RhoA-Dependent Phosphorylation and Relocalization of ERM Proteins into Apical Membrane/Actin Protrusions in Fibroblasts

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Vol. 9, Issue 2, 403-419, February 1998

RhoA-Dependent Phosphorylation and Relocalization of ERM Proteins into Apical Membrane/Actin Protrusions in Fibroblasts

Reuben J. Shaw,^* Michael Henry,^* Frank Solomon,^* and Tyler Jacks^*^¶

^*Center for Cancer Research, Department of Biology, Massachusetts Institute of Technology, Cambridge, Massachusetts 12139; and Howard Hughes Medical Institute, Cambridge, Massachusetts 02139

Submitted September 3, 1997; Accepted November 25, 1997
Monitoring Editor: Thomas D. Pollard

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

The ERM proteins (ezrin, radixin, and moesin) are a group of band 4.1-related proteins that are proposed to function as membrane/cytoskeletallinkers. Previous biochemical studies have implicated RhoA inregulating the association of ERM proteins with their membranetargets. However, the specific effect and mechanism of actionof this regulation is unclear. We show that lysophosphatidic acidstimulation of serum-starved NIH3T3 cells resulted in relocalizationof radixin into apical membrane/actin protrusions, which was blockedby inactivation of Rho by C3 transferase. An activated alleleof RhoA, but not Rac or CDC42Hs, was sufficient to induce apicalmembrane/actin protrusions and localize radixin or moesin intothese structures in both Rat1 and NIH3T3 cells. Lysophosphatidicacid treatment led to phosphorylation of radixin preceding itsredistribution into apical protrusions. Significantly, cotransfectionof RhoAV14 or C3 transferase with radixin and moesin revealedthat RhoA activity is necessary and sufficient for their phosphorylation.These findings reveal a novel function of RhoA in reorganizingthe apical actin cytoskeleton and suggest that this function maybe mediated through phosphorylation of ERM proteins.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Ezrin, radixin, and moesin (the ERM proteins) are three closely related proteins in the band 4.1 superfamily, members of whichare known to serve as membrane-cytoskeletal linkers (Tsukita andYonemura, 1997; Tsukita et al., 1997). The ERM proteins are foundin dynamic plasma membrane/actin interfaces such as ruffling membranes,cleavage furrows, and microvilli; ezrin is a component of microvilliin a number of polarized epithelia (Bretscher, 1983; Hanzel etal., 1991; Berryman et al., 1993; Franck et al., 1993; Winckleret al., 1994; Amieva and Furthmayr, 1995). Furthermore, antisenseexperiments have demonstrated that these proteins are criticalfor the formation of surface microvilli in a lymphoma cell lineas well as maintenance of cell-cell and cell-substratum adhesionin certain epithelial cells (Takeuchi et al., 1994). Expressionof a dominant negative allele of ezrin has also been shown tocause loss of microvilli in polarized epithelial cells (Crepaldiet al., 1997). It was recently reported that ezrin is involvedin the reorganization of ICAM-2 into uropods in lymphoblastomacells, sensitizing them to natural killer cells (Helander et al.,1996). This again suggests that the ERM proteins may help to reorganizeboth the cytoskeleton and membrane proteins to promote cell-celladhesion. These proteins are also closely related to the productof the neurofibromatosis type 2 (NF2) tumor suppressor gene merlin,which is mutated in certain cancer tumor types (Rouleau et al.,1993; Trofatter et al., 1993).

Several studies suggest that the ERM proteins have a bipartite structure analogous to that proposed for band 4.1, composedof an amino-terminal domain responsible for binding to integralmembrane targets [including the hyaluronic acid receptor CD44(Tsukita et al., 1994)] and a carboxyl domain that binds to theactin cytoskeleton (Turunen et al., 1994; Pestonjamasp et al.,1995). Studies performed in vitro and in vivo indicate that inresting cells the ERM proteins may exist in a head-to-tail, intramolecularassociation that masks both the membrane- and actin-binding sites(Berryman et al., 1995; Gary and Brestcher, 1995; Tsukita et al.,1997). Because all three ERM proteins have been shown to be phosphorylatedand relocalized to dynamic actin structures in a variety of celltypes in response to growth factors (Bretscher, 1989; Urishidaniet al., 1989; Fazioli et al., 1993; Nakamura et al., 1995), ithas been proposed that phosphorylation may regulate these proteinsthrough disruption of this intramolecular association; however,this has not been demonstrated experimentally.

RhoA is a member of the ras-like GTPase superfamily and has been shown to regulate the actin cytoskeleton and mitogenic signalingin response to extracellular signals (Machesky and Hall, 1996).RhoA has been tied to many cellular functions, including regulationof cell motility (Takaishi et al., 1993; Ridley et al., 1995),polarity (Strutt et al., 1997), cytokinesis (Kishi et al., 1993),and cell-cell (Tominaga et al., 1993) and cell-substratum adhesion(Laudanna et al., 1996). Of note, the ERM proteins and RhoA havebeen shown to colocalize, and moesin coimmunoprecipitates withRhoGDI, a regulator of Rho (Takaishi et al., 1995; Hirao et al.,1996). RhoA was also shown to regulate the association of ERMproteins with one potential integral membrane target, CD44 (Hiraoet al., 1996). Here, we have analyzed the relationship betweenRhoA and the ERM proteins and describe a novel morphogenetic activityof RhoA in fibroblasts: the formation of apical membrane/actinprotrusions. The ERM proteins appear to be critical componentsof these structures. Further, we report that stimulation of RhoAactivity results in phosphorylation of the ERM proteins, whichcorrelates with the formation of these structures.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Cell Lines and Transfection

