The RHO1-specific GTPase-activating Protein LRG1 Regulates Polar Tip Growth in Parallel to Ndr Kinase Signaling in Neurospora

Nico Vogt^*^,, and Stephan Seiler^*^,

*Institut für Mikrobiologie und Genetik, Abteilung Molekulare Mikrobiologie; and Deutsche Forschungsgemeinschaft Research Center of Molecular Physiology of the Brain (CMPB), Universität Göttingen, D-37077 Göttingen, Germany

Submitted December 19, 2007; Revised July 1, 2008; Accepted August 7, 2008
Monitoring Editor: Fred Chang

ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Regulation of Rho GTPase signaling is critical for cell shapedetermination and polarity. Here, we investigated the role ofLRG1, a novel member of the GTPase-activating proteins (GAPs)of Neurospora crassa. LRG1 is essential for apical tip extensionand to restrict excessive branch formation in subapical regionsof the hypha and is involved in determining the size of thehyphal compartments. LRG1 localizes to hyphal tips and sitesof septation via its three LIM domains. The accumulation ofLRG1 as an apical cap is dependent on a functional actin cytoskeletonand active growth, and is influenced by the opposing microtubule-dependentmotor proteins dynein and kinesin-1. Genetic evidence and invitro GTPase assays identify LRG1 as a RHO1-specific GAP affectingseveral output pathways of RHO1, based on hyposensitivity tothe glucan inhibitor caspofungin, synthetic lethality with ahyperactive β1,3-glucan synthase mutant, altered PKC/MAK1pathway activities, and hypersensitivity to latrunculin A. Themorphological defects of lrg-1 are highly reminiscent to theNdr kinase/RAM pathway mutants cot-1 and pod-6, and geneticevidence suggests that RHO1/LRG1 function in parallel with COT1in coordinating apical tip growth.

INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Polarized growth is a multifactorial property that is coordinatedby numerous signaling pathways, and monomeric GTPases of theRas super family have been identified as key regulators of cellpolarity (Etienne-Manneville and Hall, 2002; Jaffe and Hall,2005; Bustelo et al., 2007; Park and Bi, 2007). They act asmolecular switches that cycle between an active GTP–boundand an inactive GDP–bound form. Transition between thesetwo forms is achieved through GTPase-activating proteins (GAPs)leading to the inactive form and GDP-GTP-exchange factors (GEFs)that activate the small G-protein. Originally, GTPases of theRho subfamily were described as key regulators of the actincytoskeleton, but now it has become obvious that they influencemany cellular processes including cytoskeletal organization,vesicle transport, and transcriptional regulation. The positionof small G-proteins at the bottleneck of signal transductionpathways explains the many defects seen when these GTPases aremisregulated.

A challenging complication in determining the specific functionsof small G-proteins is the fact that the number of GAPs andGEFs is significantly larger than the number of GTPases thatthey regulate. For example, the D. melanogaster genome containsonly six Rho proteins, but $~$ 20 GEFs and more than 20 GAPs (Adamset al., 2000), indicating that understanding the specific functionsof these regulators will be the key for deciphering the temporaland spatial activity of the switches. Although considerableprogress has been made in understanding the activation of smallGTPases through their GEFs (Gulli and Peter, 2001; Schmidt andHall, 2002; Garcia et al., 2006), full activation of a specificGTPase requires not only the coordination of the "on" switch,but also the shuttling between both the active and inactivestates of the GTPase is essential for full signaling activityof the small G-protein (Vanni et al., 2005; Barale et al., 2006).Nevertheless, little is known about how the GAPs are regulatedin a spatial and temporal manner. Interestingly, the numberof GAPs present in the available fungal and animal genomes isexceeding those of the GEFs (Goffeau et al., 1996; Adams etal., 2000; Borkovich et al., 2004; Jaffe and Hall, 2005), indicatingthat fine-tuning of the "off-switch" is of high importance forproviding the necessary specificity for the Rho module.

