Cdc42 GEF Tuba regulates the junctional configuration of simple epithelial cells

doi:10.1083/jcb.200605012

Published online 2 October 2006. doi:10.1083/jcb.200605012
The Rockefeller University Press, 0021-9525 $8.00
JCB, Volume 175, Number 1, 135-146

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Cdc42 GEF Tuba regulates the junctional configuration of simple epithelial cells

Tetsuhisa Otani¹^,2, Tetsuo Ichii¹^,2, Shinya Aono¹, and Masatoshi Takeichi¹^,2

¹ Graduate School of Biostudies, Kyoto University, Yoshida-Honmachi, Sakyo-ku, Kyoto 606-8501, Japan
² RIKEN Center for Developmental Biology, Chuo-ku, Kobe 650-0047, Japan

Correspondence to Masatoshi Takeichi: takeichi{at}cdb.riken.jp

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Abstract
Introduction
Results
Discussion
Materials and methods
References

Epithelial cells are typically arranged in a honeycomb-likepattern, minimizing their cell–cell contact areas, whichsuggests that some tension operates for shaping of the cellboundaries. However, the molecular mechanisms that generatesuch tension remain unknown. We found that Tuba, which is aCdc42-specific GEF, was concentrated at the apical-most regionof cell junctions in simple epithelia via its interaction withZO-1. RNAi–mediated depletion of Tuba altered the geometricalconfiguration of cell junctions, resulting in a curved and slackappearance. At the subcellular level, Tuba inactivation modifiedthe assembly pattern of junctional F-actin and E-cadherin. TubaRNAi also retarded cell junction formation in calcium-switchexperiments. Suppression of Cdc42 activity or depletion of N-WASP,which is an effector of Cdc42, mimicked the effects of Tubadepletion. Conversely, overexpression of dominant-active Cdc42or N-WASP enhanced the junction formation of Tuba-depleted cells.These results suggest that Tuba controls the shaping of celljunctions through the local activation of Cdc42 and its effectors.

S. Aono's present address is the Institute for Frontier MedicalSciences, Kyoto University, Sakyo-ku, Kyoto 606-8507, Japan.

Abbreviations used in this paper: AJ, adherens junction; DH,Dbl homology; GEF, guanine nucleotide exchange factor; MLC,myosin light chain; N-WASP, neural Wiskott-Aldrich syndromeprotein; TJ, tight junction.

Introduction

Top
Abstract
Introduction
Results
Discussion
Materials and methods
References

Elucidation of the mechanisms controlling the shape of cellsis an important cell-biological issue. In epithelial layers,cells are arranged in an orderly honeycomb-like pattern, inwhich cell–cell boundaries exhibit a more or less stretchedmorphology that is similar to the interfaces of soap bubbles,implying that some physical tension is operating for the shapingof cell outlines (Thompson, 1917; Hayashi and Carthew, 2004).The molecular mechanisms that produce such tension, however,remain unresolved. In Drosophila melanogaster retinal cells,cadherin cell-adhesion molecules were shown to be required forminimizing the surface areas of the cells in contact with eachother (Hayashi and Carthew, 2004), suggesting that this molecularfamily controls the tensile property of cell junctions. Cadherinorganizes the complex machinery for cell adhesion by interactingwith several cytoplasmic components, including catenins. Thiscomplex is concentrated at the adherens junction (AJ), whichis located directly under the tight junction (TJ; Farquhar and Palade, 1963),and these two types of junctional structures are positionedat the apical-most margin of the entire cell–cell junction,although the cadherin–catenin complex is also distributedthroughout the lateral cell–cell contacts. The AJ is linedwith actin fibers, and cadherin requires ${alpha}$ -catenin, which isone of the catenins that is known to interact with F-actin (Rimm et al., 1995;Drees et al., 2005; Yamada et al., 2005), for its full adhesiveactivity (Watabe-Uchida et al., 1998), suggesting that cadherinand F-actin cooperate in cell junction organization. In turn,regulators of cadherin or actin are assumed to be involved inthe modulation of cell–cell boundary morphology.

Rho family small GTPases (Rho GTPases) are pivotal regulatorsof the actin cytoskeleton (Etienne-Manneville and Hall, 2002).In epithelial cells, these GTPases have also been implicatedin cadherin activities (Fukata and Kaibuchi, 2001; Braga and Yap, 2005);conversely, the GTPase activities are modulated by cadherin-mediatedadhesion (Kim et al., 2000; Noren et al., 2001; Braga and Yap, 2005),suggesting that these enzymes are important for cadherin–actininterplay. The activities of Rho GTPases are regulated by guaninenucleotide exchange factor (GEF), which exchanges GDP for GTP(Schmidt and Hall, 2002). Once activated, the small GTPasescan interact with various downstream effectors, acting as amolecular switch (Etienne-Manneville and Hall, 2002). Amongseveral classes of protein identified as Rho GEFs, the Dbl familyproteins are best characterized. The Dbl homology domain (DHdomain) has been shown to be necessary and sufficient for theGEF activity of Dbl family Rho GEFs (Hart et al., 1994). Itis thought that localized activation of GEFs contributes tothe spatiotemporal activation of Rho GTPases. Among the RhoGEFs identified, Tiam1, which is a Rac-specific GEF, has beenbest characterized as a modulator of cell junctions, and itsdepletion impairs both AJ and TJ formation (Malliri et al., 2004;Chen and Macara, 2005; Mertens et al., 2005). GEF-H1/Lfc, whichis a GEF for Rho, was also implicated in TJ functions (Benais-Pont et al., 2003).On the other hand, the role of Cdc42 and its GEFs in cell junctionassembly is poorly understood, although the activation of Cdc42was shown to increase actin accumulation at cell junctions (Kodama et al., 1999).Also, nectin, which is an AJ component, could activate Cdc42through FRG, which is a Cdc42 GEF (Fukuhara et al., 2004). Weshow that Tuba, which is a Cdc42-specific GEF that belongs tothe Dbl family (Salazar et al., 2003), plays an important rolein the regulation of cell junction configuration by becominglocalized at the apical junctions of simple epithelia.