NIH3T3 cells were obtained from American Type Culture Collection (Rockville, MD). R12 cells were a generous gift of M. Symons(Onyx Pharmaceuticals, Richmond, CA). R12 cells are a subcloneof Rat1 cells stably expressing the tTA tetracycline-repressibletransactivator (Resnitzky et al., 1994). All experiments wereperformed in the absence of tetracycline. For some indicated experiments,two previously characterized NIH3T3 cell lines stably expressingfull-length radixin with the hemagglutinin (HA) epitope tag attheir carboxyl terminus were utilized (Henry et al., 1995). Lysophosphatidicacid (1-oleoyl) was purchased from Avanti Polar Lipids (Alabaster,AL) and prepared in phosphate-buffered saline (PBS) with 0.6 mMCaCl₂, 0.5 mM MgCl₂, 1% bovine serum albumin (BSA) (essentiallyfatty acid free, Sigma, St. Louis, MO) as described by van Corvenet al. (1989). All cells were transfected by modified calciumphosphate with glycerol shock as previously described (Henry etal., 1995). For indirect immunofluorescence analysis, exponentiallygrowing NIH3T3 cells or R12 cells were seeded at 1-2 × 10⁵ cells onto ethanol-sterilized glass coverslips in a six-welldish and the next day were transfected with 5 µg total DNA perwell. For these experiments, 2.5 µg of each GTPase or empty pcDNA3were cotransfected with 2.5 µg of each ERM or merlin expressionconstruct. For immunoprecipitation experiments, exponentiallygrowing cells were plated at 1-2 × 10⁶ in a 100-mm dish and then transfected the next day with 20 µgtotal DNA. For these experiments, 15 µg of RhoAV14, C3, or emptyexpression plasmid were cotransfected with 5 µg of moesin or radixinexpression plasmids. Transfected cells were placed in DMEM supplementedwith 10% fetal calf serum (Hyclone, Logan, UT), for R12 cells,or DMEM supplemented with 10% calf serum (for NIH3T3 cells), for16 h and then rinsed in DMEM and placed in DMEM (0% serum) for8-12 additional hours. For lysophosphatidic acid (LPA) treatment,cells were starved as described by Buhl et al. (1995); cells werestarved 20-24 h in DMEM supplemented with 0.1% fetal bovine serumand then rinsed with DMEM and placed in DMEM alone (0% serum)for 16 h.

Expression Constructs

GTPase constructs (RhoAV14, RhoAN19, Rac1V12, CDC42V12) were cloned into the pcDNA3 mammalian expression vector and were obtainedfrom Lisa Stowers and John Chant (Harvard University, Cambridge,MA). Each of the GTPases carried the myc epitope tag at theiramino terminus. Expression plasmids encoding C3 transferase (EFC3)and empty vector (EFplink) were obtained from R. Triesmann (ImperialCancer Research Fund, London). Full-length radixin and RADC mutantdriven by $beta$ -actin or tetracycline-repressible promoter were previouslydescribed (Henry et al., 1995). Full-length merlin and moesinwere generated by reverse-transcriptase-polymerase chain reactionutilizing RNA from murine fetal brain and murine adult lung, respectively.Primer sequences for mouse merlin were 5 $'$ -GCCGTCGACGCCGGAGCCATCGCTTCTCG-3 $'$ and the reverse primer 5 $'$ -GCCGTCGACGAGTTCTTCAAAGAAGGC-3 $'$ . Primersequences for mouse moesin were 5 $'$ -GGCCGTCGACCCCAAAACGATCAGTGTGCG-3 $'$ and the reverse primer 5 $'$ -GGCCGTCGACCATGGACTCAAACTCATCAATGCG-3 $'$ .Reverse transcriptase-polymerase chain reaction fragments weredigested with Sal and directed cloned into pcDNA3 carrying anHA epitope tag directly following the Sal cloning site and ATGdirectly preceding it, such that the final construct expressedeach with the HA tag at their carboxyl terminus.

Primary Antibodies

Monoclonal antibody (mAb) 12CA5 and biotinylated 12CA5 were purchased from Boehringer Mannheim (Indianapolis, IN). mAb 9E10was purchased from Oncogene Science (Uniondale, NY). pAb CR22recognizes primarily moesin by indirect immunofluorescence, althoughit does cross-react with radixin and ezrin as previously described(Tsukita et al., 1994). Anti-CD44 rat monoclonal IM7 was purchasedfrom PharMingen (San Diego, CA).

Immunocytochemistry/Confocal Microscopy

Cells were grown on ethanol-sterilized glass coverslips as described above. Twenty-four to 30 h posttransfection, cells werefixed for 15 min with 3.7% paraformaldehyde in PBS at room temperature,washed three times in PBS, permeabilized with 0.5% Triton X-100in PBS for 10 min, and washed three times in PBS. Cells were thenblocked in 10% normal goat serum in PBS (Vector Laboratories,Burlingame, CA). The cells were then incubated in primary antibodydiluted in PBS containing 1% BSA for 30 min at 37°C, washed threetimes in PBS, and then incubated for 30 min at 37°C with the appropriatesecondary antibody diluted in PBS containing 1% BSA: fluoresceinisothiocyanate (FITC) or rhodamine-conjugated goat anti-mousefor 12CA5, or FITC goat anti-rat for IM7. In some experiments,during secondary antibody incubation, cells were stained withrhodamine-conjugated phalloidin (Molecular Probes, Eugene, OR)and/or 4,6-diamidino-2-phenylindole (Sigma) to reveal F-actinand DNA, respectively. For 12CA5 and 9E10 double labeling experiments,9E10 and rhodamine-goat anti-mouse incubations were performedas above; then, after secondary washes, cells were fixed in 2%paraformaldehyde, washed three times in PBS, and then incubatedwith biotinylated 12CA5 diluted in PBS containing 1% BSA as above,washed, and finally incubated with FITC-streptavidin diluted inPBS containing 1% BSA. Coverslips were mounted onto glass slidesusing Mowiol mounting medium (Hoescht Celanese, Charlotte, NC)containing the antifade agent 1,4 diaza-bicyclo[2,2,2] octane(Aldrich, Milwaukee, WI) at 15 mg/ml. Cells were examined by conventionalmicroscopy on an Axioplan microscope (Carl Zeiss, Thornwood, NY)using 63 × 1.4 N.A. and 100 × 1.3 N.A. objectives. For confocalmicroscopy, cells were examined with a MRC600 scanning laser confocalmicroscope (Bio-Rad Laboratories, Richmond, CA). Images were recordedon Tri-X-Pan400 film or Ektachrome Elite400 film (Eastman Kodak,Rochester, NY).

