Article |
Address correspondence to Philippe Chavrier, UMR144 Centre National de la Recherche Scientifique, Institut Curie, 26 rue d'Ulm, F-75248 Paris cedex 05, France. Tel.: 33-1-42-34-63-59. Fax: 33-1-42-34-63-77. email: philippe.chavrier{at}curie.fr
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Abstract |
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Key Words: ARF6; exocyst complex; recycling; endocytosis; small GTP-binding protein
Abbreviations used in this paper: ARF, ADP-ribosylation factor; NRK, normal rat kidney; RE, recycling endosome; siRNA, small interfering RNA; Tf, transferrin; TfR, transferrin-receptor.
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Introduction |
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ADP-ribosylation factor (ARF) 6, a member of the family of ARF small GTP-binding proteins, regulates membrane movement between the plasma membrane and early endocytic compartments (Chavrier and Goud, 1999). Like all small GTP-binding proteins, ARF6 cycles between active GTP and inactive GDP-bound forms, and studies from several laboratories have indicated that ARF6 activation occurs at the plasma membrane (D'Souza-Schorey et al., 1998; Frank et al., 1998; Franco et al., 1999; Vitale et al., 2002). The ARF6 GDP/GTP cycle has been shown to regulate the uptake and recycling of plasma membrane proteins to generate membrane protrusive structures concomitant with alterations in the cortical actin cytoskeleton (Radhakrishna and Donaldson, 1997; D'Souza-Schorey et al., 1998; Franco et al., 1999; Palacios et al., 2001). This specific and essential role of ARF6 is further reflected by its involvement in various cellular processes requiring transient cellular polarization such as cell spreading, cell motility and phagocytosis (Song et al., 1998; Zhang et al., 1998; Radhakrishna et al., 1999; Palacios et al., 2001; Santy and Casanova, 2001; Niedergang et al., 2003). ARF6 activity is also required for regulated secretion in adipocytes and neuroendocrine cells (Yang and Mueckler, 1999; Vitale et al., 2002). These observations point to a crucial role for ARF6 in plasma membrane and cortical actin remodeling through the regulation of membrane recycling to specialized regions of the plasma membrane. However, our understanding of the mechanism of ARF6 membrane remodeling is still limited and awaits the identification of new effector pathways.
The delivery of membrane vesicles to spatially restricted areas of the plasma membrane is a multi-step process requiring polarized transport, restricted docking and fusion of vesicles to specific plasma membrane sites (for review see Finger and Novick, 1998). Recently, an eight-subunit complex termed the exocyst complex has been shown to mediate the vectorial targeting of secretory vesicles to sites of membrane insertion in yeast (TerBush and Novick, 1995). The exocyst complex is conserved in mammals where it plays a role in vesicle delivery from a post-Golgi compartment to specific plasma membrane domains of epithelial and neuronal cells (Grindstaff et al., 1998; Hazuka et al., 1999; Lipschutz et al., 2000; Vega and Hsu, 2001; Yeaman et al., 2001). Although little is known about the regulation of exocyst complex function, interactions between small GTP binding proteins and exocyst complex subunits have been reported (for review see Lipschutz and Mostov, 2002). These interactions suggest a potential connection between signaling and modulation of polarized membrane growth by the exocyst complex. In this study, we identify the exocyst complex as a novel effector for ARF6, mediating endocytic membrane recycling to dynamic regions of the plasma membrane.
