Medical Institute of Bioregulation, Kyushu University, 3-1-1 Maidashi, Higashi-ku, Fukuoka 812-8582, Japan
* Author for correspondence (e-mail: hsumi{at}bioreg.kyushu-u.ac.jp)
Accepted 15 July 2003
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Summary |
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Key words: Formin proteins, Fhos, Diaphanous proteins, Actin, Stress fiber, Rac
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Introduction |
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In resting cells, mDia is probably folded in an inactive form, which is maintained by an intramolecular interaction between the N- and C-terminal regions (Alberts, 2001; Ishizaki et al., 2001
; Watanabe et al., 1999
). Disruption of the intramolecular interaction by deleting the N- or C-terminal region leads to the activation of mDia, thereby inducing the formation of stress fibers. On cell activation, binding of the small GTPase Rho to the N-terminal region of mDia is considered to induce a conformational change to render the protein in an open active state (Watanabe et al., 1999
). The activated mDia seems to function via the core modules FH1 and FH2 (Nakano et al., 1999
; Watanabe et al., 1999
). The FH1 region of formins is rich in proline residues, which appears to serve as a target of the actin monomer-binding protein profilin and/or proteins containing an SH3 or WW domain (Bedford et al., 1997
; Chan et al., 1996
; Evangelista et al., 1997
; Imamura et al., 1997
; Kamei et al., 1998
; Watanabe et al., 1997
). The FH2 domain, which locates C-terminal to the FH1 domain, is the most conserved region among the formin family proteins. Recent studies have shown that the FH2 domain of Bni1p, a formin required for actin cable formation in the budding yeast (Evangelista et al., 2002
; Sagot et al., 2002a
), stimulates de novo actin polymerization in vitro (Pruyne et al., 2002
; Sagot et al., 2002b
). The molecular function of FH2 domains of most formin proteins is, however, under investigation.
We had fortuitously cloned cDNA encoding a novel formin homologue, which was also identified as Fhos (formin homologue overexpressed in spleen) by other investigators during the course of the present study (Westendorf et al., 1999). Although this formin might be involved in transcription from the serum response element (Westendorf, 2001
), its role in the regulation of actin cytoskeleton has remained unknown.
Here we show that Fhos in an active form induces thick actin stress fibers, which seems to require both the FH1 and FH2 domains. Fhos localizes to the actin-based structure: the N-terminal region of Fhos probably mediates the targeting of this protein to actin stress fibers, probably via its F-actin-binding activity. We also show that the Fhos forms a homotypic complex in cells. The self-association of Fhos seems to be mediated via the FH2 domain: the domains bind to each other in a direct manner. The novel function of the FH2 domain may participate in processes that involve F-actin organization, such as promotion of actin filament assembly.
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Materials and Methods |
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Cells and fluorescence microscopy
COS-7 and HeLa cells were cultured in Dulebecco's Modified Eagle's Medium (DMEM) supplemented with 10% FCS. Cells were transfected with plasmids using Lipofectamine (Invitrogen), and cultured for 3 hours. After the addition of DMEM containing 10% fetal calf serum (FCS), cells were cultured for another 13 hours. Following three washes with PBS, cells were fixed for 15 minutes in 3.7% formaldehyde. Alternatively, cells were treated simultaneously with 1.9% formaldehyde and 0.1% Triton X-100 in PBS for the first 2 minutes, and further fixed with 3.7% formaldehyde in PBS for 15 minutes (in the case of Fig. 4D). In either case, cells were subsequently permeabilized for 4 minutes with 0.1% Triton X-100 in PBS. After being washed three times, the permeabilized cells were blocked with PBS containing 3% bovine serum albumin (BSA) for 60 minutes (Ishizaki et al., 1997; Stokoe et al., 1994
). Indirect immunofluorescence analysis was performed using an anti-Myc primary antibody (9E10, Roche, Tokyo, Japan) and AMCA (aminomethylcoumarin)-conjugated donkey anti-mouse secondary antibody (CHEMICON, Temecula, CA) or Alexa Fluor 488-labeled goat anti-mouse secondary antibody (Molecular Probes, Eugene, OR). For F-actin staining, Texas Red-X phalloidin (Molecular Probes) was used. Images were visualized with a Nikon Eclipse TE300 microscope and captured on an ORCA digital camera (Hamamatsu Photonics, Hamamatsu, Japan), with the exception of those shown in Fig. 3A and Fig. 5C, which were acquired by laser confocal microscopes LSM5 PASCAL (Zeiss, Tokyo, Japan) and Radiance 2100 (Bio-Rad), respectively.
