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© The Rockefeller University Press, 0021-9525/1997//387 $5.00
The Journal of Cell Biology, Volume 137, Number 2, , 1997 387-398

Regulated Membrane Localization of Tiam1, Mediated by the NH₂-terminal Pleckstrin Homology Domain, Is Required for Rac-dependent Membrane Ruffling and C-Jun NH₂-terminal Kinase Activation

The Netherlands Cancer Institute, Antoni van Leeuwenhoekhuis, Division of Cell Biology, 1066 CX Amsterdam, The Netherlands

Rho-like GTPases, including Cdc42, Rac, and Rho, regulate signaling pathways that control actin cytoskeletal structures and transcriptional activation. The Tiam1 gene encodes an activator of Rac1, and similarly to constitutively activated (V12)Rac1, overexpression of Tiam1 in fibroblasts induces the formation of membrane ruffles. Tiam1 contains a Dbl homology (DH) domain and adjacent pleckstrin homology (PH) domain, hallmarks for activators of Rho-like GTPases. Unique for Tiam1 are an additional PH domain and a Discs-large homology region in the NH₂-terminal part of the protein. Here we show that both in fibroblasts and COS cells, membrane localization of Tiam1 is required for the induction of membrane ruffling. A detailed mutational analysis, in combination with confocal laser scanning microscopy and immunoelectron microscopy, demonstrates that the NH₂-terminal PH domain of Tiam1, but not the DH-adjacent PH domain, is essential for membrane association. This NH₂-terminal PH domain of Tiam1 can be functionally replaced by the myristoylated membrane localization domain of c-Src, indicating that the primary function of this PH domain is to localize the protein at the membrane. After serum starvation, both membrane association of Tiam1 and ruffling can be induced by serum, suggesting that receptor stimulation induces membrane translocation of Tiam1. Similar to V12Rac1, Tiam1 stimulates the activity of the c-Jun NH₂-terminal kinase (JNK). This Rac-dependent stimulation of JNK also requires membrane association of Tiam1. We conclude that the regulated membrane localization of Tiam1 through its NH₂-terminal PH domain determines the activation of distinct Rac-mediated signaling pathways.

Rho-like GTPases, which include Cdc42, Rac1, and RhoA, control distinct signal transduction pathways that determine the organization of the actin cytoskeleton in response to various extracellular stimuli. In fibroblast cells, activation of Cdc42 and Rac results in the formation of focal complexes and filopodia or lamellipodia, respectively, while Rho is involved in the formation of stress fibers and focal contacts (Ridley and Hall, 1992; Ridley et al., 1992; Kozma et al., 1995; Nobes and Hall, 1995a). Each of these GTPases can be activated by specific growth factors, and they may also constitute a hierarchical signaling cascade (Kozma et al., 1995; Nobes and Hall, 1995a). The resulting cytoskeletal rearrangements influence both adhesion and motility of cells, implicating Rholike GTPases as key regulators of these processes (Nobes and Hall, 1995b).

Apart from their effects on the cytoskeleton, both Cdc42 and Rac1 can activate the c-Jun NH₂-terminal kinase (JNK)¹ pathway, while all three Rho-like GTPases activate serum response factor (Coso et al., 1995; Hill et al., 1995; Minden et al., 1995; Olson et al., 1995). Rho-like proteins thus may also play a role in transcriptional activation of genes. Moreover, both Rac1 and RhoA are involved in the transformation of cells by Ras (Khosravi-Far et al., 1995; Qiu et al., 1995a,b), and constitutively active mutants of Rac1 (V12Rac1) and RhoA (V14RhoA) can induce an oncogenic phenotype in NIH3T3 cells (Perona et al., 1993; Qiu et al., 1995a; Van Leeuwen et al., 1995).

Rho-like GTPases are activated by guanine nucleotide dissociation stimulators (GDSs), also known as guanine nucleotide exchange factors. Inactivation occurs by hydrolysis of bound GTP, which is stimulated by interaction with GTPase activating proteins, while guanine nucleotide dissociation inhibitors (GDIs) lock the GTPases either in the active or in the inactive state (Boguski and McCormick, 1993). The role of these regulators in the diverse signaling pathways mediated by Rho-like proteins is largely unknown.

