Guanine Nucleotide Exchange Factor-H1 Regulates Cell Migration via Localized Activation of RhoA at the Leading Edge

Perihan Nalbant^*^,, Yuan-Chen Chang^*^,, Jörg Birkenfeld^*^,, Zee-Fen Chang, and Gary M. Bokoch^*

*Departments of Immunology and Microbial Science, and Cell Biology, The Scripps Research Institute, La Jolla, CA 92037; Department of Molecular Cell Biology, Center for Medical Biotechnology, University of Duisburg-Essen, 45117 Essen, Germany; Institute of Biochemistry and Molecular Biology, College of Medicine, National Taiwan University, Taipei 100, Taiwan

Submitted January 14, 2009; Revised July 1, 2009; Accepted July 9, 2009
Monitoring Editor: Paul Forscher

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cell migration involves the cooperative reorganization of theactin and microtubule cytoskeletons, as well as the turnoverof cell–substrate adhesions, under the control of Rhofamily GTPases. RhoA is activated at the leading edge of motilecells by unknown mechanisms to control actin stress fiber assembly,contractility, and focal adhesion dynamics. The microtubule-associatedguanine nucleotide exchange factor (GEF)-H1 activates RhoA whenreleased from microtubules to initiate a RhoA/Rho kinase/myosinlight chain signaling pathway that regulates cellular contractility.However, the contributions of activated GEF-H1 to coordinationof cytoskeletal dynamics during cell migration are unknown.We show that small interfering RNA-induced GEF-H1 depletionleads to decreased HeLa cell directional migration due to theloss of the Rho exchange activity of GEF-H1. Analysis of RhoAactivity by using a live cell biosensor revealed that GEF-H1controls localized activation of RhoA at the leading edge. Theloss of GEF-H1 is associated with altered leading edge actindynamics, as well as increased focal adhesion lifetimes. Tyrosinephosphorylation of focal adhesion kinase and paxillin at residuescritical for the regulation of focal adhesion dynamics was diminishedin the absence of GEF-H1/RhoA signaling. This study establishesGEF-H1 as a critical organizer of key structural and signalingcomponents of cell migration through the localized regulationof RhoA activity at the cell leading edge.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cell migration plays key roles in the regulation of such criticalprocesses as wound healing, neuronal development, and immuneresponsiveness. It is now well established that the Rho GTPaseproteins RhoA, Rac, and Cdc42 regulate cell migration throughthe precise spatial and temporal coordination of dynamic actin-basedstructures, such as the protrusive lamellipodia found at theleading edge of migrating cells. In addition, Rho GTPases regulateintegrin-based adhesion sites to control cell attachment, spreading,and detachment (for reviews, see Hall, 1998; Ridley, 2001; Etienne-Mannevilleet al., 2002). Whereas Rac and Cdc42 promote nascent focal contactformation in dynamic protrusions at the leading edge, RhoA mediatescontractile actin stress fiber assembly, a process importantfor the maturation of focal contacts into larger focal adhesions(FAs). A strong correlation exists between the traction forcegenerated by cell–substratum adhesion and the growth andturnover of focal adhesions during cell migration (for review,see Bershadsky et al., 2003). The diversity of Rho GTPase signalingduring migration is thought to ensure a fine balance betweencell adhesion and protrusion that is critical for efficientand controlled translocation (for review, see Ridley et al.,2003).

A key event for the spatiotemporal regulation of motility isthe localized activation of Rho GTPases. Earlier studies hadlinked Rac1 activity to protrusion of the leading edge, whereasRho activity had been shown to be required for contractile activitythat supported retraction of the cell body and trailing tail(for reviews, see Etienne-Manneville, 2002; Ridley, 2001; Worthylakeand Burridge, 2001). These observations and others supporteda simple view of Rac activation primarily at the cell anterior,with Rho activation at the cell posterior. However, the activitiesof Rho proteins in migrating cells have recently been visualizedusing real-time fluorescent biosensors, and the highest levelsof activity observed with Rac1, Cdc42, and RhoA have all beenpredominantly in the dynamic leading edge (Kraynov et al., 2000;Gardiner et al., 2002; Nalbant et al., 2004; Pertz et al., 2006).Interestingly, Cdc42 and Rac1 were activated $~$ 2 µm behindthe leading edge during cell protrusion, and their activitydecreased in a broad gradient toward the cell interior (Machaceket al., 2009). In clear contrast, RhoA activity unexpectedlydisplayed a peak adjacent to the very cell edge synchronouswith edge advancement, whereas there was a delay in Cdc42 andRac1 activation relative to the initiation of protrusion (Pertzet al., 2006; Machacek et al., 2009). These data are consistentwith studies demonstrating that RhoA signaling is functionallyassociated with leading edge extension, ruffling, and motility(Fukata et al., 1999; Matsumoto et al., 2001; Palazzo et al.,2001; Kurokawa et al., 2005; El-Sibai et al., 2008). There isvery little knowledge of molecular pathways regulating localizedRho activity in migrating cells and the relevance of such signalingfor coordinated cell translocation is still unclear.

Interestingly, various studies have implicated Rho GTPase-dependentcross-talk between microtubules (MTs) and the actin cytoskeletonduring cell migration (for reviews, see Wittmann and Waterman-Storer,2001; Etienne-Manneville, 2004). Coordinated actin dynamicsrequires an intact MT cytoskeleton, because lack of a functionalmicrotubule lattice inhibits cell polarization and dynamicsof leading edge lamellipodia (Mikhailov and Gundersen, 1998;Etienne-Manneville and Hall, 2001; Baudoin et al., 2008). DynamicMTs at the leading edge of migrating cells are necessary forefficient Rac-dependent protrusive behavior, whereas in turnRac signaling promotes MT penetration into the leading edge,suggesting a positive feedback loop (Waterman-Storer et al.,1999; Wittmann et al., 2003). Nocodazole-induced depolymerizationof MTs suppresses cell protrusion, while increasing RhoA-dependentcontractility and actin stress fiber formation (Danowski, 1989;Enomoto, 1996). It is therefore conceivable that during migrationdiscrete localized Rho activities function to regulate cross-talkbetween these two cytoskeletal networks in a spatial and temporalmanner.

Multiple guanine nucleotide exchange factors (GEFs) that activateRho GTPases in vitro and in vivo have been identified (for review,see Rossman et al., 2005). The Rho-specific exchange factorGEF-H1 is of particular interest, because its catalytic activitytoward RhoA is negatively regulated by MT binding (Ren et al.,1998; Krendel et al., 2002). Chang et al. (2008) showed thata signaling cascade composed of GEF-H1/RhoA/Rho kinase (ROCK)and myosin light chain (MLC) plays a critical role in mediatingcell contractility induced by microtubule depolymerization (Changet al., 2008). In addition to this direct effect on cell contractility,GEF-H1 has also been found to be a component of tight junctionsand is important for the integrity of cell–cell adhesion(Benais-Pont et al., 2003). Although both of these processesare important in cell motility, the exact role of GEF-H1 upstreamof RhoA activity in migrating cells is not known. However, acritical role for GEF-H1 in regulating RhoA activation duringcleavage furrow initiation in dividing HeLa cells has been demonstrated(Birkenfeld et al., 2007).

Here, we investigated the effects of GEF-H1 depletion by usingsmall interfering RNA (siRNA) technology on localized RhoA activityin the context of cell motility. GEF-H1 depletion led to aberrantlocalized RhoA activation in the leading edge, accompanied byreduced migration. The lack of proper actin-myosin-based contractilityin the affected cells, along with decreased turnover of focaladhesions, gave rise to dramatic changes in actin and protrusiondynamics at the cell edge. Our data reveal GEF-H1 as a criticalcomponent of the locomotory machinery, coordinating multipleRhoA-dependent signaling pathways during the migration of cells.

MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Reagents and Antibodies
Nocodazole was purchased from Sigma-Aldrich (St. Louis, Mo.)and was dissolved in dimethyl sulfoxide. Generation and affinitypurification of the polyclonal anti-GEF-H1 antibody used inthis study has been described previously (Zenke et al., 2004).The antibody was used at 1:1000 in immunoblots and 1:100 inimmunofluorescence (IF) experiments. The following commercialantibodies were used: for immunostaining, monoclonal anti- ${alpha}$ -tubulin(clone B-5-1-2; Sigma-Aldrich) and anti-paxillin antibodies(BD Biosciences Transduction Laboratories, Lexington, KY) at1:1000 and 1:500 dilution, respectively. Alexa-labeled secondaryantibodies (Invitrogen, Carlsbad, CA) and rhodamine-labeledphalloidin (Sigma-Aldrich) were used at 1:500 dilution.

For immunoprecipitation (IP) experiments and immunoblots, thefollowing antibodies were used: monoclonal anti-paxillin (BDBiosciences Transduction Laboratories; 1:100), monoclonal anti-Myc(9E10, prepared in-laboratory; 1:200), monoclonal anti-actin(C4, MP Biomedicals, Solon, OH; 1:10,000), monoclonal anti-phosphotyrosine(clone 4G10, Millipore, Billerica, MA; 1:4000), monoclonal anti-focaladhesion kinase (FAK) (clone 4.47, Millipore; 1:1000), and anti-pFAK(rabbit, pY397, Invitrogen; 1:2000).

