The Borgs, a New Family of Cdc42 and TC10 GTPase-Interacting Proteins

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Molecular and Cellular Biology, October 1999, p. 6585-6597, Vol. 19, No. 10
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

The Borgs, a New Family of Cdc42 and TC10 GTPase-Interacting Proteins

Gérard Joberty,^* Richard R. Perlungher, and Ian G. Macara

Markey Center for Cell Signaling and Department of Pharmacology, University of Virginia, Charlottesville, Virginia 22908

Received 21 April 1999/Returned for modification 9 June 1999/Accepted 30 June 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The Rho family of GTPases plays key roles in the regulation of cell motility and morphogenesis. They also regulate proteinkinase cascades, gene expression, and cell cycle progression.This multiplicity of roles requires that the Rho GTPases interactwith a wide variety of downstream effector proteins. An understandingof their functions at a molecular level therefore requires theidentification of the entire set of such effectors. Towards thisend, we performed a two-hybrid screen using the TC10 GTPase asbait and identified a family of putative effector proteins relatedto MSE55, a murine stromal and epithelial cell protein of 55 kDa.We have named this family the Borg (binder of Rho GTPases) proteins.Complete open reading frames have been obtained for Borg1 throughBorg3. We renamed MSE55 as Borg5. Borg1, Borg2, Borg4, and Borg5bind both TC10 and Cdc42 in a GTP-dependent manner. Surprisingly,Borg3 bound only to Cdc42. An intact CRIB (Cdc42, Rac interactivebinding) domain was required for binding. No interaction of theBorgs with Rac1 or RhoA was detectable. Three-hemagglutinin epitope(HA₃)-tagged Borg3 protein was mostly cytosolic when expressedectopically in NIH 3T3 cells, with some accumulation in membraneruffles. The phenotype induced by Borg3 was reminiscent of thatcaused by an inhibition of Rho function and was reversed by overexpressionof Rho. Surprisingly, it was independent of the ability to bindCdc42. Borg3 also inhibited Jun kinase activity by a mechanismthat was independent of Cdc42 binding. HA₃-Borg3 expression causedsubstantial delays in the spreading of cells on fibronectin surfacesafter replating, and the spread cells lacked stress fibers. Wepropose that the Borg proteins function as negative regulatorsof Rho GTPasesignaling.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Motility and morphogenesis are probably among the most complicated processes that a cell performs. The proteins and molecularmechanisms that regulate these processes are only now beginningto be elucidated. Adherent cells elaborate an extracellular matrixof proteins to which they bind through receptors called integrins(8). The integrins cluster at focal adhesion complexes andtransmit signals through these complexes to the actin-myosin cytoskeleton(11; for reviews, see references 10 and 46). Signaling throughother types of receptor, such as those that bind growth factors,can be modulated by engagement of integrins with the extracellularmatrix (39). A key role in controlling focal adhesions and theactin cytoskeleton is played by the small, Rho-like GTPases (9,19, 28, 29), of which there are at least 13 types in mammaliancells (15, 36, 54). The most intensively studied membersof this family of GTPases are RhoA, Rac1A, and Cdc42. Many ofthese proteins induce dramatic changes in the actin cytoskeletonwhen expressed ectopically as gain-of-function mutants (23,35, 40, 41; reviewed in reference 16) and can perturbcell adhesion, cell spreading, motility, and cytokinesis (11,20, 44, 50; reviewed in reference 26 and 55). The replatingof fibroblasts from suspension culture onto a fibronectin-coatedsurface causes dramatic membrane ruffling and the rapid productionof lamellipodia and microspikes around the edges of the spreadingcells. These changes are mediated by the activation of the Racand Cdc42 GTPases (5). The RhoA GTPase is transiently inhibitedafter replating and then activated at a later stage of spreading,at which time actin stress fibers appear within the cytosol (11).Similar changes in the activities of these proteins may occurat the leading edge of motile cells. Additionally, the Rho GTPasescan activate protein kinases cascades and transcription factorsand can regulate entry into the cell cycle (2, 12, 24,37, 55).

Given this wealth of responses, it is not surprising that each of the Rho family GTPases has been found to interact with aplethora of target proteins that likely act as downstream effectors.These proteins include a variety of types of kinase and of adapters,plus other proteins of unknown function (for reviews, see reference51 and 55). Several of the adapter proteins interact withknown components of the actin cytoskeleton such as profilin, buttheir roles remain unclear (49, 56).

Because the Rho family GTPases mediates changes in gene expression and cell division that are independent of the actin cytoskeleton,different subsets of effectors likely participate in distinctsignal transduction pathways downstream of the GTPases (24,52). It is only through the identification and detailed analysisof the complete set of Rho family GTPases and of their effectorproteins, therefore, that we will achieve satisfactory understandingof the molecular basis for those aspects of motility and morphogenesisthat are influenced by theseGTPases.

Toward this end, we performed a large two-hybrid screen of a whole mouse embryo library, using the TC10 GTPase as bait. Althoughits cDNA was cloned almost a decade ago (14), TC10 has beencharacterized only recently (14, 33). Of the >250 positivesclones that we isolated in the screen, many contained open readingframe fragments of previously described proteins that interactwith Cdc42 (33). These proteins include the protein kinases $alpha$ -PAK, $beta$ -PAK, $gamma$ -PAK, PAK4, myotonic dystrophy kinase-related Cdc42-bindingkinase (MRCK)- $alpha$ and - $beta$ , and mixed-lineage kinase 2 (MLK2) (1,25, 48, 51). We also isolated a partial cDNA for a putativenew MRCK protein that we called MRCK- $gamma$ . In addition, the screenidentified N-WASP (30) and an uncharacterized protein calledMSE55 (marrow stromal/endothelial cell protein with a molecularmass of 55,000 Da) (3). All of these clones contained a CRIB(Cdc42, Rac interactive binding) domain, which has been shownto be necessary and sufficient to permit association with theCdc42 and/or Rac proteins when in the GTP-bound state (7).Three other downstream effectors of Cdc42 that also contain CRIBdomains, namely, WASP, p120ACK, and MLK3 (51), were not identifiedin the two-hybrid screen. These proteins do not bind TC10 (33).

We now describe a new family of five related TC10 and Cdc42 binding proteins, which we have called Borgs (binders of Rho GTPases).Three of the cDNAs for these proteins were identified in the two-hybridscreen, and two more were uncovered by database searches. Oneprotein of this family (Borg5) is identical to the previouslyreported protein MSE55 (3), which was discovered serendipitouslyas a protein cross-reacting with an anti-hemonectin antibody.A Northern blot detected MSE55 mRNA only in endothelial and bonemarrow stromal cells (3). The cDNA encodes a protein of 391amino acid residues with two regions of weak similarity to somecalcium binding domains. More recently, a database search revealedthat the protein contains a CRIB domain, and purified glutathioneS-transferase (GST)-MSE55 protein was shown to bind efficientlyto [ $gamma$ -³²P]GTP-Cdc42 and more weakly to [ $gamma$ -³²P]GTP-Rac (7). We demonstrate that the other Borg family membersare more widely expressed, that bind TC10 and/or Cdc42, and caninhibit the Cdc42-mediated activation of the c-Jun N-terminalkinase (JNK). Ectopic expression of Borg1 or Borg3 induces distinctivechanges in cell morphology and significantly delays cell spreadingon fibronectin as well as cell motility in a woundtest.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cloning of Borg cDNAs. The two-hybrid screen has been described previously (33). The bait was TC10(Q75L) $Delta$ C, a gain-of-function mutant of TC10 lackingthe C-terminal isoprenylation signal and fused to the DNA bindingdomain of the yeast GAL4 protein. The library was from a mouseembryo (day 9) fused to the activating domain of VP16 and waskindly provided by Stan Hollenberg (Seattle, Wash.). Four positiveclones encoded a protein sequence highly similar to that of thehuman protein MSE55 (amino acid residues 1 to 110) (3). Differencesin 11 amino acids residues between the clones and MSE55 most likelyrepresent interspeciesdifferences.

A set of two identical clones and another of five clones each encoded new CRIB domains which showed closer similarity to thatof MSE55 than to CRIB domains of other known Rho family GTPasebinding proteins. The complete human cDNA of the first gene wasobtained from expressed sequence tag (EST) plasmid R13749/26651and was named Borg1. Both fragments found in the screen correspondto amino acids 1 to 181 of the human open reading frame of Borg1and encompassed a complete CRIB domain. Alignments of sequenceswere by made using the clustal algorithm in the Megalign programfrom the DNAStar software package. The mouse sequence from thescreen possesses four additional amino acid residues (PSPQ) betweenpositions 143 and 144. Overall, the mouse and human sequencesare 81% identical. The set of five clones encode a reading frame,which we have termed Borg4, for which no full-length ESTs werepresent in the database. A partial human sequence of Borg4 wasobtained from EST AA013011/360199. The sequence encodes twoadditional amino acid residues (SS) located between positions68 and 69 of the mousesequence.