Tiam1 was originally identified in T-lymphoma cells as an invasion- and metastasis-inducing gene (Habets et al., 1994). The predicted Tiam1 protein consists of 1,591 amino acids and contains a Dbl homology (DH) domain. This domain is present in GDS proteins for Rho-like GTPases and is considered to be the catalytic domain (Hart et al., 1994). DH domains are found in a rapidly expanding group of proteins, many of which are encoded by transforming genes that were identified after transfection of genomic DNA or cDNA libraries into NIH3T3 cells (Cerione and Zheng, 1996; Collard, 1996). A number of these proteins, like Dbl, Ost, Cdc24, Lbc, and Vav were shown to activate Rho-like GTPases (Hart et al., 1991; Horii et al., 1994; Zheng et al., 1994, 1995; Olson et al., 1996). Tiam1 is the only GDS protein identified that specifically activates Rac in vitro as well as in vivo (Michiels et al., 1995). In fibroblasts, Tiam1 induces the formation of membrane ruffles, similarly to constitutively activated V12Rac1 (Michiels et al., 1995). The Tiam1-induced phenotype is inhibited by coexpression of dominant-negative mutant (N17)Rac1, but not by coexpression of (N17)Cdc42 or by inactivation of RhoA with C3 transferase (Michiels et al., 1995; Collard, 1996). This indicates that the Tiam1-induced membrane ruffling is primarily caused by activation of Rac and that other Rho-like GTPases are not involved. Moreover, V12Rac1, but not V14RhoA, induces an invasive phenotype in T-lymphoma cells, similar to Tiam1, suggesting that Tiam1-induced invasiveness is also caused by activation of Rac (Michiels et al., 1995).

Apart from the DH domain, Tiam1 contains several other conserved motifs, including a consensus myristoylation sequence at the NH₂ terminus, a Discs-large homology region (DHR), and two pleckstrin homology (PH) domains (Habets et al., 1994; Collard, 1996; see Fig. 1 A). One of the PH domains is present COOH-terminally adjacent to the DH domain, as found in all other GDS proteins for Rho-like GTPases (Collard, 1996), while a second PH domain is located in the NH₂-terminal part of Tiam1. DHR domains have been implicated as protein–protein interaction motifs (Ponting and Phillips, 1995). PH domains, primarily found in signaling molecules, are thought to determine the cellular localization and/or activity of these proteins by interacting with proteins or phospholipids (for review see Lemmon et al., 1996).

View larger version (55K): [in this window] [in a new window] [Download PPT slide]   Figure 1 Confocal images of NIH3T3 cells expressing truncated Tiam1 proteins. A depicts the Tiam1 constructs encoding the COOH-terminal 1,199 amino acids (C1199) or 682 amino acids (C682) that were used for transfection of NIH3T3 cells, in comparison to the full-length Tiam1 protein (FL1591). Established cell lines that express the C1199 Tiam1 protein (B) or the C682 Tiam1 protein (C) were fixed and stained with anti-Tiam1 antibodies (Habets et al., 1994), followed by FITC-coupled secondary antibodies (left) and by TRITC-labeled phalloidin for F-actin (right). Note the prominent membrane ruffling in cells that express the C1199 Tiam1 protein. Stress fibers are hardly visible in these cells, since the optical sections were made through the upper half of the cells to reveal the presence or absence of membrane ruffling. No significant differences were found in the amount or appearance of stress fibers between Tiam1-expressing cells and controls. M, myristoylation signal; P, PEST regions; PHn and PHc, NH2-terminal and COOH-terminal pleckstrin homology domains. Magnification is 250x. Bar, 40 µm.

	Materials and Methods

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Transfection Constructs
Full-length mouse Tiam1 (FL1591) and the NH₂-terminally truncated C1199 and C580 Tiam1 constructs (nomenclature refers to the number of COOH-terminal amino acids [aa] of the encoded Tiam1 proteins) contain artificial SpeI and SalI restriction sites in front of the first ATG and a hemagglutinin tag (HA-tag), followed by a SalI restriction site, at their 3' ends. They were cloned as SpeI-SalI fragments into the eukaryotic expression vector pUTSV1 (Eurogentec S.A., Belgium), which was linearized by SpeIXhoI. C1199-PHc carries a small internal PstI (aa 1377) to BsmI (aa 1390) deletion in the conserved COOH-terminal part of the DH-adjacent PH domain. C1199-DH1 carries a BamHI (aa 1103) to XbaI (aa 1130) deletion in a nonconserved part of the DH domain. C1199-DHR carries a large NotI (aa 853) to Asp718 (aa 905) deletion in the DHR region that eliminates most of the DHR region. C1199-PHn carries a small internal Asp700 (aa 513) to EarI (aa 528) deletion in the conserved COOH-terminal part of the NH₂-terminal PH domain, which is quite similar to the deletion made in the COOH-terminal PH domain (C1199-PHc). Overhangs were blunted by either Klenow end filling reactions ( Boehringer Mannheim Corp., Indianapolis, IN) or with T4 DNA polymerase ( Boehringer Mannheim Corp.) before ligation. The myristoylation sequence of c-Src, encoding the NH₂-terminal 20 amino acids, was amplified with SpeISalI adaptors by PCR with Pfu polymerase (Stratagene, La Jolla, CA) and cloned between the SpeI and SalI sites at the 5' ends of the FL1591-PHn, C1191-PHn, and C580 Tiam1 constructs. Fragments containing the COOHterminal PH domain of Tiam1, the PH domain of Dbl, or the PH domain of β-Ark were amplified by PCR with SmaI and PvuII adapters and used to replace the region containing the NH₂-terminal PH domain of Tiam1 in the C1199 construct. The exchanged regions contain 17 additional aa at the NH₂-terminal end and 36 additional aa (33 aa for β-Ark) at the COOHterminal end, in comparison to the consensus PH domain (Gibson et al., 1994). To analyze whether the NH₂-terminal PH domain is sufficient for membrane targeting, a region containing the NH₂-terminal PH domain, from SalI (aa 393) to BstX1 (aa 647), was fused to the Bsu36I site (aa 1022) at the NH₂ terminus of the C580 Tiam1 protein. All amplified fragments were sequenced with the T7 polymerase sequencing kit ( Pharmacia LKB Biotechnology Inc., Uppsala, Sweden).