Cell Culture and RNA Interference
HeLa cells were maintained in DMEM (Invitrogen) containing 8%fetal bovine serum (FBS), 2 mM L-glutamine, 100 U/ml penicillinG, and 100 U/ml streptomycin. For RNA interference experiments,nontargeting control, GEF-H1- (siGenome, ON-Target Plus), andmDia1- [si-mDia1(K2)] targeting duplex oligonucleotides werepurchased from Dharmacon RNA Technologies (Boulder, CO). ThesiRNA pool targeting GEF-H1 contained the following four oligonucleotides(oligos): oligo 6 (J-009883-06, 5'-GAAUUAAGAUGGAGUUGCAUU-3'),oligo 7 (J-009883-07, 5'-GUGCGGAGCAGAUGUGUAAUU-3'), oligo 8(J-009883-08, 5'-GAAGGUAGCAGCCGUCUGUUU-3'), and oligo 9 (J-009883-09,5'-CCACGGAACUGGCAUUACUUU-3'). The sequence of the mDia1 targetingoligonucleotide (LUJAF-000492) was 5'-GCUGGUCAGAGCCAUGGAU-3'.For the assay, $~$ 150,000 HeLa cells grown per well of a six-wellplate were transfected with control, GEF-H1 (10 nM final) ormDia1 (100 nM final) siRNA by using 4 µl of Lipofectamine2000 (Invitrogen). At 24 h after transfection, cells were trypsinizedand replated on glass coverslips, and live-cell differentialinterference contrast (DIC) imaging was conducted at 72 h aftertransfection. For assays requiring overexpression of exogenousenhanced green fluorescent protein (EGFP)-tagged proteins, cellswere transfected with the appropriate constructs at 48 h afterthe siRNA transfection, and fluorescence imaging was then performedthe next day (72 h after siRNA transfection). As control forpossible off-target effects, each single oligo was tested.

DNA Constructs
EGFP-GEF-H1-wild type (WT) and EGFP-GEF-H1-(DH) constructs inthe mammalian expression vector pCMV5 have been described previously(Krendel et al., 2002; Zenke et al., 2004). Mutant constructsresistant to the siRNA oligo 9 [EGFP-GEF-H1-WT^9R and EGFP-GEF-H1-(DH^9R)]were generated by site-directed mutagenesis as described inChang et al. (2008). The constructs encoding for EGFP-EB1 andEGFP-actin were gifts from Leif Dehmelt (TSRI). EGFP-paxillinwas a gift from Clare Waterman-Storer (National Institutes ofHealth, Bethesda, MD). The RhoA biosensor construct for live-cellfluorescence resonance energy transfer (FRET) experiments waskindly provided by Olivier Pertz (Center for Biomedicine, Universityof Basel, Basel, Switzerland) and Klaus Hahn (University ofNorth Carolina, Chapel Hill, NC). The generation of stable biosensor-expressingHeLa cell lines were described in Birkenfeld et al. (2007).

Migration Experiments
For two-dimensional (2D) migration studies, cells were replatedon glass coverslips 24 h after siRNA transfection at high density(2 x 10⁵/well of a six-well plate). At 72 h after transfection,a scratch was generated. After 30 min recovery time phase-contrasttime-lapse movies of randomly chosen regions were imaged usinga 20x objective lens and a frame rate of 1 min. Migration areawas analyzed using standard image analysis tools provided byMetaMorph (Molecular Devices, Sunnyvale, CA). Three-dimensionalmigration was assessed using a modified Boyden chamber transwellassay with 8-µm pore filters (Millipore) coated with fibronectin(10 µg/ml; Sigma-Aldrich). At 54 h post-siRNA transfection,HeLa cells were incubated in migration medium (DMEM with 1%FBS) for 18 h and then trypsinized. Cells were resuspended infresh migration medium and placed in the upper chamber of thefilter (10⁵ cells in 300 µl). The lower chamber of thetranswell was filled with 400 µl of migration medium eitherwith or without 20% FBS. After 6 h of incubation, the filterswere removed and the migrating cells on the underside of thechamber were fixed using 4% paraformaldehyde. Cells were visualizedby 0.1% crystal violet staining. Randomly, 10 images of eachfilter were captured using a 20x objective lens to calculatethe number of migrated cells (n = 6 filters for each condition;n = 3 filters to determine total cell numbers). To determinethe overall number of cells used for each transfection condition,additional transwell filters were used in parallel, and thenumber of cells in the upper side together with the number ofcells in the bottom side of the chamber was counted (n = 3 filtersfor each condition).

Immunofluorescence and Cell Imaging
For immunofluorescence staining, cells were fixed with 4% paraformaldehydefor 20 min at 37°C, permeabilized with 0.5% Triton X-100for 5 min at room temperature followed by blocking with 5% bovineserum albumin in phosphate-buffered saline (PBS) for 1 h. Specimenswere incubated with the appropriate primary and secondary antibodiesat the indicated dilutions.

Fluorescence and brightfield imaging was performed on a fullyautomated TE2000-U microscope (Nikon, Tokyo, Japan) controlledby MetaMorph software (Molecular Devices) equipped with a CoolSNAPFX camera (Roper Scientific, Trenton, NJ). Images were acquiredusing a 20x phase contrast or 60x/1.4 numerical aperture (NA)oil objective with appropriate filter sets. Time-lapse imagingof migrating cells was carried out in a sealed chamber at 37°Cand with indicated frame rates. For fluorescence experiments,live-cell imaging medium was used (F-12 medium without phenolred [Invitrogen] supplemented with 8% FBS, 2 mM L-glutamine,and 2 mM HEPES). Image processing was performed with MetaMorph(Molecular Devices), ImageJ (http://rsb.info.gov/ij/), and AdobePhotoshop software (Adobe Systems, Mountain View, CA).

FRET Imaging of RhoA Activation in Living Cells
Localized RhoA activation was visualized using a live-cell FRETprobe described previously (Pertz et al., 2006). HeLa cellsstably expressing the RhoA probe were used for FRET activityassays (Birkenfeld et al., 2007). Biosensor cells were transfectedwith nontargeting control or GEF-H1–specific siRNA for48–72 h. Live-cell FRET imaging was performed with multiplecells randomly selected from each population. Cyan fluorescentprotein (CFP) and FRET images were acquired using a 60x/1.4NA oil objective and the following fluorescence filter sets(Chroma Technology, Brattleboro, VT) for sensitized emissionFRET assay: CFP, D436/20, D470/40; and FRET, D436/20, HQ535/30.A dichroic mirror was custom manufactured (Chroma Technology)for compatibility with all the filters named above. Cells wereilluminated with a 200-W Hg lamp, and exposure times were adjustedto the expression level of the RhoA biosensor (typically 50–100ms, with 2 x 2 binning). Image analysis was performed usingMetaMorph (Molecular Devices) and ImageJ software (http://rsb.info.gov/ij/)essentially as described previously (Pertz et al., 2006; Birkenfeldet al., 2007). In brief, each image was shading corrected andbackground subtracted. A threshold based mask was generatedand applied to each CFP and FRET image. By doing so, noise outsideof the cell was eliminated. In a final step, the image representingRhoA activity was generated by dividing the processed FRET imageby the corresponding CFP image. As images were acquired sequentially,the postimaging ratiometric process might generate artifactsdue to motion between two acquisitions. To account for suchpossible artifacts a control ratio image was generated usingtwo sequentially acquired CFP images for the ratio operation.This technique reveals maximum false positive signal originatingfrom cell movement during the time lapse.

Paxillin Immunoprecipitation (IP) and Tyrosine Phosphorylation
Tyrosine phosphorylation of paxillin was assessed by IP andsubsequent immunoblotting. At 72 h after siRNA-transfection,cells in 100 mm-diameter dishes were rinsed with ice-cold PBSand scraped off into lysis buffer (50 mM Tris-HCl, pH 7.5, 1%NP-40, 0.1% SDS, 0.25% sodium deoxycholate, 10 mM NaF, 2 mMNa₂VO₄, 5 mM MgCl₂, 150 mM NaCl, 1 mM dithiothreitol [DTT],1 mM β-glycerophosphate, 1 mm phenylmethylsulfonyl fluoride[PMSF],and appropriate dilutions of the protease inhibitors leupeptin,aprotinin, and pepstatin). After syringe shearing, the insolubledebris was removed by centrifugation at 13,000 x g for 10 minat 4°C. Aliquots of lysates were incubated with the primarymouse anti-paxillin or anti-myc antibody for 2.5 h at 4°C,and protein A-agarose was added for additional 0.5 h. Immunecomplexes were washed four times in lysis buffer without SDSand sodium deoxycholate. IPs or total lysates were subjectedto SDS-polyacrylamide gel electrophoresis (PAGE) for immunoblotanalysis using the antibodies against phospho-Tyr (4G10), GEF-H1,and actin. IPs were confirmed by stripping the membrane of phospho-Tyrantibody and reprobing with anti-paxillin antibody. The proteinswere detected by enhanced chemiluminescence according to themanufacturer's instructions.

FAK Activation
After 72 h of siRNA treatment, cells were lysed in lysis buffer(50 mM Tris-HCl, pH 7.5, 1% NP-40, 10 mM NaF, 2 mM Na₃VO₄, 5mM MgCl₂, 150 mM NaCl, 1 mM EDTA, 1 mM DTT, 1 mM β-glycerophosphate,1 mM PMSF, and appropriate dilutions of the protease inhibitorsleupeptin, aprotinin, and pepstatin). Cell lysates were separatedby SDS-PAGE, transferred to membranes, and subjected to Westernblot to visualize pFAK (Tyr397), indicating the level of activeFAK.

