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© The Rockefeller University Press,
0021-9525/2000//1073 $5.00
The Journal of Cell Biology, Volume 149, Number 5,
, 2000 1073-1086
Original Article |
Zyxin, a Regulator of Actin Filament Assembly, Targets the Mitotic Apparatus by Interacting with H-Warts/Lats1 Tumor Suppressor
hsaya{at}gpo.kumamoto-u.ac.jp
The mitotic apparatus plays a pivotal role in dividing cells to ensure each daughter cell receives a full set of chromosomes and complement of cytoplasm during mitosis. A human homologue of the Drosophila warts tumor suppressor, h-warts/LATS1, is an evolutionarily conserved serine/threonine kinase and a dynamic component of the mitotic apparatus. We have identified an interaction of h-warts/LATS1 with zyxin, a regulator of actin filament assembly. Zyxin is a component of focal adhesion, however, during mitosis a fraction of cytoplasmic-dispersed zyxin becomes associated with h-warts/LATS1 on the mitotic apparatus. We found that zyxin is phosphorylated specifically during mitosis, most likely by Cdc2 kinase, and that the phosphorylation regulates association with h-warts/LATS1. Furthermore, microinjection of truncated h-warts/LATS1 protein, including the zyxin-binding portion, interfered with localization of zyxin to mitotic apparatus, and the duration of mitosis of these injected cells was significantly longer than that of control cells. These findings suggest that h-warts/LATS1 and zyxin play a crucial role in controlling mitosis progression by forming a regulatory complex on mitotic apparatus.
Key Words: Cdc2 • interaction • mitotic spindle • phosphorylation • serine/threonine kinase
© 2000 The Rockefeller University Press
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Introduction |
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The warts gene (also known as lats) was identified as a tumor suppressor of Drosophila melanogaster (Justice et al. 1995; Xu et al. 1995). The warts/lats encodes serine/threonine kinase sharing a high identity with the catalytic domain of myotonic dystrophy protein kinase (DMPK) family, many of which are known to be involved in various mitotic events. Among the DMPK family proteins, Saccharomyces cerevisiae Dbf2 was found to be required for completion of mitosis; mutation in Dbf2 results in a dumbbell-shape phenotype, which is the consequence of cell division failure (Toyn and Johnston 1994). Orb6, a DMPK homologue in Schizosaccharomyces pombe, plays a role in coordinating cell morphogenesis with the cell cycle. Orb6 is known to possess dual functions of both organizing the actin cytoskeleton and negative regulation of mitosis by affecting cdc2 (Verde et al. 1998). The human Rho-associated kinase (Rho kinase) and citron-K kinase, DMPK family members, have been shown to be involved in the regulation of cytokinesis (Madaule et al. 1998; Yasui et al. 1998).
A human homologue of the warts/lats gene, termed h-warts/LATS1, has been identified and demonstrated to negatively regulate Cdc2 activity by interacting with Cdc2 in the mitotic phase (Tao et al. 1999). Analogous to its mutant in Drosophila, mice deficient of LATS1 gene have been shown to develop malignant tumors (St. John et al. 1999). Moreover, h-warts/LATS1 protein was found to localize at the centrosome in interphase and to translocate dynamically toward mitotic spindles in metaphase-anaphase, and, finally, to the midbody by telophase (Nishiyama et al. 1999). Recently, the Sid2 kinase, structural homologue of Dbf2 and a potential counterpart of h-warts/LATS1 in fission yeast, has been demonstrated to function as part of a novel signaling pathway required for onset of cytokinesis. Sid2 is a component of the spindle pole body and by virtue of its transient localization to the division site, it appears to determine the timing of ring constriction (Sparks et al. 1999). Based on these observations, h-warts/LATS1 is speculated to be heavily involved in mitotic events in mammalian cells and that loss of its function disrupts normal cell cycle regulation, leading to the development of tumors. Therefore, identification of cellular targets of the h-warts/LATS1 protein will provide clues to its precise cell cycle function and to its involvement in tumorigenesis.