When the databases were searched by BLAST, using a region of the CRIB domains of Borg1 and MSE55/Borg5 as the query, we identifiedtwo new open reading frames for closely related proteins, whichwe named Borg2 and Borg3. EST AA046144/376758 encoded the completehuman Borg2 protein, and EST W85265/408069 encoded the completemouse Borg3 protein. In all cases, we have defined "complete"as meaning that the open reading frames begin with an initiationcodon downstream of a Kozak consensus sequence (22) and thatin-frame stop codons are found upstream of this sequence. Full-lengthBorg1, Borg2, and Borg3 cDNAs were mutagenized by PCR so as tocreate a BamHI (or, for Borg2, a BglII) site at the 5' end andan EcoRI site at the 3' end of the open reading frames. TheseDNA fragments were then cloned in frame into the pKH₃ (6),pGEX2T, and VP16 vectors that had been cut with BamHI and EcoRI.The vectors produce fusion proteins with an N-terminal triple-HA1(hemagglutinin epitope) tag, GST, or VP16 activation domain,respectively.

Two conserved residues within the CRIB domain of Borg3 (Ile²³ and Ser²⁴) were mutated to Ala residues by megaprimer PCR mutagenesis (4),to produce CRIB (I₂₃A,S₂₄A). A truncation mutant in which theC-terminal 67 amino acid residues of Borg3 were deleted was producedby PCR. Recombinant proteins were expressed and purified fromEscherichia coli as previously described (6).

Yeast conjugation assay. Conjugation assays were performed as previously described (33). Briefly, Saccharomyces cerevisiae HF7c (MATa) wastransformed with VP16 vectors that express fragments or full-lengthsequences of Borg proteins fused to the VP16 activation domain.Strain W303 (MAT $alpha$ ) was transformed with modified pGBT9 vectorsexpressing GAL4 DNA binding domain fusions with different activatedmutants of Rho family GTPases lacking the C-terminal isoprenylationsignal. The two mating types were mixed and incubated overnighton YPD plates to permit mating. The following day, the spots werereplica plated onto selective medium (L/W/H plus 10 mM 3 aminotriazole) and incubated at 30°C to permit growthof diploids containing interacting proteins. Other known targetproteins that interact with Rac(G12V) $Delta$ C and Rho(G14V) $Delta$ C were testedin the same assay as positive controls for expression of theseGTPases.

In vitro binding assays. Recombinant GST-Borg proteins were purified, and 2 µg of each, or of GST alone, was spotted onto nitrocellulose and allowedto dry for 1 h at room temperature. The nitrocellulose was blockedin binding buffer (50 mM Tris-HCl [pH 7.5], 100 mM NaCl, 5 mMMgCl₂, 0.1 mM dithiothreitol) plus 5% dried milk for 1 h at 4°C.TC10 and Cdc42 proteins (3 µg) were loaded with [ $alpha$ -³²P]GTP or [ $alpha$ -³²P]GDP (3,000 Ci/mmol) as described previously (33) and separatedfrom unincorporated nucleotide by passage over a Pharmacia PD10size exclusion column equilibrated in binding buffer. Equal amountsof radiolabeled proteins (ca. 0.5 µCi of each) were incubatedwith the nitrocellulose in 10 ml of binding buffer for 1 h at4°C. The blots were subsequently washed three times with 50 mlof binding buffer, and associated proteins were detected byfluorography.

Immunodetection, immunofluorescence, and imaging. NIH 3T3 fibroblasts were cultured on 10-cm-diameter plates or on two-well LabTek chamber slides (Nunc) in Dulbecco modifiedEagle medium (DMEM) supplemented with 5% fetal calf serum, 5%calf serum, penicillin, and streptomycin. The cells were transfectedby the calcium phosphate precipitation technique as previouslydescribed (43). For each transfection experiment, 12 µg of DNAwas mixed with the calcium phosphate reagents in a final volumeof 1.2 ml. One-sixth of the mix was added per LabTek chamber (forimmunofluorescence studies), and the remainder was added per 10-cm-diameterplate of cells (for immunoblotting). When two plasmids (12 µgof each) are mixed and cotransfected, we find that under theseconditions about 90% of the transfected cells express bothproteins.

Cell protein extracts were prepared from the plates 48 h posttransfection, submitted to sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) and transferred to nitrocellulosemembranes as described previously. Proteins were detected withmonoclonal antibody 12CA5 (anti-HA; 1/5,000) or 9E10 (anti-Myc;1/20,000) and revealed with a horseradish peroxidase-conjugatedanti-mouse secondary antibody by using chemiluminescence (Kirkegaard& Perry Laboratories, Gaithersburg, Md.). For immunofluorescence,cells were washed in phosphate-buffered saline (PBS) 40 h posttransfectionand then fixed in paraformaldehyde (4% [wt/vol] in PBS) for 15min at room temperature. Cells were washed in PBS, and residualformaldehyde was quenched with 50 mM ammonium chloride for 15min. Cells were permeabilized with Triton X-100 (0.2% [vol/vol]in PBS) for 3 min and blocked in PBS plus 3% (wt/vol) bovine serumalbumin for at least 20 min. Cells were then incubated with mousemonoclonal anti-HA antibody 12CA5 (1/500) in PBS plus 0.3% bovineserum albumin for 1 h. After being washed in the same buffer,cells were incubated for 45 min with the secondary, Texas red-coupledantibody (1/1,200) and fluorescein isothiocyanate (FITC)-phalloidin(1/1,000; Sigma). Slides were mounted in Citifluor (Ted Pella,Redding, Calif.) and imaged by using a 60× water immersion objectivelens on a Nikon inverted microscope equipped with a Hamamatsucharge-coupled device camera. Data were captured and processedby using Openlab 2.0 (Improvision) and Adobe Photoshop 5.0software.

JNK assay. Cos or NIH 3T3 cells, grown in DMEM supplemented with 5% fetal calf serum, 5% calf serum, penicillin, and streptomycin, werecotransfected with plasmids as described above. Control vectorspKH₃ and pRK7 were used as necessary to normalize the amount ofDNA transfected to 9 µg per 100-mm-diameter plate. Cells wereincubated overnight in serum-free DMEM 24 h posttransfection;then 100 µg of anisomycin was added (control), and cells wereincubated for 20 min at 37°C. Cells were washed twice with 10ml of ice-cold PBS and lysed in 400 µl of lysis buffer (25 mMHEPES [pH 7.4], 300 mM NaCl, 1.5 mM MgCl₂, 0.5 mM dithiothreitol,20 mM $beta$ -glycerophosphate, 1 mM Na₃VO₄, 0.1% Triton X-100, 20 µgof aprotinin/ml, 10 µg of leupeptin/ml, 1 mM phenylmethylsulfonylfluoride, 1 µM okadaic acid). Lysed cells were scraped off theplates, and the supernatant was cleared by centrifugation (5 minat 14,000 × g, 4°C). Equal volumes (100 µl) of the supernatantwere removed for immunoblot analysis and separated on 12% polyacrylamidegels by SDS-PAGE. The proteins were transferred to a nitrocellulosemembrane and immunoblotted. HA₃-tagged proteins were immunoprecipitatedfrom the remaining supernatant and washed three times in bufferA (2 mM Na₃VO₄ and 1% NP-40 in PBS), once in buffer B (100 mMmorpholinepropanesulfonic acid [MOPS; pH 7.5], 0.5 M LiCl), andonce in kinase buffer (12.5 mM MOPS [pH 7.5], 12.5 mM $beta$ -glycerophosphate,7.5 mM MgCl₂, 0.5 mM EGTA, 0.5 mM NaF, 0.5 mM Na₃VO₄). Immunoprecipitatedproteins were resuspended in 30 µl of kinase buffer, and 2 µgof purified GST $---$ c-Jun(1-79) plus 2 µCi of [ $gamma$ -³²P]ATP were added to each reaction tube. The reactions proceededat 30°C for 20 min and were stopped by the addition of 10 µl of4× Laemmli sample buffer. Kinase reaction complexes were separatedon 12% polyacrylamide gels by SDS-PAGE and analyzed byfluorography.