Cells and Transfection Experiments
NIH3T3 cells, stably expressing the C1199 Tiam1 protein and C682 Tiam1 protein, have been described previously (Van Leeuwen et al., 1995). NIH3T3 cells and COS-7 cells were cultured in a humidified CO₂ incubator in DME supplemented with 10% newborn calf serum or 10% fetal calf serum, respectively. For transient expression assays, NIH3T3 cells were seeded in dishes with or without coverslips (8,000 cells/cm²). 18 h after seeding, cells were transfected with lipofectamin (Life Technologies, Inc., Grand Island, NY). COS-7 cells were seeded in dishes with or without coverslips and transfected using DEAE dextran (Seed and Aruffo, 1987). 16 h after transfection, the medium was either replaced and cells were incubated for an additional 30 h before washing and fixation, or cells were incubated for 24 h in serum-free medium, followed by the addition of serum for 2 h. Western blot analyses were performed to monitor the size and expression levels of the mutant proteins, using either polyclonal antibodies directed against the COOH-terminal part of Tiam1 (Habets et al., 1994) or monoclonal antibodies against the HA-tag (12CA5; Boehringer Mannheim Corp.) at the COOH terminus of all mutant Tiam1 proteins. Proteins were visualized using the enhanced chemiluminescence protocol ( Amersham Corp., Arlingtin Heights, IL).

Immunocytochemistry
Cells on coverslips were washed and fixed in 3.7% formaldehyde in PBS. Cells were subsequently stained as described (Michiels et al., 1995) with a polyclonal rabbit antiserum against Tiam1 (Habets et al., 1994). Antibodies were visualized with FITC-labeled secondary antibodies (Zymed Labs Inc., S. San Fransisco, CA). Cells were stained simultaneously for F-actin with TRITC-labeled phalloidin (Molecular Probes, Eugene, OR) at a concentration of 2 U/ml. At least 100 positive cells were analyzed by fluorescence microscopy and confocal laser scanning microscopy. Optical sections were taken through the apical part of the cells to show the presence or absence of membrane ruffles. Confocal images were recorded separately and subsequently merged. Colocalization of green (FITC) and red (TRITC) fluorescence appears in yellow in the merged images.

Immunoelectron Microscopy
48 h after transfection, cells were fixed for 1 h on the dish with a mixture of 4% paraformaldehyde and 0.5% glutaraldehyde in 0.1 M phosphate buffer. Fixed cells were scraped with a rubber policeman, washed, embedded in 10% gelatin, and infiltrated overnight with 1 M sucrose. After a further infiltration (2 h) with 1.8 M sucrose with 20% polyvinylpyrolidone, the samples were frozen in liquid nitrogen. Frozen thin sections were collected on formvar/carbon-coated grids, preincubated with 0.15% glycine in PBS, followed by immunoincubations with antibodies for 45 min at 25°C. Subsequently, the sections were incubated with 10-nm gold-labeled secondary antibodies for 30 min at 25°C. Antibody dilutions were made in phosphate buffer with 1% BSA and sections were washed in the same buffer, before and in between the incubation steps. Finally, sections were embedded and stained with 1.5% methylcellulose containing 0.3% uranyl acetate and examined in an electron microscope (model CM10; Philips Electronic Instrs., Mahwah, NJ). Where appropriate, the distribution of immunogold particles in at least 40 cross sections of cells was analyzed.