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

GEF-H1 Depletion Inhibits Cell Migration in a Rho-dependent Manner
GEF-H1 is a Rho-specific guanine nucleotide exchange factorthat mediates cross-talk between the MT and actin cytoskeletonsthrough the MT-dependent activation of Rho/ROCK-mediated acto-myosin-dependentcontractility and stress fiber formation. Supplemental Movie1 shows that the control HeLa cells used in these experimentswere highly motile. To assess the role(s) of GEF-H1 in HeLacell migration, we used siRNA to deplete GEF-H1. GEF-H1 knockdownwas efficient, with >95% siRNA-transfected cells (SupplementalFigure S1A), and depletion of >80% of endogenous GEF-H1 routinelyobserved (Figure 1, A and B). Single cell analysis using immunostainingfor endogenous GEF-H1, as well as expression of exogenous EGFP-taggedGEF-H1 in the presence of GEF-H1 siRNA, revealed significantdecrease of GEF-H1 protein in the majority of the cells belowthe minimum levels detected in control cells (Supplemental FigureS1, B and C).

View larger version (48K):
[in this window]
[in a new window]

Figure 1. GEF-H1–depleted cells migrate slower. (A) Three-dimensional migration of HeLa cells is inhibited upon GEF-H1 depletion. At 72 h post-siRNA transfection, cells were either harvested for Western blotting or seeded on a 3D migration filter coated with fibronectin matrix to allow migration through the filter for 6 h. Left, percentage of migrated cells. Results are means ± SD from three independent transfection experiments. Middle, GEF-H1 protein level in control and GEF-H1 siRNA treated cells. GEF-H1 amount was quantified by Western blot using anti-GEF-H1 antibody at 72 h post-siRNA transfection. Results are means ± SD from n = 8 independent transfection experiments. Right, representative blot. See also Supplemental Figure 1 for single cell quantification. (B) Transfection of siRNA-resistant EGFP-GEF-H1 plasmids in HeLa cells. Cells were treated with control or GEF-H1-specific #9 siRNA and transfected with the indicated EGFP-GEF-H1 plasmids 48 h post-siRNA treatment. 9R and 9R^DHmut represent EGFP-GEF-H1 constructs resistant to GEF-H1-specific siRNA oligo #9. At 72 h post-siRNA transfection, cells were lysed to analyze GEF-H1 expression level by Western blot using anti-GEF-H1 antibody (left). In parallel, transfected cells were fixed to visualize EGFP fluorescence together with nuclear 4,6-diamidino-2-phenylindole staining to quantify the percentage of EGFP positive cells (right). Results are ±SD from three independent experiments. (C) In vitro wound healing of HeLa cells in 2D. At 72 h post-siRNA transfection, a scratch was generated into the confluent monolayer and cells were allowed to migrate for 2 h. Cell outlines were drawn along the wound edge at time = 0 h (imaging start) and 2 h, as indicated in the bottom panel. Migration was quantified by calculating the area between the two outlines by using MetaMorph software. Results are the means ± SD of four independent experiments. Bottom, representative migration area after 2 h of wound closure of control and GEF-H1–specific #9 siRNA-treated cells. *p < 0.05 and **p < 0.01.

GEF-H1–depleted cells exhibited significantly slower migrationbehavior in in vitro three-dimensional migration experimentsby using fibronectin-coated filters, as well as in wound healingassays (Figure 1, A and C). The magnitude of the effect wascomparable in both assays, suggesting that similar pathwaysdownstream of GEF-H1 might be affected in each scenario. Thedecrease in cell migration observed in the GEF-H1–depletedcells was not due to differences in cell viability (SupplementalFigure S2).

To verify that the observed migration defect was specificallycaused by the depletion of GEF-H1, we cotransfected cells expressingthe GEF-H1 siRNA with an siRNA-resistant mutant of EGFP-taggedwild-type GEF-H1 (EGFP-GEF-H1^9R). This led to increased cellmigration in the in vitro scratch assay compared with the expressionof an siRNA-sensitive GEF-H1-wt construct, confirming the specificityof the siRNA effects (Figure 1C). By introducing a mutationinto the DH-region of this siRNA-resistant construct (EGFP-GEF-H1-DH^9R),we were able to test whether the catalytic exchange activityof GEF-H1 was involved in the decreased migration efficiency.Indeed, we observed that cotransfection of the inactive construct(EGFP-GEF-H1-DH^9R) with GEF-H1 siRNA was unable to rescue cellmigration, and the migration efficiency was similar to thatof the siRNA-targeted GEF-H1-wt construct. Thus, the decreaseof migration efficiency upon GEF-H1 depletion is a result ofthe loss of GEF-H1 Rho exchange activity.

GEF-H1 Depletion Causes Aberrant RhoA Activation Dynamics at the Leading Edge
The requirement for intact Rho GEF activity of GEF-H1 for normalcell motility led us to examine the activity of its target GTPase,RhoA, during cell motility. As we had shown previously, whenwe measured bulk RhoA activity with an affinity-based pull-downassay, we could not detect any significant change of overallRhoA-GTP levels in cells depleted of GEF-H1 (Chang et al., 2008).This was perhaps not unexpected, because only a small proportionof the entire Rho GTPase protein pool might be active in cellsgrowing in serum. Moreover, Rho activation is likely to be subjectedto tight control by upstream regulators to permit highly localizedsignaling responses. Indeed, studies by us and others usingfluorescent activation biosensors in migrating cells have shownthat Rho GTPase activation is highly spatially and temporallyregulated, particularly at the cell leading edge (Kraynov etal., 2000; Gardiner et al., 2002; Kurokawa et al., 2004; Nalbantet al., 2004; Pertz et al., 2006; Machacek et al., 2009). Toassess whether GEF-H1 function is important for localized activationof RhoA during cell migration, we used a genetically encodedfluorescence biosensor based on FRET (Pertz et al., 2006). Usingthis probe, Pertz et al. (2006) previously showed that in randomlymigrating mouse embryonic fibroblasts, RhoA activity is localizedto distinct zones in dynamic protrusions. A band of high RhoAactivity was localized at the very distal part of the leadingedge in regions where protrusions were extending. In addition,high levels of RhoA activity were found on the distal side ofserum-induced membrane ruffles.

Similar to the observations by Pertz et al. (2006) in mouseembryonic fibroblasts, our studies of randomly migrating HeLacells also revealed highest RhoA activity in dynamic protrusionsand regions showing strong edge ruffling (Figure 2). This generaloverall distribution of RhoA activity was observed both in controland GEF-H1–depleted conditions (Figure 2A). Some cellsalso displayed high RhoA-GTP levels in their tail region, coincidentwith strong tail contraction. However, the latter was ratherrare (only 2 of 16 control cells) and could not be assessedstatistically. As observed with the affinity-based pull-downassay, when we compared the average cellular RhoA activity levelsusing the average RhoA FRET values in each cell, we could notdetect a significant difference in cells in which GEF-H1 hadbeen depleted (Figure 2D, top). However, when we quantifiedRhoA activity within 1 µm of the cell edge in membraneprotrusions relative to the overall activity (Figure 2D, bottom),there was a significant decrease of $~$ 50% in the GEF-H1–depletedcells.

View larger version (54K):
[in this window]
[in a new window]

Figure 2. Depletion of GEF-H1 perturbs localized activation of RhoA at the edge of migrating HeLa cells. HeLa cells stably expressing a FRET biosensor for RhoA activity were transfected with control- and GEF-H1-siRNA, respectively, with >95% efficiency, and then cells selected at random for imaging. FRET ratio images denote activity patterns of RhoA under the conditions depicted. (A) Two representative pseudocolor images for localization of RhoA activity are shown for each condition. Bar, 20 µm. n = 18 control and 14 GEF-H1–depleted cells, respectively, from three independent experiments. (B) Localized RhoA activation in cell protrusions over time was assessed using time-lapse movies and kymographs. The first frame of representative movies is shown for cells with control and GEF-H1 siRNA. Kymographs were generated using ImageJ software with a bin-width of 1 and subjected afterward to an in-built Gaussian Blur Filter ( ${sigma}$ radius = 1). Two typical kymographs per cell are shown (bar, 5 µm). The time-frame was 10 s for the duration of 4 min. (C) Motion control. False positive signals due to cell movement between the sequential CFP and FRET image acquisition. Three images were acquired: CFP-1, FRET, and CFP-2. Left, the actual ratio image was derived by dividing FRET by CFP-1. Right, the control image was obtained by dividing CFP-2 by CFP-1 to reveal maximum possible motion-related error. (D) Leading edge activity is decreased in cells depleted of GEF-H1. Top, average RhoA activation levels per cell were determined by measuring the average signal intensity of each ratio image with the built-in ImageJ "measure" tool. Results are means ± SEM from 34 (control) and 49 (GEF-H1–depleted) cells (n = 3 experiments). Bottom, RhoA activity in the leading edge relative to the cell average. A 1-µm-wide line was drawn along the border of each protrusion and average activity was measured within this region. Relative RhoA activity in the leading edge was calculated by division with overall average activity of the same cell. Only cells from time-lapse experiments were analyzed to focus on dynamic cell protrusions. Results are means ± SEM from 32 (control) and 33 (GEF-H1–depleted) cell protrusions with p value = 0.0047 (11 control and 10 GEF-H1 siRNA–treated cells).