Apical tip extension is the hallmark of filamentous fungi, andfungal hyphae share with neurons and pollen tubes the distinctionof being among the most highly polarized cells in biology (Palaniveluand Preuss, 2000; Chilton, 2006; Harris, 2006), thus makingthem attractive models for the analysis of fundamental mechanismsunderlying cellular polarity. Nevertheless, the molecular understandingof fungal morphogenesis is still a major challenge. Phylogeneticanalyses and the comparison of Saccharomyces cerevisiae morphogeneticdata with the limited results from various filamentous asco-and basidiomycetes have established that a core set of "polarityfactors" is conserved between unicellular and filamentous fungi(reviewed in Wendland, 2001; Borkovich et al., 2004; Harris,2006). Thus, the accumulated knowledge of baker's yeast is servingas an invaluable source for comparative morphogenetic studies,but it is becoming increasingly evident that subtle differencesin the wiring of these conserved components and the presenceof additional proteins that are absent in unicellular fungiresult in dramatically different morphogenetic outcomes rangingfrom budding to filamentous growth (Boyce et al., 2003, 2005;Rottmann et al., 2003; Seiler and Plamann, 2003; Li et al.,2006; Malavazi et al., 2006).

Current fungal research is focusing on the description of thevarious Rho proteins and the analysis of the interplay betweenthe different modules (Wendland and Philippsen, 2000, 2001;Boyce et al., 2003, 2005; Chen and Dickman, 2004; Leveleki etal., 2004; Rasmussen and Glass, 2005, 2007; Mahlert et al.,2006). Various studies have identified Rho1 as one key regulatorof hyphal growth and polarity. Aspergillus fumigatus Rho1 hasbeen described as part of the β1,3-glucan synthase complexthat localizes to zones of active growth at the hyphal apex(Beauvais et al., 2001). A similar role in maintaining cellwall integrity was suggested for Rho1 of Ashbya gossypii, becausedeletion mutants showed reduced filamentous growth and highrates of cell lysis (Wendland and Philippsen, 2001). Aspergillusnidulans RhoA has been implicated in polar growth, branching,and cell wall synthesis (Guest et al., 2004). Budding yeastRho1p as the best characterized representative of the Rho1 familyhas multiple functions in regulating the two main structuralfeatures of the fungal cell (reviewed in Levin, 2005; Park andBi, 2007). The organization of the actin cytoskeleton is controlledthrough the interaction of the activated GTPase with the polarisomecomponent Bni1p, whereas maintenance of the cell wall integrityis achieved via two independent mechanisms. Rho1p activatescell wall synthesis through the direct stimulation of the enzymeglucan synthase, which catalyzes the polymerization of β1,3-glucan.In addition, it activates the mitogen-activated protein (MAP)kinase pathway that monitors the cell wall integrity throughits activation of protein kinase C thereby coordinating thetranscription of several cell wall–specific enzymes.

To identify the critical components that contribute to polarizedgrowth, we developed a large-scale genetic screen for the isolationof conditional mutants defective in polar and directed growthin the Neurospora crassa (Seiler and Plamann, 2003) and haveidentified the Ndr kinase COT1 and its upstream regulator kinasePOD6 as required for hyphal tip extension. These kinases areimportant for normal cell differentiation and polar morphogenesisin various organisms, yet their specific functions are stillelusive (summarized in Hergovich et al., 2006). The buddingyeast RAM network (regulation of Ace2p activity and cellularmorphogenesis) is currently the best characterized, even thoughstill poorly understood, Ndr signaling cascade (Nelson et al.,2003; Jansen et al., 2006; and references therein). RAM-defectivecells exhibit a round morphology and fail to separate aftercytokinesis. The Ndr kinase Cbk1p is an essential componentof this pathway, whereas the STE20-like kinase Kic1p probablyfunctions as a direct upstream kinase of Cbk1p. In addition,Hym1p, Tao3p and Mob2p are required for Cbk1p activation andlocalization, The presence of these components also in highereukaryotes have established the idea that Ndr kinases and otherinteracting proteins represent the core components of a conservedsignaling network required for polarized morphogenesis. Here,we describe the characterization of a LIM and Rho-GAP domain–containingprotein (therefore named LRG1) that acts as a RHO1–specificGAP and provide genetic evidence that LRG1 functions in parallelwith COT1 in coordinating polar tip growth.