Results

Top
Abstract
Introduction
Results
Discussion
Materials and methods
References

Tuba localizes at the apical junction by interacting with ZO-1
We used Caco-2 cells throughout the present experiments, asthey exhibited typical simple epithelial morphology. Immunostainingwith a mAb specific for Tuba (Fig. 1 A) showed that this moleculewas sharply concentrated at cell junctions (Fig. 1, C–E). When Tuba cDNA had been introduced into Caco-2 cells, the intensityof junctional Tuba signals increased (Fig. 1 B), justifyingthe aforementioned observation on the endogenous Tuba localization.A similar distribution was observed in other simple epithelialcells, such as DLD-1 and MTD-1A (unpublished data). Immunostainingof Caco-2 cells at high densities showed that Tuba was strictlylocalized at the apical-most margin of cell junctions, colocalizingwith ZO-1, which is a TJ component (Fig. 1 C). Tuba also colocalizedwith l-afadin (Mandai et al., 1997), which is an AJ component(Fig. 1 D). However, although the l-afadin was also detectableat basal regions of the cell–cell contacts, to some extent,Tuba did not follow this localization of l-afadin. Tuba alsooverlapped with the apical margin population of ${alpha}$ E-catenin, althoughthe latter was distributed throughout the cell–cell contacts(Fig. 1 E). Other populations of Tuba molecules were localizedin the cytoplasm, which were most abundant at perinuclear regions.

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Figure 1. Localization of Tuba at the apical cell–cell junctions in Caco-2 cells. (A) Immunoblot detection of Tuba from a Caco-2 cell lysate with anti-Tuba mAb. Two isoforms, of 190 and 170 kD, are detected. (B) Cell junctional signals of Tuba are increased by its exogenous expression. Compare the immunofluorescence signals along cell junctions between the centrally located transfectants and surrounding nontransfectants. (C–E) Endogenous Tuba is concentrated at the apical region of cell junctions. Cells were coimmunostained for Tuba and ZO-1 (C), l-afadin (D), or ${alpha}$ E-catenin ( ${alpha}$ -catenin) (E). Tuba is colocalized with ZO-1, l-afadin, and the apical-most population of ${alpha}$ E-catenin ( ${alpha}$ -catenin). Bars: (B) 20 µm; (C–E) 10 µm.

Because Tuba closely colocalized with ZO-1, we investigatedtheir potential interactions. First, we observed the localizationof these molecules in low-calcium medium, in which cadherinmolecules became dispersed but ZO-1 remained as clusters. Evenunder these conditions, Tuba maintained its colocalization withZO-1 (Fig. 2 A). We then overexpressed Tuba and ZO-1 togetherin Caco-2 cells. Excessive Tuba molecules were localized notonly along cell junctions, but also became clustered in thecytoplasm, and ZO-1 tightly associated with all these Tuba signals(Fig. 2 B). As a control, we coexpressed Tuba and ß-catenin,but these two molecules did not colocalize (Fig. 2 C), indicatingthat the Tuba–ZO-1 colocalization was caused by theirspecific interactions.

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Figure 2. Tuba is recruited to cell–cell junctions with ZO-1. (A) Tuba and ZO-1 are colocalized with each other even after disorganization of cell–cell contacts. Caco-2 cells were cultured in low-calcium medium and coimmunostained for Tuba and ZO-1. (B and C) Clusters of overexpressed Tuba are colocalized with ZO-1 (B), but not with ß-catenin (C). (D) Tuba coimmunoprecipitates with ZO-1. Tuba and ZO-1-HA were coexpressed in human embryonic kidney 293 cells; and ZO-1 was immunoprecipitated from their lysates with anti-HA antibody, and then the coprecipitated molecules were identified by immunoblotting. (E) Schematic diagram of deletion mutants of Tuba used in this study. From the N-terminus, Tuba consists of four Src homology 3 (SH3) domains, a DH domain, a Bin1/amphiphysin/Rvs (BAR) domain, and two SH3 domains. Flag tag was attached only to ${Delta}$ C. For immunodetection of Tuba or its mutants, we generally used the anti-Tuba mAb, which had been generated against the C-terminal portion of Tuba. For detection of ${Delta}$ C, we used anti-Flag antibodies. (F) Tuba C terminus is required for the interaction between Tuba and ZO-1. Deletion mutants of Tuba were coexpressed with ZO-1, and their coprecipitates were assayed as in D. Bands were detected by using a mixture of mAbs against Tuba and Flag tag. (G) Tuba C terminus is required for junctional localization. FL, ${Delta}$ DH, and ${Delta}$ N are localized at cell junctions (arrowheads), as well as in the cytoplasm, whereas ${Delta}$ C is detected only in the cytoplasm. (H and I) Junction localization of Tuba is abolished in ZO-1 knockdown cells. Expression of ZO-1 was knocked down in Caco-2 cells by siRNA (H). ZO-1 RNAi cells were coimmunostained for Tuba and ZO-1 (I). Similar results were obtained by using three different siRNAs, siZO-1-1–3. Bars, 20 µm.

We next performed immunoprecipitation using lysates of cellscotransfected with Tuba and ZO-1 cDNAs and found that Tuba coprecipitatedwith ZO-1 (Fig. 2 D). Tuba was also able to coprecipitate withZO-2, but not with ZO-3 (Fig. S1, A and B, available at http://www.jcb.org/cgi/content/full/jcb.200605012/DC1).To determine the sites on Tuba responsible for its interactionwith ZO-1, we coexpressed a series of deletion mutants of Tubawith ZO-1, tested their binding by immunoprecipitation, andfound that their interaction required the C-terminal domainof Tuba (Fig. 2, E and F). However, the C-terminal fragmentalone was unable to bind ZO-1 (unpublished data), suggestingthat some cooperation of the C-terminus with other sites onTuba may be required for the Tuba–ZO-1 interaction. Theimportance of the C-terminal domain was confirmed by immunostainingof Tuba deletion-mutant transfectants (Fig. 2 G). Constructsin which the DH or N-terminal half region had been deleted,designated as ${Delta}$ DH or ${Delta}$ N, respectively, could become localizedat cell junctions, although ${Delta}$ N was largely cytoplasmic. In contrast, ${Delta}$ C was completely cytoplasmic. Finally, we depleted ZO-1 expressionby using RNAi, and found that Tuba could not become localizedat the cell junctions that had lost ZO-1 (Fig. 2, H and I),despite the normal appearance of the apical junctions in ZO-1–deficientcells (McNeil et al., 2006; Umeda et al., 2004). These resultsconfirmed that ZO-1 was required for the cell junction localizationof Tuba. On the other hand, ZO-2 depletion did not affect Tubalocalization (Fig. S1 C), indicating that ZO-1 plays the predominantrole in targeting Tuba to cell junctions. Whether Tuba directlybinds ZO-1 or -2 or requires a mediator remains to be determined.