During mitosis, adherent cells change morphology into a spheroid and weakly adherent form. This morphological alteration involves rearrangement of cytoskeletal systems and dissociation of the adhesion apparatus, which are under the control of biochemical status through cell cycle progression (Verde et al. 1998). Focal adhesion plaques are an adhesion apparatus for cells to contact the extracellular matrix where the growing end of actin filament attaches to the plasma membrane. At the focal adhesion complex, a number of proteins serve as linkages between transmembrane proteins and the actin cytoskeleton, regulating actin filament dynamics (Craig and Johnson 1996; Beckerle 1997). As cells proceed through mitosis, components of the focal adhesion complex are known to dissociate into the cytoplasm when bundles of actin fibers disappear. The role of these actin-regulatory proteins during mitosis, which are dispersed in the cytoplasm, remains to be established.
Zyxin is a component of the focal adhesion complex (Crawford and Beckerle 1991) and plays a central role in actin filament polymerization in mammalian cells (reviewed in Beckerle 1997). Several lines of evidence demonstrate that zyxin may function to recruit components required for the actin assembly machinery to specific sites in the cell and to stimulate spatially restricted actin polymerization (Crawford et al. 1992; Reinhard et al. 1995; Hobert et al. 1996; Prehoda et al. 1999). Interestingly, zyxin exhibits a functional nuclear export signal and has been demonstrated to shuttle between the nucleus and the sites of cell adhesion (Nix and Beckerle 1997). These findings suggest that zyxin has an unknown second function in addition to its key role in regulating actin assembly.
In this study, we have identified the interaction of h-warts/LATS1 with zyxin on the mitotic apparatus during mitosis. The localization of zyxin on the mitotic apparatus appears to be dependent on the presence of h-warts/LATS1 protein. Furthermore, we showed that zyxin is phosphorylated specifically during mitosis, most likely by Cdc2 kinase, and that this phosphorylation controls the association of zyxin with h-warts/LATS1. The interaction between zyxin and h-warts/LATS1 on the mitotic apparatus implicates a significant role for actin regulatory proteins during mitosis.
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Cell Culture, Synchronization, and Transfections
HeLa, COS7, and U2OS cells were cultured in DME/F12 supplemented with 10% fetal calf serum without antibiotics. HeLa cells were synchronized at the beginning of S phase by double thymidine block and release protocol (first 24 h incubation with 1 mM thymidine, an interval of thymidine-free incubation for 8 h, and second thymidine incubation for 14 h). Mitotic cells were collected by mechanical shake-off from the culture plate 9.5 h after release from S phase. For transient transfection, cells in 6-well plates were transfected using FuGene6 transfection reagent following the manufacturer's instructions (Boehringer Mannheim). To prepare for flow cytometry, cells were trypsinized, fixed with 70% methanol, and DNA were stained with propidium iodide. Cells were subjected to flow cytometry on FACScan® (Becton Dickinson). G1, S, and G2/M populations were calculated with ModFit 2.1 software (Varity).
Expression Plasmids
Mammalian expression plasmids were constructed by subcloning the PCR amplified fragment into hemagglutinin 1 (HA)-tagged (pCGN), FLAG-tagged (pBJ-FLAG) vectors. pBJ-FLAG, was constructed by inserting an annealed oligonucleotide between the XhoI and BamHI sites of pBJ-myc. All the PCR products were obtained using PyroBest DNA polymerase (Takara) and we confirmed their sequences. For glutathione-S-transferase (GST) fusion protein expression in bacteria, pGEX2TH-based plasmids were constructed as previously described (Masuko et al. 1999).