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An in vitro pull-down binding assay
GST (glutathione S-transferase)-, MBP (maltose-binding protein)-, or His-tagged proteins were expressed in Escherichia coli strain BL21 and purified by glutathioneSepharose-4B (Amersham Pharmacia Biotech), amylose resin (New England Biolabs), or His-bind resin (Novagen, Madison, WI), respectively, according to the manufacturer's protocol. Pull-down binding assays were performed as previously described (Ago et al., 1999). Briefly, a pair of a GST-fusion (10 µg) and an MBP- or His-tagged protein (10 µg) were mixed in 1 ml of phosphate buffered saline (PBS; 137 mM NaCl, 2.68 mM KCl, 8.1 mM Na2HPO4 and 1.47 mM KH2PO4, pH 7.4) containing 1% Triton X-100. A slurry of glutathione-Sepharose-4B or amylose resin was added to the mixture, followed by incubation for 30 minutes at 4°C. After washing three times with PBS, proteins were eluted with 10 mM glutathione or with 10 mM amylose. The eluates from the resin were subjected to SDS-PAGE and stained with CBB (Coomassie Brilliant Blue).
F-actin co-sedimentation assay
Rabbit skeletal muscle actin was purchased from Cytoskeleton (Denver, CO). The depolymerized G-actin in a G-buffer (5 mM Tris, pH 8.0, 0.2 mM ATP, 0.2 mM CaCl2, and 0.5 mM dithiothreitol) was polymerized by the addition of KCl, MgCl2, and ATP at the final concentrations of 50 mM, 2 mM, and 1mM, respectively, and incubated for 60 minutes at 25°C. His-tagged Fhos-N was diluted into a F-buffer (5 mM Tris, pH 8.0, 50 mM KCl, 2 mM MgCl2, 1 mM ATP, 0.2 mM CaCl2, and 0.5 mM DTT) and clarified by centrifugation for 1 hour at 4°C at 100,000 g. Polymerized actin and His-Fhos-N at the indicated concentrations were mixed in F-buffer and incubated for 60 minutes at 25°C. The mixture was then centrifuged for 60 minutes at 100,000 g. Both supernatants and pellets were subjected to SDS-PAGE, followed by staining with CBB. In the case of the quantification of the free and bound HisFhos-N, the amounts of the protein on the gel were estimated by the image analyzer LAS1000 (Fuji Photo Film, Tokyo, Japan).
F-actin blot overlay
F-actin blot overlays were performed by the method of Luna (Luna, 1998) with minor modifications. Briefly, lysates of E. coli expressing GST-fusion proteins or purified His-tagged proteins were subjected to SDS-PAGE, and transferred to a polyvinylidene difluoride membrane (Millipore, Bedford, MA). The membrane was incubated for 60 minutes at 25°C with 50 µg/ml of F-actin in the presence of 40 µM phalloidin in TBS (20 mM Tris, pH 7.4, and 150 mM NaCl) containing 0.1% Tween-20 and 3% BSA. The blots were washed three times for 10 minutes in the same buffer and probed with an anti-actin monoclonal antibody (Roche, Tokyo, Japan). Proteins were also analyzed by immunoblot with anti-GST polyclonal antibodies (Amersham Pharmacia Biotech) or an anti-His monoclonal antibody (Qiagen, Tokyo, Japan).
Immunoprecipitation
HeLa cells (4x106 cells) were transfected with indicated plasmids using Lipofectamine (Invitrogen) and cultured for 36 hours in DMEM supplemented with 10% FCS. The cells were broken with a lysis buffer (135 mM NaCl, 5 mM EDTA, 10% glycerol, and 20 mM HEPES, pH 7.4) containing 1% NP-40. The lysate was precipitated with an anti-Myc antibody (9E10, Roche) or anti-Flag antibody (M2, Sigma-Aldrich) in the presence of protein G-Sepharose. After washing three times with the lysis buffer, the precipitants were applied to SDS-PAGE and transferred to a polyvinylidene difluoride membrane (Millipore). The membrane was probed with the anti-Flag monoclonal antibody, anti-Myc polyclonal antibodies (Santa Cruz Biotechnology, Santa Cruz, CA), anti-GFP rabbit polyclonal antibodies (Clontech) or anti-Fhos rabbit polyclonal antibodies. The anti-Fhos antibodies were raised against the C-terminal peptide (1125-1144) of human Fhos.
