From the Department of Molecular Oncology, Genentech, Inc., South San Francisco, California 94080
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ABSTRACT |
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Wiskott-Aldrich syndrome is an X-linked hematopoietic disease that manifests itself in platelet deficiency and a compromised immune system. Analysis of hematopoietic cells from affected individuals reveals that mutations in the Wiskott-Aldrich syndrome protein (WASP) result in structural and functional abnormalities in the cell cortex, consistent with the suggestion that WASP is involved with regulation of the actin-rich cortical cytoskeleton. Here we report that WASP interacts with a recently described cytoskeletal-associated protein, PSTPIP, a molecule that is related to the Schizosaccharomyces pombe cleavage furrow regulatory protein, CDC15p. This association is mediated by an interaction between the PSTPIP SH3 domain and two polyproline-rich regions in WASP. Co-expression of PSTPIP with WASP in vivo results in a loss of WASP-induced actin bundling activity and co-localization of the two proteins, which requires the PSTPIP SH3 domain. Analysis of tyrosine phosphorylation of PSTPIP reveals that two sites are modified in response to v-Src co-transfection or pervanadate incubation. One of these tyrosines is found in the SH3 domain poly-proline recognition site, and mutation of this tyrosine to aspartate or glutamate to mimic this phosphorylation state results in a loss of WASP binding in vitro and a dissolution of co-localization in vivo. In addition, PSTPIP that is tyrosine phosphorylated in the SH3 domain interacts poorly with WASP in vitro. These data suggest that the PSTPIP and WASP interaction is regulated by tyrosine phosphorylation of the PSTPIP SH3 domain, and this binding event may control aspects of the actin cytoskeleton.
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INTRODUCTION |
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PSTPIP is a recently described coiled-coil and SH3 domain-containing protein that is homologous to CDC15p, a Schizosaccharomyces pombe phosphoprotein involved with the assembly of the cytokinetic cleavage furrow (1-3). PSTPIP is associated with protein-tyrosine phosphatase (PTP)1 HSCF, a member of the PEST family of PTPs (4), via a critical tryptophan in the PSTPIP coiled-coil domain (2), and this association mediates the dephosphorylation of tyrosine residues in PSTPIP that are modified either by co-expression of the v-Src tyrosine kinase or in the presence of the PTP inhibitor pervanadate. Throughout interphase, the coiled-coil domain localizes PSTPIP to actin-rich regions of the cell, including the cortical cytoskeleton and lammelipodia, and the protein migrates to the cleavage furrow during cytokinesis. Overexpression of PSTPIP in mammalian cells induces filapodial extension and cell rounding, and induced expression of the mammalian protein in S. pombe results in a dominant negative inhibition of cytokinesis (1). These data suggest that PSTPIP is a tyrosine phosphorylated cytoskeletal regulatory protein that may be involved with the control of cytokinesis.
Wiskott-Aldrich syndrome is an X-linked hematopoietic disease that presents with platelet abnormalities and immunodeficiency (5, 6), and mutations in the Wiskott-Aldrich syndrome protein (WASP) cause this syndrome (7-9). WASP is a multi-domain protein containing pleckstrin homology, CDC42-binding, polyproline, and actin regulatory motifs (7). Hematopoietic cells from Wiskott-Aldrich syndrome patients have abnormalities in their cortical cytoskeletons (6, 10), and overexpression of WASP induces bundling of F actin, which may be regulated by CDC42, a GTPase involved with cytoskeletal modulation (11, 12). A WASP homologue in Saccharomyces cerevisiae is involved with cortical actin assembly and cytokinesis (13, 14). In addition, WASP binds to various tyrosine kinases as well as the Nck and GRB 2 adaptor proteins, suggesting a link with cellular signal transduction pathways (15-19). These data suggest that WASP is a scaffold that mediates the assembly of various signaling and structural components involved with cytoskeletal regulation.
Together, these data suggest the involvement of both PSTPIP and WASP in the control of the cytoskeleton. Here we show a physical interaction between the SH3 domain of PSTPIP and proline-rich regions of WASP. This interaction appears to modulate the actin bundling activity localized to the C terminus of WASP (11). Analysis of the tyrosine phosphorylation of PSTPIP reveals that one of the two phosphotyrosines in this protein is within the polyproline-binding pocket of the SH3 domain, and this modification appears to regulate the binding between PSTPIP and WASP. This study describes a novel mechanism for the modulation of the interaction between two components involved with regulation of the cytoskeleton.
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MATERIALS AND METHODS |
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Two-hybrid Screening-- Yeast two-hybrid screening was performed as described previously (1), Briefly, full-length PSTPIP (1) was cloned in frame with the galactose DNA-binding domain and used as bait to screen a library derived from murine BaF3 hematopoietic progenitor cells. Yeast capable of growing in the absence of histidine were used as sources for plasmid DNA that was isolated by polymerase chain reaction. The resultant fragments were sequence by dye terminator sequencing.