Tuba depletion perturbs junctional configuration
To elucidate the function of Tuba in Caco-2 cells, we examinedthe effect of its RNAi-mediated depletion, either by isolatingstable transfectants expressing small hairpin Tuba RNAs or bytreating cells with a siRNA specific for Tuba, and the resultsconsistently observed in these transfectants (Tuba-RNAi cells)are described in this study. Efficient and specific knockdownof Tuba was confirmed by Western blotting and immunofluorescence(Fig. 3, A and B). Immunostaining for ZO-1 and l-afadin revealedthat, in Tuba-RNAi cells, the overall outlines of TJ and AJwere distorted; their cell–cell boundaries were overlybent and less strained, compared with those in the controls(Fig. 3, C and D), suggesting that those junctions had acquiredreduced tension. We quantified this difference by measuringthe ratio of junction length to the distance between vertices,defining a "linearity index," and confirmed that the junctionsof Tuba-RNAi cells were excessively curved (Fig. 3 E). Concomitantly,some of the Tuba-RNAi cells exhibited unusually small apicalareas (Fig. 3 D, arrows). Quantification showed that the variationin the apical surface area increased after Tuba depletion (Fig. 3 F).

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Figure 3. Tuba regulates the junctional configuration. (A) Immunoblot detection of Tuba from control, pSUPER-Tuba–transfected, and Tuba siRNA–treated cells by use of anti-Tuba mAb. (B) Immunostaining of control and pSUPER-Tuba–transfected cells with anti-Tuba mAb. (C and D) Distorted apical junctions in Tuba-RNAi cells. Control and Tuba-RNAi cells were stained for ZO-1 (C) or l-afadin (D). In Tuba-RNAi cells, the apical junctions are more irregularly curved than in the controls. Some cells exhibit abnormally small apical surface areas, as outlined by these markers (arrows). (E) Quantification of junction linearity. Junction length (blue) and the distance between vertices (red) were measured. Linearity index is defined by the ratio of junction length to the distance between vertices. (right) This index increases in Tuba-RNAi cells. *, P < 0.05. n = 3 independent experiments, in each of which >150 junctions were measured; t test. (F) Apical area is more variable in Tuba-RNAi cells. The apical area of each cell was measured, and the ratio of the SD of apical area to mean apical area was quantified. *, P < 0.05; n = 3 independent experiments, in each of which >100 cells were measured; t test. (G) Cell junction outlines are distorted in ${Delta}$ DH- or ${Delta}$ C-expressing cells, but not in FL- or ${Delta}$ N-expressing ones. Stable transfectants were immunostained for ZO-1. (right) Quantification confirms these differences. Error bars represent the mean ± the SD. *, P < 0.05; **, P < 0.001. n = 4 independent experiments, in each of which >30 junctions were measured; t test. Bars, 20 µm.

We also tested the effects of overexpression of Tuba deletionmutants in Caco-2 cells (Fig. 3 G). ${Delta}$ DH lacking the catalyticdomain perturbed the junction linearity, as found in Tuba RNAicells, and ${Delta}$ C expression showed an effect similar to that of ${Delta}$ DH, suggesting that these mutant molecules compete with endogenousTuba for interactions with partners required for their functions.These results corroborated the observation that Tuba inactivationled to the distortion of junctional morphology.

Impaired distribution of E-cadherin and F-actin after Tuba depletion
Despite the deformed outlines of the apical cell–cellcontacts, E-cadherin and F-actin appeared normally concentratedalong the AJ in Tuba RNAi cells (Fig. 4 A). The expressionlevels of E-cadherin and other junctional proteins were alsonot changed (Fig. 3 A). However, their distributions in lower(lateral) portions of cell–cell boundaries were affected.In normal Caco-2 cells, E-cadherin was concentrated at theseareas in a peculiar networklike pattern, overlapping with actinfibers with a similar network (Fig. 4 A). Close-up views showedthat the lateral populations of E-cadherin or overlapping F-actinorganized strands that were linked with their AJ components.In Tuba-RNAi cells, E-cadherin strands became fragmented anddiscontinuous with the AJ, with a concomitant disturbance ofactin filaments, which appeared less polymerized than in thecontrols. Quantification of F-actin density at cell junctionsconfirmed that the lateral actin fibers less densely distributedin the RNAi cells, although the apical actin filaments wereonly slightly affected (Fig. 4 B). In addition, Tuba depletionreduced the colocalization of E-cadherin and actin fibers, althoughthe Triton X-100 solubility of E-cadherin was not particularlydifferent between control- and Tuba-RNAi cells (Fig. 4 C).

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Figure 4. Disorganization of F-actin and E-cadherin networks by Tuba suppression. (A) Double-staining for F-actin (green) and E-cadherin (red). F-actin and E-cadherin form an AJ at the apical-most margin of the junction (arrowheads), and the AJ is linked with the lateral networks of these molecules in the case of control cells. In Tuba-RNAi cells, F-actin appears to have been dispersed at the lateral portions, and the E-cadherin networks have become fragmented and discontinuous with the AJ; the colocalization of E-cadherin and F-actin is also reduced. (B) Quantification of F-actin density at cell junctions. (left) F-actin density at apical and lateral cell junctions was measured as shown. (right) Quantification shows that lateral F-actin density is reduced in Tuba-RNAi cells. Error bars represent the mean ± the SD. n > 40 junctions. (C) Triton X-100 solubility of E-cadherin is not altered in Tuba-RNAi cells. S, soluble fraction; I, insoluble fraction. (D) Effects of Tuba deletion mutants on E-cadherin distribution. Immunostaining for E-cadherin shows that, in ${Delta}$ DH- or ${Delta}$ C-expressing cells, E-cadherin localization at lateral cell–cell contacts is more diffuse compared with that in FL-expressing cells. In ${Delta}$ N-expressing cells, E-cadherin was most highly concentrated at lateral cell–cell contacts. Bars, 10 µm.

We also generated stable transfectants expressing Tuba deletionmutants, and examined E-cadherin distribution in them (Fig. 4 D).In ${Delta}$ DH- and ${Delta}$ C-expressing cells, E-cadherin at the lateral membranesappeared more diffuse or fragmentary, as compared with thatof FL-expressing cells. Thus, these two constructs not onlyimpaired apical junctional linearity (see above) but also perturbedthe lateral distribution of E-cadherin, as in the case of Tuba-depletedcells. On the other hand, in ${Delta}$ N-expressing cells, E-cadherinbecame more highly concentrated at the cell–cell contacts.This implies that the N-terminal half region has an inhibitoryactivity for Tuba.