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Results |
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The DAD of Fhos in the C-terminus appears to regulate the Fhos activity probably by interacting with the N-terminus
Deletion of the C-terminus of Fhos seems to render the protein in an active form, as described above (Fig. 1). Alberts has recently reported that the diaphanous-related formin homology proteins, such as mDia1-3 and Bni1p, contain a conserved module in the C-termini, designated the Dia-autoregulatory domain (DAD), in which several residues situated towards the C-termini are basic ones (Fig. 2C): the DAD seems to interact intramolecularly with the N-terminus, thereby regulating the protein activity (Alberts, 2001). Alignment of the sequence of Fhos revealed that the C-terminal region of this protein (amino acids 1101-1132) exhibits a modest homology with the DAD sequences of the Diaphanous-related proteins, as shown in Fig. 2C; this was also raised by Westendorf (Westendorf, 2001
). To study the role of the DAD in the regulation of Fhos, we prepared some C-terminally truncated mutants and expressed them in HeLa cells (Fig. 2A,B). Fhos-
C3 (1-1120), which lacks the polybasic region of the DAD, could promote actin fiber formation, suggesting that the DAD plays an important role.
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We next purified GSTFhos-DAD (1081-1145) and performed an in vitro pull-down binding assay to investigate whether the DAD of Fhos is responsible for the head-to-tail interaction. As shown in Fig. 2D, GSTFhos-DAD directly interacted with HisFhos-N, whereas it was incapable of binding to HisFhos-FH1FH2. In addition, GST-Fhos (1081-1120), which lacks the polybasic region in the DAD, failed to interact with HisFhos-N (Fig. 2E), suggesting that the polybasic region is essential for the binding to the N-terminus of Fhos. On the basis of these findings, we propose that Fhos probably occurs in a closed inactive form via the DAD-mediated intramolecular interaction, and that disruption of the interaction appears to lead to activation of Fhos, thereby promoting the formation of actin stress fibers.
Fhos in an active form localizes to actin stress fibers
Active forms of Fhos, such as Fhos-C and Fhos-
N
C, not only induce stress fiber formation but also appear to be recruited to the actin-based structure (Fig. 1). To verify the localization of activated Fhos, we expressed GFPFhos-
N
C in HeLa cells and performed optical sectioning by confocal microscopy. The analysis revealed that Fhos-
N
C exactly localized to these thick actin fibers that mainly aligned with the long axis of the spindle-shaped cells, in sections throughout from the bottom to the top of the cells (Fig. 3A). The localization of this protein provides a remarkable contrast to a cytoplasmic distribution pattern of an active mDia, which can also induce the formation of actin stress fibers (Watanabe et al., 1999
). In some cells, thick actin fibers were observed to wind round and Fhos was still targeted to such unusual fibers (Fig. 3B). Furthermore, also in COS-7 cells, the active mutant protein Fhos-
N
C induced the formation of thick actin fibers and localized to the induced actin-based structure (Fig. 3C).
Localization of active Fhos to actin stress fibers is probably mediated via its N-terminal F-actin-binding region
Although a mutant protein comprising only the entire FH1 and FH2 domains (amino acids 533-1053) could induce the formation of actin stress fibers, it failed to localize to the fibers in HeLa cells (Fig. 1) and COS-7 cells (data not shown), in contrast with Fhos-C and Fhos-
N
C. Because the protein Fhos-FH1FH2 lacks a fragment N-terminal to the FH1 domain (amino acids 415-532) compared with Fhos-
N
C, it seems possible that the N-terminal region is responsible for the targeting to actin filaments. To test this possibility, we prepared the N-terminal region (amino acids 1-569), Fhos-N, as a His-tagged protein, and carried out an F-actin co-sedimentation assay. As shown in Fig. 4A, Fhos-N was pelleted together with F-actin but not precipitated in the absence of F-actin, indicative of its direct interaction with F-actin. We next titrated in different amounts of the formin to estimate a dissociation constant, and found that Fhos-N bound to actin in a dose-dependent manner with an apparent Kd of about 2 µM (Fig. 4B). The Kd value is similar to those of actin-binding proteins such as
-actinin and talin (Bennett et al., 1984
; McCann and Craig, 1997
). The specific interaction of Fhos-N with F-actin was confirmed by an F-actin overlay assay: after the lysate of E. coli expressing GSTFhos-N, GSTFhos-FH2 or GST alone was subjected to SDS-PAGE, proteins were transferred to a membrane and probed with F-actin. As shown in Fig. 4C, F-actin bound solely to Fhos-N on the filter membrane in a direct manner; F-actin did not interact with GSTFhos-FH2, GST alone or bacterial proteins.