Protein-Protein Interaction Analysis-- Fragments of PSTPIP and WASP were subcloned by either the polymerase chain reaction or by restriction enzyme digestion. These fragments were incorporated either into a plasmid encoding the glutathione S-transferase (GST) protein, the green fluorescent protein (GFP), or an N-terminal ExpressTM epitope tag. The resultant plasmids were transfected into Escherichia coli (GST), COS, or CHO cells (GFP and ExpressTM) and were analyzed as described previously (1, 2). Coprecipitation experiments were performed as described previously (1, 2).
Confocal Microscopy-- Constructs expressing either GFP (WASP) or FLAGTM epitope-tagged (PSTPIP) proteins were co-transfected into CHO cells grown in glass chamber slides as described previously (1, 2). Transfected cells were than stained with either rhodamine phalloidin (for F actin) or Cy-3-labeled anti-FLAGTM (for PSTPIP) and were visualized using laser-scanning confocal microscopy.
PSTPIP Mutagenesis-- Full-length PSTPIP or its SH3 domain was mutagenized by polymerase chain reaction-directed mutagenesis as described previously (1, 2). Tyrosine phosphorylation was analyzed by either co-transfection with a plasmid encoding v-Src or incubation of transfected cells with the tyrosine phosphatase inhibitor pervanadate as described previously (1, 2).
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RESULTS AND DISCUSSION |
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Characterization of the PSTPIP Interaction with WASP-- Screening of a murine BaF3 library using the yeast two-hybrid system with murine PSTPIP as bait resulted in the isolation of a murine homologue of WASP. Analysis of this interaction by yeast two-hybrid assays revealed that the full-length form of PSTPIP interacted in vivo with murine and human WASP, but a form of the protein lacking the SH3 domain did not (data not shown). These results suggested that the SH3 domain of PSTPIP was responsible for the original yeast two-hybrid interaction by recognition of a proline-rich motif in WASP (20-22). To test this hypothesis, full-length and deleted forms of WASP were expressed in COS cells, and the proteins were analyzed for interaction with the SH3 domain of PSTPIP expressed as a GST fusion. As Fig. 1 illustrates, two regions of WASP corresponding to residues 1-321 (WASP 5) and 321-502 (WASP 4) were able to interact with the GST SH3 fusion of PSTPIP, although the full-length protein (WASP FL) containing both of these regions appeared to bind significantly better. The proline-rich regions within WASP 4 and WASP 5 appeared to be required for this interaction, because WASP 1 (deleted for the proline-rich domain) did not interact. The binding sites were mapped to a finer level using oligopeptides derived from each of the proline-rich regions of WASP. Fig. 1 illustrates that two overlapping oligopeptides corresponding to residues 350-384 (peptides j and k) within the second binding site completely blocked the interaction in vitro at relatively low peptide concentrations, whereas another peptide derived from the other binding site (residues 302-325, peptide f) was able to partially inhibit this interaction at higher peptide concentrations. Although both of these regions contain stretches of prolines, Fig. 1 shows that polyproline is able to only weakly inhibit the interaction in vitro at relatively high concentrations. However, short stretches of proline were not alone sufficient to block the interaction, because such regions are found in other WASP-derived peptides tested (Fig. 1). Thus, the interaction between the PSTPIP SH3 domain and WASP is mediated by polyproline-containing regions that differ significantly from previously described SH3 recognition sites.