JNK Assay
Semiconfluent COS-7 cells or NIH3T3 cells were transfected with pCMVFlag-JNK1 and pcDNA-neo-Rac1– or Tiam1-expression vectors as described above. 48 h after transfection, cells were washed with ice-cold PBS and lysed on ice in a buffer containing 50 mM Tris-HCl, pH 7.5, 1% NP40, 100 mM NaCl, 5 mM EDTA, 100 µM sodium orthovanadate, 1 mM sodium fluoride, 20 µM aprotonin, 20 µM leupeptin, and 1 mM Pefabloc. After centrifugation (10 min, 10,000 g), flag-tagged c-Jun kinase was immunoprecipitated using 2 µg/ml of M2 monoclonal antibody (Kodak, Rochester, NY) for 1 h (4°C). Immune complexes were captured using protein A–Sepharose beads ( Pharmacia LKB Biotechnology Inc.) coated with rabbit anti–mouse immunoglobulins (Nordic Immunological Labs, Capistrano Beach, CA). Beads were washed three times in lysis buffer and once in kinase buffer (20 mM Hepes, 10 mM MgCl₂). Dried beads were incubated for 20 min at 30°C with 5 µg bacterially expressed glutathione S–transferase (GST)-c-Jun (amino acids 1–135) in 40 µl kinase buffer containing 1 mM DTT, 20 µM ATP, 5 µCi [-³²P]ATP (5,000 Ci/mmol), and 0.5 mM para-nitrophenylphosphate. Reactions were stopped with SDSsample buffer, and the amount of radioactive GST-c-Jun was quantified after SDS-PAGE by phosphorimaging. The level of expression of Tiam1, mutant Rac, and tagged JNK in the NIH3T3 or COS-7 cells was monitored by Western blotting.

	Results

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Membrane Association of Tiam1 Is Required for Membrane Ruffling
We have shown previously that full-length Tiam1 (FL1591) or a large COOH-terminal fragment of the Tiam1 protein (C1199) causes Rac1-dependent induction of membrane ruffling in NIH3T3 fibroblast cells (Michiels et al., 1995). Established NIH3T3 cell lines expressing either of these proteins are flat and epithelial-like and contain many membrane ruffles (Fig. 1 B), a phenotype that is also induced by transfection or microinjection of constitutively activated (V12)Rac1 (Ridley et al., 1992; Michiels et al., 1995; Van Leeuwen et al., 1995). In contrast, a smaller COOH-terminal part of the Tiam1 protein (C682), which contains only the DH domain and the adjacent PH domain, did not induce this phenotype (Fig. 1 C). As shown by confocal laser scanning immunofluorescence microscopy, the truncated large C1199 Tiam1 protein was present in the cytoplasm and colocalized with F-actin in membrane ruffles (Fig. 1 B). In contrast, the short C682 Tiam1 protein seemed to be restricted to the cytoplasm (Fig. 1 C). Western blot analyses (see Fig. 4, lanes 1–3) indicated that both proteins were intact and equally expressed. This suggested that the difference in phenotypes induced by these truncated proteins is probably caused by a different intracellular localization, and not by differences in stability. Immunoelectron microscopy (immuno-EM) indeed confirmed that the C1199 Tiam1 protein is present in the cytoplasm as well as at the cell membrane and particularly in the membrane ruffles, whereas the C682 Tiam1 protein is almost exclusively located in the cytoplasm (Fig. 2). We hypothesized, therefore, that membrane localization of Tiam1 is required for morphological transformation of NIH3T3 cells, including the formation of membrane ruffles.

View larger version (16K): [in this window] [in a new window] [Download PPT slide]   Figure 4 Immunoblotting of mutant Tiam1 proteins. Cell lysates were separated on a 7.5% SDS-polyacrylamide gel and blotted to nitrocellulose. All mutant C1199 and C682 Tiam1 proteins were detected with a polyclonal anti-Tiam1 antibody (Habets et al., 1994). Mutant C580 Tiam1 proteins were detected with a monoclonal antibody against the HA-tag (12CA5). Proteins were visualized using enhanced chemiluminescence ( Amersham Corp.). Molecular mass markers (in kD) are shown. The arrow indicates the position of the mutant C1199 Tiam1 proteins.

View larger version (45K): [in this window] [in a new window] [Download PPT slide]   Figure 2 Immunoelectron microscopic localization of truncated Tiam1 proteins. Frozen sections of established NIH3T3 cell lines expressing either C1199 Tiam1 (A) or C682 Tiam1 (B) were stained with anti-Tiam1 antibodies followed by gold-conjugated secondary antibodies. The C682 Tiam1 protein is almost exclusively located in the cytoplasm, whereas the C1199 Tiam1 protein is also present at the plasma membrane and in the membrane ruffles. Bar, 400 nm.

View larger version (72K): [in this window] [in a new window] [Download PPT slide]   Figure 3 Confocal images of COS-7 cells expressing mutated C1199 Tiam1 proteins. In this figure, the first column depicts the mutant Tiam1 proteins that were used. The second column shows the FITC-staining for Tiam1 expression. The third column shows the TRITClabeled phalloidin staining for F-actin, while the merged images of Tiam1 (green) and F-actin (red) are shown in the fourth column. Colocalization appears in yellow. Deletions within the conserved domains are indicated by arrowheads. See Materials and Methods section for a description of the mutations. For abbreviations, see legend to Fig. 1. Magnification is 200x. Bar, 40 µm.