To evaluate the dynamics of RhoA activation in randomly migratingcells, time-lapse movies were subjected to kymograph analysisin which line-scans of RhoA activity were plotted over time.In the control cells, RhoA activity remained restricted to adistinct "activity zone" at the leading edge, often with a peakof activity at the very cell edge (Figure 2B and SupplementalMovie S3A). This band of activity reflected high rates of rufflingand protrusive behavior in these regions. Indeed, there wasa good correlation between membrane protrusions that were eitheractively growing or stable and the maintenance of high RhoAactivity (Supplemental Figure S3). In contrast, although manyGEF-H1–depleted cells displayed relatively higher levelsof RhoA activity at the leading edge, they usually lacked thepeak activity zone seen in the control cells. In addition, theRhoA activity in this region was not stable in the absence ofGEF-H1 but displayed highly variable patterns with time (Figure 2Band Supplemental Movie S3B). Thus, depletion of GEF-H1 functionin HeLa cells disrupted the persistent localization of activeRhoA at the leading edge.

GEF-H1 Depletion Alters Leading Edge Behavior during Cell Migration
Because of the loss of concentrated RhoA activity at the leadingedge of randomly migrating cells, we wondered whether alterationsof leading edge morphology might be associated with the depletionof GEF-H1, providing a possible underlying cause for defectsin the motility of the cells. We used brightfield imaging andkymograph analysis of phase-contrast and DIC movies to assessthe integrity and dynamics of control cells and GEF-H1–depletedHeLa cells (Figure 3 and Supplemental Movie S2). Control cellsusually displayed a very characteristic and highly organizedleading edge: individual small protrusions of routinely uniformsize and appearance were extended, which subsequently convertedinto dense ruffles with a regular rearward flow. The distancecovered by each ruffle during the inward flow was relativelysteady, leading to a highly regular appearance of the kymograph(Figure 3A, control kymograph). In contrast, the leading edgeof GEF-H1–depleted cells was extremely disorganized: Themembrane extensions seemed to be less regular than in controlcells and were often extremely large (Figure 3A, GEF-H1 siRNAkymograph; and B). Based on these observations we quantifiedthe percentage of cells with protrusions >2.5 µm. Significantlyhigher numbers of GEF-H1–depleted cells generated theselarge extensions compared with control cells (Figure 3C). Inaddition, the ruffling was more random than in control cells.Both effects were accompanied by a decreased persistency ofthe generated protrusions, which tended to collapse to the pointof origin rather than adhere (Supplemental Movie S2, GEF-H1depleted). This behavior was detected in 70.0 ± 2.6%of GEF-H1–depleted cells, whereas only 20.8 ± 8.3%of control cells exhibited disorganized ruffling (n = 3 experiments,with 73 control and 95 GEF-H1 siRNA-treated cells). Interestingly,we also noted that GEF-H1 depletion not only changed the dynamicbehavior of the leading edge, but also increased the overallnumber of cells that displayed a ruffling phenotype (control,66 ± 9.9% vs. GEF-H1 depleted, 91.4 ± 1.5). Specificityof this phenotype was confirmed by using each individual oligonucleotideincluded in the siRNA mix targeting GEF-H1 (Supplemental FigureS4). This finding suggests that the molecular pathways necessaryfor initiation of protrusion and ruffle generation might beintact, albeit poorly controlled, in GEF-H1–depleted cells.

View larger version (69K):
[in this window]
[in a new window]

Figure 3. Dynamics of the leading edge is altered in GEF-H1 depleted cells. Cells were replated on glass coverslips 24 h post-siRNA transfection and subjected to time-lapse DIC microscopy at 72 h after transfection. Ruffling cells were chosen randomly for imaging purposes. Ruffling was defined by three-dimensional movement of the cell membrane inward from the leading edge. (A) Kymograph analysis of control- and GEF-H1–depleted cells. Left, representative images (first frame) of control- and GEF-H1–depleted cell movies. Bar, 10 µm. Right, representative kymographs. Kymographs of 73 control and 95 GEF-H1–depleted cells were generated using a built-in macro in MetaMorph software (n = 3 independent experiments). Frame rate, 5 s. The bottom two panels show a representative region of a control and GEF-H1–depleted cell, respectively. The maximum size of individual protrusions is indicated by yellow arrows. (B) Kymographs were used to measure maximum protrusion size during time-lapse recordings. n = 11 control and 10 GEF-H1–depleted cells from two independent experiments were analyzed. In total, 695 (control) and 602 (GEF-H1 siRNA) protrusions were measured. (C) Percentage of cells forming extensions >2.5 µm. Extensions were measured using the line tool. Each cell observed by time-lapse imaging was analyzed to avoid bias. Cells which formed neither ruffles, nor protrusions were neglected. Results are means ± SD of 76 control and 87 GEF-H1–depleted cells from three independent DIC time-lapse experiments. Significance between the two conditions was tested using t test analysis (**p < 0.01).

GEF-H1 Depletion Alters Dynamics of the Leading Edge Actin Cytoskeleton
We used fluorescence imaging to assess whether the effects onleading edge behavior observed when GEF-H1-RhoA signaling wasperturbed were reflected by changes in the actin cytoskeleton.The most striking difference between control and GEF-H1–depletedcells regarding the actin cytoskeleton was the morphology anddensity of actin within the leading edge. Concomitant with thebrightfield studies (Figure 3), the leading edge of controlcells was well defined and contained a very dense populationof actin rich membrane ruffles (Figure 4, A and B). The widthof this F-actin–enriched area was relatively constantalong the entire protrusion. In contrast, cells lacking theRhoA GEF displayed a nonuniform, irregular actin staining, inwhich the actin-rich ruffles were neither densely packed, norcontinuous along the leading edge as in control cells (Figure 4,A and B, and Supplemental Figure S5). Interestingly, immunostainingwith an antibody against GEF-H1 showed strong colocalizationof endogenous GEF-H1 with F-actin in the ruffling membrane protrusionsof control cells, supporting a potential regulatory role ofGEF-H1 in the leading edge, presumably attenuating membraneruffling (Figure 4C; also see Supplemental Figure S6 for confocalimages).

View larger version (51K):
[in this window]
[in a new window]

Figure 4. The actin cytoskeleton is altered in cells lacking GEF-H1. (A) Actin cytoskeleton of control and GEF-H1–depleted cells. Cells were stained using rhodamine-conjugated phalloidin. Left, two cells during wound healing. Right, single migrating cells (see also Supplemental Figure S5 for quantification of actin staining in the leading edge). Bar, 5 µm. (B) Leading edge integrity is compromised in cells depleted of GEF-H1. Imaging was performed along the wound at randomly chosen regions, and every cell in each image was analyzed. For each individual cell, the length of the entire leading edge region was measured using the line tool (ImageJ). In a second step, length of ruffling regions within the leading edge was measured (depicted in red in the schematic). Ruffling was defined as actin accumulation in a typically curled shape similar to three-dimensional membrane folds observed in DIC movies. "Ruffling at cell border" was calculated as fraction of the leading edge. Results are means ± SD of n = 2 independent experiments with 179 control and 232 GEF-H1–depleted cells. Statistical significance of the difference between the two conditions was assessed using t test analysis of all control versus GEF-H1–depleted cells (p = 7.17 e^–11). (C) Colocalization of endogenous GEF-H1 and actin in membrane ruffles of migrating cells at the wound edge. (D) Stress fiber organization in the leading edge during wound healing. At low focus, actin fibers perpendicular to the cell edge were visible. (E) Example frames derived from the EGFP-actin movie of a control cell showing the formation of an actin bundle (red arrow) from an inward ruffling region (see also Supplemental Movie S4 and text). Frame rate, 5 s.

HeLa cells do not display very pronounced internal stress fiberscompared with fibroblasts. However, there were distinct differencesin the orientation of stress fibers between control and theGEF-H1–depleted condition. During wound healing, controlcells often displayed hemi-circumferential actin bundles whichwere localized in parallel to the leading edge and only visibleat low focus (Figure 4D, control). In contrast to the controls,GEF-H1–depleted cells rarely displayed ordered actin bundles(Figure D, GEF-H1 depleted). Both in wound healing experimentsand in single migrating cells, stress fibers were sparse andseemed randomly organized in cells lacking GEF-H1, without apreferential orientation with respect to the leading edge (Figure 4,A and D, GEF-H1 siRNA).

The half-rings observed in the control cells were reminiscentof the "actin arcs" described by other groups in neuronal growthcones and fibroblasts (Figure 4D, control) (Heath, 1983; Schaeferet al., 2002, 2008). The persistent flow of such actin arcshas been implicated in the dynamics and retrograde transportof MTs (Gupton et al., 2002; Schaefer et al., 2002, 2008). Time-lapsestudies with control cells using EGFP-tagged actin indicatedthat these actin fibers might indeed derive from the leadingedge and move rearward to align eventually with the stress fiberpopulation already existent in the cell body (Figure 4E andSupplemental Movie S4). Thus, GEF-H1 depletion severely disruptedthe actin cytoskeleton in HeLa cells, leading to a significantloss of F-actin organization both at the leading edge and towardthe cell interior.

GEF-H1 Depletion Alters Organization of the Microtubule Cytoskeleton
We could not detect significant changes in the microtubule-organizingcenter orientation in GEF-H1–depleted cells, indicatingthat the diminished migration observed was not due to defectsin cellular directionality (Supplemental Figure S7). However,we wondered whether in cells depleted of GEF-H1 the lack oftransverse actin bundles would affect the organization and dynamicsof the MT cytoskeleton. Anti-tubulin antibody staining of MTsshowed that MTs were more densely packed at the cell edge incells lacking GEF-H1 (Figure 5). In control cells the bulk ofdistinguishable MTs were present as an intertwined network oftenaligned parallel to, but localized in a considerable distancefrom, the leading edge (Figure 5A). This MT boundary regionwas defined by the arch-like parallel F-actin bundles presentin the control cells (Figure 5A). In contrast, MTs in GEF-H1–depletedcells were oriented perpendicular to the cell edge and extendedwell into the leading edge area (Figure 5, A and B).