Cell spreading and motility assays. NIH 3T3 cells in 10-cm-diameter plates were transfected with 10 µg of DNA. Forty hours after transfection, cells were trypsinized,maintained in suspension for 15 to 20 min, and then replated onLabTek chambers that had been coated with fibronectin (0.5 mlof a 50-µg/ml solution). At different times (18, 45, or 180 min)after replating, cells were fixed with paraformaldehyde and processedfor immunofluorescence as described above. Transfected cells wereanalyzed by using Openlab 2.0 software to measure cell surfaceareas in contact with the fibronectin surface. For each time point,the areas of 100 cells were counted. To compare expression levelsof the Borg proteins within the transfected cells, images werecaptured under conditions such that no camera pixels were saturated,and the mean fluorescence of the counted cells was determinedfor each experiment. Differences in mean cell area at 18 min postplatingwere analyzed by an unpaired t test assuming equal variances (varianceswere calculated for each data set and found to be approximatelyequal). Probabilities (P values) were also calculated for thet-test values and degrees of freedom (i.e.,198).

To quantitate cell mobility, a wounding assay was used. Cells were cotransfected with the plasmid of choice plus pK7-GFP,which expresses a bright mutant of green fluorescent protein (GFP).Cells were split and replated at high density and low densityonto two 35-mm-diameter plates. After 3 days, when the cells wereconfluent, an aspirator was drawn across the center of the high-densityculture, to produce a clean 1-mm-wide wound area free of celldebris. After a further 24 h of incubation to permit migrationof cells into the empty area of the plate, the numbers of greenand nonfluorescent cells in the cleared area were counted andcompared to the ratio of green to nonfluorescent cells in thelow-density, unwounded culture. Cells cotransfected with pK7-GFPand the pRK7 empty plasmid gave a ratio close to 1.0, a valueexpected if the GFP itself has no effect on motility. Statisticalsignificance of the data was assessed by a two-sample ttest.

Nucleotide sequence accession numbers. Accession numbers for the Borg open reading frame sequences are AF163840 (Borg1), AF164118 (Borg2), AF164119 (Borg3),and AF165114(Borg4).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Cloning of Borg family cDNAs. A two-hybrid screen of a 9-day mouse embryo library using an activated TC10 GTPase as bait identified numerous clones thatencoded protein fragments incorporating a CRIB domain. Three groupsof clones had almost identical CRIB domains and similar flankingsequences, suggesting that they belonged to a family of relatedproteins that interact with Rho family GTPases (Fig. 1). Databasesearches using the protein sequence of each group uncovered fivesets of human ESTs encoding proteins with a high degree of similarityto the two hybrid clones. One of these clones was almost identicalto the previously reported human MSE55 protein (3) and is mostlikely the mouse counterpart of MSE55. We obtained from differentESTs the complete open reading frames for three proteins of thisnew family but found no ESTs encompassing the 3' end of one cDNAfound in the screen.

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FIG. 1. (A) Schematic of Borg protein domain structures. Bars showing the regions of similarity within the primary sequences of the Borg proteins are aligned according to the CRIB domains. The C-terminal sequence of Borg4 is not known. Borg5 is the putative mouse homolog of human protein MSE55. (B) Alignment of BH1, BH2, and BH3 domains. The N-terminal region comprises the CRIB domain and the BH1 domain.

Because the predicted sizes of the members of this family are all lower than 55 kDa, because the tissue expression of thecorresponding mRNAs is not restricted to endothelial and stromalcells (see below), and because the name MSE55 does not indicatefunction, we decided to rename the whole family Borg proteins.Borg1 is the complete new protein of which a part was revealedin the two-hybrid screen, Borg2 and Borg3 are the two proteinsfor which DNA sequences were found in the EST database, Borg4corresponds to the incomplete cDNA identified in the screen, andBorg5 is MSE55. Two uncharacterized sequences which correspondto Borg1 have been deposited by others in the GenBank database(accession no. AF001436 and AF094521).

Surprisingly, the mouse sequence of Borg1 contains four additional amino acids after position 143 that are a repeat of thefour previous amino acids (PSPQ). This discrepancy is confirmedin two other independent mouse EST clones. Additionally, the humansequence of Borg4 contains an insertion of two amino acids betweenpositions 68 and 69 of the mouse sequence (SSSK versus SK). Thesedifferences in otherwise well-conserved sequences might reflectthe presence of different splice variants of the sameproteins.

The domain structures of the Borg proteins are diagrammed in Fig. 1A. Borg1, Borg2, and especially Borg3 (210 [22.5 kDa],254 [27.5 kDa], and 150 [15.5 kDa] amino acid residues, respectively)are smaller than Borg5/MSE55 (which consists of 379 amino acidresidues, for a predicted molecular mass of 39 kDa). Bahou etal. (3) described MSE55 as a 391-amino-acid protein, but theinitiation codon that they indicated corresponds, at the mRNAlevel, to a very unlikely translation start. The Kozak context(22) for translation is unfavorable: CUGAUGC versus the bestconsensus described, ACCAUGG (the first adenine being presentin 90% of cases) (initiation codon indicated by underlining).The context of the second in-frame Met codon (ACCAUGA) is closerto the Kozak consensus motif and aligns naturally with the initiationcodon of the other Borg proteins (Fig. 1B). We suggest, therefore,that it most probably represents the true start site for translationof Borg5 and have numbered residues in Fig. 1 accordingly. TheN-terminal regions of all five Borg proteins are highly similar,comprising a short basic region (from 13 amino acids for Borg1to as short as 3 amino acids for Borg5) followed by a CRIB domainsequence, ISXPLGDFRHTXH(I/V)G. This sequence matches the consensusmotif, I(S/G)XPXXFXHXXHVG (7), with an additional residue inthe Borg CRIB domains between the P and Fresidues.

A well-conserved, short domain of about 12 amino acids that is not found in any other known protein follows the CRIB domain.We therefore call it Borg homology 1 (BH1) domain. The centraland C-terminal parts of the proteins are more divergent. Two otherwell-conserved motifs that we call the BH2 and BH3 domains canbe defined (Fig. 1). The BH2 domain is not present in Borg3; theBH3 domain has a central location in Borg5, whereas it is localizedat the C-terminal parts of Borg1, Borg2, and Borg3. Neither domainis present within the N-terminal fragment of Borg4 for which wehave sequence information. A proline-rich domain (about 40% ofPro in each case) can be observed in the central regions of Borg1,Borg3, and Borg5. The four amino acid residues insertion of themouse Borg1 sequence is located within this region. Borg5 alsocontain eight in-tandem heptad repeats (consensus PAANPPA) locatedat the C-terminal side of the BH3domain.

Borg mRNAs show distinct expression patterns. The MSE55 gene is expressed in endothelial and bone marrow stromal cells but not in monkey liver, spleen, brain, lung, andkidney (3). To determine the tissue expression patterns ofother members of the family, fragments of cDNA encoding humanBorg1, Borg2, or Borg4 or mouse Borg3 were used to probe a humantissue poly(A)⁺ mRNA blot (Fig. 2). Borg1, Borg2, and Borg3 mRNAs were detectedin all eight tissues studied, though at very different levels.For all three genes, multiple transcripts were observed. Borg1is expressed as two transcripts of about 1.8 and 2 kb and at highlevels in heart. Borg1 mRNA is less abundant in pancreas and especiallyliver. The Borg2 probe revealed four different transcripts ofvarious sizes (from 2 to 5.5 kb). Borg2 is also expressed at highlevels in heart but at low levels in brain, and the largest transcriptwas not detected in liver. The Borg3 probe was not of human originand gave a weaker signal. However, transcripts of about 1 and2 kb are visible (Fig. 2) and were more clearly seen in a ratcardiomyocyte mRNA extract (data not shown). In addition to thesetwo messengers, present in all examined tissues, a more abundanttranscript of about 3.5 kb is detectable specifically in skeletalmuscle. The presence of multiple transcripts suggests the possibleexistence of differentially spliced mRNAs and of Borg proteinvariants. Indeed, two slightly different mRNAs of MSE55 have beendescribed (3). No transcripts were found in any tissues probedwith the Borg4 probe. The Borg4 gene might, like Borg5, be expressedin only a few, specific tissues or cell types. However, it isstriking that all available ESTs are of embryonic or fetal origin.Therefore, Borg4 may not be expressed in adult tissues.

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FIG. 2. Tissue-specific expression of Borg genes. A nylon membrane containing human poly(A)⁺ mRNAs from different tissues (Clontech) was hybridized with $alpha$ -³²P-labeled human (mouse for Borg3) cDNA probes encoding the Borg proteins. Ran GTPase cDNA was used as a loading control. The same membrane was used in all four Northern blots. Molecular sizes of RNA standards are indicated (in kilobases) on the left. Arrows indicate the multiple transcripts that hybridized with each probe.