Antibody Preparation
Two polyclonal antibodies against h-warts/LATS1 were generated by injecting rabbits with two synthetic peptides, C1 (PVDPDKLWSDDNEEENVNDTLNG), and C2 (SDEDDQNTGSEIKNRDLVYV), coupled to keyhole limpet-hemocyanin (KLH) via the added NH2-terminal cysteine. GST–h-warts amino acids 136–700 and amino acids 136–410 were also used for immunizing rats, generating G3 and G4 antisera, respectively. The polyclonal antibody against zyxin was generated in rabbit as previously described (Macalma et al. 1996), or purchased from Santa Cruz. Monoclonal antibodies for HA-epitope (12CA5) and FLAG-epitope (M5) were obtained from Boehringer Mannheim and Sigma-Aldrich, respectively. Monoclonal antibodies for 
-tubulin (clone B512), vinculin and cyclin B were purchased from Sigma-Aldrich and Transduction Laboratories, respectively.
Immunoprecipitation
Cells were lysed on ice for 30 min with 0.5% NP-40 lysis buffer consisting of 0.5% NP-40, 25 mM Tris-Cl, pH 7.5, 137 mM NaCl, 1 mM EDTA, 1 mM EGTA, 5% glycerol, 2 µg/ml aprotinin, 20 mM β-glycerophosphate, 1 mM ABSF, 10 µM leupeptin, 1 µM pepstatin, and 1 mM Na3VO4. Lysates were centrifuged at 14,000 g for 20 min. Aliquots of supernatant (200 µg, 
2.0 mg/ml) were incubated for 1 h at 4°C with specific antibodies, and another 1 h incubation after adding 30 µl of protein G/A agarose beads (50% slurry; Calbiochem). After being washed, the bound proteins were analyzed by immunoblotting.
For coimmunoprecipitation of h-warts/LATS1 and zyxin, HeLa cells were lysed on ice for 30 min with five cell volumes of the 0.1% NP-40 lysis buffer (0.1% NP-40, 100 mM NaCl, 25 mM Tris-Cl, pH 8.0, 5 mM EGTA, 1 mM MgCl2 and 5% glycerol supplemented with 1 mM DTT, 2 µg/ml aprotinin, 20 mM β-glycerophosphate, 1 mM ABSF, 10 µM leupeptin, 1 µM pepstatin, 1 mM Na3VO4, 1 mM benzamidine, and 1 µM microcystin), and centrifuged at 14,000 g for 20 min. Precleared 400 µg quantities of cell lysate (4 mg/ml) were mixed with 3 µl of anti-zyxin antibody for 3 h on ice, then 15 µl of protein A–Sepharose beads (Amersham Pharmacia) were added and incubated for another 2 h at 4°C. After washing five times with the 0.1% NP-40 lysis buffer, the lysate was eluted by boiling for 3 min in 62.5 mM Tris-Cl, pH 6.8, containing 2% SDS and 10% glycerol. The elute was removed, made to 10 mM DTT and 0.1% bromophenol blue, boiled again and then subjected to immunoblotting. Quantification analysis was performed by MacBAS v2.5 software.
In Vitro Pull-Down Assay and Solution-Binding Assay
For pull-down assay, 30 µg of GST fusion protein was immobilized on glutathione-agarose, and equilibrated with 0.5% NP-40 lysis buffer. Aliquots of cell lysate (200 µg, 2.0 mg/ml) were incubated with the glutathione-agarose for 1 h. The bound proteins were analyzed by immunoblotting. In vitro solution binding assay was performed as described (Jin et al. 1998). In brief, 10 µg of GST fusion proteins was immobilized on the glutathione-agarose and equilibrated with buffer B (20 mM Hepes-KOH, pH 7.9, 50 mM NaCl, 1 mM MgCl2, 17% glycerol, and 2 mM DTT). The glutathione-agarose were incubated with 1 µg of His-h-warts in 200 µl of buffer B for 1 h at 4°C. After extensive washing with buffer B, the bound proteins were analyzed by immunoblotting.