To see the effects of Tuba depletion on more dynamic phasesof cell contact, we observed the behavior of E-cadherin andF-actin during the recovery process of cell–cell adhesionby conducting a "calcium-switch" experiment (Fig. 5 A). Inlow-calcium medium, E-cadherin disappeared from cell–cellboundaries, and actin fibers irregularly ran along cell peripheriesin both control and Tuba-RNAi cells. By 1 h after calcium restoration,E-cadherin and actin became sharply colocalized at cell–cellboundaries. In Tuba-RNAi cells, however, this E-cadherin accumulationwas retarded. At 1 h, although we could detect junctional E-cadherin,its signals were fragmented, and actin fibers did not sharplydelineate cell–cell boundaries. Furthermore, E-cadherinsignals did not fully colocalize with F-actin ones. The retardationof E-cadherin accumulation was confirmed by quantifying thejunctional fluorescence intensity of E-cadherin at 5 min aftercalcium switch (Fig. 5 B). In contrast to E-cadherin, ZO-1 recruitmentto cell junctions was not severely affected in Tuba-RNAi cells(Fig. 5 C), although the outlines of these cells appeared tobe less tense compared with those of control cells. These resultssuggest that the junctional recruitment of ZO-1 occurs independentlyof the Tuba signaling, whereas the organization of E-cadherinand actin at cell junctions is under the control of Tuba. Meanwhile,we found no difference in the composition of catenins coprecipitatingwith E-cadherin between the control and Tuba-RNAi cell lysates(unpublished data), indicating that Tuba deficiency did notaffect cadherin–catenin complex formation.

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Figure 5. Junctional recruitment of F-actin and E-cadherin after calcium switch. (A) Cells were cultured in low-calcium medium overnight, and then cadherin-mediated junction assembly was initiated by the addition of calcium. In Tuba-RNAi cells, the relocation of E-cadherin to cell junctions was retarded, and F-actin could not be reorganized into sharp lines at cell–cell boundaries by 1 h. (B) Immunofluorescence intensity of E-cadherin at cell junctions was quantified for the samples incubated for 5 min with calcium. Error bars represent the mean ± the SD. n = 60 junctions. (C) ZO-1 relocation to cell junctions was not severely effected in Tuba-RNAi cells. Bars, 10 µm.

The effects of ZO-1 knockdown on junctional configuration
As ZO-1 knockdown depleted Tuba from cell junctions, we expectedthat ZO-1–RNAi and Tuba-RNAi cells would display similarphenotypes. However, this was not the case. The outlines ofapical junctions appeared rather straighter in ZO-1–RNAicells than in the controls (Fig. S2 A, available at http://www.jcb.org/cgi/content/full/jcb.200605012/DC1),which is opposite to what we had anticipated. We noticed thatmyosin IIA or IIB became strongly up-regulated along the apicaljunctions of ZO-1–depleted cells (Fig. S2 B); furthermore,phosphorylation of serine 19 of myosin light chain (MLC), whichreflects its activation, was also up-regulated at ZO-1–depletedcell junctions (Fig. S2 C). In Tuba-RNAi cells, on the otherhand, neither myosin localization nor MLC phosphorylation wasup-regulated at cell junctions (Fig. S2, E and F). From theseobservations, we reasoned that ZO-1 depletion up-regulated myosinII activities via unknown mechanisms, and enhanced the contractilityof junctional actin fibers, hiding the opposite effect of Tubadepletion. To test this possibility, we examined the effectof Y-27632, which is an inhibitor of Rho kinase (Uehata et al., 1997)that can suppress MLC activation (Amano et al., 1996), and foundthat this reagent abolished the up-regulation of myosin II inZO-1–RNAi cells (Fig. S2 D). Importantly, in the presenceof Y-27632, the cell junctions now became more severely distortedin ZO-1–RNAi cells than in the controls (Fig. S2 A), indicatingthat, provided myosin II is inactive, ZO-1 and Tuba depletionsexhibit similar junctional phenotypes. These findings suggestthat there are at least two pathways downstream of ZO-1, a Rho–Rhokinase–myosin pathway and a Tuba pathway, and that ZO-1depletion affected both pathways. As Y-27632 alone can distortcell junctions to some extent (Fig. S2 A), a balance betweenthese pathways may determine the overall junction morphology.Collectively, we can conclude that the phenotypes observed inZO-1–depleted cells do not contradict with the proposedrole of the interaction between ZO-1 and Tuba in cell junctionconfiguration. It is of note that cell junction formation isdelayed in ZO-1–depleted cells (McNeil et al., 2006; Umeda et al., 2004),which is similar to the properties of Tuba-RNAi cells, supportingthe idea that ZO-1–dependent localization of Tuba at celljunctions is required for its functions.

Tuba signals through Cdc42
Next, we studied the functions of Tuba as a Cdc42 GEF. We firstconfirmed that Tuba preferentially activated Cdc42 by conductingan in vitro guanine nucleotide exchange assay (Fig. S3, availableat http://www.jcb.org/cgi/content/full/jcb.200605012/DC1). Asthe activation of Rho GTPases has been correlated with its membraneassociation (Bokoch et al., 1994), we examined the subcellularlocalization of Cdc42 in Caco-2 cells by immunostaining. Inconfluent Caco-2 cells, immunostaining signals for Cdc42 wereweakly, but consistently, detected at the apical cell–celljunctions, and this localization of Cdc42 became less visiblein Tuba-RNAi cells (Fig. 6 A). When cells had been subjectedto calcium-switch experiments, Cdc42 was rapidly recruited tocell–cell contact sites upon the restoration of normalcalcium concentration in the control cells, and this redistributionof Cdc42 was retarded in the Tuba-RNAi cells (Fig. 6 B). TheCdc42 immunofluorescence signal per cell junction was reducedby $~$ 30% in the Tuba-RNAi cells, when measured at the 30 min incubationpoint (Fig. 6 C). These observations suggest that Tuba has theability to facilitate the recruitment of Cdc42 to cell junctions.Because Cdc42 was shown to be activated during cell junctionassembly (Kim et al., 2000; Noren et al., 2001), we measuredits activity by pull-down assays. The results showed that Cdc42was transiently activated at 5 min after calcium switch, butthis activation did not occur in Tuba-RNAi cells (Fig. 6 D).We could not detect any other differences in the overall activityof Cdc42 between control and Tuba-RNAi cells by this biochemicalmethod; the Tuba-mediated Cdc42 regulation might represent onlya small portion of the entire regulatory systems for this smallGTPase.