Borg3 interacts specifically with Cdc42. Partial cDNAs for Borg1, Borg4, and Borg5 were found in the two-hybrid screen. All clones of these cDNAs contained the 5'coding region including the region corresponding to the CRIB andBH1 domains of the proteins. In a yeast two-hybrid conjugationassay, the expressed protein fragments of Borg1, Borg4, and Borg5interacted specifically with the activated TC10 GTPase deletedof its isoprenylation signal [TC10(Q75L) $Delta$ C] and not with the GDP-boundTC10 mutant [TC10(T31N) $Delta$ C] (Fig. 3A shows data for Borg4 and Borg5).They also bound to an activated mutant of Cdc42 [Cdc42(Q61L) $Delta$ C].To check that the interaction was not an artifact of the use offragments rather than full-length proteins, we repeated the conjugationassay using the complete open reading frames of Borg1 to Borg3.Surprisingly, although the Borg1 and Borg2 interacted specificallywith TC10, Borg3 did not (Fig. 3A). Borg3 did, however, interactstrongly with Cdc42. Burbelo et al. reported a weak binding ofMSE55/Borg5 to GTP-loaded Rac1 in a dot blot assay (7), butin our hands, no member of the Borg family gave a positive responsein the two-hybrid assay with activated mutants of either Rac1or RhoA (Fig. 3A).

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FIG. 3. Binding of Borg proteins to different Rho-like GTPases. (A) Yeast two-hybrid conjugation assays. S. cerevisiae HF7c (MATa) was transformed with VP16 empty vector or with VP16 containing Borg cDNAs (the complete open reading frame of Borg1, Borg2, or Borg3 or a fragment obtained from the two-hybrid screen for Borg4 and Borg5). The transformants were then conjugated to S. cerevisiae W303 (MAT $alpha$ ) which had been transformed with pGBT9 plasmids containing cDNA encoding different Rho-like GTPases. Each GTPase open reading frame had been truncated to remove the C-terminal isoprenylation signal. Results show the growth of diploids after replica plating onto selective medium (L/W/H plus 10 mM 3-aminotriazole). For the three Borg cDNAs identified in the screen, the number of independent clones identified is noted. (B and C) Binding of GST-Borg proteins to TC10-GTP, Cdc42-GTP, or Cdc42-GDP. Purified recombinant GST or GST-Borg1, GST-Borg2, GST-Borg3, GST-Borg3(I₂₃A,S₂₄A), and GST-Borg3(1-83) (2 µg of each) were spotted onto a nitrocellulose membrane, which was then incubated with TC10-[ $alpha$ -³²P]GTP, Cdc42-[ $alpha$ -³²P]GTP, or Cdc42-[ $alpha$ -³²P]GDP (0.5 µCi; 3,000 Ci/mmol). Interactions were revealed by fluorography after the membranes were washed in binding buffer as described in Materials and Methods.

To determine whether the observed interactions between the small GTPases and the Borgs is direct, we spotted equal amountsof recombinant GST-Borg1, GST-Borg2, and GST-Borg3 fusion proteinsonto nitrocellulose and incubated them with recombinant TC10 orCdc42 that had been loaded with [ $alpha$ -³²P]GTP. After washing, the GST-Borg1 and GST-Borg2 proteins showedstrong binding to both Cdc42 and TC10. Binding of GST-Borg3 toTC10 was undetectable, although it bound the GTP-loaded Cdc42with high affinity (Fig. 3B). [ $alpha$ -³²P]GDP-Cdc42 did not bind to GST-Borg3, demonstrating that, asexpected, the binding of Cdc42 to Borg3 is nucleotide dependent(Fig. 3C). These results confirm the validity of the yeast two-hybridconjugation assay and demonstrate that the original two-hybridscreen was unable to identify Borg3 not because it was absentfrom the library but because it does not recognize TC10. It isinteresting that the Borg3 CRIB domain, though closely relatedto the CRIB domains of the other Borg family members, nonethelesscontains determinants that can differentiate TC10 from Cdc42,despite the fact that these GTPase effector domain sequences arealmost identical. Similarly, we have found that while MLK2 andN-WASP interact with TC10, MLK3 and WASP do not, though all seemto bind with similar affinity to Cdc42 (33).

To confirm that the CRIB domain constitutes the only binding site on Borg proteins for Cdc42, we created a GST-Borg3 mutantin which the two first, highly conserved amino acid residues (Ileand Ser) of the CRIB motif were converted to Ala residues [Borg3(I₂₃A,S₂₄A)].This fusion protein did not detectably bind [ $alpha$ -³²P]GTP-loaded Cdc42 (Fig. 3B). We also created a C-terminal truncationmutant of Borg3, GST-Borg3(1-83), which lacks BH3 and part ofthe Pro-rich domain. This mutant bound Cdc42 as well as did thewild-type protein. These results argue that the CRIB domain regionof Borg3 is necessary and sufficient for interaction with theCdc42GTPase.

Borg3 inhibits JNK independently of Cdc42 binding. JNK is the terminal protein kinase of a cascade that can be activated by numerous stress-related signal inputs and by a varietyof seven-transmembrane domain receptors that couple to heterotrimericG proteins (31). The $beta$ $gamma$ subunits released from the G proteinupon activation of these receptors are believed to activate exchangefactors for Rho family GTPases (13). Cdc42 can then activatethe protein kinase cascade that switches on JNK. The mixed-lineagekinase MLK2 may mediate this activation (18). However, thereremains the possibility that other downstream effectors of Cdc42participate in the pathway. We therefore tested the effects ofBorg expression on the activity of JNK in transfected Coscells.

As shown in Fig. 4, the coexpression of HA₃-Borg3 suppressed the basal activity of HA-JNK. Anisomycin stimulated both thebasal JNK and Borg-inhibited JNK activities by about the samedegree, indicating that Borg3 does not interfere with the stress-mediatedsignaling pathway that regulates JNK. The inhibition by HA₃-Borg3was not a result of changes in the level of expression of theHA-JNK or of competition for the anti-HA antibody. In fact, HA₃-Borg3is not efficiently immunoprecipitated by the anti-HA₃ tag antibody,perhaps because the tag is hidden by interaction of the Borg withother proteins or because it is partially buried within the foldedprotein (not shown). To assess whether this inhibition is dependenton the binding of Cdc42, we used in the same assay a CRIB domainmutant, Borg3(I₂₃A,S₂₄A), that cannot bind Cdc42. Expression ofthis mutant inhibited basal JNK activity to the same extent asthe wild-type Borg3 (Fig. 4B). In each case, we checked the presenceof all ectopically expressed proteins in the lysates by immunoblotting(Fig. 4). A similar inhibition of JNK activity by HA₃-Borg3 andHA₃-Borg3(I₂₃A,S₂₄A) was observed in transfected NIH 3T3 cells(not shown).

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FIG. 4. Inhibition of JNK by Borg3. Cos cells were transfected as described in Materials and Methods and incubated overnight in serum-free DMEM. After 24 h, 100 µg of anisomycin (Anis.) was added (control) and the cells were incubated for 20 min at 37°C. Cells were lysed in 400 µl of lysis buffer. After clearing, equal volumes (100 µl) of the supernatant were removed for immunoblot analysis and separated by SDS-PAGE. Proteins were transferred to a nitrocellulose membrane and immunoblotted as described in Materials and Methods. HA₃-tagged proteins were immunoprecipitated from the remaining supernatant and resuspended in 30 µl of kinase buffer, and 2 µg of purified GST-c-Jun(1-79) as the substrate plus 2 µCi of [ $gamma$ -³²P] ATP were added to each reaction tube. The reactions proceeded at 30°C for 20 min and were stopped by the addition of 10 µl of 4× Laemmli sample buffer. Kinase reaction complexes were separated by SDS-PAGE and analyzed by fluorography.

These data indicate that the inhibition of the JNK pathway by Borg proteins is independent of the binding to Rho-like GTPasesand therefore is not a result of competition for another downstreameffector such as MLK2, which is required for JNKactivation.