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Results |
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These antibodies were used to determine the intracellular distribution of Sec10 and the exocyst complex by immunofluorescence and immuno-EM. In nonpolarized MDCK cells and in NRK cells, Sec10 localization was predominantly perinuclear and partially overlapped with the distribution of the Golgi marker GM130 (Fig. 2, AC and DF, respectively). Immuno-EM of nonpolarized MDCK cells and NRK cells revealed localization of endogenous Sec10 to tubulo-vesicular structures close to Golgi cisternae and corresponding presumably to the TGN (Fig. 3, A and D, respectively; arrows). These observations are in agreement with reported association of the Sec6, Sec8, and Exo70 exocyst subunits with the TGN (Vega and Hsu, 2001; Yeaman et al., 2001). Interestingly, Sec10 was also detected in scattered vesicular structures visible by immunofluorescence microscopy in MDCK (Fig. 2 B, arrows) and in NRK cells (Fig. 2, E and H; arrows). By immuno-EM, some of the Sec10-positive structures appeared as peripheral vesicles closely apposed to endosomal organelles (Fig. 3, BD; asterisks) with a characteristic vacuolar region and few intraluminal vesicles (Fig. 3, B and C, MDCK cells; Fig. 3 D, NRK cells, arrowheads point to Sec10 labeling). As shown in Fig. 3 C, these vesicular elements are likely to correspond to endosomal buds. The localization of Sec10 to endocytic compartments was studied by double-labeling immunofluorescence microscopy analysis of NRK cells with a combination of anti-TfR mAb and anti-Sec10 antibodies. A significant overlap of Sec10 and TfRs was observed in perinuclear compartments (Fig. 2, GI; arrowheads). To ascertain the presence of Sec10 in recycling endocytic compartments, we used whole-mount immuno-EM as initially described by Stoorvogel et al. (1996). NRK cells were incubated with HRP-conjugated transferrin (Tf) to fill the entire recycling pathway, and were processed for whole-mount immuno-EM as described in the Materials and methods section. Anti-Sec10 antibodies decorated vesicular endosomal structures and appeared enriched in endosomal buds (Fig. 3, E and F; arrows), some of which were also labeled for TfRs (Fig. 3 F, arrow). Based on these data, we conclude that beside its previously known localization to the TGN and to some specialized sites at the plasma membrane (Grindstaff et al., 1998; Hazuka et al., 1999; Lipschutz et al., 2000; Vega and Hsu, 2001), the exocyst complex is also present in the recycling endocytic pathway.
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Discussion |
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We report that a domain comprising the last 330 residues of Sec10 interacts with ARF6 by a two-hybrid screen and in pull-down assays. This association is direct, and occurs preferentially with activated GTP-ARF6 (Fig. 1). The association of GTP-ARF6 with Sec10 is reminiscent of interactions reported recently in yeast and mammalian cells between the exocyst subunits and several members of the Rab, Rho, and Ral small GTP-binding protein subfamilies (for review see Lipschutz and Mostov, 2002; Novick and Guo, 2002). In yeast, the exocyst complex acts presumably by targeting secretory vesicles to sites of exocytosis (Finger and Novick, 1998). Recruitment of Sec15p to secretory vesicles requires its interaction with GTP-Sec4p, a Rab protein functioning in Golgi to plasma membrane transport in yeast (Finger et al., 1998; Guo et al., 1999b). At a later stage on the secretory pathway, interaction of Sec3p with GTP-Cdc42p and GTP-Rho1p, two Rho proteins essential for cell polarity establishment and maintenance, is probably required to direct exocytosis to the bud (Grote et al., 2000; Guo et al., 2001; Zhang et al., 2001). In mammalian cells, Sec5 interacts with GTP-Ral (Moskalenko et al., 2002), which may regulate complex assembly (Moskalenko et al., 2002), whereas interaction of Exo70 with the Rho protein TC10 has recently been implicated in trafficking of Glut4 to the plasma membrane (Inoue et al., 2003). The mammalian exocyst complex is found at specialized sites of the plasma membrane along the axon and in the growth cone of neuronal cells, as well as at epithelial cellcell contacts (Grindstaff et al., 1998; Hazuka et al., 1999; Lipschutz et al., 2000).
An intracellular pool of the complex is also detected on the TGN (Vega and Hsu, 2001; Yeaman et al., 2001; Fig. 3, A and D). Interestingly, expression of dominant-inhibitory Sec10 and Sec8 blocks neurite outgrowth in PC12 cells and trafficking to the basolateral membrane in MDCK cells, respectively (Lipschutz et al., 2000; Vega and Hsu, 2001). In addition, Sec10 overexpression stimulates tubule formation in an in vitro model of kidney tubulogenesis (Yeaman et al., 2001). All together, these results support the idea that the exocyst complex is required for transport between the TGN and sites of plasma membrane growth. Our data indicate that the perinuclear distribution of the exocyst complex in mammalian cells is not restricted to the TGN (Vega and Hsu, 2001; Yeaman et al., 2001), but extends into REs. Here, we demonstrate that TfR-containing endocytic buds that are abundant on REs (Stoorvogel et al., 1996) carry endogenous Sec10. This is consistent with data showing that Exo70 and Sec8 exocyst subunits are associated with TfR-positive REs in MDCK cells (Folsch et al., 2003). However, it is unlikely that the recruitment of Sec10 to the RE requires GTP-bound ARF6, as perinuclear Sec10 localization is not affected by dominant-inhibitory ARF6 that lowers GTP-ARF6 level. Rather, our observations indicate that GTP-ARF6, which accumulates at the plasma membrane (D'Souza-Schorey et al., 1998; Frank et al., 1998; Franco et al., 1999; Vitale et al., 2002), triggers the localization of Sec10, and the exocyst complex, to plasma membrane protrusions and invaginations that form upon ARF6 activation (Fig. 7).