In Vitro Kinase Assay
Synchronized HeLa cells were washed with ice-cold PBS and lysed on the plate with RIPA buffer as previously described (Izawa et al. 1996). Lysates were centrifuged at 14,000 g for 20 min, and the supernatant was used for the kinase assays. Kinase reaction were conducted at 25°C for 30 min in a final volume of 50 µl containing 20 mM Tris, pH 7.4, 10 mM MgCl2, 10 µCi of 
-[32P]ATP (3,000 Ci/mmol; Amersham Pharmacia), 1 µM microcystin, 8 µg of cell lysates, and 10 µg of GST-zyxin. Each reaction mixture was then chilled and mixed with 30 µl of glutathione-agarose beads (50% slurry) and 0.5 ml of ice-cold TNE buffer, followed by rocking for 30 min at 4°C. The glutathione-agarose beads were washed and boiled in 30 µl of Laemmli sample buffer to elute GST fusion proteins. The samples were resolved by 8% SDS-PAGE and visualized by autoradiography. The result of gel analyses were quantified by MacBAS (Fujifilm).
Depletion of Cdc2
Aliquots of 150 µl of mitotic cell lysate (1.0 mg/ml) were incubated with 50 µl of p13-suc1 agarose beads (50% slurry; Upstate Biotechnology) at 4°C for 45 min. After centrifugation, 50 µl of fresh p13 suc1-beads was added to the supernatant and incubated for an additional 30 min. The Cdc2 kinase assay was performed by the SignaTECT assay system (Promega) in which biotinylated peptide derived from histone H1 was used as a substrate and radiolabeled phosphorylated substrate was recovered with streptoavidin matrix. The purified active Cdc2 kinase was prepared as previously described (Kusubata et al. 1992).
Immunofluorescence Microscopy
U2OS cells were grown on a 35-mm petri dish to 70% confluence, fixed with 4% paraformaldehyde/PBS, pH 7.4, for 15 min at room temperature, followed by permeabilization with 0.2% Triton X-100/PBS, otherwise fixed with a methanol/acetone solution for 10 min on ice. A preextraction protocol was performed either with 7.5 µg/ml digitonin in KHM buffer (25 mM Hepes-KOH, pH 7.2, 125 mM potassium acetate, 2.5 mM magnesium acetate) or with microtubule stabilizing buffer (MSB; 80 mM Pipes-KOH, pH 6.8, 5 mM EGTA, 1 mM MgCl2 containing 0.5% Triton X-100) for 5 min at room temperature before fixing with chilled absolute methanol for 10 min at –20°C as described (Terada et al. 1998). After being washed, cells were incubated with the following antibodies: rabbit anti-zyxin antibody, rat anti–h-warts antibody (G3), and monoclonal mouse anti–-tubulin antibody (B512). This was followed by incubation with FITC-conjugated anti–rabbit/mouse IgG antibody (Amersham Pharmacia), Cy3-conjugated anti-rat IgG antibody (Amersham Pharmacia), and Texas red–conjugated anti-mouse IgG antibody (Molecular Probes). The stained cells were mounted with 1,4-diazabicyclo-[2,2,2]-octane/glycerol, and observed with confocal microscopy (Fluoview; Olympus). Images were obtained separately by independent excitation at 488/568 nm to minimize overlapping signals, and were processed using Photoshop software (Adobe).
Microinjection
U2OS cells were grown on 35-mm petri dishes to 75% confluency and microinjected using semi-automatic micro-manipulator/injector (Eppendorf 5171/5246). Cells in prometaphase were selected for injection on the basis of morphology by phase contrast images, and injected with a 1.0 mg/ml solution of purified GST fusion proteins and rhodamine-tubulin (Cytoskeleton) in PBS, pH 6.9, supplemented with a final concentration of 0.5 mM GTP. The microscopical stage was maintained at 37°C and the procedure was completed within 20 min to minimize pH changes. After injection, cells were incubated at 37°C for 20 min for rhodamine-tubulin to be distributed to the mitotic spindle, followed by detergent preextraction (7.5 µg/ml digitonin in KHM buffer) and a methanol fixation protocol as described above.