β

Immuno-EM analyses of transfected COS cells showed that all mutant proteins were equally present in the cytoplasm and at the plasma membrane (Fig. 5), except for mutant C1199 Tiam1, which contains a deletion in the NH₂terminal PH domain (C1199-PHn). This protein was almost exclusively localized in the cytoplasm (Fig. 5 D), similar to the C682 Tiam1 protein (Fig. 2 B). The C1199-DH Tiam1 protein, which carries a deletion in the catalytic DH domain and does not induce membrane ruffling, was still capable of associating with the plasma membrane (Fig. 5 B). This clearly shows that membrane localization of Tiam1 is not a consequence of the induction of membrane ruffling. Therefore, it can be concluded that the NH₂-terminal PH domain is essential for the membrane localization of C1199 Tiam1 and that this membrane localization is required for the formation of membrane ruffles.

View larger version (47K): [in this window] [in a new window] [Download PPT slide]   Figure 5 Ultrastructural localization of mutant C1199 Tiam1 proteins in COS-7 cells. Immunogold labeling of mutant C1199 Tiam1 proteins with a deletion in the COOH-terminal PH domain (A), a deletion in the DH domain (B), a deletion in the DHR domain (C), and a deletion in the NH2-terminal PH domain (D). C1199-PHn Tiam1 is almost exclusively localized in the cytoplasm, while other mutant Tiam1 proteins also associate with the plasma membrane. Bar, 400 nm.

View larger version (76K): [in this window] [in a new window] [Download PPT slide]   Figure 6 Confocal images of COS-7 cells expressing mutant Tiam1 proteins. Confocal laser scanning microscopic images of COS-7 cells expressing C580 Tiam1 (A), MS-C580 Tiam1 (B), full-length Tiam1 (FL1591) (C), full-length Tiam1 with a deletion in the NH2-terminal PH domain (FL-PHn) (D), and FL-PHn containing a Src myristoylation signal at the NH2 terminus (MS-FL-PHn) (E). The insert in E is a higher magnification of the framed region showing the vesicle-like structures that are surrounded by the MS-FL-PHn Tiam1 protein. Indicated in blue is the myristoylation signal from c-Src (MS), containing the NH2-terminal 20 amino acids. In the merged images, Tiam1 is shown in green and F-actin in red. Magnification is 200x. Bar, 40 µm.

View larger version (46K): [in this window] [in a new window] [Download PPT slide]   Figure 7 Immunoelectron microscopic localization of mutant C580 Tiam1 proteins. Immunogold labeling of transiently transfected COS cells expressing C580 Tiam1 (A) or MS-C580 Tiam1 (B). Note that the MS-C580 Tiam1 protein is located at and underneath the plasma membrane. Bar, 400 nm.

To analyze the specificity of the NH₂-terminal PH domain of Tiam1, a region containing this PH domain was exchanged for the corresponding regions containing the PH domain of DbL, the PH domain of β-ARK, or the COOHterminal PH domain of Tiam1 (see Materials and Methods). However, none of these mutant Tiam1 proteins localized at the plasma membrane and induced membrane ruffling (data not shown). This means either that additional sequences are required for correct functioning of these PH domains or that the primary function of the NH₂terminal PH domain, namely to localize Tiam1 through specific interactions with components of the plasma membrane, cannot be substituted for by other PH domains.

The NH₂-terminal PH Domain Is Required for the Induction of Membrane Ruffles by the Full-Length Tiam1 Protein
The full-length Tiam1 protein (FL1591) carries a consensus myristoylation sequence at the NH₂ terminus. By labeling with [³H]myristate, we have confirmed that the NH₂ terminus of Tiam1 is myristoylated (not shown). To test whether the myristoylation is sufficient for the membrane association of full-length Tiam1, a small deletion was also made in the NH₂-terminal PH domain of full-length FL1591 Tiam1. However, similar to C1199-PHn, mutant fulllength Tiam1 (FL1591-PHn) was unable to induce membrane ruffling in NIH3T3 cells or COS cells (Fig. 6, C and D), and immuno-EM showed that the protein was not localized at the plasma membrane (data not shown). Apparently, the NH₂-terminal myristoylation of full-length Tiam1 alone is not sufficient for membrane localization. To further substantiate this, the NH₂-terminal c-Src sequences were fused in front of the FL1591-PHn1 Tiam1 protein. This region of Src contains a basic region that is required for optimal membrane translocation in addition to the myristoylation sequence, whereas other Src-like tyrosine kinases contain a palmitoylated cysteine in this region (Superti-Furga and Courtneidge, 1995). Both additional sequences are absent in Tiam1. Cells expressing the M^S-FL1591-PHn1 Tiam1 protein again showed membrane ruffling, although less extensive than cells expressing FL1591 Tiam1 (Fig. 6, C–E). Again, no main differences in expression levels were observed between these proteins (data not shown). Immuno-EM confirmed that the M^S-FL1591-PHn1 Tiam1 protein was present at and close to the plasma membrane, as found for M^S-C580 Tiam1 (data not shown). Apparently, the accessory basic region of c-Src also functions to properly localize M^S-FL1591PHn1 Tiam1. Similar to M^S-C580, the expression of M^SFL1591-PHn Tiam1 led to the formation of small cytoplasmic vesicle-like structures, and the protein was also located around these structures (Fig. 6 E). These observations indicate that the NH₂-terminal PH domain also serves as an essential membrane tag, or perhaps membrane anchor, for full-length Tiam1.