MATERIALS AND METHODS

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INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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Strains, Media, and Growth Conditions
N. crassa strains used in this study are summarized in the Table 1.General genetic procedures and media used in the handling ofN. crassa have been described (Davis and DeSerres, 1970) orare available through the Fungal Genetic Stock Center (www.fgsc.net).Growth tests to determine the sensitivity of mutant strainsin comparison to wild type against cytoskeletal, cell wall,and protein kinase C (PKC) inhibitors were performed on minimalmedium supplemented with 0.5% sorbose to enhance colonial growthof the strains and to allow a better comparison of the differentstrains on a single plate. The hygromycin B and nourseothricinconcentrations were adjusted to 200 and 30 µg/ml, respectively,to select for transformants. Homologous recombination eventsin the heterokaryotic strain HP1 containing the ${Delta}$ lrg-1–deletednucleus were verified by phenotypic analysis of transformantsgrown on 400 µM p-fluorophenylalanine (fpa) and 200 µg/mlhistidine or 5 µg/ml benomyl and 200 µg/ml pantothenicacid and by the complementation of the growth defect of potential ${Delta}$ lrg-1 strains with a 6-kb genomic SacII fragment containinglrg-1 (pNV16).

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Table 1. Neurospora crassa strains used in this study

Plasmid Construction
Primer sequences are summarized in the Supplementary Table S1.The lrg-1 deletion cassette in pNV46 was obtained by plasmidgap repair in S. cerevisiae (Orr-Weaver and Szostak, 1983

).pRS416 was linearized with XbaI and XhoI, the Nat^R cassettewas amplified by PCR with primers NV_gpd1 and NV_nat5 and pNV1as template (Seiler et al., 2006

), and the 5' and 3' flankingregions of lrg-1 were amplified from cosmid X8D4 using the oligonucleotidesNV_KOlrg5f, NV_KOlrg5r, NV_KOlrg3f, and NV_KOlrg3r. These primerscontained 25-bp homologous overhangs at their 5' ends and allowedrecombination of the four linear DNA fragments into the functionaldeletion cassette in yeast. To generate the GAP and LIM domaindeletion constructs, a 6-kb genomic SacII fragment containinglrg-1 coding region and 1.5- and 1-kb 5' and 3' regions, respectively,was inserted in pBluescript SK+ (Stratagene, Amsterdam, Netherlands)to obtain pNV16. The hygromycin cassette, amplified with theprimers Hyg5'Xba and Hyg3'Xba and plasmid pMP6 as template,was inserted into the unique XbaI site. LRG1^1–847 wasgenerated by deleting the C-terminal domain of lrg-1 in pNV16with ApaI and by inserting the hygromycin B resistance cassette(hph; which was amplified via ApaI-containing primers). ForLRG1^781–1279, the lrg-1 promoter was amplified using oligonucleotidesthat introduce NcoI and SacI sites and inserted together withan NcoI/SacII fragment harboring the GAP domain (aa 781-1279)into SacI/SacII-digested pBluescript SK+. The hygromycin cassettewas introduced into XbaI. Point mutations in the three LIM domainswere generated with the QuickChange Site-Directed MutagenesisKit (Stratagene) according to manufacturer's instruction usingthe oligonucleotides NV_LIM1mut_f, NV_LIM1mut_r, NV_LIM1mut2_f,NV_LIM1mut2_r, NV_LIM2mut_f, NV_LIM2mut_r, NV_LIM2mut2_f, NV_LIM2mut2_r,NV_LIM3mut_f, NV_LIM3mut_r, NV_LIM3mut2_f, NV_LIM3mut2_r. Thezinc-finger coordinating cysteines and histidines were substitutedby amino acids that lack the zinc-binding capability (LIM1:C121S, C124S, C98L, C101S; LIM2: H185V, C188S, C162S, C165A;LIM3: C492S, C495S, C469G, and C472S). The triple LIM domainmutation construct was generated by multiple mutagenesis PCRsto obtain all eight mutations of the first and second LIM domain.The third LIM domain was mutated in a parallel construct. AMscI/SacI fragment containing mutated LIM1*/2*, and a SacI/MluIfragment of LIM3* was ligated into pNV16 digested with MscI/MluI.The hygromycin cassette harboring Bsp120I restriction siteswas subsequently introduced into the unique NotI site of thevector. The K910A exchange in the GAP domain was generated usingthe primers NV_GAPmut_f and NV_GAPmut_r, and the hygromycinresistance cassette introduced via Bsp120I/NotI. The R847L pointmutation in the GAP domain was generated using the primers NV_LRG20and NV_LRG21, and the hygromycin resistance cassette introducedvia XbaI. N-terminal MYC-tagged version of LRG1 and LRG1^1–847were constructed by inserting a ninefold MYC-tag into the uniqueMscI right after the start codon with primers NV_myc4 and NV_myc3with pYM6 (Knop et al., 1999