Synchronized HeLa cells were injected into the cytoplasm with a combination of 1.0 mg/ml solution of purified GST fusion proteins together with 1.0 mg/ml β-galactosidase (Sigma-Aldrich). Cells were fixed with 0.5% glutaraldehyde/PBS, pH 7.2, at subsequent time points, followed by incubation with 1 mg/ml of 5-bromo-4-chloro-3-indolyl-β-D-galactopyranoside (X-gal) in 150 mM NaCl, 0.01% sodium deoxycholate, 0.02% NP-40, 2 mM MgCl2, 5 mM K3Fe(CN)6, and 5 mM K4Fe(CN)6 for 12 h at 37°C. After removing the X-gal solution, cells were overlaid with acreto-orcein (Merck) in 60% acetic acid to visualize chromatin.
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An additional experiment to confirm the interaction of zyxin with h-warts/LATS1 was performed. Two polyclonal antibodies were raised against h-warts/LATS1 by injecting two KLH-conjugated synthetic polypeptides, C1 (amino acids 1,041–1,063) and C2 (amino acids 1,111–1,130), into rabbits. Endogenous h-warts/LATS1 was immunoprecipitated by the anti-C1 antibody and was detected at immunoblotting by the anti-C2 antibody (Fig. 1 D, lane 8). When the COS7 cell lysate expressing HA-tagged zyxin (full-length) was immunoprecipitated with the anti-C1 antibody, HA-zyxin (full-length) was coprecipitated with endogenous h-warts/LATS1 (Fig. 1 E, lane 3).
Furthermore, we tested whether endogenous zyxin and h-warts/LATS1 interact in vivo. Using anti-zyxin antibody generated in rabbits, zyxin was immunoprecipitated from HeLa cell lysate. The endogenous h-warts/LATS1 was detected in the immunoprecipitate (Fig. 1 F). Although comparison of the band profiles revealed that the small fraction of h-warts/LATS1 (9%) interacts with zyxin, these results indicate the association of h-warts/LATS1 and zyxin in intact cells.
Since zyxin harbors three copies of LIM domain in the COOH-terminal third of the molecule (Fig. 2 A), known as a protein–protein interacting structure, we first examined whether the LIM domain of zyxin serves as a binding interface for h-warts/LATS1 interaction. COS7 cell lysates expressing HA-tagged zyxin either full-length, NH2-terminal two-thirds (
1) or COOH-terminal third (2), which contains three LIM domains, were incubated with GST–h-warts/LATS1 (amino acids 136–700) fusion protein bound to glutathione-agarose beads (Fig. 2 B, lanes 1–3). The pull-down assay revealed that HA-zyxin2 coprecipitated with GST–h-warts/LATS1 but HA-zyxin1 did not (Fig. 2 B, lanes 7 and 9). Unexpectedly, the full-length HA-zyxin was hardly detectable in the GST–h-warts precipitate (Fig. 2 B, lane 5).
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3) and GST-zyxin-LIM1/2/3 (2) were found to bind with purified h-warts protein, the other GST-zyxin mutants did not (Fig. 2 C). This in vitro binding experiment demonstrated that zyxin directly interacts with h-warts/LATS1 and that the region containing both LIM1 and LIM2 domains of zyxin is essential for their binding. Interestingly, consistent with the findings shown in Fig. 2 A, GST-zyxin (full-length) did not interact with His-tagged h-warts/LATS1. However, their association was detected in in vivo binding assays (Fig. 1C, Fig. E, and Fig. f). Based on these findings, we speculated that the LIM1/2 domains are masked in full-length zyxin and that an intramolecular and/or intermolecular modification may regulate the interaction between zyxin and h-warts/LATS1.