Scanning Electron Microscopy (SEM)

SEM was performed on transfected RhoAV14, CDC42V12, and pcDNA3 vector control NIH3T3 cells. Transfections were performed asabove using 2.5 µg RhoAV14 or CDC42V12 and 2.5 µg pcDNA3 or 5µg pcDNA3. Three independent transfections were examined by SEMwith more than 200 cells examined per transfection. Coverslipsfrom the same transfections were processed for anti-myc immunofluorescenceto gauge the transfection efficiency per sample. The percentageof cells demonstrating the phenotype as shown in Figure 5 forRhoV14 or CDc42V12 was nearly identical to the percentage shownto be transfected by these GTPases by anti-myc indirect immunofluorescenceon parallel coverslips. Moreover, the exact same phenotype ofhundreds of apical projections was observed in nearly all cellsof an NIH3T3 cell line stably expressing RhoAV14 and never inthe parental NIH3T3 cell line. Cells plated as described abovewere fixed in 2% gluteraldehyde (EM grade, Sigma) in PBS for 15min at 0°C, washed three times in PBS, incubated in 1% OsO₄ at0°C for 30 min, washed three times in PBS, and then dehydratedin a graded series of ethanol and dried in a critical point drierafter substitution with liquid CO₂. Dried samples were coatedwith approximately 200 Å gold/paladium using a gold sputter coater(Technics, Alexandria, VA) and were examined under a scanningelectron microscope (Amray, Bedford, MA).

Immunoprecipitation and Immunoblotting

For LPA treatment, parallel sets of NIH3T3 cells stably expressing HA-radixin were starved as above until the last incubationin DMEM alone. After 10 h in DMEM alone, cells were washed inDMEM without methionine and cysteine or DMEM without phosphateand then placed in these media for 40 min, at which time 500 µCi[³⁵S]methionine, cysteine (New England Nuclear, Boston, MA) or 1mCi ]³²P]orthophosphate (NEN) was added, respectively, and incubatedfor an additional 5 h. Cells were then treated with vehicle orLPA for indicated times. Treated cells were washed with PBS andlysed in 1 ml of RIPA-PIP buffer (50 mM Tris, pH 7.5, 1% TritonX-100, 0.5% sodium deoxycholate, 10% glycerol, 2 mM EDTA, 150mM NaCl, 0.5% SDS) with protease and kinase/phosphatase inhibitors50 mM NaF, 1 mM NaOVO₄, 50 µm phenylarsine oxide, 20 mM NaMoO₄,1 µm staurosporine, 100 nM calyculin A. Lysates were rocked at4°C for 15 min, scraped with a rubber policeman, and microcentrifugedat 14,000 × g for 15 min. An aliquot of the supernatant was thentrichloroacetic acid precipitated to equilibrate incorporatedcounts. Equilibrated supernatants were precleared with normalrabbit serum and 50% protein A-Sepharose beads (Pierce Chemical,Rockford, IL) for 1 h. After preclearing, each lysate were incubatedwith 1 µg 12CA5 (preincubated for 2 h with 50% protein A-Sepharose).After 3 h incubation with 12CA5/protein A-Sepharose, immunocomplexeswere pelleted at 1000 × g and washed three times in RIPA-PIP bufferwithout inhibitors. Sample buffer (5×) was added, and sampleswere incubated at 100°C for 5 min. Samples were resolved on 7%SDS-PAGE gels and visualized by autoradiography (after fixationand fluorometric enhancement of the ³⁵S gel).

For Rho/C3 transfection experiments, 16 h posttransfection, cells were washed in DMEM without phosphate and incubated withDMEM without phosphate for 40 min after which 1 mCi [³²P]orthophosphate was added to each plate as above and incubatedat 37°C for 8 h. Cells were then lysed and immunoprecipitatedas above. After resolving on a 7% SDS-PAGE gel, immunoprecipitateswere transferred to polyvinyl diflouride membranes (PVDF) as previouslydescribed (McClatchey et al., 1997). After Western transfer, thePVDF blot was wrapped in saran wrap, and autoradiography was usedto visualize the ³²P signal. After a sufficient exposure (2 d in Figure 8), the blotwas equilibrated in TBS-T (10 mM Tris, pH 8.0, 150 mM NaCl, 0.1%Tween 20) and immunoblotted with 12CA5, followed by a horseradishperoxidase-conjugated goat anti-mouse secondary antibody, andthe signal was visualized by enhanced chemiluminescence, as previouslydescribed (Henry et al., 1995).

Detergent Extraction Analysis

Parallel plates of NIH3T3 cells were transfected with 15 µg of either pcDNA3 or RhoAV14, along with 5 µg of HA-moesin as describedabove. At 16 h posttransfection, one set of plated cells was washedin DMEM without phosphate and incubated with DMEM without phosphatefor 40 min, and 1 mCi [³²P]orthophosphate was added to each plate as described above andincubated at 37°C for 8 h. The other set of cells was washed inDMEM without cysteine or methionine and incubated with DMEM withoutcysteine or methionine for 40 min, and 0.5 mCi [³⁵S]methionine-cysteine mix was added to each plate and incubatedat 37°C for 8 h. To obtain the detergent-soluble and -insolublefractions, cells were rinsed once in PBS, and then incubated in1 ml of Triton X-100 lysis buffer (80 mM piperazine-N,N-bis[ethanesulfonicacid], pH 6.4, 5 mM EGTA, 1 mM MgCl₂, 0.5% Triton X-100) withprotease and kinase/phosphatase inhibitors (see above) for 40s. Solubilized material was collected as the detergent-solublefraction. The material remaining on the tissue culture dish wasincubated in RIPA-PIP buffer as described above and designatedthe detergent insoluble fraction. Samples were then immunoprecipitatedwith 12CA5 antibody (see above).

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

LPA-induced Relocalization of Radixin Is Blocked by C3 Transferase

LPA induces the formation of focal adhesions and stress fibers in quiescent Swiss3T3 fibroblasts in a manner dependent onRhoA activity (Ridley and Hall, 1992). To investigate the roleof Rho in the regulation of ERM proteins, we examined the effectof LPA treatment on radixin localization, utilizing NIH3T3 cellsstably expressing full-length radixin, epitope-tagged at its carboxylterminus (Henry et al., 1995). Serum deprivation of these cellsresulted in decreased radixin immunostaining and diffuse localizationwith a reduction (although not total disappearance) of actin stressfibers (Figure 1A, panels a and b). Within 3-5 min after LPA treatment,radixin was redistributed into short apical membrane protrusionsgrossly similar to microvilli and to peripheral actin protrusionsas well (Figure 1A, panels c-h). This result was confirmed usinga polyclonal antibody that recognizes all three ERM proteins endogenouslyin NIH3T3 cells (Figure 1B, a and c). These apical structuresalso contained F-actin as visualized by rhodamine phalloidin (seearrows in Figure 1A, panels e-h; Figure 1B, panels c and d).