) as template. The C-terminal MYC⁹-tagin LRG1^781–1279 was inserted via the EcoRI and SacII sitesof pNV16 using the primers NV_myc1 and NV_myc2. Western blotanalysis using a monoclonal 9E10-anti-cMYC antibody (Santa CruzBiotechnology, Santa Cruz, CA) verified the expression of theMYC-tagged LRG1 constructs. The enhanced green fluorescent protein(eGFP) coding region was amplified from pSM1 (Poggeler et al.,2003

) using oligonucleotides NV_GFP1 and NV_GFP2 and subsequentlyligated via EcoRV into MscI-digested pNV16 to generate GFP::LRG1.cDNAs of the six Rho GTPases were generated by reverse transcriptionwith RevertAid M-MuLV Reverse Transcriptase (Fermentas, Vilnius,Lithuania) from mRNA prepared with PolyATtract (Promega, Madison,WI), amplified by PCR using primers covering the genes fromATG to stop codon using oligonucleotides mentioned in SupplementaryTable S1. Sequences were inserted via primer-based restrictionsites (NotI-NotI for Rho1 to Rho4 or SalI-NotI for CDC42 andRAC) into modified pETM-30 (EMBL-Heidelberg, Protein ExpressionFacility). The GAP domain of LRG1 (aa 650-1035) was amplifiedwith primers NV_lrg14 and NV_lrg18 and introduced via SalI/XhoIand NotI into pETM-30. The N. crassa overexpression constructswere controlled by a modified CPC promoter derived from plasmidpMP6 harboring BglII and SpeI as unique cloning sites (Seileret al., 2006

). Genomic coding regions of the six Rho proteinswere amplified with primers containing the mentioned restrictionsites.