Controlled Cellular Localization of Tiam1
PH domains have been identified in other signaling molecules as protein–protein and/or protein–phospholipid interaction motifs that are required for the controlled targeting of these proteins to the plasma membrane (Lemmon et al., 1996). In tissue sections of skin and certain carcinomas, endogenous Tiam1 is predominantly present in the cytoplasm. Also in some cell lines, where we can envision endogenous Tiam1 by Western blotting, including T-lymphoma cells and neuronal cells, it is mainly localized in the cytoplasmic fraction (data not shown), suggesting that Tiam1 may translocate to the plasma membrane after receptor stimulation. So far, however, we have not been able to identify a receptor-mediated signaling pathway involving Tiam1 activation. To investigate whether membrane translocation of exogenous Tiam1 could be visualized in NIH3T3 cells, we analyzed whether serum could affect the localization and capacity of Tiam1 to induce membrane ruffling. As shown in Fig. 8 A, NIH3T3 cells transiently expressing the C1199 Tiam1 protein showed no membrane ruffling after serum starvation for 24 h. Almost no Tiam1 protein was present at the plasma membrane, and F-actin was mostly concentrated in lamellipodia in the Tiam1-expressing cells. Since these optical sections were taken at the basal site of the cells to illustrate the lamellipodia, stress fibers are also visible. Note that after serum starvation for 24 h, NIH3T3 cells still contain some stress fibers, in contrast to Swiss 3T3 cells. Immuno-EM confirmed that most of the cells contained significantly less Tiam1 at the plasma membrane after serum starvation (Fig. 8, D and F). The residual membrane-associated Tiam1 might be sufficient for the presence of lamellipodia under these conditions. Addition of serum induced membrane localization and subsequent ruffling of C1199 Tiam1-expressing cells after 2 h (Fig. 8, B and E), at which time point seruminduced stress fibers have already decreased. A quantification of these results is presented in Fig. 8 F. Similar results were obtained with FL1591 Tiam1, C1199-PHc, and C1199DHR Tiam1 (data not shown). In contrast, after 24 h of serum starvation the M^S-C580 Tiam1 protein remained at the plasma membrane and still induced membrane ruffling (Fig. 8 C). This suggests that the serum-induced membrane translocation of Tiam1 is mediated by the NH₂-terminal PH domain.

View larger version (94K): [in this window] [in a new window] [Download PPT slide]   Figure 8 Serum-dependent localization of Tiam1. Confocal images of NIH3T3 cells expressing C1199 Tiam1 (A and B) or MS-C580 Tiam1 (C) proteins. Cells were serum starved for 24 h (A and C), followed by stimulation with serum for 2 h (B). In the merged pictures, Tiam1 proteins are shown in green and F-actin in red. These optical sections were taken at the basal sites of the cells and reveal the presence of stress fibers in serum-starved NIH3T3 cells. Magnification is 300x. (D and E) Immuno-EM localization of C1199 Tiam1 after serum starvation (D) or after readdition of serum for 2 h (E). In F, the distribution of gold particles in at least 40 cross sections of cells were scored and presented as the percentage of cross sections with gold particles being predominantly at the membrane (M) or in the cytoplasm (C). Bars: (A–C) 40 µm; (D and E) 400 nm.

Membrane-associated Tiam1 Activates JNK
To investigate whether membrane association of Tiam1 is also required for the induction of other Rac-mediated signaling pathways besides membrane ruffling, the activity of JNK was determined after cotransfection with different Tiam1 mutants (see Materials and Methods). Both in COS-7 cells and NIH3T3 cells, cotransfection of fulllength Tiam1 led to an almost sevenfold stimulation of JNK activity, similar to constitutively activated (V12)Rac1 (Fig. 9 A). Cotransfection of tagged mitogen-activated protein kinase (MAPK) with full-length or mutant Tiam1 or (V12)Rac did not result in activation of MAPK (not shown). The stimulation of JNK by Tiam1 was dependent on the activation of Rac, since cotransfection of dominantnegative (N17)Rac1 partly blocked the activation of JNK by Tiam1 (Fig. 9 A). Higher amounts of (N17)Rac interfered with the expression of JNK. Furthermore, a deletion in the catalytic DH domain of Tiam1 prevented JNK activation (not shown). Cotransfection of dominant-negative (N17)Cdc42 did not interfere with the activation of JNK by Tiam1 (data not shown). Transfection of C1199 Tiam1 stimulated JNK activity to a similar extent as FL1591 (Fig. 9 B). However, shorter COOH-terminal Tiam1 fragments such as C682 and C580 Tiam1, which did not localize to the plasma membrane, were not able to activate JNK above background levels. Also, mutant C1199-PHn Tiam1, which did not localize to the plasma membrane because of the deletion in the NH₂-terminal PH domain, was unable to activate JNK (Fig. 9 B). M^S-C580 Tiam1 caused no stimulation of JNK activity (Fig. 9 B), and neither did M^S-C1199-PHn or M^S-FL1591-PHn Tiam1 proteins (data not shown). These proteins, however, induced membrane ruffling and were present at the plasma membrane (Fig. 6). A possible explanation for this somewhat unexpected result is that activation of endogenous Rac by M^S-containing Tiam1 proteins is sufficient for induction of membrane ruffling but not for stimulation of JNK. Alternatively, the lack of induction of JNK activity is caused by the different ultrastructural localization of the M^S-C580 Tiam1 protein (compare Figs. 5 and 7) or may reflect the need for an intact NH₂-terminal PH domain. Interestingly, similar results were obtained with membrane-targeted p110 phosphoinositide-3-kinase which was able to stimulate membrane ruffling but not gene transcription from the Jun-inducible Fos promoter (Reif et al., 1996). Whatever the mechanism, these results indicate that the localization of Tiam1 at the plasma membrane is also required for Rac-mediated stimulation of JNK activity.