Effects of ectopic expression of Borg proteins on cell shape. To examine whether Borgs might, like many downstream effectors of Cdc42/Rac, play a role in the elaboration or remodelingof the actin cytoskeleton, we expressed Borg1, Borg2, and Borg3as HA₃-tagged fusion proteins in NIH 3T3 fibroblasts. As a negativecontrol, cells were transfected with the empty vector, pKH₃. Expressionof the Borg protein was detected with the monoclonal anti-HA antibody12CA5 and a secondary Texas red-coupled antibody. The F-actinframework was revealed by using FITC-phalloidin. Expression ofHA₃-Borg1 did not cause any dramatic changes in cell shape, butthere was a substantially reduced abundance of stress fibers inmost of the transfected cells, and unusually long, thin extensionswere common (Fig. 5b and c). Similar but more pronounced morphologicalchanges were seen when we ectopically expressed HA₃-Borg2 andespecially HA₃-Borg3. Most of the transfected cells displayeda disturbed shape, in which the cell bodies had pulled in, butalso extended long, sometimes beaded processes and protrusivelamellipodia (Fig. 5d to g). This phenotype is reminiscent ofthat produced by the overexpression of RhoGDI or RhoGAPs suchas p190 or by injection of C3 botulinum toxin which inhibits Rhofunction (40, 53). The HA₃-Borgs were all localized mainlyin the cytosol but also in filopodia and at the edges of lamellipodia,where they were coincident with cortical F-actin structures (Fig.5b to g). These phenotypes were also seen in other cell typesthat were tested, including baby hamster kidney (BHK21) and Swiss3T3 cells (data not shown). We confirmed by immunoblotting thatBorg1 to Borg3 were expressed and were of the expected size (Fig.5h). To verify the preferential targeting of the Borg proteinsto the ruffles of lamellipodia, we coexpressed a Myc-tagged, activatedRac1 [Rac1(G12V)] with HA₃-Borg3. Expression of activated Rac1in NIH 3T3 fibroblasts induces the formation of rounded cellswith large, multilayered ruffles around the entire edge of thecell (41). Ectopic expression of HA₃-Borg3 did not perturb thisphenotype, as shown by phalloidin staining (Fig. 5j), but theBorg protein was concentrated in the ruffles (Fig. 5i). However,the interaction of the Borg with these structures is relativelyweak, because treatment with 0.008% digitonin to permeabilizethe plasma membrane resulted in the loss of all detectable HA₃-Borg3from the cells, though it did not visibly perturb the actin cytoskeleton(data not shown).

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FIG. 5. Cell morphologies induced by ectopic expression of HA₃-tagged Borg proteins. NIH 3T3 fibroblasts were transfected with pKH₃ empty vector (a) or with pKH₃ or pKMyc vector containing cDNA encoding either Borg1 (b and c), Borg2 (d and e), Borg3 (f and g), or Cdc42 (k). Some cells were cotransfected with pKH₃-Borg3 plus pKMyc-Rac(G12V) (i and j) or with pKH₃-Borg3 plus pKMyc-Cdc42 (l). Cells were fixed 40 h after transfection and processed for immunofluorescence using either the monoclonal mouse anti-HA antibody 12CA5 and a secondary, Texas red-coupled anti-mouse antibody to detect Borg proteins (b, d, f, and i) or with FITC-phalloidin to reveal F-actin (a, c, e, g, j, k, and l) as described in Materials and Methods. Lysates from transfected cells were analyzed by immunoblotting using anti-HA antibody 12CA5. Detection was by chemiluminescence (h). For panels k and l, expression of Myc-Cdc42 (k) and HA₃-Borg3 (l) was checked by immunofluorescence using monoclonal antibodies 9E10 (anti-Myc) and 12CA5, respectively, and a secondary Texas red-coupled antibody (not shown). In panel k, arrow indicates a transfected cell. Bar = 40 µm.

We then wanted to assess whether the ectopic expression of Borgs would inhibit the cytoskeletal remodeling induced by Cdc42.Overexpression of wild-type HA₃-tagged or Myc-tagged Cdc42 inducesthe formation of lamellipodia bordered with microspikes aroundthe cell edge and a partial loss of stress fibers (Fig. 5k). Thecoexpression of HA₃-Borg3 with Myc-Cdc42 did not inhibit thisphenotype but instead produced a different, "porcupine" phenotype,in which the cells radiated an abundance of actin-filled spikesthat were sometimes branched and the cell bodies were devoid ofstress fibers (Fig. 5l). Equivalent results were obtained whenHA₃-Borg1 or HA₃-Borg2 was coexpressed with Myc-Cdc42 (not shown).This phenotype is not caused by a Borg-mediated enhancement ofCdc42 function, for the following reasons. First, the phenotypeis not induced by expression of a gain-of-function mutant of Cdc42.Second, we observed a similar phenotype when the p190 RhoGAP wascoexpressed with Myc-Cdc42 (data not shown). We conclude, therefore,that Borgs neither inhibit Cdc42 function nor act downstream ofCdc42 to trigger filopodia formation, but that the results areconsistent with an inhibition of Rho function induced by Borgproteins. To test this hypothesis, we examined whether the Borgphenotype could be reversed by the coexpression of wild-type Rho.NIH 3T3 cells were transfected either with HA₃-Borg3 alone, withMyc-tagged RhoA alone, or with HA₃-Borg3 plus Myc-RhoA. As canbe seen in Fig. 6c and f, the Borg3 produced a characteristicdistortion of the normal cell morphology, with loss of stressfibers and the extension of protrusive lamellipodia. Coexpressionof the Myc-RhoA dramatically increased stress fiber formationand the restoration of a more normal fibroblast appearance. Thisresult supports the hypothesis that Borg3 inhibits Rho functionand suggests that it acts upstream of or parallel to Rho ratherthan by inhibiting a downstream effector of Rho.

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FIG. 6. Borg phenotype is abolished by coexpression of Myc-RhoA. NIH 3T3 fibroblasts were transfected with either pKMyc containing cDNA encoding for RhoA protein (a and d) or pKH₃ containing cDNA encoding Borg3 protein (c and f) or were cotransfected with plasmids encoding HA₃-Borg3 and Myc-RhoA proteins (b and e). Cells were fixed and processed for immunofluorescence. Tagged proteins were detected with either monoclonal anti-HA antibody 12CA5 (b and c) or monoclonal anti-Myc antibody 9E10 (a). Both antibodies were revealed with a secondary, Texas red-coupled anti-mouse antibody. F-actin was revealed with FITC-phalloidin (d to f). Bar = 40 µm.

Finally, to determine whether the effect of the Borg proteins on the cell phenotype is dependent on binding to Cdc42, we usedthe CRIB (I₂₃A,S₂₄A) mutant of Borg3, which is defective in Cdc42binding (Fig. 3B). Surprisingly, when transfected into NIH 3T3fibroblasts, the CRIB-defective mutant induced the same dramaticphenotype as did wild-type HA₃-Borg3, with loss of stress fibersand the extension of large, protrusive lamellipodia (Fig. 7b ande). The expression of a C-terminal deletion of Borg3 (residues1 to 83) gave a weaker phenotype, similar to the one obtainedwhen Borg1 is overexpressed. Few cells produced protrusive lamellipodia,but many cells extended long processes (Fig. 7c). Although theCRIB-defective mutant was expressed at levels equivalent to thoseof the wild-type HA₃-Borg3, the Borg3(1-83) fragment did not expresswell, and only few cells expressed the protein at a high level.However, no degradation of the protein could be detected (Fig.7g). The data suggest that the characteristic phenotype inducedby expression of Borg3 is independent of its interaction withCdc42.

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FIG. 7. Borg3 phenotype is independent of Cdc42 binding. NIH 3T3 fibroblasts were transfected with pKH₃ vector containing cDNA encoding either Borg3 (a and d), Borg3(I₂₃A,S₂₄A) (b and e), or Borg3(1-83) (c and f). Cells were fixed and processed for immunofluorescence by using either monoclonal mouse anti-HA antibody 12CA5 revealed with a secondary, Texas red-coupled anti-mouse antibody to detect HA₃-Borg proteins (a to c) or FITC-phalloidin to reveal F-actin (d to f). Bar = 40 µm. In parallel the expression levels of the different proteins were checked by immunoblotting with anti-HA antibody after transfer of cell lysate proteins to a nitrocellulose membrane (g). Proteins were revealed by chemiluminescence using a secondary anti-mouse antibody coupled to horseradish peroxidase. A control with cells transfected with pKH₃ empty vector is also included. For cell lysates containing HA₃-Borg3(1-83), a 10-fold longer exposure of the membrane is shown (×10). Arrows indicate the different Borg3 proteins.