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Figure 6. Role of Cdc42 in junction assembly. (A) Cdc42 is localized at cell–cell boundaries, and this localization is diminished in Tuba-RNAi cells. (B and C) Delayed redistribution of Cdc42 to Tuba-RNAi cell junctions in calcium-switch experiments. Cdc42 was immunostained at the indicated times after calcium restoration (B). Immunofluorescence intensity of Cdc42 at cell junctions was quantified for the samples incubated for 30 min (C), in which the intensity of control-RNAi cells was adjusted to 100. Error bars represent the mean ± the SD. *, P < 0.05. n = 3 independent experiments, in each of which >10 junctions were measured; paired t test. (D) Delayed activation of Cdc42 in Tuba-RNAi cells. After Cdc42 pull-down assays using GST-PAK-CRIB, the intensity of electrophoretic bands of Cdc42 was quantified. In brief, each band was encircled by a box, and the signal density of the band was measured. The ratio of the Cdc42 signals in GST-PAK-CRIB pull-down samples to those in the total lysates was defined as "active Cdc42/total Cdc42." The ratio in control-RNAi cells at 0 min was adjusted to 1. Error bars represent the mean ± the SEM. *, P < 0.05; n = 3 independent experiments; one-tailed t test. (E and F) Effects of Cdc42 mutants on junction assembly in calcium-switch assays. Dominant-negative (N17-Cdc42) or constitutive-active (V12-Cdc42) Cdc42 was expressed in control or in Tuba-RNAi cells. In N17-Cdc42–transfected control cells (E), the junctional recruitment of F-actin and E-cadherin was delayed (compare with Fig. 5). (F) In contrast, V12-Cdc42 strongly promoted the junctional accumulation of these molecules in Tuba-RNAi cells. (G) Linearity index in control or Tuba-RNAi cells, expressing either GFP (control) or dominant-negative or constitutive-active Cdc42, measured at 1 h. Error bars represent the mean ± the SD. *, P < 0.005; **, P < 0.0005. n = 3 independent experiments, in each of which >40 junctions were measured; t test. Bars: (A) 10 µm; (B, E, and F) 20 µm.

To test if the cellular phenotypes observed in Tuba-RNAi cellswere caused by reduced Cdc42 activities, we examined if dominant-negativeCdc42 expression could mimic Tuba depletion. Caco-2 cells transfectedwith Cdc42 mutants were unable to grow to form cell colonies,and for this reason, we observed only early cell–cellcontact events by using calcium-switch assays. In the cellstransfected transiently with dominant-negative N17-Cdc42, E-cadherinand actin accumulation were perturbed in a fashion similar tothose found in Tuba-RNAi cells. E-cadherin remained punctateand F-actin irregularly delineated cell junctions at 1 h afterthe calcium restoration (Fig. 6 E). Conversely, when dominant-activeV12-Cdc42 had been expressed in Tuba-RNAi cells, the E-cadherinand actin reassembly was dramatically facilitated, resultingin the formation of junctions with a tightened appearance (Fig. 6 F).Measurement of the junction linearity confirmed that dominant-negativeN17-Cdc42 was able to loosen the cell boundaries of the controlcells, but could not significantly enhance the phenotype ofTuba-RNAi cells, and dominant-active V12-Cdc42 enhanced therectilinear organization of cell junctions in both control andTuba-RNAi cells (Fig. 6 G). Thus, Cdc42 inactivation mimickedthat of Tuba, and activation of Cdc42 could rescue the TubaRNAi phenotypes. The effect of V12-Cdc42 appeared excessive,as it facilitated even the control cell junction formation,reflecting its dominant-active nature.

Previous studies showed that Tuba interacted with neural Wiskott-Aldrichsyndrome protein (N-WASP; Salazar et al., 2003). As N-WASP isan effector of Cdc42 (Rohatgi et al., 1999), we studied itspotential role in the Tuba–Cdc42 signaling system. Wefirst confirmed that Tuba could coprecipitate with N-WASP (Fig. 7 A). Next, we knocked down N-WASP by using RNAi (Fig. 7 B). In N-WASP–RNAicells, the outlines of cell junctions became distorted in apattern comparable to that in Tuba-RNAi cells (Fig. 7 C). Forcomparison, we also knocked down the expression of IQGAP1, whichis another Cdc42 effector implicated in cell junctions (Kuroda et al., 1998;Noritake et al., 2004), and found that IQGAP1 depletion hadno effects on the junction linearity (Fig. 7, B and C), suggestingthat these effectors have distinct roles. Tuba and Cdc42 wereable to localize normally to cell–cell junctions in theN-WASP–depleted cells (Fig. 7 D), suggesting that thesemolecules function upstream of N-WASP.

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Figure 7. Role of N-WASP in junctional configuration. (A) Tuba interacts with N-WASP. Tuba and myc-N-WASP were coexpressed in human embryonic kidney 293 cells, N-WASP was immunoprecipitated from their lysates with anti-myc antibody, and the coprecipitated molecules were identified by immunoblotting. (B, left) Immunoblot detection of N-WASP from control and N-WASP–RNAi cells with anti–N-WASP antibody. (right) Immunoblot detection of IQGAP1 from control and IQGAP1-RNAi cells with anti-IQGAP1 antibody. (C) Distortion of cell–cell boundaries in N-WASP–RNAi cells, detected by ZO-1 immunostaining. (right) Linearity index. Error bars represent the mean ± the SD. *, P < 0.005. **, P < 0.0005. n = 3 independent experiments, in each of which >100 junctions were measured; t test. (D) Localization of Tuba and Cdc42 is not altered in N-WASP–RNAi cells. (left) Tuba localization in confluent N-WASP–RNAi cells. (right) Cdc42 localization in N-WASP–RNAi cells at 30 min after calcium restoration. Bars, 20 µm.

We also examined E-cadherin and actin organization in N-WASP–RNAicells. In them, E-cadherin strands became fragmented at thelateral cell–cell contacts, as seen in Tuba-RNAi cells,and their colocalization with F-actin was dramatically reduced(Fig. 8 A). The fibrous organization of actin itself appearedto have been suppressed at the lateral cell–cell contactregions, although the apical AJ-associated bundles were notaffected. In calcium-switch assays, N-WASP depletion perturbedthe organization of E-cadherin and F-actin at early cell–cellcontacts (Fig. 8 B), which is a phenocopy of the effects ofTuba depletion. Finally, by using the calcium-switch assay,we examined whether N-WASP overexpression could rescue the defectsof junction assembly that are induced by Tuba depletion. Theresults showed that overexpression of full-length N-WASP facilitatedthe accumulation of E-cadherin and F-actin at cell–cellcontacts in Tuba RNAi cells (Fig. S4, A and C, available athttp://www.jcb.org/cgi/content/full/jcb.200605012/DC1), althoughthis effect was most evident at 5 min after calcium restoration,and became less clear at 1 h. In contrast, overexpression of ${Delta}$ cof-N-WASP, which cannot activate Arp2/3 complex–dependentactin nucleation in vitro (Rohatgi et al., 1999), did not facilitateE-cadherin or F-actin accumulation at cell–cell contacts(Fig. S4, B and D).

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Figure 8. Role of N-WASP in cadherin or actin distribution. (A) Double-staining for F-actin (green) and E-cadherin (red) in N-WASP–RNAi cells. Arrowheads indicate the AJ. Note the diffuse actin signals at the lateral cell junctions, and reduced colocalization of F-actin and E-cadherin, in N-WASP–RNAi cells. Actin fibers along the AJ appear normal. (B) Control and N-WASP–RNAi cells were subjected to calcium-switch assays and stained for F-actin or E-cadherin. N-WASP depletion delayed cell junction assembly. Linear reorganization of actin filaments was impaired, and E-cadherin accumulation was irregular at 1 h. Bars, 10 µm.