Depending on the cell types, ARF6 has been shown to control the recycling of proteins endocytosed through the clathrin-dependent pathway (D'Souza-Schorey et al., 1995, 1998), or to transport proteins that are endocytosed independently of clathrin (Radhakrishna and Donaldson, 1997; Naslavsky et al., 2003). Although it has not been clarified whether these pathways intersect and whether recycling materials follow a common route back to the plasma membrane, ARF6 activity has consistently been associated with the formation of actin-based plasma membrane protrusions (Song et al., 1998; Franco et al., 1999; Radhakrishna et al., 1999; Palacios et al., 2001). Accordingly, ARF6 is implicated in the regulation of cellular processes requiring a transient mechanism to deliver membranes to regions of the cell surface reorganization. A common feature of these processes (including membrane ruffling, cell spreading, cell motility, and phagocytosis; Song et al., 1998; Zhang et al., 1998; Radhakrishna et al., 1999; Palacios et al., 2001; Santy and Casanova, 2001; Niedergang et al., 2003) is that polarized endocytic recycling contributes to cellular polarization. Directional recycling of TfRs and integrins to the leading edge has been reported during cell spreading and motility in fibroblasts (Hopkins et al., 1994; Pierini et al., 2000; Laukaitis et al., 2001; Roberts et al., 2001). Similarly, recycling endocytic vesicles positive for VAMP3 insert at the site of pseudopod extension during phagocytosis in macrophages, in a process that is under ARF6 control (Bajno et al., 2000; Niedergang et al., 2003). Here, we found that spreading of ARF6-Q67Lexpressing NRK cells is strongly inhibited by coexpression of dominant-inhibitory Sec10. This observation, together with the reported inhibition of NRK and HeLa cell spreading upon inhibition of ARF6 function (Radhakrishna and Donaldson, 1997; Song et al., 1998), suggests that membrane delivery from internal endocytic reservoirs is a major player during cell spreading in a process that involves the ARF6/exocyst complex machinery controlling membrane insertion at the plasma membrane.
Therefore, we favor a model that considers that local ARF6 activation at the plasma membrane is required for polarized membrane recycling and insertion through interaction of GTP-ARF6 with the vesicle-tethering exocyst complex. According to this model, interfering with exocyst complex activity is expected to impair docking of recycling transport intermediates with the plasma membrane. Indeed, we observed a partial inhibition of Tf recycling in Sec5-depleted cells, consistent with the observation that only a fraction of Tf recycles to the plasma membrane through REs (Sheff et al., 1999). In addition, the observation that dominant inhibition of Sec10 function triggers the formation of an extensive endocytic tubular network is also consistent with an essential role of the exocyst complex in endocytic recycling. Analogous to findings in yeast where inhibition of Sec10p leads to intracellular membrane accumulation (Roth et al., 1998), we believe that this morphological change is produced by interfering with the docking of recycling transport intermediates with the plasma membrane. Although our findings bring novel insights as to how ARF6 may control delivery of recycling vesicles, they do not explain how the exocyst complex can operate simultaneously in post-Golgi and endocytic recycling pathways without mixing. One possibility is that specificity is provided earlier when the exocyst complex is recruited to donor compartments or vesicles.