Expression of Borg proteins delays cell spreading in a CRIB domain-dependant manner. Recent evidence has implicated several Rho family GTPases in cell motility and in spreading on fibronectin-coated surfaces(11, 34). Engagement of integrin receptors by fibronectinresults in a rapid and dramatic activation of Cdc42 and Rac, whichpromotes their interaction with a plethora of downstream effectors(11, 55). The function of many of these interactions in motilityand spreading remains unclear. To determine whether the expressionof Borg proteins would affect the ability of cells to spread,NIH 3T3 fibroblasts were transfected with either the empty pKH₃vector, pKH₃-Borg1, or pKH₃-Borg3. Forty hours after transfection,cells were trypsinized, maintained in suspension for 15 to 20min, and then replated onto fibronectin-coated slides. Cells werefixed with paraformaldehyde at intervals and processed for immunofluorescencelabeling. Spreading was quantitated by measuring total cell surfaceareas of transfected or control cells. Results are shown in Fig.8. At early times after replating (18 min), control cells wererounded, with lamellipodia encircling the cell bodies. Cells wereat this stage devoid of stress fibers (Fig. 8a, untransfectedcells). On the other hand, many of the cells expressing HA₃-Borg1or HA₃-Borg3 remained very small (cell area < 500 µm²), whereas almost no control cells were of that size (Fig. 8m).By 45 min, control cells were still rounded but had formed somestress fibers (Fig. 8b). In contrast, although the Borg-expressingcells began to spread, most of them were still small and completelydevoid of stress fibers. Three hours after replating, controlcells possessed abundant stress fibers and had attained a normalfibroblastic shape (Fig. 8c). Curiously, although the majorityof Borg-expressing cells had by 3 h reached surface areas similarto those of the control (Fig. 8m), they exhibited an unusual phenotype,with a highly convoluted perimeter. These cells contained fewstress fibers (Fig. 8c).

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FIG. 8. Borg3 expression delays cell spreading of NIH 3T3 cells on fibronectin-coated surface in a Cdc42-binding-dependent manner. NIH 3T3 fibroblasts were transfected with pKH₃ empty vector or with pKH₃ containing cDNA encoding either Borg1, Borg3, Borg3(I₂₃A,S₂₄A), or Borg3(1-83); 40 h after transfection, cells were trypsinized and replated on fibronectin-coated slides. Cells were fixed and processed for immunofluorescence at specific times. FITC-phalloidin was used to reveal F-actin (a to c), and anti-HA antibody 12CA5 and a secondary, Texas Red-coupled anti-mouse antibody were used to reveal Borg proteins (d to l). Arrows in panels a to c show HA₃-Borg3-expressing cells. Bar = 40 µm. For quantitation of cell surface area at 18 and 180 min following replating (m and n), cells were visualized by FITC-phalloidin (Control) or anti-HA staining. Measurement were made on 100 cells for each time point, using the Openlab 2.0 software. Cells were then grouped according to size. Results of one representative experiment are shown. Two to four independent experiments were carried out. Data for the 18-min time point were analyzed by an unpaired t test. Variances were approximately equal for all data sets. Mean areas for Borg1- and Borg3-transfected cells were very highly significantly different from those of the control (P << 0.001) and Borg3(I₂₃A,S₂₄A)-transfected (P << 0.001) cells.

These results suggest that the ectopic expression of Borg1 or Borg3 can interfere with the normal process of spreading, bothby delaying the rate of spreading and by interfering with theattainment of a normal fibroblastic shape after spreading is complete.The Rho GTPase is initially inhibited after engagement of integrinreceptors by fibronectin but is activated at later stages of cellspreading. The effect of the Borg3 on cell shape is thereforeconsistent with the proposal that the Borgs partially inhibitRhofunction.

As discussed above, the loss of stress fibers and changes in cell shape induced by Borg3 are independent of Cdc42 binding.To determine whether the reduction in spreading rate or alterationin cell shape is mediated by a Borg3-Cdc42 interaction, we assessedthe effect of the mutant protein Borg3(I₂₃A,S₂₄A) and of Borg3(1-83).Ectopic expression of HA₃-Borg3(I₂₃A,S₂₄A) significantly reducedthe delay in cell spreading seen with the wild-type HA₃-Borg3(Fig. 8g and h). Within 18 min following replating, 48% of thecells expressing HA₃-Borg3(I₂₃A,S₂₄A) were larger than 10³ µm² (Fig. 8n), a proportion similar to that for the control cells(54%) and substantially higher than that for the cells expressingwild-type HA₃-Borg3 (13%). These differences were very highlysignificant, as determined by an unpaired t test (equal variances).Borg3(1-83) gave an intermediate result. The effects of the twomutants are not additive since the results obtained with a doublemutant, HA₃-Borg3(I₂₃A,S₂₄A,1-83), was similar to that of cellsexpressing the CRIB(I₂₃A,S₂₄A) mutant (not shown). The differencesin spreading rate were not due to differences in expression levelsof the various proteins, as judged by quantitation of the immunofluorescenceof transfected cells counted in the assay (notshown).

These data indicate that the inhibition of spreading by Borg3 depends largely on its ability to bind Cdc42 and to a lesserextent on an intact BH3 and/or Pro-rich domain. The inhibitionmay be partially explained by a competition with other downstreameffectors for Cdc42, which is rapidly activated upon integrinreceptor engagement byfibronectin.

Contrary to the effects on spreading rate, however, the two Borg3 mutants remained fully capable of interfering with the attainmentof a normal fibroblastic cell shape. As can be seen in Fig. 8iand l, the transfected cells after 3 h on fibronectin possesshighly convoluted, lace-like peripheries with several holes neartheir edges. These cells also lack stress fibers (not shown).This result is consistent with the possibility that a domain nearthe N terminus of Borg3 (e.g., BH1) can inhibit Rho function independentlyof Cdc42binding.

Dynamic regulation of Rho is also required for cell migration (34). We therefore examined whether the ectopic expressionof HA₃-Borg3 could inhibit the movement of cells into a clearedarea of a monolayer. This wounding assay is expected to be lesssensitive to small changes in signaling functions, because itoccurs over a prolonged time period (24 h). Thus, cells that havea reduced motility rate might still have time to migrate intothe cleared area. Nonetheless, as shown in Table 1, HA₃-Borg1,HA₃-Borg3, and HA₃-Borg3(I₂₃A,S₂₄A), when coexpressed with GFP,did significantly reduce the fraction of green fluorescent cellsthat migrated.

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TABLE 1. Effects of ectopic expression of Borg proteins on fibroblasts migration in a wound test

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We have described a new family of proteins, named Borg1 to Borg5, that are putative downstream effectors of Cdc42 and/or TC10.Borg1, Borg4, and Borg5 were identified from a two-hybrid screenusing the TC10 GTPase as bait; Borg2 and Borg3 were discoveredfrom database searches for Borg-related ESTs. Borg5 is most likelythe human homolog of a previously reported protein called MSE55that was shown to interact with Cdc42 and Rac through a conservedCRIB domain (3). Each member of the Borg family contains ahighly related CRIB domain near the N terminus of the proteinand several further regions of close similarity to one another,which we have called BH1, BH2, and BH3 domains, that were notfound in any other proteins in the database. Remarkably, althoughBorg1, Borg2, Borg4, and Borg5 appear to bind with similar affinitiesto both Cdc42 and TC10, Borg3 does not interact detectably withTC10. Compared with the other members of the family, the Borg3protein sequence lacks three amino acids immediately upstreamof the CRIB domain. This deletion might account for the differentialbinding to the small GTPases. This result extends our previousobservations that closely related pairs of effectors, such asMLK2-MLK3 and WASP-N-WASP, interact differentially with TC10 (33).TC10 has also been reported to be insensitive to the nucleotideexchange factor Dbl (17). Thus, TC10 may be designed to respondin a restricted way to only a subset of upstream signals and toactivate only a specific subset of the downstream effectors thatare regulated by Cdc42. Such restrictions may be essential ifTC10 operates mainly in highly differentiated tissues such asmuscle, where proliferative signals could be deleterious tofunction.

The tissue distribution of Borgs varies with the isoform. Borg1 mRNA was detected in all tissues examined, while Borg2 wasexpressed only at very low levels in brain and liver. Borg3 mRNAappears to be present at very low levels in most tissues, buta much longer transcript was clearly detectable in skeletal muscle.Whether the multiple Borg transcripts represent splice variantsor partially processed mRNAs remains to be determined. We wereunable to clone the full-length sequence of Borg4, and no mRNAwas detected for this protein in any of the adult human tissuestested. It may therefore be expressed only in fetal or embryonictissues.

We studied Borg1 and Borg3 in more detail. When expressed ectopically in NIH 3T3 cells (or in BHK cells), the proteins appearedto be predominantly cytoplasmic and induced a characteristic phenotypethat included the formation of long thin extensions and protrusivelamellipodia as well as the partial loss of stress fibers. Theeffect may be related to the loss of stress fibers caused by inhibitionof Rho function, which permits a more extensive remodeling ofthe F-actin into filopodia (35). The idea that there is competitionbetween different GTPase-mediated signals for structuring thefinite amount of actin present within the cell has been also proposedby others (32). We tested this hypothesis further by coexpressingBorg3 with wild-type Rho. The overexpression of Rho restored stressfibers and a more normal fibroblastic cell shape, supporting theidea that Borg3 can inhibit Rhofunction.