	Discussion

Top Abstract Introduction Results Discussion Materials and methods References

We have demonstrated that Tuba is concentrated at the apical-mostmargin of the epithelial cell junctions by binding to the TJprotein ZO-1 (or its associated proteins), suggesting that thismolecule is localized around the TJ. Depletion of Tuba distortedthe outlines of the apical TJ–AJ complex. Closer observationsof F-actin and E-cadherin revealed that although the AJ structureitself appeared normal, the distributions of these moleculeslocated lower than the AJ were disorganized. In normal Caco-2cells, F-actin organized a fibrous network at the lateral portionsof the cell junction, and this actin network was linked withthe apical actin fibers forming the AJ, and E-cadherin showedan overlapping distribution. As a result of Tuba depletion,the E-cadherin networks became fragmented, with a concomitantreduction of thick, lateral actin filaments. These observationssuggest a scenario in which Tuba functions at the level of theTJ, but its effects spread to the lower portions of the junction.As such apical-specific localization has never been reportedfor other Cdc42 or Rac GEFs, Tuba may play a unique, position-specificrole in junctional organization.

Our results suggest that Tuba is required for the regulationof geometrical configuration of the apical junctions. Althoughthe mechanism that generates the linear morphology of the apicaljunctions is poorly understood, we can speculate that the surfacetension supported by the cortical actin cytoskeleton is important,as the actin cytoskeleton is a critical regulator of the viscoelasticityof the cell cortex (Petersen et al., 1982). The role of Tubais likely to regulate actin polymerization via Cdc42 and itseffectors, and E-cadherin follows the actin distribution, assuggested by their colocalization. The lateral networks of F-actinand E-cadherin strands, thus formed, may increase the surfacetension for minimizing the surface area of cell junctions, orstabilize the linear morphology of cell junctions, and thismolecular status is disrupted by the loss of Tuba. On the otherhand, through the experiments of ZO-1 knockdown, we found thatZO-1 functioned not only as a partner for Tuba but also as aregulator of myosin activity, and the latter activity influencedthe morphology of cell junctions. In contrast to the case ofZO-1 depletion, Tuba-depletion did not affect myosin distributionor activity, suggesting that actomyosin contractility may notprimarily be involved in the loosened appearance of Tuba-depletedcell junctions. It is likely that cooperations of the myosin-dependentcontractility and Tuba-mediated actin organization determinethe overall shape of cell junctions. As an alternative roleof Tuba, it may regulate the dynamics of cadherin molecules,such as their trafficking and endocytosis, thus affecting junctionmorphology; this possibility remains to be tested in the future.

Supporting the hypothesis that Tuba functions via Cdc42, Tubapromoted recruitment of Cdc42 to cell junctions, transientlyactivating it during cell junction recovery processes. Dominant-negativeand -active Cdc42 mimicked the Tuba depletion and rescued theTuba RNAi phenotypes, respectively, which is consistent withthe idea that Cdc42 acts downstream of Tuba signaling. Furthermore,Tuba was shown to interact with proteins to regulate the actincytoskeleton, including N-WASP, which is a well-known effectorof Cdc42 (Salazar et al., 2003). We demonstrated that N-WASPdepletion induced distorted apical junctions, just like Tubadepletion, and also that N-WASP was required for normal accumulationof E-cadherin and F-actin at cell junctions, confirming earlierobservations (Ivanov et al., 2005). In addition, N-WASP overexpressionrestored rapid recruitment of E-cadherin and F-actin to thejunctions in Tuba RNAi cells. These results suggest that N-WASPmay be one of the components working downstream of the Tuba–Cdc42pathway; this idea is also supported by a recent study withmelanoma cells (Kovacs et al., 2006). N-WASP activates the Arp2/3complex, which creates branched actin filaments (Blanchoin et al., 2000;Rohatgi et al., 1999); and the Arp2/3 complex was shown to benecessary for cells to assemble cadherin-based cell contacts(Kovacs et al., 2002; Verma et al., 2004). When consideringall of the data together, we can imagine a scheme in which N-WASP,activated by Tuba–Cdc42, enhances actin polymerizationat the level of the apical junctions. This process then leadsto the delivery of polymerized actin filaments to the lowerportions of cell junctions, and these actin filaments may serveas a scaffold on which the E-cadherin–catenin complexmay be anchored. Although other mechanisms, such as traffickingof E-cadherin might also be involved, this scheme accounts forthe putative mechanism as to how Tuba, which is confined tothe apical region, can organize F-actin and E-cadherin throughoutthe lateral cell–cell contacts. Meanwhile, the rescuingeffect of N-WASP overexpression on Tuba-depleted cells appearedto have been transient, indicating that other factors are alsoinvolved in the Tuba–Cdc42 signaling system.

Calcium-switch experiments showed that Tuba was also requiredfor the initial processes of junction formation. Both E-cadherinand F-actin assemblies were impaired during the reestablishmentprocess of cell–cell contacts. ZO-1 has been shown toform a complex with the cadherin–catenin complex at theearly stages of cell junction assembly (Rajasekaran et al., 1996;Ando-Akatsuka et al., 1999), implying that, in nascent cell–cellcontacts, Tuba may be in closer proximity to cadherins thanin mature junctions, and thus could directly control cadherin-mediatedadhesion. Even at early cell–cell contacts, however, cellboundaries always displayed a less-tensed appearance, not onlyin Tuba-RNAi cells but also in N-WASP–RNAi cells or thoseexpressing dominant-negative Cdc42. These observations suggestthat a common function of Tuba governs the initial, as wellas the mature, phases of cell–cell contact.

Several GEFs other than Tuba have been implicated in cell–celladhesion, including Tiam1, which is a Rac-specific GEF (Chen and Macara, 2005;Hordijk et al., 1997), and Asef, which is also a Rac GEF (Kawasaki et al., 2003).FRG participates in nectin-induced activation of Cdc42 (Fukuhara et al., 2004),and GEF-H1 regulates TJ permeability (Benais-Pont et al., 2003).It is likely that many GEFs are sequentially involved in celljunction assembly in a redundant or independent manner. Tiam1deficiency was reported to disrupt epithelial junctions (Malliri et al., 2004;Mertens et al., 2005). Not only Tuba depletion, but also Tiam1depletion impairs both AJ and TJ organization. In future studies,it is therefore important to define how Rac and Cdc42 GEFs sharetheir roles in the regulation of cell assembly.