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Figure 1. LPA-induced relocalization of radixin into apical membrane/actin protrusions in NIH3T3 cells. (A) Indirect immunofluorescencewas performed on NIH3T3 cells stably expressing HA-epitope-taggedradixin. These cells were serum starved, and then treated withvehicle for 15 min (a and b), or with LPA (6 µM) for 3 min (cand d), 5 min (e and f), or 15 min (g and h). HA-radixin localization(using the 12CA5 mAb against the HA epitope) is shown in panelsa, c, e, and g, and F-actin localization (using rhodamine phalloidin)is shown in b, d, f, and h. Starting 3-5 min after LPA treatment,radixin was relocalized into peripheral and apical membrane protrusionsthat also contain actin. These results were observed in threeindependent stable cell lines. Arrows denote colocalization ofHA-radixin and actin in LPA-induced membrane protrusions. (B)NIH3T3 cells were serum starved and then treated with vehicle(a and b) or LPA for 15 min (c and d) and visualized for endogenousERM proteins (a and c) using the CR22 polyclonal antibody or F-actinusing rhodamine phalloidin (b and d). Arrows indicate the colocalizationof ERM proteins and actin in membrane protrusions. Similar resultswere observed when a radixin-specific antibody was used as well.These results demonstrate that endogenous ERM proteins are similarlyrelocalized after LPA treatment as the exogenous epitope-taggedform of radixin. Bar, 10 µm.

Given that RhoA is a major mediator of LPA-induced actin rearrangement (Ridley and Hall, 1992; Jalink et al., 1994; Chrzanowska-Wodnickaand Burridge, 1996; Kozma et al., 1997), we examined whether inactivationof RhoA by C3 transferase might inhibit the LPA-induced radixinrelocalization. C3 transferase catalyzes the ADP ribosylationof RhoA on asparagine 41, which is thought to cause its functionalinactivation (Aktories et al., 1989; Sekine et al., 1989). Tointroduce C3 into the radixin-expressing cell lines, we transientlycotransfected expression plasmids carrying the C3 cDNA and a lacZcDNA, or the lacZ plasmid with an empty vector into NIH3T3 cellsstably expressing HA-radixin. The cells were then serum starvedand treated with LPA. Double immunostaining for $beta$ -gal and radixindemonstrated that the presence of C3 significantly reduced thelocalization of radixin in apical structures after LPA treatment;only 15% of the C3-transfected cells showed the relocalizationcompared with 66% in the lacZ-only control (Figure 2). It shouldbe noted, however, that prolonged C3 treatment leads to cell roundingand loss of adhesion in fibroblasts (Paterson et al., 1990), raisingthe possibility that the inhibition of radixin relocalizationcould be a secondary consequence of other changes in cell shapeor adhesion. 4,6- Diamidino-2-phenylindole staining of DNA wasperformed in all these experiments, and examination of the C3-expressingcells revealed that their nuclei are morphologically intact, incontrast to those treated with many other stimuli that induceapoptosis, suggesting that the inhibition of radixin relocalizationis not simply a consequence of C3 inducing apoptosis.

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Figure 2. C3 pretreatment blocks LPA-induced relocalization of radixin in NIH3T3 cells. (A) NIH3T3 cells stably expressing HA-radixinwere transfected with expression plasmids encoding lacZ and C3transferase (a and b) or lacZ alone (c and d) and then serum-starvedand treated with LPA for 15 min. LacZ (b and d) localization (red)is shown to indicate transfected cells, and HA-radixin localization(green) is shown in panels a and c. C3-transfected cells (arrowsin panel a) show a lack of radixin localization into apical protrusionsafter LPA treatment. Bar, 10 µm. (B) Percentage of cells in lacZonly or lacZ plus C3 transfections displaying relocalization ofradixin to apical protrusions after LPA treatment. Results ofthree independent experiments are shown. One hundred transfectedcells were counted for each sample. Errors bars denote SD of themean.

RhoA Is Sufficient to Relocalize ERM Proteins to Apical Membrane/Actin Protrusions

Given that C3 treatment reduced LPA-induced relocalization of radixin, we next addressed whether activated RhoA might be sufficientfor radixin relocalization. Expression plasmids encoding myc epitope-taggedactivated (RhoAV14) or dominant negative (RhoAN19) alleles ofRhoA were cotransfected with radixin (tagged with the HA epitope)into NIH3T3 cells. The cells were then starved and visualizedfor RhoA and radixin localization by indirect immunofluorescenceusing the myc and HA epitope tags, respectively. Radixin alonein serum-starved NIH3T3 cells colocalized with peripheral actin,including a few apical protrusions (Figure 3a). In cells cotransfectedwith RhoAV14, radixin was highly concentrated in approximately100-200 apical membrane/actin protrusions in >80% of the transfectedcells. These protrusions were morphologically similar to the apicalstructures induced by LPA treatment (Figure 3, c and d; see alsoFigure 5b, described below). All cells displaying the radixinrelocalization also contained profuse stress fibers, a hallmarkfeature of activated Rho in fibroblasts (Figure 6d and our unpublishedresults). Relocalization of endogenous ERM proteins by transfectionof RhoAV14 was also observed (our unpublished results). The localizationof radixin to apical protrusions was not observed in cells transfectedwith the dominant-negative RhoAN19 (Figure 3, panels e-f). Importantly,transfection with activated alleles of two other small GTPasesin the Rho subfamily, Rac and CDC42, also failed to induce radixinrelocalization to apical structures but did alter radixin's subcellulardistribution (Figure 3, panels b, g, and h). Activated CDC42 inducedfilopodial structures in a large percentage of transfected cellsas previously reported (Kozma et al., 1995; Nobes and Hall, 1995),but these projections were larger in length and diameter thanthe RhoA-induced structures and were always located in the ventralplane of the cell along the substratum, rather than on the apicalsurface (see Figures 3b and 5c).