By what mechanism might the Borg proteins exert their effects on the cell? Conceivably, the Borg CRIB domain might bind toCdc42 and/or TC10 and compete out other downstream effectors forthese GTPases. We do not favor this mechanism, however, becausea CRIB mutant of Borg3 that is unable to bind Cdc42 was fullycapable of inducing the characteristic Borg phenotype. The CRIBmutant data also rule out the possibility that the phenotype mightresult from the interaction of GTP-bound Cdc42 and/or TC10 withBorg, which activates a downstream signal. Moreover, the coexpressionof Borg3 with wild-type Cdc42 did not inhibit the formation offilopodia by Cdc42 but caused a dramatic increase in their length.A similar phenotype could be induced by the coexpression of theRhoGAP, p190, with Cdc42, supporting the proposal that Borgs caninhibit Rho function. Therefore, the Borg proteins most likelyinduce the observed effects on the cytoskeleton independentlyof a direct interaction with the small GTPases, although bindingto Cdc42 may well modify these effects, either by changing thesubcellular distribution of the Borg proteins or by inducing conformationalchanges which would alter their interactions with otherproteins.

It is important to note that changes in stress fiber formation can occur independently of Rho activity. For example, the drugcytochalasin D activates Rho but causes the dissolution of stressfibers (38). Rho is believed to regulate stress fiber formationthrough its downstream effector, ROCK, which phosphorylates andinhibits the myosin light-chain (MLC) phosphatase. Phosphorylationof MLC mediates the formation of actomyosin bundles and stimulatescontraction (21). A protein kinase effector of Cdc42 and Rac(PAK1) has been reported to phosphorylate and inhibit the MLCkinase, thereby reducing MLC phosphorylation and reducing actomyosinbundling (45), but these results have been disputed, and inanother system PAK1 appears to be able to stimulate MLC phosphorylation(47). Our present data do not, therefore, definitively provethat Borg proteins cause disassembly of stress fibers throughan inhibition of Rho function, but they are consistent with thishypothesis.

The cytoskeletal responses of cells to Rac have been shown to be independent of the effects of this GTPase on other signalingpathways such as that which activates JNK (24). A similar situationprobably holds for other Rho family GTPases, including Cdc42.To determine whether Borg proteins participate in these otherpathways, we examined whether the expression of Borg3 interfereswith or potentiates JNK activation. We showed that wild-type HA₃-taggedBorg3 inhibited the basal JNK activity. Surprisingly, like itseffects on the cytoskeleton, the Borg3-mediated inhibition ofJNK was independent of its ability to bind Cdc42. It remains tobe determined whether the mechanism by which the Borg proteininterferes with JNK is the same as that by which it inhibits Rhofunction.

Our observations on the effects of Borg3 on cell spreading revealed two distinct responses, only one of which was independentof Cdc42 binding. After replating onto fibronectin, the cellsthat expressed HA₃-Borg3 spread very slowly, and the spread cellspossessed an unusual cell shape and lacked stress fibers. Usingthe CRIB mutant which is defective in Cdc42 binding, we were ableto partially restore the normal spreading rate but did not restorenormal cell shape. We propose that the rate of spreading is atleast partially dependent on the activation of Cdc42 and its interactionwith a set of downstream effectors, which may be inhibited bycompetition with the Borg protein. WASP and N-WASP interact withthe Arp2-Arp3 complex. This complex, which enhances actin nucleation,branching, and cross-linking of actin filaments in vitro, is involvedin the formation of lamellipodia (27, 42). However, competitioncannot completely account for the inhibition in cell spreading,because expression of the mutant Borg3(1-83), which can bind Cdc42,was also relatively ineffective in inhibiting spreading. Borg3(1-83)is expressed much less efficiently than wild-type protein, buteven when only cells that expressed similar amounts of proteinwere compared, the Borg3(1-83) mutant did not show the same degreeof inhibition of spreading as did the wild-type protein. It islikely, therefore, that protein-protein interactions involvingthe C-terminal domains of Borg are required, in addition to Cdc42binding, to inhibit cell spreading on fibronectin. The abnormalcell shape caused by expression of either the CRIB mutant or theC-terminal deletion mutant is consistent with our other data thatimplicate Borgs in Rho inhibition and with evidence from othergroups that Rho is switched on at a late stage in cell spreadingand may be necessary for the assumption of a normal fibroblasticcell shape (5, 11).

The wounding assay for cell motility was less sensitive to ectopic expression of Borg3. Although a small inhibition was consistentlyobserved, it was much less dramatic than the inhibition of spreading.This difference may reflect the very different times over whichthe two experiments were conducted. Motility was estimated after24 h, during which time the cell could compensate for partialinhibition of endogenous functions either by changes in gene expressionor by adaptation in the responsiveness to externalsignals.

Overall, our studies suggest that Borg proteins may interfere with the activity of the Rho GTPase and function as negativeregulators in cross talk between Cdc42- and Rho-mediated signalingpathways. The mechanism by which Borg proteins inhibit actin stressfiber formation remains to be determined. They could inhibit signalingthrough the lysophosphatidic acid receptor or through the G $alpha$ proteinsthat couple to Rho-specific guanine nucleotide exchange factors,or they could inhibit the exchange factors themselves. Alternatively,they may interfere with the phosphorylation of MLC. It will beof interest, therefore, to identify binding partners for the Borgproteins other than Cdc42 and TC10 as a first step toward a completedescription of theirfunction.

	ACKNOWLEDGMENTS

We thank Stan Hollenberg, Rick Cerione, Mark Rush, and Gary Bokoch for their kind gifts of reagents, and we thank Cheryl Neudauer,Nia Tatsis, and Tom Parsons for helpfuldiscussions.

This work was supported by the Markey Center for Cell Signaling and by grant CA 56300 from the National Institutes ofHealth.

	FOOTNOTES

^* Corresponding author. Mailing address: Room 7191 Hospital West, Box 577, HSC, University of Virginia School of Medicine, Charlottesville,VA 22908. Phone: (804) 982-0083. Fax: (804) 924-1236. E-mail:gmj4h{at}virginia.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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15. Guasch, R. M., P. Scambler, G. E. Jones, and A. J. Ridley. 1998. RhoE regulates actin cytoskeleton organization and cell migration. Mol. Cell. Biol. 18:4761-4771[Abstract/Free Full Text].

16. Hall, A. 1998. Rho GTPases and the actin cytoskeleton. Science 279:509-514[Abstract/Free Full Text].

17. Hart, M. J., A. Eva, D. Zangrilli, S. A. Aaronson, T. Evans, R. A. Cerione, and Y. Zheng. 1994. Cellular transformation and guanine nucleotide exchange activity are catalyzed by a common domain on the dbl oncogene product. J. Biol. Chem. 269:62-65[Abstract/Free Full Text].

18. Hirai, S., M. Katoh, M. Terada, J. M. Kyriakis, L. I. Zon, A. Rana, J. Avruch, and S. Ohno. 1997. MST/MLK2, a member of the mixed lineage kinase family, directly phosphorylates and activates SEK1, an activator of c-Jun N-terminal kinase/stress-activated protein kinase. J. Biol. Chem. 272:15167-15173[Abstract/Free Full Text].

19. Hotchin, N. A., and A. Hall. 1995. The assembly of integrin adhesion complexes requires both extracellular matrix and intracellular Rho/Rac GTPases. J. Cell Biol. 131:1857-1865[Abstract/Free Full Text].

20. Keely, P. J., J. K. Westwick, I. P. Whitehead, C. J. Der, and L. V. Parise. 1997. Cdc42 and Rac1 induce integrin-mediated cell motility and invasiveness through Pi(3)K. Nature 390:632-636[Medline].

21. Kimura, K., M. Ito, M. Amano, K. Chihara, Y. Fukata, M. Nakafuku, B. Yamamori, J. Feng, T. Nakano, K. Okawa, A. Iwamatsu, and K. Kaibuchi. 1996. Regulation of myosin phosphatase by Rho and Rho-associated kinase (Rho-kinase). Science 273:245-248[Abstract].

22. Kozak, M. 1986. Point mutations define a sequence flanking the AUG initiator codon that modulates translation by eukaryotic ribosomes. Cell 44:283-292[Medline].

23. Kozma, R., S. Ahmed, A. Best, and L. Lim. 1995. The Ras-related protein Cdc42Hs and bradykinin promote formation of peripheral actin microspikes and filopodia in Swiss 3T3 fibroblasts. Mol. Cell. Biol. 15:1942-1952[Abstract].

24. Lamarche, N., N. Tapon, L. Stowers, P. D. Burbelo, P. Aspenstrom, T. Bridges, J. Chant, and A. Hall. 1996. Rac and Cdc42 induce actin polymerization and G1 cell cycle progression independently of P65(Pak) and the JNK/SAPk map kinase cascade. Cell 87:519-529[Medline].