View larger version (14K): [in this window] [in a new window] [Download PPT slide]   Figure 9 Stimulation of JNK activity by Tiam1. (A) COS-7 cells were transfected with pCMV-Flag-JNK1 and empty vector (pcDNA-neo), full-length Tiam1 (FL1591), or constitutively activated (V12)Rac1. Cotransfection with dominant-negative (N17)Rac1 was performed as indicated. The activity of immunoprecipitated Flag-JNK was determined 48 h after transfection by an in vitro kinase assay using bacterially expressed GST-Jun as a substrate. The expression of Tiam1, Myc-tagged (N17)Rac, and Flag-tagged JNK was analyzed by Western blotting and is shown underneath the graph. (B) NIH3T3 cells were transfected with pCMV-Flag-JNK1 and mutant Tiam1 constructs. JNK activity was determined as described. All data are presented as fold stimulation of empty vector controls. Equal amounts of expressed Flag-JNK1 and Tiam1 proteins, as determined by Western blotting, were used. Data represent mean ± standard deviation of at least two independent experiments.

	Discussion

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A short COOH-terminal fragment of Tiam1, C682 Tiam1, which lacks the NH₂-terminal PH domain, did not associate with the plasma membrane in NIH3T3 cells or COS-7 cells and was unable to induce membrane ruffling (see Figs. 1 and 2). Similar to C1199 Tiam1 and (V12)Rac1, the C682 Tiam1 protein induces a tumorigenic phenotype in NIH3T3 cells (Van Leeuwen et al., 1995). This indicates that the Tiam1-induced formation of membrane ruffles and induction of a tumorigenic phenotype are triggered by two distinct signaling pathways. Since JNK activity could not be stimulated by C682 Tiam1 and none of the truncated or mutant Tiam1 proteins activated MAPK, it is unlikely that the induction of a tumorigenic phenotype is due to activation of JNK or MAPK. An explanation could be that tumorigenicity is caused by activation of cytoplasmic Rac, although we cannot exclude that cytoplasmic Tiam1 activates another, yet unknown GTPase. Both the C1199 and C682 Tiam1 proteins were also able to induce an invasive phenotype in T-lymphoma cells (Habets et al., 1994). As the localization of Tiam1 might be differently regulated in lymphoid cells compared to adherent COS and fibroblast cells, we are currently testing whether or not JNK is involved in the Tiam1/Rac-mediated induction of an invasive phenotype in T-lymphoma cells.

A detailed structural analysis showed that a small deletion in the NH₂-terminal PH domain, but not the DHadjacent COOH-terminal PH domain, abolished the membrane localization of Tiam1 and the subsequent induction of membrane ruffling. In all DH domain–containing GDS proteins analyzed thus far, the DH domain is flanked by a PH domain (Cerione and Zheng, 1996; Collard, 1996), suggesting that the DH–PH combination is a functional unit. Indeed, deletions in either the DH domain or the flanking PH domain of the protooncogenes Dbl, Ost, Dbs, and Lfc result in loss of transforming capacity (Ron et al., 1991; Horii et al., 1994; Whitehead et al., 1995a,b; Zheng et al., 1996). The transforming capacity of a mutant of Lfc, which carried a deletion in the PH domain, could be restored by the addition of a COOH-terminal Ras CAAX motif, suggesting that the localization of Lfc at the plasma membrane is required for its transforming capacity (Whitehead et al., 1995b). In contrast, the Ras-CAAX motif was not sufficient to replace the PH domain of Dbl, which is required for the presence of Dbl in the particulate fraction of cells (Zheng et al., 1996). Corresponding results were obtained for the NH₂-terminal PH domain of Ras-guanine nucleotide release factor (GRF), suggesting that the association of Ras-GRF and Dbl in the particulate fraction is a prerequisite for their activity (Buchsbaum et al., 1996; Zheng et al., 1996). Together with pleckstrin and RasGRF, Tiam1 is one of a few proteins that contains two PH domains (Habets et al., 1994). Similarly to Ras-GRF, only the NH₂-terminal PH domain of Tiam1 is involved in the localization of the protein. The COOH-terminal PH domain of Tiam1 has only moderate homology with other PH domains and lacks a highly conserved tryptophan residue in the COOH-terminal -helix (Habets et al., 1994). Although a complete deletion of the DH-adjacent PH domain of Tiam1 abolished membrane ruffling, it did not interfere with the membrane localization of the protein (data not shown). What other functions can be attributed to this PH domain remains to be elucidated.