View larger version (46K):
[in this window]
[in a new window]

Figure 5. Microtubule organization is perturbed upon GEF-H1 depletion. (A) Costaining of the actin and the MT cytoskeleton. The figure shows cells migrating into the wound. Cells were fixed at 2 h after wound and stained with rhodamine-conjugated phalloidin and anti- ${alpha}$ -tubulin antibody. To visualize the stress fibers, cells were imaged at low focus. A red line depicting the leading edge was generated based on the actin image and pasted onto the MT image to demonstrate the distance of MTs to the cell edge (enlarged box shown at right). (B) MT alignment with respect to the leading edge in migrating cells. Red line represents the actin boundary. (C) Quantification of MT tips approaching the leading edge. Cells were transfected with EGFP-EB-1 construct and subjected to fluorescence time-lapse imaging (frame rate, 5 s). The average number of EGFP-EB-1–decorated MT tips within a defined edge region was quantified as described in the bottom panels and in Supplemental Material. Results are means ± SD of four (control) and five (GEF-H1–depleted) cells, with each three analyzed regions. Statistical significance was assessed using Student's t test. p = 0.0048 (see also Supplemental Figure S9 for measurements with a significant number of fixed cells). (D) The velocity of EGFP-EB-1–decorated tips was measured using the Particle Tracker tool (ImageJ). Results are means ± SD of 196 (control) and 137 (GEF-H1–depleted) particles tracked in each five cells.

To measure the density of MT ends in the leading edge we performedtime-lapse imaging of EGFP-EB1—the MT plus-end bindingprotein (Supplemental Movie S5) (Morrison et al., 2002

). Usingthe image analysis software ImageJ (http://rsb.info.gov/ij/),we quantified plus-end tips in the leading edge, determiningthe average number of plus-end tips ([per square micrometer,per frame]) within a defined region along the edge (for protocol,see Supplemental Figure S8 and Supplemental Movie S6). In GEF-H1–depletedcells, we observed a highly significant increase in the numberof tips detected along the cell edge as compared with controlconditions (Figure 5C). In addition, quantitation of MT densityin the leading edge of fixed cells (Supplemental Figure S9)also showed a statistically significant difference between thetwo conditions.

To test whether MT growth was affected by GEF-H1 depletion aswell, we tracked EGFP-EB1 particles for each time-point to determinethe average tip velocity. Although there was a slight increasein GEF-H1–depleted cells, the difference in the velocityof MT tips between cells lacking the GEF and control cells wasnot significant (Figure 5D). Together, these observations suggestthat GEF-H1 depletion impacts on MT behavior at the leadingedge, perhaps resulting from deficient actin organization.

GEF-H1 Depletion Inhibits Focal Adhesion Turnover
RhoA signaling has been shown to regulate FA dynamics in variouscellular systems (for reviews, see Ridley, 2001; Etienne-Mannevilleand Hall, 2002; Kaverina et al., 2002). In particular, growthand maturation of focal complexes is driven by mechanical forcegenerated by the actin- and myosin-containing contractile stressfibers (for review, see Bershadsky et al., 2003). As shown inFigures 4 and 5A, stress fiber alignment during cell migrationis aberrant in GEF-H1–depleted cells, and we showed previouslythat RhoA/ROCK-dependent phosphorylation of myosin II is inhibitedin nocodazole-treated GEF-H1–deficient cells (Chang etal., 2008). Brightfield analysis of migrating cells revealedthat cells lacking GEF-H1 formed large protrusions at the leadingedge (Figure 2 and Supplemental Movie S2) that often failedto adhere; instead, they folded back and gave rise to a largeruffle. This observation suggested that aberrant RhoA activationat the leading edge might lead to defects in cell-substrateadhesion in the absence of GEF-H1.

We initially assessed FA organization by examining the FA-associatedprotein paxillin. Small focal complex-like structures were detectedin the leading edge of control migrating cells (Figure 6A, enlargedbox; and Supplemental Movies S8 and S9A). Behind this regionand under the cell body, we detected larger FAs of varying sizethat were often associated with actin stress fibers. In contrast,the general appearance of the FAs differed in the GEF-H1–depletedcells: first, the leading edge rarely displayed focal complexes(Figure 6A, enlarged box). Second, we often noted an increasednumber of large FAs in the body of GEF-H1–depleted cellscompared with control conditions (Figure 6A; data not shown).Overall, these observations suggested to us that FA turnovermight be affected in cells lacking the GEF-H1–RhoA pathway.

View larger version (66K):
[in this window]
[in a new window]

Figure 6. Turnover of focal adhesions is perturbed in GEF-H1-depleted cells. (A) Control or GEF-H1–depleted cells were fixed 2 h after wound and immunostained using antibody for paxillin together with rhodamine-labeled phalloidin. Arrow in enlarged control image indicates small focal complexes in the leading edge, whereas the arrow in the GEF-H1 siRNA-treated cell points to an extension deficient in paxillin-containing foci. (B) Left, representative EGFP-paxillin time-lapse images showing generation (red arrows) and dissolution (yellow arrows) of focal adhesions (see also Supplemental Movie S7). Right, frequency (percentage) of detected focal adhesions with the indicated "live-time" (detection duration). Particles were detected with IMARIS 5.0 software (Bitplane) and analyzed using Excel software (Microsoft, Redmond, WA). Binning, 4 min. Results are means ± SE of 10 regions in five control cells and 12 regions in six GEF-H1–depleted cells. Significance between the two conditions was tested for each time range. p < 0.05, **p < 0.01, and ***p < 0.001. (C) Focal adhesion sliding in GEF-H1–depleted cells is slower than in control cells. Time-lapse videos of EGFP-paxillin–expressing cells were recorded for 40 min and analyzed to track EGFP-paxillin containing focal adhesions by IMARIS 5.0. Representative snapshots: gray dots show detected EGFP-paxillin foci. Colored lines display the tracked path of each dot during the time-lapse experiment. (D) Accumulated distance of tracked focal adhesion dots as measured using Image-Pro Plus software. Figures show representative analyses in which the slope is indicative of the speed of the detected adhesion point. Each colored line represents a detected and traced focal adhesion.

We performed fluorescence live-cell imaging using EGFP-paxillinto assess FA dynamics. As seen in Figure 6B, the FAs in controlcells matured and dissolved over the period of observation,whereas the adhesions in GEF-H1–depleted cells did notchange their size over a long period (yellow arrows) (also seeSupplemental Movie S7). To quantify the effect on FA dynamics,we used the IMARIS-Autoquant software (Bitplane, St. Paul, MN)to measure the FA turnover. This software allows the detectionand tracking of FA in each frame of a time-lapse movie, as shownin Figure 6B, and can determine the period of time that eachdetected FA was visible in the movie. In the example shown inFigure 6C, small dots in gray represent the detected FA andthe colored lines display the path of the FA during the movie.This analysis revealed that in GEF-H1–depleted cells thenumber of "long-lived" FAs was significantly increased, indicativeof decreased turnover (Figure 6B, right).

As larger FAs were associated with the ends of acto-myosin–decoratedstress fibers, we measured FA "sliding" by using the Image-ProPlus software (MediaCybernetics, MediaCybernetics, Bethesda,MD). Using this analysis, we found that FAs in GEF-H1–depletedcells slide significantly slower throughout the duration ofthe experiment than in control cells, as reflected by the smallerslope of the colored lines (Figure 6D). This may mirror thereduced contractility of associated acto-myosin–basedstress fibers.

A GEF-H1/RhoA/mDia Pathway Is Involved in Focal Adhesion Turnover
FA turnover has been shown to be regulated by a variety of mechanisms(for review, see Bershadsky et al., 2003). Contact of MT plusends with peripheral FAs is one means of regulating their turnover(for review, see Small and Kaverina, 2003). However, we foundthat in GEF-H1–deficient cells there were greater numbersof MTs extending into the leading edge (Figure 5C), and we coulddetect no evident difference in their association with FA (datanot shown). Similarly, the activity of p21-activated kinases(PAKs) has been shown to regulate FA lifetime and turnover (Manseret al., 1997). We could detect no differences in the levelsof phosphorylated active PAK1/2 between control and GEF-H1–depletedcells (Supplemental Figure S10).

Tyrosine phosphorylation of FAK occurs during generation ofFAs (for review, see Schlaepfer et al., 1999). Phosphorylationof FAK Tyr397 is not only important for FA assembly but alsofor their turnover during cell migration (Webb et al., 2004;Hamadi et al., 2005). Western blot analysis of control and GEF-H1–depletedcells revealed that there was a substantial decrease in FAKTyr397 phosphorylation in cells lacking GEF-H1, concomitantwith the decreased turnover of FAs (Figure 7A).