25. Leung, T., X. Q. Chen, I. Tan, E. Manser, and L. Lim. 1998. Myotonic dystrophy kinase-related Cdc42-binding kinase acts as a Cdc42 effector in promoting cytoskeletal reorganization. Mol. Cell. Biol. 18:130-140[Abstract/Free Full Text].

26. Machesky, L. M., and A. Hall. 1996. Rho $---$ a connection between membrane receptor signalling and the cytoskeleton. Trends Cell Biol. 6:304-310. [Medline]

27. Machesky, L. M., and R. H. Insall. 1998. Scar1 and the related Wiskott-Aldrich syndrome protein, WASP, regulate the actin cytoskeleton through the Arp2/3 complex. Curr. Biol. 8:1347-1356[Medline].

28. Machesky, L. M., and A. Hall. 1997. Role of actin polymerization and adhesion to extracellular matrix in Rac- and Rho-induced cytoskeletal reorganization. J. Cell Biol. 138:913-926[Abstract/Free Full Text].

29. Mackay, D. J., F. Esch, H. Furthmayr, and A. Hall. 1997. Rho- and Rac-dependent assembly of focal adhesion complexes and actin filaments in permeabilized fibroblasts: an essential role for ezrin/radixin/moesin proteins. J. Cell Biol. 138:927-938[Abstract/Free Full Text].

30. Miki, H., T. Sasaki, Y. Takai, and T. Takenawa. 1998. Induction of filopodium formation by a Wasp-related actin-depolymerizing protein N-Wasp. Nature 391:93-96[Medline].

31. Minden, A., A. Lin, F. X. Claret, A. Abo, and M. Karin. 1995. Selective activation of the JNK signaling cascade and c-Jun transcriptional activity by the small GTPases Rac and Cdc42Hs. Cell 81:1147-1157[Medline].

32. Moorman, J. P., D. Luu, J. Wickham, D. A. Bobak, and C. S. Hahn. 1999. A balance of signaling by Rho family small GTPases RhoA, Rac1 and Cdc42 coordinates cytoskeletal morphology but not cell survival. Oncogene 18:47-57[Medline].

33. Neudauer, C. L., G. Joberty, N. Tatsis, and I. G. Macara. 1998. Distinct cellular effects and interactions of the Rho-family GTPase TC10. Curr. Biol. 8:1151-1160[Medline].

34. Nobes, C., D., and A. Hall. 1999. Rho GTPases control polarity, protrusion, and adhesion during cell movement. J. Cell Biol. 144:1235-1244[Abstract/Free Full Text].

35. Nobes, C. D., and A. Hall. 1995. Rho, rac, and cdc42 GTPases regulate the assembly of mult

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12.	Coso, O. A., M. Chiariello, J. C. Yu, H. Teramoto, P. Crespo, N. Xu, T. Miki, and J. S. Gutkind. 1995. The small GTP-binding proteins Rac1 and Cdc42 regulate the activity of the JNK/SAPK signaling pathway. Cell 81:1137-1146[Medline].
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14.	Drivas, G. T., A. Shih, E. Coutavas, M. G. Rush, and P. D'Eustachio. 1990. Characterization of four novel ras-like genes expressed in a human teratocarcinoma cell line. Mol. Cell. Biol. 10:1793-1798[Abstract/Free Full Text].
15.	Guasch, R. M., P. Scambler, G. E. Jones, and A. J. Ridley. 1998. RhoE regulates actin cytoskeleton organization and cell migration. Mol. Cell. Biol. 18:4761-4771[Abstract/Free Full Text].
16.	Hall, A. 1998. Rho GTPases and the actin cytoskeleton. Science 279:509-514[Abstract/Free Full Text].
17.	Hart, M. J., A. Eva, D. Zangrilli, S. A. Aaronson, T. Evans, R. A. Cerione, and Y. Zheng. 1994. Cellular transformation and guanine nucleotide exchange activity are catalyzed by a common domain on the dbl oncogene product. J. Biol. Chem. 269:62-65[Abstract/Free Full Text].
18.	Hirai, S., M. Katoh, M. Terada, J. M. Kyriakis, L. I. Zon, A. Rana, J. Avruch, and S. Ohno. 1997. MST/MLK2, a member of the mixed lineage kinase family, directly phosphorylates and activates SEK1, an activator of c-Jun N-terminal kinase/stress-activated protein kinase. J. Biol. Chem. 272:15167-15173[Abstract/Free Full Text].
19.	Hotchin, N. A., and A. Hall. 1995. The assembly of integrin adhesion complexes requires both extracellular matrix and intracellular Rho/Rac GTPases. J. Cell Biol. 131:1857-1865[Abstract/Free Full Text].
20.	Keely, P. J., J. K. Westwick, I. P. Whitehead, C. J. Der, and L. V. Parise. 1997. Cdc42 and Rac1 induce integrin-mediated cell motility and invasiveness through Pi(3)K. Nature 390:632-636[Medline].
21.	Kimura, K., M. Ito, M. Amano, K. Chihara, Y. Fukata, M. Nakafuku, B. Yamamori, J. Feng, T. Nakano, K. Okawa, A. Iwamatsu, and K. Kaibuchi. 1996. Regulation of myosin phosphatase by Rho and Rho-associated kinase (Rho-kinase). Science 273:245-248[Abstract].
22.	Kozak, M. 1986. Point mutations define a sequence flanking the AUG initiator codon that modulates translation by eukaryotic ribosomes. Cell 44:283-292[Medline].
23.	Kozma, R., S. Ahmed, A. Best, and L. Lim. 1995. The Ras-related protein Cdc42Hs and bradykinin promote formation of peripheral actin microspikes and filopodia in Swiss 3T3 fibroblasts. Mol. Cell. Biol. 15:1942-1952[Abstract].
24.	Lamarche, N., N. Tapon, L. Stowers, P. D. Burbelo, P. Aspenstrom, T. Bridges, J. Chant, and A. Hall. 1996. Rac and Cdc42 induce actin polymerization and G1 cell cycle progression independently of P65(Pak) and the JNK/SAPk map kinase cascade. Cell 87:519-529[Medline].
25.	Leung, T., X. Q. Chen, I. Tan, E. Manser, and L. Lim. 1998. Myotonic dystrophy kinase-related Cdc42-binding kinase acts as a Cdc42 effector in promoting cytoskeletal reorganization. Mol. Cell. Biol. 18:130-140[Abstract/Free Full Text].
26.	Machesky, L. M., and A. Hall. 1996. Rho $---$ a connection between membrane receptor signalling and the cytoskeleton. Trends Cell Biol. 6:304-310. [Medline]
27.	Machesky, L. M., and R. H. Insall. 1998. Scar1 and the related Wiskott-Aldrich syndrome protein, WASP, regulate the actin cytoskeleton through the Arp2/3 complex. Curr. Biol. 8:1347-1356[Medline].
28.	Machesky, L. M., and A. Hall. 1997. Role of actin polymerization and adhesion to extracellular matrix in Rac- and Rho-induced cytoskeletal reorganization. J. Cell Biol. 138:913-926[Abstract/Free Full Text].
29.	Mackay, D. J., F. Esch, H. Furthmayr, and A. Hall. 1997. Rho- and Rac-dependent assembly of focal adhesion complexes and actin filaments in permeabilized fibroblasts: an essential role for ezrin/radixin/moesin proteins. J. Cell Biol. 138:927-938[Abstract/Free Full Text].
30.	Miki, H., T. Sasaki, Y. Takai, and T. Takenawa. 1998. Induction of filopodium formation by a Wasp-related actin-depolymerizing protein N-Wasp. Nature 391:93-96[Medline].
31.	Minden, A., A. Lin, F. X. Claret, A. Abo, and M. Karin. 1995. Selective activation of the JNK signaling cascade and c-Jun transcriptional activity by the small GTPases Rac and Cdc42Hs. Cell 81:1147-1157[Medline].
32.	Moorman, J. P., D. Luu, J. Wickham, D. A. Bobak, and C. S. Hahn. 1999. A balance of signaling by Rho family small GTPases RhoA, Rac1 and Cdc42 coordinates cytoskeletal morphology but not cell survival. Oncogene 18:47-57[Medline].
33.	Neudauer, C. L., G. Joberty, N. Tatsis, and I. G. Macara. 1998. Distinct cellular effects and interactions of the Rho-family GTPase TC10. Curr. Biol. 8:1151-1160[Medline].
34.	Nobes, C., D., and A. Hall. 1999. Rho GTPases control polarity, protrusion, and adhesion during cell movement. J. Cell Biol. 144:1235-1244[Abstract/Free Full Text].
35.	Nobes, C. D., and A. Hall. 1995. Rho, rac, and cdc42 GTPases regulate the assembly of mult