Localization of h-warts/LATS1–Zyxin Complex to Mitotic Apparatus
Next, we compared the subcellular localization of h-warts/LATS1 and zyxin by immunocytochemical analysis. We raised antibody against zyxin (amino acids 24–35) in rabbits by the procedure described by Macalma et al. 1996. Consistent with their previous characterization, this antibody recognized a single band of 82 kD, which is described as the molecular mass of full-length zyxin by immunoblotting (Fig. 3 A). Indirect immunofluorescent studies revealed that the antibody specifically detected concentrated zyxin at the focal adhesion plaques, where the bundles of actin filaments end (Fig. 3 B). In the mitotic cells, the characteristic staining of zyxin was found to disappear from focal adhesions and was seen as a diffuse cytoplasmic distribution (Fig. 3 C). A similar change in subcellular distribution was observed in vinculin, another focal adhesion protein with a proline-rich stretch functionally related to zyxin, as cells retracted and rounded up during mitosis (data not shown). Notably, with careful observation of the zyxin immunostaining, a zyxin signal was barely seen at the mitotic apparatus (Fig. 3 C, b, arrows). This signal became more distinct when cells were fixed with acetone/methanol solution (Fig. 3 D).
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1 and GST-zyxin2 were processed for the in vitro kinase assay. GST-zyxin1, which corresponds to the NH2-terminal two thirds of zyxin, was significantly phosphorylated with mitotic cell lysate whereas no phosphorylation was detected in GST-zyxin2 (Fig. 5 D).
Characterization of Zyxin-Kinase during Mitosis
To address the class to which zyxin-kinase belongs, we used various specific inhibitors that have been developed for kinases. The kinase assay was performed with mitotic cell lysates which were preincubated with various kinase inhibitors (Fig. 6 A). GST-zyxin phosphorylation activity in the cell lysate was specifically inhibited not only when the mitotic cell lysate was preincubated with the broad serine/threonine kinase inhibitor staurosporine (100 nM), but also after preincubation with olomoucine, which is a specific inhibitor of Cdc2 (Fig. 6 A). Therefore, to examine whether Cdc2 kinase is the responsible kinase for zyxin phosphorylation in the mitotic cell lysate, we prepared mitotic cell lysate depleted of Cdc2, which should contain the full complement of mitotically active kinases except for Cdc2, including kinases activated downstream of Cdc2 (Fig. 6 B). By monitoring the total protein concentration and the Cdc2 kinase activity of the depleted mitotic cell lysate (Fig. 6 C), we found that phosphorylation of GST-zyxin was significantly inhibited by depleting Cdc2 from the mitotic cell lysate (Fig. 6 D, lane 3). Addition of active Cdc2 complex to the Cdc2-depleted mitotic cell lysate restored the phosphorylation activity (Fig. 6 D, lane 4), indicating that loss of zyxin phosphorylating activity was due to removal of Cdc2 but not to other components in the lysate. Furthermore, the purified Cdc2 kinase complex was sufficient for zyxin phosphorylation without requiring any other components (Fig. 6 E). These data demonstrate that Cdc2 is a kinase responsible for the mitosis-specific phosphorylation of zyxin in vitro, even though other active kinases are present in the mitotic lysate.
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Zyxin Is Targeted to the Mitotic Apparatus by Interacting with h-warts/LATS1
To test whether dynamic changes in zyxin localization on the mitotic apparatus is dependent on h-warts/LATS1 distribution, we attempted to disrupt endogenous zyxin localization by injecting excessive amounts of an h-warts/LATS1 fragment (amino acids 136–700) that is shown to bind preferentially to zyxin (Fig. 2 B). Prophase/prometaphase U2OS cells were microinjected with purified GST–h-warts/LATS1(136–700) fusion protein, or control GST protein. Rhodamine-labeled tubulin was injected together with the GST fusion proteins not only to distinguish injected cells but to monitor mitotic spindle organization as the cell cycle proceeds. After injection, cells were subjected to the detergent-preextraction immunostaining with anti-zyxin antibody. Signal of endogenous zyxin on the mitotic apparatus was diminished or disappeared in 64% of the GST–h-warts/LATS1(136–700)–injected cells (n = 11), whereas it was decreased in only 18% of the GST-injected control cells (n = 12; Fig. 8). These observations indicate that association of zyxin with h-warts/LATS1 is essential for targeting as well as dynamic localization of zyxin on the mitotic apparatus during mitosis.