View larger version (41K):
[in this window]
[in a new window]

Figure 7. Tyrosine phosphorylation of focal adhesion components is altered in cells lacking GEF-H1. (A) Tyrosine phosphorylation of focal adhesion kinase is decreased in cells lacking GEF-H1. Cell lysates of control and GEF-H1–depleted cells were collected and examined by immunoblot for pFAK(Y397) and total FAK. For quantification, phosphorylated FAK was normalized to the amount of total FAK from whole cell lysates. Results are from n = 3 independent experiments, means ± SD. (B) Depletion of mDia1 leads to decreased FAK tyrosine phosphorylation during in vitro wound healing. Cells were transfected with control, GEF-H1 or mDia1 siRNA. At 72 h post-siRNA transfection, multiple scratch wounds were generated (18/3.5-cm dish), and cells were allowed to migrate for 6 h. Protein samples were collected and subjected to immunoblotting for pFAK(Y397) and total FAK. Left, quantification of pFAK(Y397) normalized to total FAK protein. Results are from n = 2 independent experiments, means ± SD (C) Tyrosine phosphorylation of paxillin is decreased in GEF-H1–depleted cells. Cell lysates of control and GEF-H1–depleted cells were IPed by using anti-paxillin antibody. Immunoprecipitates and total cell lysates were separated by SDS-PAGE and subjected to immunoblotting with the anti-phospho-tyrosine antibody 4G10 (Tyr-P). The membrane was stripped and reprobed with anti-paxillin antibody. Left, relative quantification of phospho-tyrosine paxillin to total paxillin from two independent IP experiments (means ± SD).

The RhoA effector mDia is involved in the recruitment of Srckinase to focal adhesions and its activation by FAK (Yamanaet al., 2006

). We therefore tested whether this effector mightplay a role in cellular effects observed upon depletion of GEF-H1.Using siRNA technology, we depleted mDia1 protein in HeLa cellsand assessed phosphorylation of FAK Tyr397: Tyr397 phosphorylationwas comparably decreased in cells lacking mDia1, implicatinga possible involvement of this RhoA effector in the phenomenaobserved when GEF-H1 is lacking (Figure 7B).

The phosphorylation of FAK at the Tyr397 site is prerequisitefor tyrosine phosphorylation of the downstream FA adaptor proteinpaxillin (Schaller and Parsons, 1995). Immunoprecipitation ofpaxillin and subsequent Western blot analysis with a tyrosine-specificantibody showed that there was indeed a strong decrease of paxillintyrosine phosphorylation in cells lacking GEF-H1 (Figure 7C).Together, depletion of the Rho GEF, GEF-H1, strongly impairsthe turnover of focal adhesions by perturbing tyrosine phosphorylationof key FA proteins, possibly due to the lack of proper RhoAeffector signaling.

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

GEF-H1 Regulates RhoA Activity at the Leading Edge
During cell migration, RhoA GTPase activity regulates the actincytoskeleton to efficiently coordinate leading edge protrusivenessand contractility of the cell body. Recent studies have detecteda major region of RhoA activation at the front of migratingfibroblasts, reflecting such critical roles (Kurokawa and Matsuda,2005; Pertz et al., 2006). Indeed, RhoA activation in this regiontemporally correlates with edge advancement (Machacek et al.,2009). However, it is still unknown how such localized RhoAactivation is achieved by upstream mechanisms.

In the current study, visualization of RhoA activity with alive cell biosensor showed that GEF-H1 is a major regulatorof localized RhoA activation in the leading edge of migratingHeLa cells. In contrast to the effects on localized activity,the overall RhoA activation level in cells was not significantlyaltered, as measured either by glutathione transferase-Rhotekinaffinity-based assay (Chang et al., 2008) or by FRET (SupplementalFigure S3A). GEF-H1 thus controls the localized activation dynamicsof the RhoA pool at the front of the migrating cell, ratherthan bulk RhoA activity. In agreement with this finding, wehad recently shown that GEF-H1, acting in concert with Ect2,can regulate localized RhoA activation at the cleavage furrowduring cytokinesis (Birkenfeld et al., 2007).

The role of the RhoA activity zone in the leading edge is stillunder investigation, but regulatory functions during cell migrationare likely. Machacek et al. (2009) found a strict spatiotemporalcorrelation between RhoA, Rac1, and Cdc42 GTPases in the leadingedge of migrating mouse embryo fibroblasts. In their study,RhoA was consistently activated first with respect to expansionof the protrusion, before Rac1 and Cdc42, suggesting a potentiallydominant role for RhoA in initiating protrusion. In MTln3 cancercells, EGF-induced leading edge RhoA activity was also foundto function upstream of Rac1 and Cdc42 activation to regulatecell motility and actin dynamics in the leading edge (El-Sibaiet al., 2008). Here, RhoA activity critically modulated protrusionsize during MTln3 cell migration, with inhibition of RhoA causingan increase in basal cell area and formation of large, randomlyoriented protrusions. These findings also support a criticalrole for RhoA in the tight balance between extension and contractionin order to achieve efficient cell migration.

The present data suggest a key role of GEF-H1–regulatedRhoA activity in leading edge cytoskeletal regulation. Our time-lapseanalysis of single migrating cells revealed strongly perturbedleading edge dynamics upon depletion of GEF-H1. In control cellsGEF-H1 was found to accumulate in membrane ruffles within thisregion, consistent with a localized GEF-H1-RhoA signaling pathway(Figure 4C and Supplemental Figure S6).

GEF-H1 Regulates Cell Migration
As a consequence of unstable RhoA activity in the leading edge,the siRNA-mediated depletion of GEF-H1 led to a decrease inHeLa cell migration efficiency. Migration was inhibited to asimilar extent in both a two-dimensional wounding assay andin a three-dimensional (3D) filter assay, suggesting similarGEF-H1 function in both types of cell migration. As single cellswere used to study migration in 3D, aberrant regulation of cell–cellcontacts is unlikely to explain our findings. Indeed, we couldnot detect significant alterations of cell-cell contacts incells lacking GEF-H1 in in vitro scratch assays (SupplementalFigure S11). In contrast, our studies revealed multiple othermigration-related cellular perturbations upon GEF-H1 depletion.

The aberrant leading edge dynamics in cells lacking GEF-H1 stronglycorrelated with alterations in the organization of the actincytoskeleton at the cell edge. Both centripetal flow of leadingedge ruffles and the spatial alignment of stress fibers wereperturbed in the absence of GEF-H1. In control cells, we observeda distinct zone behind the leading edge in which curved actinbundles were aligned parallel to the cell boundary; such orderedactin structures were rarely detected in the absence of GEF-H1.In time-lapse studies with control cells, we were able to observeactin bundle generation associated with the rearward flow ofactin from the leading edge. Transverse actin bundles, alsotermed actin arcs, have been reported in multiple cell types(Heath, 1983; Schaefer et al., 2002; Hotulainen and Lappalainen,2006) and have been implicated in controlling dynamics and retrogradetransport of MTs (Schaefer et al., 2002). Similarly, in ourstudy only few MTs were found extending into the leading edgeof control cells, with most MTs localized just behind the regionwhere transverse actin bundles were located. In that area, manyMTs were bent and aligned parallel to the leading edge, suggestingthat actin bundles in HeLa cells might also guide MTs and confinetheir spatial organization. In agreement with this, the lackof transverse actin fibers in GEF-H1–depleted cells wasparalleled by a substantial increase in MTs extending outwardto the cell edge. Our measurements of MT tip movement suggestthat MT growth per se was not affected by depletion of GEF-H1.Rather, the orientation of MTs mostly perpendicular with respectto the cell edge support the hypothesis that GEF-H1 might facilitatethe controlled approach of MTs to the leading edge by modulatingthe dynamics of guiding actin fibers.

The observed accumulation of MTs in the leading edge could accountfor the uncontrolled protrusion observed upon RhoA inhibition.As reported previously, dynamic MTs promote protrusion via theactivation of Rac in the leading edge (Waterman-Storer et al.,1999; Wittmann et al., 2003, 2004), and the MT-mediated increaseof Rac1 activity in the leading edge might be the underlyingcause for enhanced protrusion. Our preliminary data indicatethat the overall cellular levels of Rac1, as measured by p21-bindingdomain pull-down experiments, are not significantly increasedafter depletion of GEF-H1 (data not shown). In support of this,the overall levels of PAK phosphorylation, a downstream effectorof Rac, are also unchanged (Supplemental Figure S10). Rather,inhibition of RhoA-dependent actin bundling might allow theenhanced localization of MTs in the leading edge, leading tolocalized increase of Rac activity. In future studies, it willbe interesting to use in vivo activity biosensors to examinelocalized Rac activity patterns at the leading edge in a GEF-H1–depletedbackground.

Focal Adhesion Turnover Is Decreased in the Absence of Active GEF-H1
FAs provide a crucial link between the actin cytoskeleton andthe substrate to enable efficient force generation and transmittanceduring cell migration (Hu et al., 2007). In turn, maturationof FAs has been shown to be altered by external mechanical force,indicative of mechanosensitive regulatory pathways (Rivelineet al., 2001). The perturbed contractility observed in GEF-H1–depletedcells was paralleled by alterations in FA behavior (Figures 6and 7). The overall numbers of focal adhesions did not seemto be decreased, suggesting that formation of FA per se wasunaffected. This is consistent with another study where inhibitionof GEF-H1 function (GEF-H1-DH mut) in mouse embryonic fibroblastsdid not interfere with the generation of focal adhesions (Limet al., 2008). Time-lapse movies in the present study showedthat FAs grew slower in cells depleted of GEF-H1, suggestingthat loss of RhoA-dependent contractility might perturb theFA maturation process. Consistent with this, there was a dramaticincrease in the average focal adhesion lifetime (Figure 6B,right). We also observed a decrease in FA "sliding" in GEF-H1–depletedcells during migration, indicating reduced stress fiber contractility.Taken together, dysfunctional GEF-H1-RhoA signaling impairsFA turnover in migrating cells.