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Figure 3. Cotransfection of RhoAV14, but not RhoAN19, RacV12, or CDC42V12, with radixin is sufficient to cause relocalization to apicalmembrane/actin protrusions in NIH3T3 cells. NIH3T3 cells weretransiently transfected with radixin (a and b), radixin and RhoAV14(c and d), radixin and RhoAN19 (e and f), radixin and RacV12 (gand h), and radixin and CDC42V12 (b). All GTPase constructs weremyc epitope tagged. HA-radixin (a, b, c, e, and g) and myc-taggedGTPases (d, f, and h) localizations are shown. Cotransfectionsfollowed by immunolocalization were performed in 12 independentexperiments. Radixin localization in the presence of activatedRhoA was further verified by transfection of radixin into twoindependent NIH3T3 cell lines stably expressing the RhoAV14 allele.In all experiments, at least 100 transfected cells were examinedfor each condition, and cells shown are representative of > 80%of the transfected cell population. In the presence of activatedRhoA, but not dominant negative RhoA, activated Rac, or activatedCDC42, radixin localized into apical membrane protrusions. $alpha$ -mycand actin staining were used in all experiments to verify functionalexpression of RhoAV14. Bar, 10 µm.

To determine whether the RhoA-induced radixin localization was unique to this protein or was a more general property of theERM family, we examined the localization of moesin under theseconditions. We also tested the effect on the product of the NF2tumor suppressor gene, merlin, which is a more distantly relatedmember of this family. In addition, we addressed whether thiswas a unique property of NIH3T3 cells by performing parallel transfectionswith R12 cells (a Rat1 cell derivative). In both serum-starvedNIH3T3 and R12 cells, exogenous moesin and radixin were concentratedin apical actin protrusions when cotransfected with RhoAV14, butnot with RhoAN19, RacV12, or CDC42V12, or when transfected withouta GTPase (Figure 4). In all experiments, the localization of moesinor radixin was indistinguishable. In contrast, merlin, which localizesvery similarly to radixin and moesin when transfected alone inthese cells (compare panels a and g of Figure 4), was not presentin apical protrusions in the presence of activated RhoA (Figure4h), suggesting that the redistribution of ERM proteins in thesestructures is a specific effect. Interestingly, however, merlinbecame less clearly plasma membrane-associated in cells expressingRhoAV14. Using antiCD44 staining as a marker for the RhoA-inducedapical structures (see below), we confirmed that these were stillformed in the merlin plus RhoAV14 cotransfectants (our unpublishedresults). Additionally, experiments using a HA-tagged murine ezrinconfirmed that it behaved as moesin and radixin in these experiments(our unpublished results).

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Figure 4. Cotransfection with RhoV14 relocalizes moesin, but not merlin, to apical membrane protrusions in R12 cells. Cells were transientlytransfected with moesin (a), moesin and RhoAV14 (b and c), moesinand RhoAN19 (d), moesin and RacV12 (e), moesin and CDC42v12 (f),merlin (g), or merlin and RhoAV14 (h). Moesin and merlin weretagged with HA-epitope tag at their C termini. HA-moesin (a-f)or HA-merlin (g and h) immunolocalization using the 12CA5 mAbis shown. Panels b and c represent two different focal planesof the same cell to better illustrate the nature of the apicalprotrusions. All cells presented here were also shown to be positivefor GTPase expression (where applicable) by $alpha$ -myc immunostaining.These transfections were performed seven independent times, andat least 100 transfected cells were examined for each condition.Cells shown are representative of >90% of the transfected cellpopulation. Bar, 10 µm.

To characterize the RhoA-induced apical structures more completely, and to clarify the difference between the protrusionsinduced by CDC42 and RhoA, we performed SEM on NIH3T3 cells transfectedwith RhoAV14, CDC42V12, or empty vector (see MATERIALS AND METHODS).As shown in Figure 5, SEM revealed that serum-starved cells transfectedwith empty vector only had a smooth apical surface, while theRhoAV14 transfectants were covered with 100-200 apical membraneprotrusions and villus-like blebs. Moreover, the same phenotype,consisting of hundreds of apical projections, was observed in>75% of all cells of an NIH3T3 cell line stably expressing RhoAV14(our unpublished results). The number and size of the protrusionsin RhoAV14-transfected cells observed by SEM correlated extremelyclosely with the immunostaining of the ERM proteins in the presenceof RhoAV14, suggesting that these proteins are localized in themembrane protrusions visualized by this technique. Furthermore,as suggested by indirect immunofluorescence, the CDC42V12 transfectantsshowed longer, peripherally localized filopodia, and these cellsdisplayed an absence of apical surface structures (Figure 5c).

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Figure 5. SEM of RhoAV14-induced apical membrane structures and CDC42-induced filopodia. SEM was performed on serum-starved vector control(a), RhoAV14-transfected (b), and CDC42V12-transfected (c) NIH3T3cells. Note the number and length of the apical membrane protrusionsinduced by the presence of activated RhoA. Three independent transfectionswere examined by SEM with more than 200 cells examined per transfection.The percentage of cells demonstrating the phenotype as shown forRhoAV14 or CDC42V12 was nearly identical to the percentage shownto be transfected by either GTPase when a parallel coverslip wasanalyzed by indirect immunofluorescence. Furthermore, <2% of vector-onlytransfectants had apical structures similar to those seen withRhoAV14, and they were highly reduced in number and size (ca.20 per cell as opposed to 100-200). Bar, 10 µm.

A Carboxyl Domain of Radixin Modulates the RhoA-dependent Apical Protrusions

Given that activated RhoA induced the localization of ERM proteins to apical protrusions and the previous demonstration thatERM proteins are critical for microvilli formation in polarizedepithelial and lymphoma cells (Takeuchi et al., 1994; Crepaldiet al., 1997), we tested whether the ERM proteins may be criticalmodulators of the membrane protrusions formed in response to Rhoactivation. We utilized a previously characterized mutant composedof the carboxyl-terminal domain of radixin, denoted RADC, whichcorresponds roughly to the second half of the protein. This fragmentis capable of inducing long apical processes when transfectedinto HeLa cells and NIH3T3 cells in the presence of full serum(Henry et al., 1995). A similar mutant of ezrin induced analogousprocesses in other cell types (Martin et al., 1995). This activityof the C-terminal domains was not observed upon transfection ofthe full-length molecules and was suppressed by the N-terminaldomain in trans in some instances, suggesting the protein maynormally be found in an inactive intramolecular association (Henryet al., 1995; Martin et al., 1995). This model is further supportedby several studies in vitro (Gary and Bretscher, 1995; Magendantzet al., 1995).