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Regulation of the Interaction between h-warts/LATS1 and Zyxin
We have shown a physical association of zyxin with h-warts/LATS1 and that a region containing the first and second LIM domains (LIM1/2) of zyxin is responsible for the interaction. The LIM domain is a protein binding motif which is found in a wide variety of proteins involved in transcription, cell adhesion, and cytoskeletal organization (Schmeichel and Beckerle 1994; Dawid et al. 1998). Proteins with multiple LIM domains, such as zyxin, are considered to function as scaffolds for the assembly of protein complexes. To date, only cysteine-rich protein 1 (CRP1) has been reported to associate with the LIM1 domain of zyxin (Sadler et al. 1992). Our findings demonstrated that a combination of LIM1 and LIM2 domains, but not that of LIM2 and LIM3, is essential for zyxin to interact with h-warts/LATS1, suggesting that a specific protein recognition mechanism is used for their interaction. The association of h-warts/LATS1 with the full-length zyxin has been detected by in vivo but not by in vitro binding experiments. However, the deletion of the NH2-terminal region of zyxin has allowed the LIM1/2 domain to interact with h-warts/LATS1 in vitro. Therefore, we speculate that the LIM1/2 domains are masked in full-length zyxin and that the posttranslational modification, such as phosphorylation and/or proteolysis, gives rise to the conformational alterations in zyxin, exposing the LIM domains on the surface of the molecule, which allows h-warts/LATS1 to approach.
Although zyxin was first described as a phosphoprotein (Crawford and Beckerle 1991), both the mechanism and the biological significance of the phosphorylation have remained elusive. In this study, we demonstrated that the NH2-terminal region of zyxin is mitotically phosphorylated. Three lines of evidence presented here suggest that the mitotic phosphorylation of zyxin is mediated by Cdc2, a primary kinase to drive mitosis. First, depletion of Cdc2 from mitotic cell lysates completely abolished phosphorylation of zyxin. Second, purified active Cdc2 complex phosphorylated zyxin. Third, zyxin is phosphorylated during mitosis when Cdc2 is active. A number of studies have focused on the role of Cdc2 in the coordination of cellular and biochemical events during mitosis, and identification of its physiological substrates continues to represent a major challenge (Nigg et al. 1996; Nurse 2000). It cannot be completely ruled out the possibility that another kinase phosphorylates zyxin in vivo. However, the previous findings that a fraction of the cellular pool of Cdc2 is associated with the mitotic spindle, where it forms an active kinase complex with cyclin B (Bailly et al. 1989), also supports our present observations.
As predicted by our hypothesis, the Cdc2-dependent phosphorylation has been shown to allow the full-length zyxin to interact with h-warts/LATS1 (Fig. 7 A). In fact, zyxin associates with h-warts/LATS1 preferentially during mitosis (Fig. 7 B), and this interaction might be significant for the subsequent cellular events in cell division. However, the binding of phosphorylated full-length zyxin to h-warts/LATS1 was not as efficient as that of the 2 protein (Fig. 7 A), so the possibility can not be excluded that the interaction is regulated by not only phosphorylation but other unknown modifications of full-length zyxin.