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Mapping the Phosphorylated Tyrosines in PSTPIP-- PSTPIP was previously shown to be tyrosine phosphorylated in cells either expressing the v-Src tyrosine kinase or incubated with the PTP inhibitor, pervanadate (1). To analyze a possible regulatory role of tyrosine phosphorylation in the interactions between PSTPIP and WASP, each tyrosine in PSTPIP was individually mutated to phenylalanine. The mutants were then analyzed for phosphotyrosine content and mobility shifts by SDS-polyacrylamide gel electrophoresis and immunoblotting with an anti-phosphotyrosine antibody after either co-transfection of v-Src tyrosine kinase or incubation of transfected cells in the presence of pervanadate. Fig. 3 illustrates that mutation of two tyrosines of murine PSTPIP, at positions 344 and 367, to phenylalanine resulted in modifications of PSTPIP tyrosine phosphorylation in both v-Src-transfected and pervanadate-treated cells, whereas mutation of the other tyrosines to phenylalanine showed no change in banding patterns or phosphotyrosine content (data not shown). Mutation of tyrosine residue 367 alone resulted in the disappearance of the slower migrating phosphotyrosine forms of PSTPIP under both phosphorylation conditions, suggesting that the slower migrating bands are due to phosphorylation of tyrosine 367. Mutation of tyrosine 344 alone resulted in a complete loss of phosophotyrosine in the protein (Fig. 3). This result implied that phosphorylation of tyrosine 344 was required for the subsequent phosphorylation of tyrosine residue 367. In addition, the data imply that the residual single tyrosine phosphorylated band in the form of PSTPIP mutated at position 367 is due to tyrosine residue 344, whereas the more slowly migrating forms are due to phosphorylation at both the 344 and 367 positions. Examination of the sequence surrounding tyrosine 344 revealed that it is a significant consensus site for modification by Src family member tyrosine kinases (23),2 consistent with the possibility that tyrosine residue 344 is directly phosphorylated by either transfected v-Src or by an endogenous Src family tyrosine kinase that is activated by pervanadate treatment. Tyrosine residue 367 is within the polyproline recognition site of the SH3 domain of PSTPIP (20-22), and structure-function analyses of the SH3 domains in several other proteins has shown that this tyrosine is involved with binding of the proline-rich ligand. These data thus suggest that PSTPIP is sequentially phosphorylated, first at residue 344 by a Src family member tyrosine kinase and subsequently at a tyrosine within the SH3 polyproline-binding site.
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Modification of Tyr367 Modulates the PSTPIP Interaction with WASP-- The above data suggested that binding of PSTPIP to WASP might be regulated by phosphorylation of tyrosine 367 in the PSTPIP SH3 domain, because this residue is found within the polyproline-binding pocket (20-22). To test this possibility, tyrosine 367 was mutated to either an aspartate or a glutamate to mimic the incorporation of the negatively charged phosphate group at this position. Structural analysis of other SH3 domains (20-22) suggests that this tyrosine is solvent exposed and does not interact with other residues, suggesting that these mutations should not globally affect the structure of the PSTPIP SH3 domain. GST fusion proteins containing these mutations were tested for their ability to interact with WASP in an in vitro binding assay. In addition, a GST fusion containing the second proline-rich PSTPIP-binding site of WASP (residues 357-443) was also tested for its ability to bind to mutated forms of PSTPIP. As Fig. 4 illustrates, neither the two mutants containing acidic residues at the tyrosine 367 position nor the form of PSTPIP missing the SH3 domain were able to interact strongly with WASP, whereas both the wild type SH3 motif as well as an SH3 domain with phenylalanine substituted at position 367 were bound to WASP, suggesting that the incorporation of an acidic side chain at this site negatively regulates the interaction between PSTPIP and WASP. This result suggests that the incorporation of a negatively charged phosphate at position 367 would inhibit PSTPIP-WASP binding and that the SH3 domain interacts with WASP as predicted from previous structure-function studies (20-22). To examine the effects of these mutations in vivo, co-transfection experiments were performed in conjunction with confocal microscopy. Fig. 4 illustrates that although wild type PSTPIP was able to co-localize with WASP in vivo, PSTPIP with either the aspartate or glutamate mutations at position 367 showed the same lack of co-localized staining as was found for the form of the protein that was lacking the SH3 domain (Fig. 2). Finally, Fig. 4 illustrates that a GST fusion protein containing the second proline-rich PSTPIP-binding site of WASP is able to interact only with the more rapidly migrating tyrosine phosphorylated form of PSTPIP corresponding to tyrosine 344 and does not precipitate the slower migrating bands corresponding to PSTPIP tyrosine phosphorylated at both positions 344 and 367. These data suggest that phosphorylation of tyrosine 367 in the SH3 domain of PSTPIP modulates the interaction between this cytoskeletal-associated protein and WASP.
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ACKNOWLEDGEMENTS |
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We thank Dr. K. Siminovitch for graciously making results about WASP-PSTPIP interactions available before publication and for the human WASP cDNA clone. We also thank Dr. Clifford Quan for peptide synthesis, Dr. Wenlu Li for help with confocal microscopy, and Lorraine Sarullo for help with figures. We also thank Dr. Emma Lasky for fruitful discussions during the course of this project.
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FOOTNOTES |
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* The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
To whom correspondence should be addressed: Dept. of Molecular
Oncology, Genentech, Inc., 460 Pt. San Bruno Blvd., South San Francisco, CA 94080. Tel.: 650-225-1123; Fax: 650-225-6127; E-mail: lal{at}gene.com.
1 The abbreviations used are: PTP, protein-tyrosine phosphatase; WASP, Wiskott-Aldrich syndrome protein; GST, glutathione S-transferase; GFP, green fluorescent protein; CHO, Chinese hamster ovary; BTK, Bruton's tyrosine kinase; aa, amino acids; HSCF, hematopoietic stem cell fraction.
2 L. Cantley, personnel communication.
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REFERENCES |
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