First, we investigated whether the RADC polypeptide alone would induce apical membrane protrusions in the absence of serumfactors (which activate endogenous Rho and other GTPases) in NIH3T3or R12 cells. As shown in Figure 6, a and b, this mutant localizedto actin stress fibers in these cells, without causing formationof long apical protrusions. However, upon cotransfection of RhoAV14with RADC, the formation of long apical protrusions was readilyobserved (Figure 6, c and d). This result demonstrates that activatedRhoA is sufficient to reproduce the effect of this mutant in fullserum, suggesting that activation of endogenous RhoA by serummay be necessary for the previously reported activity of thismutant. Moreover, we observed that the protrusions induced byRhoA in the presence of this radixin mutant appeared distinctfrom those normally induced by RhoA. Confocal imaging analysisutilizing combined optical sections revealed a decreased numberand increased diameter and length of protrusions induced in thepresence of RhoAV14 and RADC, as compared with those caused byRhoAV14 and full-length radixin (Figure 6, e and f).

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Figure 6. Modulation of RhoA-dependent apical protrusions by a radixin carboxyl-terminal domain mutant. R12 cells were transfected withthe RADC mutant alone (a and b), or RADC and RhoAV14 (c and d).HA-RADC localization shown in panels a and c, and F-actin as visualizedby rhodamine phalloidin are shown in b and d. Note colocalizationof RADC with stress fibers in absence of RhoAV14 (arrows in aand b) and localization of actin into profuse stress fibers andlong apical processes containing RADC in the presence of RhoAV14(arrows in c and d). NIH3T3 cells were transfected with RhoAV14and full-length radixin (e) or RhoAV14 and RADC mutant (f) andthen serum-starved and subjected to confocal microscopy analysis.Panels e and f represent combined optical sections of HA-radixin(e) or HA-RADC (f) immunolocalization. NIH3T3 cells were transfectedwith lacZ and RhoAV14 (g) or lacZ, RhoAV14, and RADC (h) and thenserum-starved and subjected to double immunostaining for lacZand another marker of RhoA-induced apical structures, CD44. CD44immunolocalization is shown in g and h. LacZ-positive cells (i.e.,transfectants) are indicated by arrows. Transfections were performedin four independent experiments. Twenty-five percent of the cellstransfected with RADC and RhoAV14 displayed the extremely longapical protrusions as seen in panels c, f, and h, whereas cellstransfected with RhoA alone or RhoA plus full-length radixin nevershowed this phenotype. These results suggest that the presenceof a mutant form of radixin can directly alter the size and numberof RhoA-induced apical protrusions, but that additional factors(e.g., cell cycle) may control the full expressivity of this phenotype.Bar, 10 µm.

To examine whether the longer protrusions caused by RhoA and RADC were formed in addition to those induced by endogenous ERMproteins, we utilized immunostaining for CD44, a protein thatwe have found to be specifically enriched in the Rho-induced apicalstructures. CD44 has been proposed to be a integral membrane targetfor the ERM proteins (Tsukita et al., 1994; Hirao et al., 1996).Cells were cotransfected with lacZ, lacZ, and RhoV14, or lacZ,RhoAV14, and RADC, and processed for double immunofluoresenceto detect lacZ and CD44. We observed that the fine layer of CD44-richapical protrusions induced by RhoAV14 alone was disrupted in thepresence of the RADC mutant. Instead, fewer, longer CD44-positiveprocesses were present in these cells (Figure 6, panels g andh). These data suggest that by introducing a mutant form of radixin,the character of the RhoA-induced apical membrane protrusionscan be altered, both in size and quantity.

Rho Is Necessary and Sufficient for Serine/Threonine Phosphorylation of ERM Proteins

To investigate further whether the ERM proteins are downstream targets of RhoA in the formation of the apical membrane protrusionsand to elucidate the mechanism by which this regulation mightoccur, we examined the phosphorylation of radixin in responseto LPA treatment. Parallel plates of NIH3T3 cells stably expressingHA-radixin were metabolically labeled with [³⁵S]methionine or [³²P]orthophosphate during serum starvation, and then stimulatedwith 6 µM LPA. As shown in Figure 7, LPA led to a rapid and prolongedthreefold increase in the level of phosphorylation of radixinwithin one minute after treatment. The increase in radixin phosphorylationclearly preceded relocalization of radixin in these cells (seeabove, Figure 1A), and the level of phosphorylation remained constantbetween 1 and 15 min after LPA treatment (Figure 7). There wasno increase in the steady-state level of radixin in these experiments,as revealed by ³⁵S-labeled controls (Figure 7). Radixin phosphorylated under theseconditions did not react with anti-phosphotyrosine antibodiesin Western blots, suggesting that the modification occurred onserine/threonine residues (our unpublished results).

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Figure 7. LPA treatment of NIH3T3 cells induces phosphorylation of radixin within 1 min. Metabolically labeled NIH3T3 cells stably expressingHA-radixin or parental (mock) NIH3T3 cells were serum-starved,then treated with LPA (6 µM) for various timepoints as indicated.Cell lysates were immunoprecipitated with 12CA5 ( $alpha$ -HA) mAb. Radixinis indicated by arrowhead at left. Radixin phosphorylation wasincreased threefold within 1 min of LPA treatment and remainedconstant for 15 min. Note background band (*) whose orthophosphatecontent was not apparently modulated by LPA. Molecular size standardsare indicated at right. The data shown are representative of fourindependent experiments.