Materials and methods

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Abstract
Introduction
Results
Discussion
Materials and methods
References

Plasmid construction
A partial cDNA clone of human Tuba (KIAA1010) was obtained fromthe Kazusa DNA Institute (Chiba, Japan). The 5' sequence wasdetermined by 5'-RACE, using a SMART RACE cDNA amplificationkit (CLONTECH Laboratories, Inc.), with cDNA from Colo205 cellsused as the template. The 5' fragment was subsequently clonedby RT-PCR. The 40–amino acid deletion in the originalKIAA1010 cDNA clone (Salazar et al., 2003) was also amplifiedby RT-PCR. pSUPER vectors were generated as previously described(Brummelkamp et al., 2002). pGK-neo was further inserted atthe EcoRI–NotI site of pSUPER to obtain stable transfectants.The RNAi target sequence of Tuba was designed and inserted intothe BglII–HindIII site of pSUPER, as previously described(Brummelkamp et al., 2002). The target sequences were as follows:Tuba-RNAi-1, 5'-AGTCAAGACCTCGTCAAAG-3'; Tuba-RNAi-2, 5'-ACCTTGATGCTCACTAGAA-3';and cytokeratin 19 (as a specificity control), 5'-GCTAACCATGCAGAACCTC-3'.Stealth siRNAs with the following target sequences were synthesizedby Invitrogen: siZO1-1, 5'-GCAGCTCCAAGAGAAATCTTCGAAA-3'; siZO1-2,5'-GGCAAGAGAAGAACCAGATATTTAT-3'; siZO1-3, 5'-CCCTGGATTTAAGCCAGCCTCTCAA-3'; siZO2-1, 5'- CCCTAAAGGTGAAATGGTGACCATT-3'; siZO2-2, 5'-CCCATAGCTGATATAGCAATGGAAA-3';siZO2-3, 5'-GGCTAATGAGTTACCTGACTGGTTT -3'; siTuba, 5'-GAGCTTGAGGGAACATACAAGATTT-3'; siNWASP-1, 5'-TCAAATTAGAGAGGGTGCTCAGCTA-3': siNWASP-2,5'-TCTGTGGCTGATGGCCAAGAGTCTA-3'; siNWASP-3, 5'-CCCTCTTCACTTTCCTCGGCAAGAA-3';siIQGAP1-1, 5'-GGCCCTACAGATTCCTGCAGCTAAA -3'; siIQGAP1-2, 5'-GACAGGAAATCCTACGGTTATTAAA-3'; and siIQGAP1-3, 5'-CCAATAAGATGTTTCTGGGAGATAA -3'. Negative-controlstealth siRNAs were also obtained from Invitrogen. ${Delta}$ DH (aminoacids 1–734 and 993–1,577), ${Delta}$ N (amino acids 747–1,577),and ${Delta}$ C (amino acids 1–1,276) with or without stop codonswere generated by PCR and, subsequently, subcloned into thepCA-Sal-Flag-IRES-hygromycin vector to obtain stable transfectants.Mouse ZO-1 cDNA (a gift from S. Tsukita, Kyoto University, Kyoto,Japan) was subcloned in a pCA-Sal-HA vector. The ZO-2 expressionvector CAG-NHA-ZO2-Ipuro and ZO-3 expression vector pME18S-ZO3-7mycwere also gifts from S. Tsukita. pCA-ß-catenin-HAwas constructed by K. Tanabe in our laboratory. The N-WASP expressionvectors pEF-BOS-myc-N-WASP and pEF-BOS-myc- ${Delta}$ cof-N-WASP were donatedby T. Takenawa (University of Tokyo, Tokyo, Japan). Recombinantadenoviruses expressing myc-N17-Cdc42 and myc-V12-Cdc42 wereprovided by H. Bito and S. Narumiya (Kyoto University, Kyoto,Japan).

Cell culture and transfection
Caco-2 cells were obtained from the American Type Culture Collection.All cell lines were cultured in a 1:1 mixture of DME and Ham'sF12 supplemented with 10% FCS. To enhance cell spreading, wecultured the cells on collagen-coated dishes. Cells at 70% confluencewere transfected by use of Effectene (QIAGEN), according tothe manufacturer's protocol. For siRNA treatments, cells weretransfected by the use of Lipofectamine 2000 (Invitrogen), accordingto the manufacturer's protocol. We obtained >90% reductionin the protein level for all siRNAs at 3–4 d after transfection,and all experiments were performed during this period. Adenovirusinfection was performed by incubating cells with a viral solutionfor 3–6 h. More than 80% of the cells were infected, andthe maximal expression of the transgene was observed at 24–48h after infection, the timeframe in which all experiments wereconducted. For isolating stable transfectants, transfected cellswere selected by exposure to 400 µg/ml G418 or 100 µg/mlhygromycin. In the case of RNAi-stable lines, the survivingcolonies were picked up and cloned, and then examined for theexpression of targeted proteins by Western blotting. Multipleclones were isolated for each target sequence, in which >90%knockdown of protein expression was achieved. For the stabletransfectants of deletion mutants, the cells were maintainedas uncloned populations. For calcium-switch experiments, cellswere cultured overnight in calcium-free DME (Invitrogen) supplementedwith 10% dialyzed FCS. Cell adhesion was initiated by adding1.8 mM CaCl₂ to the medium. Y-27632 (Calbiochem) was added tocultures at a final concentration of 10 µM, and the cellswere fixed after 30 min.

Antibodies
Mouse mAb 5G6 against Tuba was raised by the standard proceduredescribed in this section. The C-terminus of human Tuba (aminoacids 1,288–1,552) was amplified by PCR and subclonedin the pGEX4T-2 vector (GE Healthcare). The fusion protein waspurified by using a GSTrap column (GE Healthcare) accordingto the manufacturer's protocol. BDF-1 mice (CLEA Japan) wereimmunized at 4-wk intervals by the i.p. injection of 15 µgper mouse of GST–human Tuba C terminus emulsified withRIBI adjuvant. 5 d after the final immunization, the splenocyteswere recovered and fused with P3-X63-Ag-U1 myeloma cells. Culturesupernatants were screened by immunofluorescence and Westernblotting for their reactivity to Tuba-GFP–stable transfectants,and positive wells were cloned by limited dilution.

