, 20 mM MgCl2, 1 mM phenylmethylsulfonyl fluoride, 10 µg/mL leupeptin, 10 µg/mL aprotinin, and 1 µg/mL pepstatin A; pH 7.4). Insoluble material was removed by centrifugation (5 minutes, 13000 rpm, 4°C), freshly prepared GST-PAK1 previously incubated with glutathione agarose was added and the samples incubated for 1 hour at 4°C. The beads were then washed with 1 × Rac assay lysis buffer and the bound protein taken up into Laemmli buffer. The resulting samples were separated by 12% SDS-PAGE and transferred to PVDF membranes for immunoblotting as described above. PAK2 activity was measured using an in-gel kinase technique as described in Borsch-Haubold et al41 with myelin basic protein (MBP) as the substrate.Measurement of F-actin levels The level of F-actin was measured as previously described.42 Basal or activated platelets (2 × 108/mL) were fixed with an equal volume of 3.6% formaldehyde-PBS at 37°C for 45 minutes. Fixed cells were permeabilized and stained with 0.1 volume 1% Triton X-100 containing 10 µM FITC-phalloidin at 25°C for 60 minutes. Platelets were gated by forward and side scatter in a flow cytometer and mean fluorescence of 10 000 cells quantitated per sample.Analysis of data Experiments were carried out on at least 3 occasions and are shown as representative data from one experiment. Where applicable, results are shown as mean plus SEM.
Vav1 is tyrosine-phosphorylated downstream of GPVI. Tyrosine
phosphorylation of Vav1 has been shown to be critical for its GTP
exchange function and to support its association with a number of
signaling proteins. Vav1 undergoes rapid tyrosine phosphorylation in
human platelets in response to the GPVI-specific agonist CRP that peaks
by 30 seconds and is sustained for at least 180 seconds (Figure
1A and not shown). In comparison, the G
protein-coupled receptor agonist thrombin stimulated a weaker increase
in tyrosine phosphorylation in human platelets but with a similar time
course (Figure 1B). Importantly, these studies were performed under
conditions that prevented the binding of fibrinogen to GPIIb-IIIa and
the action of the secondary mediators, ADP and thromboxanes,
demonstrating that the increase in phosphorylation was the direct
consequence of receptor activation. Tyrosine phosphorylation of Vav1 by
CRP was not significantly altered in the presence of the inhibitors wortmannin and Ly294002 but was abolished by the Src kinase inhibitor PP1 (Figure 1C). Similar results were observed for thrombin (not shown).
CRP also stimulated tyrosine phosphorylation of Vav1 in murine platelets (Figure 1D). In contrast, thrombin did not stimulate a significant increase in tyrosine phosphorylation of Vav1 in mouse platelets (Figure 1D). Phosphorylation of Vav1 by CRP was abolished in Syk-deficient platelets (Figure 1D). Role of Vav1 in platelet functional responses induced by GPVI To assess the role of Vav1 in platelets, we analyzed responses of platelets from mice carrying a mutation disrupting the Vav1 gene resulting in no Vav1 production.36 The number of platelets, red cells, and leukocytes in whole blood from Vav1-deficient mice is no different than wild type (Table 1). Bleeding problems, such as the intraperitoneal hemorrhage seen in Syk- and SLP-76-deficient mice, were not observed.
The role of Vav1 in the activation of PLC by CRP and thrombin was
analyzed by measuring formation of [32P]phosphatidic acid
and [32P]phosphorylation of pleckstrin, a substrate for
protein kinase C. There was no significant difference in the level of
[32P]phosphatidic acid or
[32P]phosphorylation of pleckstrin between
Vav1
A possible role of Vav1 in response to CRP and thrombin was
investigated by monitoring shape change, the earliest response that
takes place upon platelet activation. Shape change induced by CRP is
entirely dependent on the elevation of intracellular Ca++
in the presence of inhibitors of the action of thromboxanes and ADP.43 In contrast, shape change induced by thrombin is
mediated through a combination of Ca++- and rho-activated
pathways.43,44 The magnitude and time course of shape
change to low and high concentrations of thrombin and CRP was
maintained in the Vav1-deficient platelets (Figure
3A) as measured by an increase in optical
density. To confirm these observations, we performed scanning electron
microscopy of Vav1
In contrast to the above, aggregation of Vav1
Spreading on fibrinogen is not altered in
Vav1
Regulation of Rac and PAK2 activity in platelets Vav1 has been shown to lie upstream of the low-molecular-weight G protein Rac and the low-molecular-weight G protein-activated serine-threonine kinase PAK2 in a number of cell types. Importantly, both proteins are implicated in regulating actin polymerization in platelets and other cell types,17,18,45 an event that may contribute to the reduction in aggregation observed in Vav1-deficient platelets. To address this, we have investigated the role of Vav1 in the regulation of Rac and PAK2 and actin polymerization in platelets.Rac activity was assessed using a method based on that of Benard et
al34 utilizing a GST fusion protein incorporating the CRIB
domain of PAK1 to bind GTP-Rac but not GDP-Rac. We confirmed the
specificity of this assay by showing that the fusion protein bound to a
constitutively active, GTP-bound form of Rac (L61 Rac) expressed in Hel
cells but not to the endogenous, inactive Rac present within the cells
(not shown). CRP and the stronger GPVI agonist, the snake venom toxin
convulxin, did not cause a detectable activation of Rac (Figure
6A-B). By contrast, thrombin caused a
rapid and sustained level of activation of Rac with maximal activity
reached within 30 seconds (Figure 6A). Importantly, these experiments
were carried out in the presence of apyrase and indomethacin to block
the effects of the G protein-coupled secondary mediators ADP and
thromboxanes. In the absence of these inhibitors, CRP stimulates Rac
activation (Figure 6B). Thrombin-induced Rac activity was not blocked
by the PI 3-K inhibitors, wortmannin and Ly294002, or the Src kinase
inhibitor PP1 (Figure 6C).