Several reports have demonstrated that isolated PH domains can bind in vitro to G_β subunits and phospholipids like phosphatidylinositol (4,5)bisphosphate (PIP2) and inositol (3,4,5)trisphosphate (IP3) (Harlan et al., 1994; Ferguson et al., 1995; Mahadevan et al., 1995; Touhara et al., 1995). Phosphoinositide-3-kinase, which stimulates the synthesis of phosphatidylinositol (3,4,5)trisphosphate (PIP3) from PIP2 (Hiles et al., 1992), has been implicated in the activation of Rac by PDGF and insulin (Wennstrom et al., 1994; Hawkins et al., 1995) and might be required for the activation of Rac by Ras (Rodriguez-Viciana et al., 1994). Although we have shown that the association of Tiam1 with the plasma membrane is induced by serum, neither PDGF nor insulin could substitute for serum in NIH3T3 cells. G_β subunits and phospholipids represent potential downstream effectors of G-protein–coupled receptors and/or activated tyrosine kinase receptors. Based on the in vitro binding data of PH domains, it is tempting to speculate that G_β subunits and/or specific phospholipids regulate the association of Tiam1 with the plasma membrane, as depicted in Fig. 10. The fact that we were not able to functionally exchange the NH₂-terminal PH domain of Tiam1 for other PH domains argues for a specific targeting function for this PH domain, and similar results have been reported for PH domains in other signaling proteins (Buchsbaum et al., 1996; Kolanus et al., 1996). However, at the moment we cannot determine whether PH domains can function as independent modules or whether additional sequences are required for their activity.

View larger version (24K): [in this window] [in a new window] [Download PPT slide]   Figure 10 Model for activation of Rac by Tiam1. Activation of Rac requires membrane translocation of Tiam1 and might be analogous to activation of Ras by receptor-induced translocation of SOS. Membrane association of Tiam1 could be mediated by interactions between the NH2-terminal PH domain and putative effectors of activated G-protein coupled receptors (GPCR), tyrosine kinase receptors (TKR), or Ras, which may include Gβ subunits, PIP2, PIP3, IP3, and perhaps G subunits. Activation of Rac by membrane-associated Tiam1 leads to membrane ruffling and JNK activation. It is unlikely that JNK is involved in the induction of an oncogenic phenotype in NIH3T3 cells, since mutant C682 Tiam1 induces an oncogenic phenotype without activation of JNK. Which Tiam1/Rac-mediated signaling pathways are involved in the induction of an invasive phenotype in T-lymphoma cells remains to be established.

Given the importance of PH domains in Tiam1 and other GDS proteins, it is conceivable that phospholipids and/or G_β subunits are involved in their intracellular localization and/or activation. The next challenge will be to identify the upstream signaling pathways and molecules that translocate and activate these GDS proteins.

	Acknowledgments

 
We thank Drs. M. Karin, A. Eva, and T. van Biezen for their gift of constructs; G. Habets and F. van Leeuwen for their help in the initial studies; L. Oomen for his assistance with the confocal microscope; L. Oomen and N. Ong for preparation of some of the figures; and F. van Leeuwen, E. Roos, and R. Engers for critically reading the manuscript.

This work was supported by grants from the Netherlands Organization for Scientific Research and the Dutch Cancer Society to J.G. Collard.

Submitted: 8 October 1996

Revised: 23 January 1997

1. Abbreviations used in this paper: aa, amino acids; DH, Dbl homology; DHR, Discs-large homology region; GDI, guanine nucleotide dissociation inhibitors; GDS, guanine nucleotide dissociation stimulator; GRF, guanine nucleotide release factor; GST, glutathione S-transferase; HA, hemagglutinin; IP3, inositol (3,4,5)trisphosphate; JNK, c-Jun NH₂-terminal kinase; MAPK, mitogen-activated protein kinase; PH, pleckstrin homology; PIP2 and PIP3, phosphatidylinositol (4,5)bisphosphate and (3,4,5)trisphosphate.

Address all correspondence to Dr. J.G. Collard, The Netherlands Cancer Institute, Division of Cell Biology (H1), 121 Plesmanlaan, 1066 CX Amsterdam, The Netherlands. Fax: (31) 20 5121944. E-mail: JCOLL@NKI.NL

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