Decreased PAK activity did not seem to play a significant rolein the observed aberrant FA turnover in cells depleted of GEF-H1(Supplemental Figure S10). Tyrosine phosphorylation of key FAproteins has been associated with focal adhesion disassemblyand efficient cell migration (Webb et al., 2004; Hamadi et al.,2005). In agreement, we observed significantly decreased tyrosinephosphorylation of FAK and paxillin in cells lacking GEF-H1(Figure 7). Integrin-triggered auto-phosphorylation of FAK onTyr397 is critical for FAK activation and leads to further maturationof FAs. In addition, Tyr397 of FAK is not only important forthe maturation of FAs but is also involved in the mDia-dependentrecruitment of active Src kinase to the adhesion complex site(Yamana et al., 2006). Src recruitment is inseparably linkedto FAK activity. We found that depletion of mDia1 induced asubstantial decrease in FAK Tyr397 phosphorylation, suggestingthat the RhoA effector mDia might be involved in focal adhesionregulation through a FAK–Src signaling axis.

Downstream of FAK-Src signaling, paxillin phosphorylation atTyr31 and Tyr118 is crucial for focal adhesion disassembly andefficient cell migration (Zaidel-Bar et al., 2007; for reviews,see Schoenwaelder and Burridge, 1999; Brown and Turner, 2004).We observed a significant decrease in the overall tyrosine phosphorylationof paxillin in cells lacking GEF-H1. Paxillin itself is implicatedin the localization of Tyr397-phosphorylated FAK into focaladhesions, indicating a possible positive feedback loop betweenFAK and paxillin tyrosine phosphorylation. The RhoA effectormDia might be involved in this scenario as an integrating factorto link FAK, Src and paxillin signaling and facilitate properfocal adhesion turnover in migrating cells. Gupton et al. (2007)reported highly disorganized leading edge dynamics and abnormalgeneration of protrusions when mDia function was inhibited.Interestingly, the protrusions described in this study weresimilar to the phenotype observed in our GEF-H1 depletion studies.Another study by Riveline et al. (2001) revealed that localapplication of external force enhanced directional FA growthin an mDia-mediated manner. These reports are consistent withour data, and strongly support the conclusion that the observedeffects of GEF-H1 depletion on FA dynamics and protrusion aredue to aberrant RhoA signaling.

The localization of RhoA/mDia signaling might be mediated bytargeted release of GEF-H1 protein from MTs at or in the closevicinity of FAs. Persistent targeting of FAs by MTs has beenreported to promote FA disassembly (Kaverina et al., 1998, 1999).It was suggested that MTs release relaxation factors that arecritical for the proper turn-over of FAs (Efimov et al., 2008).GEF-H1 has been shown to activate RhoA upon release from MTsand, together with data from our study, this suggests that GEF-H1might mediate such localized regulation of RhoA function. Forfuture studies it will be intriguing to visualize localizedRhoA activation together with FA dynamics to assess spatiotemporalcorrelation during cell migration.

In summary, we have established GEF-H1 as a major regulatorof localized leading edge RhoA signaling in migrating HeLa cells.Our data reveal a GEF-H1–dependent route for cytoskeletalreorganization and FA dynamics via leading edge RhoA activation.Future studies will establish the potential connection(s) betweenGEF-H1-RhoA signaling and the localized regulation of leadingedge Rac1 and Cdc42 activity.

ACKNOWLEDGMENTS

We thank Dr. Leif Dehmelt for helpful discussions throughoutthe study and critical reading of the manuscript. The technicalassistance of Bruce Fowler is appreciated. This work was supportedby National Institutes of Health grant GM-39434 (to G.M.B.).

Footnotes

This article was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E09-01-0041)on July 22, 2009.

Present address: DIREVO Biotech AG, 50829 Cologne, Germany.

Address correspondence to: Gary M. Bokoch (bokoch{at}scripps.edu) or Perihan Nalbant (perihan.nalbant{at}uni-due.de).

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Baudoin, J. P., Alvarez, C., Gaspar, P., and Métin, C. (2008). Nocodazole-induced changes in microtubule dynamics impair the morphology and directionality of migrating medial ganglionic eminence cells. Dev. Neurosci 30, 132–143.[CrossRef][Medline]

Benais-Pont, G., Punn, A., Flores-Maldonado, C., Eckert, J., Raposo, G., Fleming, T. P., Cereijido, M., Balda, M. S., and Matter, K. (2003). Identification of a tight junction-associated guanine nucleotide exchange factor that activates Rho and regulates paracellular permeability. J. Cell Biol 160, 729–740.[Abstract/Free Full Text]

Bershadsky, A. D., Balaban, N. Q., and Geiger, B. (2003). Adhesion-dependent cell mechanosensitivity. Annu. Rev. Cell Dev. Biol 19, 677–695.[CrossRef][Medline]

Birkenfeld, J., Nalbant, P., Bohl, B. P., Pertz, O., Hahn, K. M., and Bokoch, G. M. (2007). GEF-H1 modulates localized RhoA activation during cytokinesis under the control of mitotic kinases. Dev. Cell 12, 699–712.[CrossRef][Medline]

Brown, M. C., and Turner, C. E. (2004). Paxillin: adapting to change. Physiol. Rev 84, 1315–1339.[Abstract/Free Full Text]

Chang, Y. C., Nalbant, P., Birkenfeld, J., Chang, Z. F., and Bokoch, G. M. (2008). GEF-H1 couples nocodazole-induced microtubule disassembly to cell contractility via RhoA. Mol. Biol. Cell 19, 2147–2153.[Abstract/Free Full Text]

Danowski, B. A. (1989). Fibroblast contractility and actin organization are stimulated by microtubule inhibitors. J. Cell Sci 93, 255–266.[Abstract/Free Full Text]

Efimov, A., Schiefermeier, N., Grigoriev, I., Ohi, R., Brown, M. C., Turner, C. E., Small, J. V., and Kaverina, I. (2008). Paxillin-dependent stimulation of microtubule catastrophes at focal adhesion sites. J. Cell Sci 121, 196–204.[Abstract/Free Full Text]

El-Sibai, M., Pertz, O., Pang, H., Yip, S. C., Lorenz, M., Symons, M., Condeelis, J. S., Hahn, K. M., and Backer, J. M. (2008). RhoA/ROCK-mediated switching between Cdc42- and Rac1-dependent protrusion in MTLn3 carcinoma cells. Exp. Cell Res 314, 1540–1552.[CrossRef][Medline]

Enomoto, T. (1996). Microtubule disruption induces the formation of actin stress fibers and focal adhesions in cultured cells; possible involvement of the rho signal cascade. Cell Struct. Funct 21, 317–326.[Medline]

Etienne-Manneville, S., and Hall, A. (2001). Integrin-mediated Cdc42 activation controls cell polarity in migrating astrocytes through PKCzeta. Cell 106, 489–498.[CrossRef][Medline]

Etienne-Manneville, S., and Hall, A. (2002). Rho GTPases in cell biology. Nature 420, 629–635.[CrossRef][Medline]

Etienne-Manneville, S. (2004). Actin and microtubules in cell motility: which one is in control? Traffic 5, 470–477.[CrossRef][Medline]

Fukata, Y., Oshiro, N., Kinoshita, N., Kawano, Y., Matsuoka, Y., Bennett, V., Matsuura, Y., and Kaibuchi, K. (1999). Phosphorylation of adducin by Rho-kinase plays crucial role in cell motility. J. Cell Biol 145, 347–361.[Abstract/Free Full Text]

Gardiner, E. M., Pestonjamasp, K. N., Bohl, B. P., Chamberlain, C., Hahn, K. M., and Bokoch, G. M. (2002). Spatial and temporal analysis of Rac activation during live neutrophil chemotaxis. Curr. Biol 12, 2029–2034.[CrossRef][Medline]

Gupton, S. L., Salmon, W. C., and Waterman-Storer, C. M. (2002). Converging populations of f-actin promote breakage of associated microtubules to spatially regulate microtubule turnover in migrating cells. Curr. Biol 12, 1891–1899.[CrossRef][Medline]

Gupton, S. L., Eisenmann, K., Alberts, A. S., and Waterman-Storer, C. M. (2007). mDia2 regulates actin and focal adhesion dynamics and organization in the lamella for efficient epithelial cell migration. J. Cell Sci 120, 3475–3487.[Abstract/Free Full Text]

Hall, A. (1998). Rho GTPases and the actin cytoskeleton. Science 279, 509–514.[Abstract/Free Full Text]

Hamadi, A., Bouali, M., Dontenwill, M., Stoeckel, H., Takeda, K., and Philippe, R. (2005). Regulation of focal adhesion dynamics and disassembly by phosphorylation of FAK at tyrosine 397. J. Cell Sci 118, 4415–4425.[Abstract/Free Full Text]

Heath, J. P. (1983). Direct evidence for microfilament-mediated capping of surface receptors on crawling fibroblasts. Nature 302, 532–534.[CrossRef][Medline]

Hotulainen, P., and Lappalainen, P. (2006). Stress fibers are generated by two distinct actin assembly mechanisms in motile cells. J. Cell Biol 173, 383–394.[Abstract/Free Full Text]

Hu, K., Ji, L., Applegate, K. T., Danuser, G., and Waterman-Storer, C. M. (2007). Differential transmission of actin motion within focal adhesions. Science 315, 111–115.[Abstract/Free Full Text]