In yeast, Sec4p acts as a bridge between the exocyst and post-Golgi transport vesicles by interacting with Sec15p (Finger et al., 1998; Guo et al., 1999b). Interestingly, two sec15 genes have been identified in mammalian cells encoding two related proteins (Sec15A and Sec15B; Kee et al., 1997; Brymora et al., 2001). These observations suggest the existence of at least two forms of the exocyst complex that may interact with specific Rab GTPases on distinct membranes. Directionality and specificity may also be achieved by polarized vesicle transport. Recently, it has been shown that a subset of microtubules could serve as a track to facilitate export from the RE to the cell surface (Lin et al., 2002), and a direct association of the exocyst complex with microtubules has been reported (Vega and Hsu, 2001). Future experiments should define the function of ARF6 in coordinating these various mechanisms that target post-endocytic recycling to sites of membrane growth during cell polarization.
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Materials and methods |
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Yeast two-hybrid screening
Two-hybrid screening was performed using a mating protocol with L40 and Y187 yeast strains, using a fusion of LexA with ARF6-Q67L as a bait and a human placenta random-primed cDNA library fused to the Gal4 activation domain, using standard procedures (Vojtek and Hollenberg, 1995).
ARF6Sec10 binding assays
Sequences encoding full-length Sec10 or its amino-terminal region (Sec10NTer; aa 378708) were subcloned into pGEX4T1 at the carboxy terminus of GST and transformed in E. coli BL21(DE3) strain. Expression was induced with 0.5 mM isopropyl ß-D-thiogalactopyranoside for 5 h at 25°C. The fusion protein was purified by affinity chromatography on glutathione-Sepharose beads (Amersham Biosciences). After elution with glutathione, the purified protein was dialyzed against 20 mM Tris, pH 7.4, 100 mM NaCl, 2 mM EDTA, 2 mM ß-mercaptoethanol, and 10% glycerol, and was stored at -80°C.
For the in vitro binding assay, recombinant ARF6 (rARF6) was purified from E. coli mostly as a GTP-bound form as described previously (Chavrier and Franco, 2001). Loading with GDP was obtained by the addition of 2 mM EDTA (free Mg2+ 1 µM) in the presence of 5 mM excess GDP for 60 min at 25°C, followed by addition of 2 mM MgCl2. In these conditions,
50% of rARF6 was converted in the GDP-bound form. Separation of the GTP- and GDP-bound forms of ARF6 (5 mg total rARF6) was performed by chromatography on a cation exchange column (Mono S HR5/5; Amersham Biosciences) equilibrated in buffer A (50 mM Tris-HCl, pH 7.5, 1 mM MgCl2, 1 mM DTT, and 10 µM GDP) at a flow rate of 1 ml/min. Elution was performed with a linear gradient of 01 M NaCl in buffer A, GTP- and GDP-ARF6 eluting at
70 mM and 110 mM NaCl, respectively. 8 µM GTP- or GDP-bound rARF6 was incubated together with GST or GST-Sec10, and was bound to glutathione-Sepharose beads (4 µM) for 60 min at 4°C in binding buffer (50 mM Tris-HCl, pH 7.5, 100 mM NaCl, 2 mM MgCl2, 1 mM DTT, and 0.5% Triton X-100) containing 100 µM GDP (GDP-ARF6 binding experiment) or GTP (GTP-ARF6 binding experiment) and 0.5% BSA (wt/vol). Beads were washed twice with binding buffer plus 0.5% BSA and twice with binding buffer. Bound proteins were eluted in SDS sample buffer and separated by SDS-PAGE. rARF6 in the bound (10% of total) and unbound (1% of total) fraction was detected by immunoblotting analysis using anti-ARF6 antibodies.
For the in vivo binding assay, HeLa cells were transfected with plasmids encoding HA-tagged ARF1 and ARF6 variants using the calcium-phosphate method. Cells were lysed 36 h after transfection with 50 mM Tris, pH 7.4, 100 mM NaCl, 1 mM EDTA, 1% Triton X-100, and a cocktail of protease inhibitors (Roche), and centrifuged at 13,000 rpm for 5 min at 4°C. Supernatants were incubated with GST or GST-Sec10 for 30 min at 4°C in the presence of 0.1% BSA, and then glutathione-Sepharose beads were added for 1 h further. Beads were washed three times with 1 ml 50 mM Tris, pH 7.4, 100 mM NaCl, 1 mM EDTA, and 1% Triton X-100. Bound proteins were eluted using SDS sample buffer, and were separated by SDS-PAGE. The presence of ARF on the beads was detected by Western blot analysis using anti-HA antibodies.