To examine whether RhoA activity was necessary and sufficient for ERM phosphorylation, we cotransfected R12 and NIH3T3 cellswith HA-tagged radixin or moesin along with C3, RhoV14, or anempty expression vector. The cells were then serum starved andradiolabeled with [³²P]orthophosphate, and the transfected ERM proteins were immunoprecipitatedand resolved by SDS-PAGE. To ensure that equivalent levels ofHA-radixin or moesin were produced and immunoprecipitated undereach condition, immunoprecipitates were transferred to PVDF afterSDS-PAGE. After exposure of the ³²P signal, the blots were probed with anti-HA antisera and thesignal was detected by chemiluminescence (Figure 8). In both celltypes, coexpression of C3 transferase reduced the level of phosphorylationof both radixin and moesin by at least 50% below the basal levelobserved in cells transfected with vector alone; protein levelswere not affected (Figure 8; our unpublished results). Moreover,cotransfection with RhoAV14 led to strong induction (sevenfoldin Rat1 cells; 2.5 fold in NIH3T3 cells) of moesin and radixinphosphorylation, again without affecting protein levels (Figure8; our unpublished results). These results indicate that RhoAactivity is necessary and sufficient to induce phosphorylationof the ERM proteins.

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Figure 8. RhoA activity is necessary and sufficient for phosphorylation of moesin. R12 or NIH3T3 cells were transfected with vectoronly, HA-moesin only, HA-moesin and RhoAV14, or HA-moesin andC3 transferase, as indicated. Cells were then serum starved andmetabolically labeled with [³²P]orthophosphate; cell lysates were immunoprecipitated as in Figure7. To ensure that equivalent levels of HA-moesin were expressedand immunoprecipitated, immunoprecipitated samples were transferredto PVDF after SDS-PAGE and immunoblotted with 12CA5 antibody;signal was detected by enhanced chemiluminescence. Moesin is indicatedby arrowhead at left. The presence of RhoA increased the basallevel of moesin phosphorylation by 7-fold in R12 cells and 2.5-foldin NIH3T3 cells, while C3 treatment reduced the basal level ofphosphorylation by at least 50% in both cell types (top panel).Protein levels were approximately equivalent in all conditionstested (bottom panel). The data shown are representative of threeindependent experiments.

As a first step in addressing the functional consequence of this Rho-dependent phosphorylation, we examined the detergentextractibility of phosphorylated and unphosphorylated moesin.Specifically, we compared the Triton X-100 extractibility of moesinmetabolically labeled with either [³⁵S]methionine or [³²P]orthophosphate, in the presence or absence of RhoAV14. As shownin Figure 9, in sharp contrast to ³⁵S- labeled moesin, ³²P-labeled moesin was found predominantly in the Triton X-100 insolublefraction. This result is consistent with the phosphorylated formof the protein having a greater affinity for the cytoskeleton.Furthermore, coexpression of RhoAV14 increased the percentageof total (³⁵S-metabolically labeled) moesin found in the insoluble fraction,which presumably reflects the increase in moesin phosphorylationcaused by the activated RhoAV14 allele.

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Figure 9. ³²P-labeled moesin partitions with the Triton X-100 insoluble fraction. NIH3T3 cells were transfected with HA-moesin only orHA-moesin and RhoAV14 as indicated. Cells were then serum starvedand metabolically labeled with [³²P]orthophosphate or [³⁵S]methionine/cysteine as described in Figure 8, and then subjectedto 0.5% Triton X-100 detergent extraction. Soluble (S) and insoluble(I) fractions were immunoprecipitated with 12CA5 antibody. Incontrast to total (³⁵S) moesin, ³²P-labeled moesin was found almost exclusively in the insolublefraction. Also, coexpression of RhoAV14 increases the percentageof moesin in the insoluble fraction. The data shown are representativeof three independent experiments.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Previous studies have demonstrated that RhoA and the ERM proteins colocalize in sites of cell-cell adhesion and in membraneruffles in epithelial cells (Takaishi et al., 1995). Furthermore,a detailed biochemical analysis has indicated that in cell lysates,RhoA modulates the affinity of the ERM proteins with a membranefraction and specifically its association with the integral membraneprotein CD44 (Hirao et al., 1996). However, the mechanism of actionor physiological consequence of the connection between RhoA andthe ERM proteins has remained unclear. Here, we have more closelyexamined the relationship between the ERM family of membrane/cytoskeletallinkers and the RhoA GTPase. We found that in NIH3T3 cells, treatmentwith LPA induced the rapid phosphorylation and subsequent dramaticrelocalization of radixin into peripheral and apical membraneprotrusions. Notably, LPA-induced relocalization of the ERM proteinswas blocked by C3 transferase. Furthermore, we have shown thatRhoA activity is both sufficient and necessary for ERM proteinphosphorylation. Under these conditions, RhoA activity was alsosufficient for the relocalization of radixin and moesin into apicalmembrane protrusions in two different cell types. These data suggestthat growth factors may mediate the localization of the ERM proteinsvia a RhoA-dependent kinase, such as protein kinase N, Rho-kinase,or PRK2 (Amano et al., 1996; Leung et al., 1996; Watanabe et al.,1996; Amano et al., 1997; Vincent and Settleman, 1997). One ormore of these kinases may serve either alone or in concert withother RhoA-dependent signals to cause ERM proteins to alter theircytoskeletal localization into the microvilli-like protrusions.Furthermore, the fact that a mutant form of radixin was able toalter the number and size of the Rho-dependent protrusions mayindicate the ERM proteins are critical components and/or regulatorsof these structures. Interestingly, we have found that phosphorylationof the related merlin protein is regulated by stimuli known toactivate Rho (Shaw et al., submitted), although the localizationof this protein in the presence of activated Rho is clearly distinctfrom that of the ERM proteins. This difference may be explainedby the presence of an actin-binding motif in the ERM proteinsthat is not well conserved in merlin.

The ERM proteins have previously been demonstrated to be essential components of microvillar structures on polarized epithelialas well as lymphocyte cell surfaces (Takeuchi et al., 1994; Crepaldiet al., 1997), and the concentration of these proteins into microvilli-likestructures in a diverse array of cell types in response to growthfactor activation or viral infection is firmly established (Gouldet al., 1986; Bretscher, 1989; Pakkanen and Vaheri, 1989; Hanzelet al., 1991; Dransfield et al., 1997). Our results may implicateRhoA in the growth factor-induced relocalization of ERM proteinsinto apical structures such as microvilli. In this manner, theERM proteins may serve as regulatable scaffolding proteins, localizingand perhaps clustering adhesion receptors such as CD44, ICAM-2,and ICAM-3 with signaling enzymes such as protein kinase A andc-yes, which have recently been reported to associate with ERMproteins (Crepaldi et al., 1997; Dransfield et al., 1997), toimportant sites of action.