The following primary antibodies were used: rabbit polyclonalantibody against ${alpha}$ -catenin (C-2081; Sigma-Aldrich), rabbit polyclonalantibody against ZO-1 (61–7,300; Invitrogen), mouse mAbT8-754 specific for ZO-1 (a gift from S. Tsukita; Itoh et al., 1991),rabbit polyclonal antibody against ZO-2 (H-110; Santa Cruz Biotechnology,Inc.), rabbit polyclonal antibody against l-afadin (Sigma-Aldrich),mouse mAb 5H10 against ß-catenin (a gift from M.J.Wheelock, University of Nebraska, Omaha, NE; Johnson et al., 1993),mouse mAb HECD-1 specific for human E-cadherin (Shimoyama et al., 1989),mouse mAb against p120-catenin (BD Biosciences), mouse mAb againstCdc42 (BD Biosciences), rabbit polyclonal antibody against N-WASP(H-100; Santa Cruz Biotechnology, Inc.), mouse mAb against MLCs(Sigma-Aldrich), mouse mAb specific for phospho-MLC 2 (Ser19;Cell Signaling Technology), rabbit polyclonal antibody againstIQGAP1 (H-109; Santa Cruz Biotechnology, Inc.), mouse mAb DM1Aagainst ${alpha}$ -tubulin (Sigma-Aldrich), mouse mAb AC-15 against ß-actin(Sigma-Aldrich), rabbit polyclonal antibody reactive with myosinIIA (Sigma-Aldrich), rabbit polyclonal antibody against myosinIIB (Sigma-Aldrich), mouse mAb M2 against Flag (Sigma-Aldrich),rabbit polyclonal antibody specific for Flag (Sigma-Aldrich),rabbit polyclonal antibody against myc (for immunofluorescence;Santa Cruz Biotechnology, Inc.), rabbit polyclonal antibodyagainst myc (for immunoprecipitation; Sigma-Aldrich), mousemAb 16B12 reactive with HA (CRP), and rabbit polyclonal antibodyagainst HA (Millipore). The following secondary antibodies wereused: goat Alexa Fluor 488/594–conjugated anti–mouseor anti–rabbit IgG (Invitrogen) and sheep HRP-conjugatedanti–mouse or anti–rabbit IgG (GE Healthcare). F-actinwas visualized by using Alexa Fluor 488–conjugated phalloidin(Invitrogen).

Immunofluorescence staining
For staining Tuba, ZO-1, ZO-2, and l-afadin, cells were fixedwith 100% methanol at –20°C for 20 min. For stainingCdc42, cells were fixed in 10% TCA at 4°C for 15 min, andpermeabilized with 0.2% Triton X-100 for 15 min at RT (Hayashi et al., 1999).Otherwise, cells were fixed with 4% PFA for 20 min or 1.25%PFA for 5 min (for phospho-S19-MLC) by directly adding a 1/4or 1/16 volume of prewarmed 20% PFA/HBSS to the medium, andpermeabilized with 0.1% Triton X-100 for 15 min. Blocking wasdone by incubating the fixed cells with 5% skim milk in TBSfor 10 min at RT. After the antibodies had been diluted withthe blocking solution, the cells were incubated at RT for 1h with the primary antibody, and then for 30 min with the secondaryantibody. Samples were mounted in FluorSave (Calbiochem), andimaged by use of a laser scanning confocal microscope (LSM510)mounted on an inverted microscope (Axiovert 100M), using Plan-Neofluar40x/1.30 NA and Plan-Apochromat 63x/1.40 NA objectives (allCarl Zeiss MicroImaging, Inc.). All images were processed byuse of Photoshop (Adobe) software.

Quantification of immunofluorescent signal intensity was doneby Scion Image (Scion Corp.). In brief, the junctional regionswere manually encircled (see Fig. 4 B for example), and thesignal density of each region was measured. The measurementof linearity index was done by LSM 5 Image Browser (Carl ZeissMicroImaging, Inc.). All statistical analysis was performedby using Excel (Microsoft).

Biochemical assays
For immunoprecipitation, the cells were lysed in lysis buffer(50 mM Tris-HCl, pH 7.5, containing 150 mM NaCl, 0.5% NP-40or Triton X-100, 1 mM EDTA, and 10% glycerol); NP-40 was usedin the myc-N-WASP immunoprecipitation experiments. Lysates wereprecleared with protein G–Sepharose 4FF beads (GE Healthcare)and incubated with anti-myc polyclonal antibody or anti-HA mAbfor 1 h, followed by incubation with protein G–Sepharosebeads for 1 h. The beads were subsequently washed three timesin the lysis buffer.

For Cdc42 pull-down assays, cells were lysed in HS-buffer (20mM Tris-HCl, pH 7.4, containing 500 mM NaCl, 5 mM MgCl₂, and1% Triton X-100). 10 µg of GST-PAK CRIB domain (a giftfrom S. Narumiya) was added to the lysate. After 1 h incubation,the lysate was incubated for another 1 h with glutathione–Sepharose4B beads (GE Healthcare). The beads were subsequently washedthree times in HS buffer.

For the Triton X-100 solubility experiments, cells were lysedin lysis buffer (50 mM Tris-HCl, pH 7.5, containing 150 mM NaCl,and 0.5% Triton X-100), and incubated for 30 min on ice. Lysateswere centrifuged at 17,000 g for 10 min, and the supernatantswere recovered (soluble fraction). The remaining pellet wasresuspended to Laemmli sample buffer (insoluble fraction).

All samples were eluted by boiling them in the Laemmli samplebuffer, resolved by SDS-PAGE using 10–20% gradient gels(Daiichi Pure Chemicals) for MLC, phospho-S19-MLC, and Cdc42,and using 7.5% gel for others, and transferred to nitrocellulosemembrane. Blocking was done using 5% skim milk in TBS. Primaryand secondary antibodies were diluted in either the blockingsolution or Can Get Signal (TOYOBO), and the membranes wereincubated for 1 h with each. Membranes were washed with 0.05%Tween-20 in TBS three times after each antibody incubation,and signals were detected by use of the ECL-plus system (GEHealthcare).

Online supplemental material
Fig. S1 shows that Tuba interacts with ZO-2, but not with ZO-3.Fig. S2 shows the effects of ZO-1 knockdown on junction morphologyand myosin localization in comparison with Tuba depletion. Fig.S3 shows that the DH domain of Tuba preferentially activatesCdc42 in vitro. Fig. S4 shows the effects of N-WASP expressionon Tuba-RNAi cells. Online supplemental material is availableat http://www.jcb.org/cgi/content/full/jcb.200605012/DC1.

Acknowledgments

We thank S. Yonemura, S. Narumiya, H. Bito, T. Takenawa, M.J.Wheelock, and S. Tsukita for reagents; M. Furuse, and Y. Takaifor valuable suggestions; M. Negishi and T. Tanoue for criticalreading of the manuscript; and H. Ishigami, M. Harata, M. Uemura,and C. Yoshii for technical assistance.

This work was supported by a grant (to M. Takeichi) from theprogram Grants-in-Aid for Specially Promoted Research of theMinistry of Education, Science, Sports, and Culture of Japan.

Submitted: 2 May 2006

Accepted: 6 September 2006

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