Generation of stable MDCK cell lines
cDNAs encoding HA-tagged ARF6-T27N and -Q67L have been described previously (Franco et al., 1999). Tet-OffTM MDCK cells were transfected with FuGENETM 6 reagent with the cDNA-encoding HA-tagged ARF6-Q67L subcloned in pTRE expression vector (CLONTECH Laboratories, Inc.) and pSPGK-Hygro. Resistant clones were maintained in medium containing 400 µg/ml hygromycin, 200 µg/ml G418, and 1 µg/ml doxycycline. Regulated expression of HA-tagged ARF6-Q67L in resistant clones was assessed by immunoblotting analysis with anti-ARF6 antibodies after 72 h of culture with or without doxycycline. Two clones (named clone 15 and 17) were selected, and gave identical results.
Transient transfection and Tf uptake
Expression plasmid for dominant inhibitory Sec10 (aa 1537) was generated by PCR from human Sec10 cDNA (a gift of Dr. P. De Camilli, Yale University School of Medicine, New Haven, CT) and by in-frame insertion at the carboxy terminus of E-GFP in the pEGFP-C1 expression vector (CLONTECH Laboratories, Inc.).
For transient transfection, MDCK I cells were trypsinized and resuspended at a density of 2.5 x 107 cells/ml in culture medium supplemented with 15 mM Hepes, pH 7.5. 5 x 106 cells were electroporated in a 0.4-cm cuvette (Equibio) with 20 µg plasmid DNA encoding HA-tagged ARF6-Q67L variants (Franco et al., 1999) with a Gene Pulser II apparatus (950 µF, 240 V; Bio-Rad Laboratories). Cells were usually analyzed 36 h after transfection. NRK cells grown on coverslips were transfected with FuGENETM 6 reagent (Roche) according to the manufacturer's procedure. For Tf uptake, 30 h after transfection, cells were incubated in internalization medium (DME supplemented with 20 mM Hepes, pH 7.4, and 1% wt/vol BSA) for 30 min at 37°C. Then, cells were incubated in internalization medium containing 10 µg/ml Alexa® 546conjugated human Tf (Molecular Probes, Inc.) for 30 min. Cells were fixed and processed for immunofluorescence labeling.
Immunofluorescence microscopy
Cells on coverslips were fixed, permeabilized, immunolabeled, and visualized for fluorescence staining as described previously (Guillemot et al., 1997). Optical sections were taken with a confocal microscope (TCS SP2; Leica). For determination of projected cell area, images were analyzed with the Integrated Morphometry Analysis module of MetaMorph® 5.04 software (Universal Imaging Corp.).
Quantification of Tf recycling
HeLa cells were transfected with siRNA duplex (Dharmacon) specific for human Sec5 with Oligofectamine® according to the manufacturer's instruction (Invitrogen; Elbashir et al., 2001; Sec5 siRNA duplex: (Sec51), 5'-CGGCAGAAUGGAUGUCUGC-3'; (Sec52), 5'-GGUCGGAAAGACAAGGCAGAU-3'). After 72 h, cells were detached in 1% EDTA/PBS and pelleted. Cells were resuspended in internalization medium (DME, 10 mM Hepes, pH 7.4, and 0.1% BSA) supplemented with 50 nM Alexa® 488labeled human Tf and incubated at 37°C. After 30 min, cells were diluted with cold internalization medium, pelleted, and resuspended in cold internalization medium supplemented with 1.5 µM human holo-Tf. An aliquot of cells was taken and kept on ice (time 0), and the remaining cells were incubated at 37°C. At the indicated time during the recycling period, aliquots of cells were taken, diluted four times in 0.1% BSA/PBS, and kept on ice. All time points were done in duplicate. FACS® analysis was performed using a FACScanTM (Becton Dickinson) measuring Alexa® 488 in FL1. Live cells were selected using a forward scatter/side scatter gate, and data from at least 2 x 103 live cells were acquired. The mean Alexa® 488 fluorescence was calculated as the averaged means of duplicate samples.