Spatial Control of Zyxin Localization during Mitosis
Zyxin has been shown to dissociate from focal adhesion plaques and to distribute diffusely into the cytoplasm coincidentally with the mitotic disappearance of focal adhesions. Subsequently, a fraction of this free cytoplasmic zyxin becomes colocalized with h-warts/LATS1 on the mitotic apparatus (Fig. 3 and Fig. 4). Since zyxin plays a critical role in the actin filament assembly at focal adhesions (Beckerle 1998, Beckerle 1997), dissociation of zyxin may contribute to actin stress fiber disassembly in the mitotic cells. The other focal adhesion components, such as paxillin (Yamaguchi et al. 1997) and p130CAS (Yamakita et al. 1999), have been reported to be phosphorylated during mitosis when focal adhesions dissociate. As for zyxin, it can be speculated that the mitotic phosphorylation is a signal for triggering detachment of zyxin from adhesion sites. However, two observations presented here support the possibility that mitotic phosphorylation is required mainly to recruit zyxin to the mitotic spindle. First, although most of the zyxin became dissociated during mitosis, both phosphorylated and dephosphorylated zyxin were detected in the cells at mitosis (Fig. 5A and Fig. B). Second, the immunolocalization study demonstrated that a subfraction of zyxin localized to the mitotic apparatus (Fig. 3C and Fig. D), which was clearly detected by the preextraction method (Fig. 4 B).
Dynamic Interaction of h-warts/LATS1–Zyxin Protein Complex on the Mitotic Apparatus
The interaction between zyxin and h-warts/LATS1 on the mitotic apparatus implicates a significant role of actin regulatory proteins during mitosis. Zyxin serves as a scaffold for gathering actin regulatory proteins, such as Ena/VASP–profilactin complex or vav-small GTPase complex, at focal adhesion plaques (Beckerle 1997). In fission yeast and Drosophila, defects in profilin, which is shown to be essential to form the actomyosin contractile ring, results in the failure of cytokinesis (Balasubramanian et al. 1994; Giansanti et al. 1998). Rho GTPase-mediated signal is required for the organization of cortical components to form the contractile ring in mammalian cells (O'Connell et al. 1999). Moreover, a number of genetic analyses converge on the idea that components associated with mitotic spindle may cooperate in formation of the contractile ring by mediating the biochemical signaling or the physical interaction between two structures (Williams et al. 1995; Adams et al. 1998). All these findings support the idea that zyxin also plays a role in cell division by regulating actin filament assembly at midzone of the dividing cell.
The duration of mitosis in cells injected with h-warts/LATS1(136–700) fragment, which significantly perturbed zyxin specifying to the mitotic apparatus, was significantly longer than that of control cells, mainly due to delay in exit from mitosis (Fig. 9). An intriguing explanation for the observation is that the mislocalization of zyxin, as well as zyxin-binding partners for actin polymerization, induces discoordination of contractile ring in dividing cells, and thereby delays their exit from mitosis. Alternatively, h-warts/LATS1 enzymatic activity may be modulated by zyxin, so that disruption of their interaction results in inactivation of h-warts/LATS1 itself. It can not be excluded, however, that another, as yet unknown, protein(s) is also functionally impaired by h-warts/LATS1(136–700) fragments to produce these results.
To maintain genomic stability and proper ploidy, it is crucial that cell division occurs at the end of anaphase after chromosome segregation. The molecular mechanism through which h-warts/LATS1 serves as a tumor suppressor is unknown, but one possible explanation is that h-warts/LATS1 may play a critical role in cell division processes by forming a complex with zyxin on the mitotic apparatus. Abrogation of this interaction may involve failure in normal mitotic progression, leading to chromosomal instability, which is a hallmark of malignant tumors.
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Acknowledgments |
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This work was supported by a grant for Cancer Research from the Ministry of Education, Science and Culture of Japan (H. Saya).
Submitted: 16 November 1999
Revised: 14 April 2000
Accepted: 19 April 2000
Abbreviations used in this paper: DMPK, myotonic dystrophy protein kinase; GST, glutathione-S-transferase; HA, hemagglutinin 1; KLH, keyhole limpet-hemocyanin; X-gal, 5-bromo-4-chloro-3-indolyl-β-D-galactopyranoside.
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