Ezrin is known to be serine/threonine phosphorylated concomitant with its localization into microvilli in response to growthfactors in a variety of cell types, including gastric parietalcells where it may participate in histamine-mediated secretion(Urishidani et al., 1989; Hanzel et al., 1991). Indeed, it hasbeen argued that phosphorylation may serve as the physiologicalactivator to release the intramolecular association of the inactiveERM proteins, allowing them to bind to both their membrane targetand actin (Tsukita et al., 1997). Furthermore, there is a strongcorrelation between ezrin serine/threonine phosphorylation andits association with the cytoskeleton in the kidney epithelium(Chen et al., 1995). We have demonstrated that phosphorylationof moesin correlates with its association with the Triton X-100insoluble fraction in vivo, and consistent with this, activatedRhoA increases the percentage of total moesin that is detergentinsoluble. Therefore, our results provide a connection betweena modulator of growth factor signaling (RhoA) and the downstreameffects on ERM localization and phosphorylation, again suggestingthe two may be functionally linked.

Additional pathways downstream of RhoA may also be involved in the relocalization of ERM proteins. RhoA is known to activatea PI5 kinase activity in fibroblasts leading to increased phosphotidylinositol4,5-bisphosphate (PIP₂) production (Chong et al., 1994; Ren etal., 1996). It has been recently demonstrated that the ERM proteinshave a PIP₂ binding site (Niggli et al., 1995), and the abilityof full-length ERM proteins to interact with CD44 in vitro isdependent on the presence of PIP₂ (Hirao et al., 1996). It ispossible that synergy between PIP₂ binding and RhoA-dependentphosphorylation fully activates the ERM proteins, or perhaps oneof the two stimuli serve as a molecular targeting signal for apicalprotrusions. Indeed, it has recently been shown that pleckstrincan induce membrane protrusions in COS cells, in a manner dependenton its ability to bind PIP₂ via one of its PH domains (Ma et al.,1997). Moreover, phosphorylation was demonstrated to regulatethe membrane association and protrusion-inducing activity of thePH domain of pleckstrin. Perhaps the ERM proteins are regulatedin a similar manner, whereby serine/threonine phosphorylationdownstream of Rho activation causes a conformation change unmaskingthe PIP₂ binding site in the amino terminus. Clearly, the identificationof the sites of RhoA-dependent phosphorylation is necessary tofurther explore these possibilities.

Several studies have indicated that the ERM proteins may be regulated by a head-to-tail intramolecular association, whichserves to mask the affinity of both the N- and C-termini fromtheir respective targets (Gary and Bretscher, 1995). It has beenproposed that upon disruption of the intramolecular association,the ERM proteins can form homodimers, heterodimers, and oligomersthat may be critical for their role in microvilli formation inthe placenta (Berryman et al., 1995). It would be very interestingto determine whether such oligomeric species were induced in aRhoA-dependent manner in the fibroblasts employed here. In fact,the mechanism by which the carboxyl terminal fragment of radixinalters the size of the Rho-A-induced apical membrane structuresmay be by altering the lattice of oligomers, which could contributedirectly to the size of the protrusions. Interestingly, vinculin,another molecule whose localization is regulated by RhoA, is alsothought to be controlled by a similar head-to-tail intramolecularassociation (Johnson and Craig, 1995; Gilmore and Burridge, 1996).It has been suggested that a combination of phosphorylation andPIP₂ binding may unmask vinculin from its inactive conformation(Gilmore and Burridge, 1996; Jockusch and Rudinger, 1996). Indeed,the effects of RhoA on the cytoskeleton may be mediated througha common mechanism of phosphorylation and PIP₂ binding leadingto the enhanced activity of a diverse group of cytoskeletal effectors,including pleckstrin, vinculin, and the ERM proteins.

Recently, two reports have further suggested connections between Rho and the ERM proteins. Mackay and colleagues (1997) utilizeda biochemical screen for proteins necessary for RhoA- and Rac-inducedactin rearrangement and identified the ERM proteins, althoughthe mechanism by which the ERM proteins act in this permeabilizedcell system is unclear at present. Conversely, Takai and colleagueshave suggested that Rho may lie upstream of ERM proteins in abiochemical pathway, as the amino terminus of the ERM proteinshave been shown to bind and negatively regulate Rho-GDI, a proteinthat keeps Rho in its inactive, GDP-bound state (Takahashi etal., 1997). While the precise nature of ERM modulation of Rho-dependentpathways remains to be determined, our results strongly suggestthat the ERM proteins can serve as downstream effectors of RhoAin its modulation of the apical actin cytoskeleton in fibroblasts.Perhaps the ERM proteins also act to localize Rho via RhoGDI toa subset of its potential effectors at these specialized apicalmembrane cytoskeleton sites.

Taken altogether, these results suggest a novel function of RhoA in the induction of apical membrane/actin protrusions andintroduce the possibility that through RhoA-dependent phosphorylation,the ERM proteins may be critical regulators and components ofthese structures. The ability of ERM proteins to target specificadhesion molecules to unique cytoskeletal regions such as uropodsin T lymphocytes ( Helander et al., 1996; Serrador et al., 1997)or differentiated microvilli in epithelial cells may be similarlyinduced by a pathway downstream of RhoA or a related GTPase.

	ACKNOWLEDGMENTS

The authors thank Karen Cichowski for many helpful suggestions; Andi McClatchey, John Chant, Lisa Stowers, Rick Cerione, JohnErickson, Sheila Thomas, Jeff Settleman, and Richard Hynes forhelpful discussions during the course of this study and/or forcomments on the manuscript; Sachiro Tsukita for the kind giftof CR22 polyclonal antibody; Ed Seling at Harvard University Museumof Comparative Zoology for helping with the SEM; and Richard Triesmann,Marc Symons, and John Chant for kindly supplying reagents.

	FOOTNOTES

Present address: University of Iowa College of Medicine, Department of Physiology and Biophysics, 400 EMRB, Iowa City, IA52245.

^¶ Corresponding author: Howard Hughes Medical Institute, MIT Center for Cancer Research, E17-517, 40 Ames Street, Cambridge,MA 02139.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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