We analyzed PAK2 activity by means of an in-gel kinase assay with MBP incorporated into the gel. Treatment of platelets with CRP resulted in weak activation of PAK2 at 90 seconds and stronger activation at 180 seconds (Figure 6D). Thrombin caused a more rapid and higher degree of PAK2 activation, which peaked at 90 seconds (Figure 6D). Activation of PAK2 by thrombin was weakly inhibited by PP1 and more strongly reduced by the PI 3-K inhibitors wortmannin and Ly294002 (Figure 6E). Activation of PAK2 by CRP was abolished by PP1 and wortmannin (Figure 6E). Vav1 These results demonstrate that Vav1 does not lie upstream of sequential
activation of Rac and PAK2 by thrombin and CRP. CRP does not stimulate
activation of Rac, whereas robust activation of Rac and PAK2 by
thrombin is largely maintained in Vav1 Actin polymerization was measured in platelets using a FACS-based assay
in which FITC-conjugated phalloidin binds to F-actin in fixed,
permeabilized platelets.42 CRP- and thrombin-induced formation of F-actin was not altered in Vav1
Vav2 is not activated in human platelets In consideration of recent reports showing that Vav1 and Vav2 play redundant roles in signaling by the B-cell receptor, we extended the present study to analyze Vav2 function in platelets. The presence of a low level of Vav2 in platelets was shown by immunoprecipitation from lysates and Western blotting (Figure 8A, lower panel, and not shown). K562 cells served as a positive control for these studies (not shown). Western blotting with an antiphosphotyrosine antibody demonstrated that Vav2 is not tyrosine phosphorylated in platelets in response to CRP or thrombin (Figure 8A, top panel). Because tyrosine phosphorylation of Vav2 has been shown to be critical for its RhoGEF activity,8 these results suggest that platelet activation does not lead to activation of Vav2.
In order to investigate the role of Vav2 in GPVI and thrombin receptor
signaling, we used platelets from mice deficient in Vav2 as well as
Vav1 The stimulation of shape change and aggregation by CRP and
thrombin was not altered in Vav2
The primary aim of this study was to investigate the role of Vav1
and Vav2 in transducing signals from the platelet collagen receptor
GPVI, with particular emphasis on the regulation of PLC The phosphorylation of Vav1 by Syk and its association with SLP-76
further suggested a role for Vav1 in GPVI signaling.28 However, neither tyrosine phosphorylation of PLC The lack of a role for Vav1 and Vav2 in the regulation of PLC The observation that GPVI stimulation does not lead to activation of
Rac was unexpected, especially in light of 2 recent reports describing
the activation of the low-molecular-weight G protein by
collagen in platelets.20,48 The likely explanation for
this apparent discrepancy is the role of secondary mediators ADP and thromboxanes in the activation of Rac downstream of GPVI. In the study
by Soulet et al,20 inhibitors of thromboxanes and ADP were
not used, and in the study by Suzuki-Inoue et al,48 an inhibitor of ADP was not used. It is therefore likely that the stimulation of Rac by collagen in these 2 studies was mediated downstream of thromboxanes and/or ADP. The demonstration of robust activation of Rac by thrombin in the present study confirms the ability
of G protein-coupled receptors to activate Rac in platelets, as
originally reported by Azim et al,19 and serves as a
positive control for the absence of a response to CRP under the same
conditions of secondary mediator blockade. Moreover, we also
demonstrate that Rac is activated following CRP stimulation in the
absence of blockers of ADP and thromboxanes. An alternative
explanation, however, for the apparent differences between this study
and those by Suzuki-Inoue et al and Soulet et al is the possible