We also tested whether the N-terminal region of Fhos associates with F-actin in vivo. When expressed in HeLa cells, Fhos-N was targeted to the stress fibers elicited by Fhos-FH1FH2 (Fig. 4D), although a part of Fhos-N was distributed in the cytoplasm. Thus, Fhos-N appears to interact with F-actin in vivo as well as in vitro.
To verify the role of the F-actin-binding activity in the localization of Fhos, we performed the F-actin overlay assay using HisFhos-N
C (533-1053) and HisFhos-FH1FH2 (415-1053); the former localized to stress fibers, but the latter did not (Fig. 1). As shown in Fig. 4E, F-actin bound directly to HisFhos-
N
C, whereas it failed to interact with HisFhos-FH1FH2, which lacks the N-terminal region. Taken together, the present findings indicate that the N-terminal region of Fhos mediates the targeting of this protein to actin stress fibers via its F-actin-binding activity.
Fhos forms a homotypic complex via the FH2 domain
It is known that the organization of individual actin filaments into higher ordered structures is controlled by bivalent actin-crosslinking proteins that contain two discrete F-actin-binding sites or by noncovalently dimerized F-actin-binding proteins (Ayscough, 1998; Janmey, 2001
; Puius et al., 1998
). To test the possibility that the F-actin-binding protein Fhos functions as a dimer, we expressed both GFP- and Myc-tagged Fhos proteins in HeLa cells and assessed the ability of the proteins to interact with each other. As shown in Fig. 5A, GFPFhos-F was co-immunoprecipitated with MycFhos-F, indicating that the full-length Fhos formed a homotypic complex in cells.
We next examined which region mediates the homotypic interaction using truncation mutants of Fhos. The truncated proteins Fhos-N
C and Fhos-FH1FH2 were co-precipitated with Fhos-F, whereas neither Fhos-N nor Fhos-FH1 interacted with Fhos-F (Fig. 5A). In addition, Myc-tagged Fhos-FH1FH2, but not Fhos-N, was coprecipitated with Flag-tagged FH2 (Fig. 5B). These findings indicate that the FH2 domain is required for formation of the homotypic complex of Fhos. The role of the FH2 domain in the intermolecular interaction was corroborated by the analysis for subcellular colocalization of truncated proteins. The protein Fhos-FH2 distributed in a cytoplasmic pattern when it is solely expressed in HeLa cells (Fig. 1A, Fig. 5C). However, when Fhos-FH2 was co-expressed with Fhos-
N
C, Fhos-FH2 became colocalized with Fhos-
N
C at thick actin fibers (Fig. 5C), supporting the idea that the FH2 domain plays a crucial role in the self-association of Fhos.
To determine whether the FH2 domains interact with each other in a direct manner, we performed an in vitro pull-down binding assay using purified proteins. As shown in Fig. 5D, MBPFhos-FH2 on the one hand was capable of directly binding to GSTFhos-FH2. On the other hand, MBPFhos-FH2 failed to interact with GST-DAD, and MBP alone did not associate with GST-FH2 (Fig. 5D). Furthermore, we prepared another FH2-containing protein with a distinct tag, HisFhos-FH1FH2, and confirmed that the FH2 domains directly bind to each other (Fig. 5E). It is thus likely that the FH2 domains homotypically interact in a direct manner, thereby mediating the self-association of Fhos.