Kaverina, I., Rottner, K., and Small, J. V. (1998). Targeting, capture, and stabilization of microtubules at early focal adhesions. J. Cell Biol 142, 181–190.[Abstract/Free Full Text]

Kaverina, I., Krylyshkina, O., and Small, J. V. (1999). Microtubule targeting of substrate contacts promotes their relaxation and dissociation. J. Cell Biol 146, 1033–1043.[Abstract/Free Full Text]

Kaverina, I., Krylyshkina, O., and Small, J. V. (2002). Regulation of substrate adhesion dynamics during cell motility. Int. J. Biochem. Cell Biol 34, 746–761.[CrossRef][Medline]

Kraynov, V. S., Chamberlain, C., Bokoch, G. M., Schwartz, M. A., Slabaugh, S., and Hahn, K. M. (2000). Localized Rac activation dynamics visualized in living cells. Science 290, 333–337.[Abstract/Free Full Text]

Krendel, M., Zenke, F. T., and Bokoch, G. M. (2002). Nucleotide exchange factor GEF-H1 mediates cross-talk between microtubules and the actin cytoskeleton. Nat. Cell Biol 4, 294–301.[CrossRef][Medline]

Kurokawa, K., Itoh, R. E., Yoshizaki, H., Nakamura, Y. O., and Matsuda, M. (2004). Coactivation of Rac1 and Cdc42 at lamellipodia and membrane ruffles induced by epidermal growth factor. Mol. Biol. Cell 15, 1003–1010.[Abstract/Free Full Text]

Kurokawa, K., Nakamura, T., Aoki, K., and Matsuda, M. (2005). Mechanism and role of localized activation of Rho-family GTPases in growth factor-stimulated fibroblasts and neuronal cells. Biochem. Soc. Transact 33, 631–634.[CrossRef][Medline]

Kurokawa, K., and Matsuda, M. (2005). Localized RhoA activation as a requirement for the induction of membrane ruffling. Mol. Biol. Cell 16, 4294–4303.[Abstract/Free Full Text]

Lim, Y. et al. (2008). PyK2 and FAK connections to p190Rho guanine nucleotide exchange factor regulate RhoA activity, focal adhesion formation and cell motility. J. Cell Biol 180, 187, 203.

Machacek, M., Hodgson, L., Welch, C., Elliot, H., Pertz, O., Nalbant, P., Abell, A., Johnson, G. L., Hahn, K. M., and Danuser, G. (2009). Coordination of Rho GTPase activities during cell protrusion. Nature (in press).

Manser, E., Huang, H. Y., Loo, T.-H., Chen, X.-Q., Dong, J.-M., Leung, T., and Lim, L. (1997). Expression of constitutively active alpha-Pak reveals effects of the kinase on actin and focal complexes. Mol. Cell. Biol 17, 1129–1143.[Abstract/Free Full Text]

Matsumoto, Y., Tanaka, K., Harimaya, K., Nakatani, F., Matsuda, S., and Iwamoto, Y. (2001). Small GTP-binding protein, Rho, both increased and decreased cellular motility, activation of matrix metalloproteinase 2 and invasion of human osteosarcoma cells. Jpn. J. Cancer Res 92, 429–438.[CrossRef]

Mikhailov, A., and Gundersen, G. G. (1998). Relationship between microtubule dynamics and lamellipodium formation revealed by direct imaging of microtubules in cells treated with nocodazole or Taxol. Cell Motil. Cytoskeleton 41, 325–340.[CrossRef][Medline]

Morrison, E. E., Moncur, P. M., and Askham, J. M. (2002). EB1 identifies sites of microtubule polymerization during neurite development. Brain Res. Mol. Brain Res 98, 145–152.[Medline]

Nalbant, P., Hodgson, L., Kraynov, V., Toutchkine, A., and Hahn, K. M. (2004). Activation of endogenous Cdc42 visualized in living cells. Science 305, 1615–1619.[Abstract/Free Full Text]

Palazzo, A. F., Cook, T. A., Alberts, A. S., and Gundersen, G. G. (2001). mDia mediates Rho-regulated formation and orientation of stable microtubules. Nat. Cell Biol 3, 723–729.[CrossRef][Medline]

Pertz, O., Hodgson, L., Klemke, R. L., and Hahn, K. M. (2006). Spatiotemporal dynamics of RhoA activity in migrating cells. Nature 440, 1069–1072.[CrossRef][Medline]

Ren, Y., Li, R., Zheng, Y., and Busch, H. (1998). Cloning and characterization of GEF-H1, a microtubule-associated guanine nucleotide exchange factor for Rac and Rho GTPases. J. Biol. Chem 273, 34954–34960.[Abstract/Free Full Text]

Ridley, A. (2001). Rho GTPases and cell migration. J. Cell Sci 114, 2713–2722.[Abstract/Free Full Text]

Ridley, A. J., Schwartz, M. A., Burridge, K., Firtel, R. A., Ginsberg, M. H., Borisy, G., Parsons, J. T., and Horwitz, A. R. (2003). Cell migration: integrating signals from front to back. Science 302, 1704–1709.[Abstract/Free Full Text]

Riveline, D., Zamir, E., Balaban, N. Q., Schwarz, U. S., Ishizaki, T., Narumiya, S., Kam, Z., Geiger, B., and Bershadsky, A. D. (2001). Focal contacts as mechanosensors: externally applied local mechanical force induces growth of focal contacts by and mDia-1 dependent and ROCK-independent mechanism. J. Cell Biol 153, 1175–1186.[Abstract/Free Full Text]

Rossman, K. L., Der, C. L., and Sondek, J. (2005). GEF means go: turning on RHO GTPases with guanine nucleotide-exchange factors. Nat. Rev. Mol. Cell Biol 6, 167–180.[CrossRef][Medline]

Schaefer, A. W., Kabir, N., and Forscher, P. (2002). Filopodia and actin arcs guide the assembly and transport of two populations of microtubules with unique dynamic parameters in neuronal growth cones. J. Cell Biol 158, 139–152.[Abstract/Free Full Text]

Schaefer, A. W., Schoonderwoert, V. T., Ji, L., Mederios, N., Danuser, G., and Forscher, P. (2008). Coordination of actin filament and microtubule dynamics during neurite outgrowth. Dev. Cell 15, 146–162.[CrossRef][Medline]

Schaller, M. D., and Parsons, J. T. (1995). pp125FAK-dependent tyrosine phosphorylation of Paxillin creates a high-affinity binding site for Crk. Mol. Cell. Biol 15, 2635–2645.[Abstract/Free Full Text]

Schlaepfer, D. D., Hauck, C. R., and Sieg, D. J. (1999). Signaling through focal adhesion kinase. Prog. Biophys. Mol. Biol 71, 435–478.[CrossRef][Medline]

Schoenwaelder, S. M., and Burridge, K. (1999). Bidirectional signalling between the cytoskeleton and integrins. Curr. Opin. Cell Biol 11, 274–286.[CrossRef][Medline]

Small, J. V., and Kaverina, I. (2003). Microtubules meet substrate adhesions to arrange cell polarity. Curr. Opin. Cell Biol 15, 40–47.[CrossRef][Medline]

Waterman-Storer, C. M., Worthylake, R. A., Liu, B. P., Burridge, K., and Salmon, E. D. (1999). Microtubule growth activated Rac1 to promote lamellipodial protrusion in fibroblasts. Nat. Cell Biol 1, 45–50.[CrossRef][Medline]

Webb, D. J., Donais, K., Leanne, A. W., Thomas, S. M., and Turner, C. E. (2004). FAK-Src signalling through Paxillin, ERK and MLCK regulates adhesion disassembly. Nat. Cell Biol 6, 154–161.[CrossRef][Medline]

Wittmann, T., Bokoch, G. M., and Waterman-Storer, C. M. (2003). Regulation of leading edge microtubule and actin dynamics downstream of Rac1. J. Cell Biol 161, 845–851.[Abstract/Free Full Text]

Wittmann, T., Bokoch, G. M., and Waterman-Storer, C. M. (2004). Regulation of microtubule destabilizing activity of Op18/stathmin downstream of Rac1. J. Biol. Chem 279, 6196–6203.[Abstract/Free Full Text]

Wittmann, T., and Waterman-Storer, C. M. (2001). Cell motility: can Rho GTPases and microtubules point the way? J. Cell Sci 114, 3795–3803.[Abstract/Free Full Text]

Worthylake, R. A., and Burridge, K. (2001). Leukocyte transendothelial migration: orchestrating the underlying molecular machinery. Curr. Opin. Cell Biol 13, 569–577.[CrossRef][Medline]

Yamana, N. et al. (2006). The Rho-mDia pathway regulates cell polarity and focal adhesion turnover in migrating cells through mobilizing Apc and c-Src. Mol. Cell. Biol 26, 6844–6858.[Abstract/Free Full Text]

Zaidel-Bar, R., Milo, R., Kam, Z., and Geiger, B. (2007). A paxillin tyrosine phosphorylation switch regulates the assembly and form of cell-matrix adhesions. J. Cell Sci 120, 137–148.[Abstract/Free Full Text]

Zenke, F. T., Krendel, M., DerMardirossian, C., King, C. C., Bohl, B. P., and Bokoch, G. M. (2004). p21-activated kinase 1 phosphorylates and regulates 14–3-3 binding to GEF-H1, a microtubule-localized Rho exchange factor. J. Biol. Chem 279, 18392–18400.[Abstract/Free Full Text]