regulation of Rac by collagen downstream of Interestingly, platelets from Vav1-deficient mice were found to have a weak impairment in aggregation to CRP and thrombin, which was delayed in onset. Vav1/Vav2-deficient platelets display the same defect, whereas aggregation of Vav2-deficient platelets to CRP and thrombin is identical to wild-type platelets. Potentially, this could be explained by a role of Vav1 in inside-out regulation of GPIIb-IIIa or a role in outside-in signaling by the integrin. There is substantial evidence for a role of Vav1 in outside-in signaling downstream of GPIIb-IIIa. Vav1 undergoes tyrosine phosphorylation upon platelet adhesion to fibrinogen.15,16 Studies in A5 CHO cells, which stably express GPIIb-IIIa, have shown that Vav1 is regulated downstream of Src and Syk tyrosine kinases and lies upstream of Rac activation and formation of lamellapodia.17,18 Surprisingly, there was no discernable difference in the spreading of wild-type, Vav1-, and Vav1/Vav2-deficient platelets on fibrinogen. It is conceivable that this might reflect a redundant role for Vav3 in this system which has recently been shown to undergo tyrosine phosphorylation following platelet adhesion to fibrinogen.16 On the other hand, the limited degree of lamellapodia formation may reflect limited activation of the Rho family proteins in platelets spread on fibrinogen in the presence of inhibitors of ADP and thromboxanes. In conclusion, we have demonstrated that neither Vav1 nor Vav2 participates in the regulation of PLC downstream of the ITAM-coupled collagen receptor GPVI, thereby demonstrating a novel difference with respect to most other ITAM-coupled receptors. Further, we have provided evidence for a role of Vav1 but not Vav2 in the late stages of platelet aggregation, although the mechanism of this event is unclear. The surprisingly mild nature of the phenotype of Vav1/Vav2-deficient platelets with regard to signaling through GPVI and GPIIb-IIIa might reflect an important role for Vav3. Experiments on mice deficient in this member of the Vav family are of considerable interest.
We would like to thank Peter Wonerow for critical evaluation of this manuscript and Jenny Corrigan (Department of Zoology, University of Oxford) for assistance with the scanning electron microscopy.
Submitted October 2, 2001; accepted June 24, 2002.
Supported by the Wellcome Trust and the British Heart Foundation (S.P.W.), the Biotechnology and Biological Sciences Research Council (M.T.), and the Medical Research Council (V.L.J.T.). A.C.P. is a Wellcome Trust Prize student.
A.C.P. and J.I.W. contributed equally to this work.
The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked "advertisement" in accordance with 18 U.S.C. section 1734.
Reprints: Andrew C. Pearce, Department of Pharmacology, University of Oxford, Oxford, OX1 3QT, United Kingdom; e-mail: andrew.pearce{at}spc.ox.ac.uk.
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  R. A. Bartolome, I. Molina-Ortiz, R. Samaniego, P. Sanchez-Mateos, X. R. Bustelo, and J. Teixido Activation of Vav/Rho GTPase Signaling by CXCL12 Controls Membrane-Type Matrix Metalloproteinase-Dependent Melanoma Cell Invasion Cancer Res., January 1, 2006; 66(1): 248 - 258. [Abstract] [Full Text] [PDF]
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T. Kawakatsu, H. Ogita, T. Fukuhara, T. Fukuyama, Y. Minami, K. Shimizu, and Y. Takai Vav2 as a Rac-GDP/GTP Exchange Factor Responsible for the Nectin-induced, c-Src- and Cdc42-mediated Activation of Rac J. Biol. Chem., February 11, 2005; 280(6): 4940 - 4947. [Abstract] [Full Text] [PDF]
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A. C. Pearce, Y. A. Senis, D. D. Billadeau, M. Turner, S. P. Watson, and E. Vigorito Vav1 and Vav3 Have Critical but Redundant Roles in Mediating Platelet Activation by Collagen J. Biol. Chem., December 24, 2004; 279(52): 53955 - 53962. [Abstract] [Full Text] [PDF]
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M. L. Jones, J. D. Craik, J. M. Gibbins, and A. W. Poole Regulation of SHP-1 Tyrosine Phosphatase in Human Platelets by Serine Phosphorylation at Its C Terminus J. Biol. Chem., September 24, 2004; 279(39): 40475 - 40483. [Abstract] [Full Text] [PDF]
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Top
Abstract
Introduction
/
IIb
3) to fibrinogen
leads to a strong increase in Vav1 phosphorylation.