Both FH1 and FH2 domains of Fhos are required for promoting actin fiber formation
The present study has shown that the N-terminal region of Fhos interacts with F-actin and that the FH2 domain mediates the homotypic interaction of this protein. However, the role for the FH1 domain of Fhos in vivo has remained uncertain. As shown in Fig. 1A, the FH1 domain alone was incapable of promoting the stress fiber formation. To address the question of whether this domain is necessary for actin reorganization in vivo, we expressed the FH1-truncated protein FH1
C (amino acids 1-566 plus 639-1053) (Fig. 6A). This mutant protein failed to induce the formation of actin stress fibers (Fig. 6B), albeit it retained the activity to form a homotypic complex (Fig. 6C). Thus, the FH1 domain of Fhos appears to be required for the actin reorganization, but not for the homotypic interaction.
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It seems likely that the FH2 domain of Fhos is also indispensable to actin stress fiber formation, given that the formation was elicited by Fhos-FH1FH2 but not by Fhos-FH1 (Fig. 1). To further study the function of the FH2 domain, we prepared the FH2-truncated proteins Fhos-C4 (1-886) and Fhos-
C5 (1-721) (Fig. 6A). As shown in Fig. 6B, the two proteins failed to induce the formation of actin stress fibers, supporting the idea that the FH2 domain is crucial for stress fiber formation.
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Discussion |
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In the case of mDia, binding of GTP-bound RhoA to the N-terminus is considered to induce the disruption of the DAD-mediated intramolecular interaction, i.e. activation of mDia (Alberts, 2001; Watanabe et al., 1999
). However, the N-terminus of Fhos can interact with the small GTPase Rac1 but in a guanine nucleotide-independent manner (Westendorf, 2001
). However, the interaction with Rac1 does not appear to lead to activation of Fhos, because the wild-type full-length Fhos was incapable of inducing the formation of actin stress fibers, even when co-expressed with a constitutively active or a dominant negative form of Rac (data not shown). It also seems unlikely that RhoA directly activates Fhos; GTP-RhoA was incapable of interacting with Fhos under the conditions where it bound to mDia (data not shown), which is consistent with a previous observation (Westendorf, 2001
). In addition, the possibility that Fhos acts upstream of RhoA may be also excluded, as neither expression of a dominant negative form of Rho (T19N) nor inactivation of Rho with C3 exotoxin affected the stress fiber formation induced by Fhos (data not shown). Further studies are necessary to know how Fhos is converted into the active state.
We show here that Fhos in the active state localizes to actin stress fibers (Fig. 1); by contrast, active mDia is not recruited to the actin-based structure (Alberts, 2001; Watanabe et al., 1999
). Furthermore, the present study shows that the targeting of Fhos to the stress fibers is mediated by the N-terminal region (Figs 1, 4), which can directly bind to F-actin (Fig. 4). The N-terminal regions of other formin proteins also seem to be involved in their subcellular localization: for instance, the N-terminus of the yeast formin fus1 is responsible for its recruitment to the projection tip that contains F-actin, whereas the N-terminal region of mDia is required for its localization to mitotic spindles, which are composed of microtubules in dividing cells (Kato et al., 2001
; Petersen et al., 1998
). It is, however, unknown at present whether the N-termini of these proteins directly interact with the cytoskeletal components, except that the N-terminal region of Fhos exhibits an F-actin-binding activity (Fig. 4).
As shown in this study, the FH2 domain is capable of directly mediating a homotypic interaction of Fhos (Fig. 5D,E), which is probably responsible for the present finding that Fhos exists as a homotypic complex in cells (Fig. 5A-C). Although the physiological role of the homotypic complex formation is currently obscure, the function of the FH2 domain as a mediator of homotypic interaction might underlie the actinnucleating activity of this modular domain. The self-association of Fhos may also participate in processes involving F-actin organization, such as promotion of actin filament bundling. The formation of linear actin structures is considered to be divided into two molecular processes, i.e. actin polymerization and bundling of the formed actin filaments. It has recently been shown that yeast formins Bni1p and Cdc12p are required for the actin-polymerizing step in the assembly of actin cables or contractile actin rings, respectively (Evangelista et al., 2002; Pelham and Chang, 2002
; Sagot et al., 2002a
). However, it is currently unclear whether formins regulate the bundling of the actin filaments directly or indirectly. The bundling of actin filaments can be caused by dimerization of F-actin-binding proteins, such as
-actinin (Ayscough, 1998
; Janmey, 2001
; Puius et al., 1998
). It seems thus possible that, in addition to the process of actin polymerization, Fhos may be also involved in the process of F-actin bundling via the formation of a homotypic complex.
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Acknowledgments |
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