Electron microscopy
For immunogold labeling on ultrathin cryosections, cells were fixed with 2% PFA in PBS for 2 h at RT. Fixed cells were processed for ultrathin cryosectioning, and were immunogold labeled (Raposo et al., 1997). Antibodies were visualized with Protein Agold conjugates (purchased from the Department of Cell Biology, Utrecht University, Utrecht, Netherlands). After staining and embedding with a mixture of uranyl acetate and methylcellulose, sections were viewed at 80 kV with a transmission electron microscope (Philips CM120; FEI Company).
For whole-mount EM, immunogold labeling of Sec10 and TfR on entire NRK cells was performed as described by Stoorvogel et al. (1996) on cells grown for 2 d on formvar-coated gold grids. In brief, after washing with MEM, 20 mM Hepes, pH 7.4, cells were starved for 45 min in the same medium at 37°C and then incubated for 45 min with 50 µg/ml of HRP-conjugated mouse Tf (Pierce Chemical Co.). Cells were rapidly cooled at 4°C and incubated in DAB-H2O2containing buffer in order to fill Tf-containing compartments with DAB polymer that served as an electron-dense marker for endosomes. Soluble cytosolic proteins were removed by permeabilization with saponin, and cells were then fixed with 3% PFA in 0.1 M phosphate buffer, pH 7.4, for 2 h. Immunogold labeling was performed at RT in the presence of saponin and using cold fish gelatin as blocking buffer. After labeling, cells on grids were fixed with 2% glutaraldehyde, rinsed in water, dehydrated in increasing concentrations of ethanol, and critical point dried in a critical point dry apparatus (Balzers). Samples were viewed with a transmission electron microscope (Philips CM120; FEI Company).
Subcellular fractionation, immunoprecipitation, and immunoblotting analysis
For subcellular fractionation, MDCK Tet-OffTM cells from two selected clones stably transfected with HA-tagged ARF6-Q67L (clones 15 and 17) were cultured in the presence of 1 µg/ml doxycycline (+Dox), or switched to doxycycline-free (-Dox) medium for 72 h. Cells from the different populations (4 x 106 cells from two 10-cm-diam dishes) were washed and scraped in PBS and homogenized in 250 mM sucrose, 3 mM imidazole, pH 7.4, with protease inhibitors by repeated passages through a 25G5/8 needle. Homogenate was subjected to a 1,000-g spin to yield a postnuclear supernatant (PNS). PNS was subjected to a 100,000-g spin to yield soluble (S) and pellet (P) fractions. Pellets were resuspended in sample buffer to volumes equal to that of the corresponding supernatants, and equal volumes of P and S fractions were loaded per lane (corresponding to 25 µg total protein from the soluble fraction). For immunoprecipitation analysis, 2 x 106 MDCK cells were lysed in 1% Triton X-100, 150 mM NaCl, 2 mM EDTA, and 30 mM Tris, pH 7.6, with protease inhibitors at 4°C. Lysates were cleared by centrifugation at 13,000 g for 10 min at 4°C, and 5 µg affinity-purified rabbit anti-Sec10 antibodies or 2.5 µg mAb against Sec8 were added for 30 min at 4°C. Then, protein GSepharose beads (Amersham Biosciences) were added, incubated for 5 h at 4°C, and washed three times in lysis buffer and once in 50 mM Tris, pH 7.5. Proteins were separated on 8% polyacrylamide gels and transferred to PVDF membranes. Detection of bound antibodies was performed with the ECL procedure (Amersham Biosciences).
Online supplemental material
Fig. S1 shows the characterization of anti-Sec10 pAbs. Fig. S2 shows the characterization of MDCK Tet-OffTM cells (clone 15) stably transformed with HA-tagged ARF6-Q67L. The online supplemental material is available at http://www.jcb.org/cgi/content/full/jcb.200305029/DC1.
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Acknowledgments |
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This work was supported by institutional funding from Centre National de la Recherche Scientifique (CNRS) and Institut National de la Santé et de la Recherche Médicale (INSERM), and by grants from Institut Curie, the Fondation BNP Paribas, and the Ligue Nationale contre le Cancer (équipe labellisée) to P. Chavrier. T. Dubois was the recipient of a post-doctoral fellowship from Association pour la Recherche sur le Cancer.
Submitted: 7 May 2003
Accepted: 16 October 2003
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