Microscopy
Immunolocalization for N. crassa hyphae was conducted followinga protocol adapted from Minke et al. (1999). Conidia were germinatedon a small piece of GN-6 cellulose filter (Gelman Sciences,)placed on the surface of an agar plate. Filters were plunge-frozenin liquid propane and transferred to fixative (3% formaldehydein 100% ethanol precooled to –80°C). Samples weremaintained at –80°C for at least 2 d and then slowlytransferred to room temperature (2 h at 20°C, 2 h at 4°C).Filters were rehydrated in a series of ethanol:buffer (100 mMphosphate, pH 7.0) solutions starting at a ratio of 90:10 andending at 10:90. The cell wall was digested by incubating thefilters for 0.5–8 min in 2 mg/ml lysing enzymes from Trichodermaharzianum (Sigma, Munich, Germany) in 100 mM potassium citrate(pH 6.0, 20 mM EGTA, 5% BSA). To block nonspecific binding ofantibody, the filters were incubated for 1 h in 5% BSA. Sampleswere immersed in the primary antibody for at least 8 h, washedseveral times in phosphate buffer, incubated in the secondaryantibody for $≥$ 8 h, and visualized using standard rhodamine andFITC filter sets. For immunolocalization, samples were viewedwith an ORCA ER digital camera (Hamamatsu, Hamamatsu City, Japan)mounted on an Axiovert S100 microscope (Carl Zeiss, Jena, Germany).Image acquisition was done using the Openlab 5.01 software (Improvision,Coventry, United Kingdom), and images were further processedusing Photoshop CS2 (Adobe, San Jose, CA). For localizationstudies of GFP::LRG1 and GFP::LRG1*, an AxioObserverZ.1 microscopeequipped with an ApoTome unit, an AxioCam MRm r3.0 CCD cameraand X-Cite (EXFO) illumination source was used with AxioVisionSoftware 4.6. For confocal imaging an Axiovert 100M microscopewith the confocal module LSM 510 and LSM 510-Software was used(all from Zeiss). To determine the kinetics of septum formation,DIC imaging of a hyphal segment was randomly started, and thefluorescence images were manually recorded at time points whenthe LRG::GFP localization had visibly changed to reduce photobleaching.The absolute time points of the GFP images were used for thecalculation of septation kinetics. Low magnification documentationof fungal hyphae or colonies was performed with a SZX12 stereomicroscope(Olympus, Tokyo, Japan) and a PS30 video camera (Kappa, Gleichen,Germany).

Enzymatic Assays
The RHO GTPases were purified as glutathione S-transferase (GST)fusion proteins. Transformed Rosetta2(DE3) cells (Novagen, Schwalbach,Germany) were grown at 20°C and induced for 12 h with 0.1M IPTG. Cell extracts generated by sonification in lysing buffer(50 mM Tris, pH 7.5, 10% saccharose, 5 mM MgCl₂, 1 mM PMSF,0.008% β-mercaptoethanol, and 0.02% NP40), were bound toGSH Sepharose (Amersham, Amersham, Buckinghamshire, United Kingdom),washed (50 mM Tris, pH 7.5, 250 mM NaCl, 5 mM MgCl₂, 1 mM PMSF,0.008% β-mercaptoethanol, 0.02% NP40) and eluted (50 mMTris, pH 8.0, 250 mM NaCl, 5 mM MgCl₂, 5 mM DTT, 20 mM glutathionereduced, and 0.02% NP40). GTPase assays were performed as described(Gibbs et al., 1988). Pre-equilibration of the RHO proteinswas for 15 min at 25°C in 30 µl buffer A (20 mM HEPES,pH 7.6, 25 mM sodium chloride, 2 mM EDTA, 1 mg/ml BSA, 0.5 mMDTT, and 0.005% sodium cholate) including 0.5 µM GTPaseand 5 µCi (0.17 µM) [ ${gamma}$ -³²P]GTP. GTP loading was stoppedon ice by adding 1 µl 0.5 M MgCl₂. GTPase, 5 µl,was added to start the reaction (final concentration: 20 mMHEPES, pH 7.6, 1 mg/ml BSA, 0.1 mM DTT, 1 mM GTP, and 4 µMGST::GAP or purified GST) at 25°C. Samples of 5 µlwere stopped in 1 ml ice-cold wash buffer (50 mM Tris, pH 7.5,50 mM sodium chloride, and 5 mM MgCl₂) and filtered trough BA85nitrocellulose membranes (Whatman, Clifton, NJ). The filterswere washed with 6 ml wash buffer, dried, and measured by scintillationcounting in a QuantaSmart scintillation counter (Perkin Elmer-Cetus,Norwalk, CT). The phospho-p44/42 MAP kinase (Thr202/Tyr204)antibodies (Cell Signaling Technology, Beverly, MA) were usedaccording to manufacturer's instructions.

RESULTS

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INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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LRG1 Is Essential for Hyphal Tip Extension
The phenotypic analysis of lrg-1(12-20) indicated no major differencesin hyphal morphology or branching frequency compared with wildtype when the strains were grown at permissive temperature (25°C;Figure 1, A and B). However, within 30 min of transferring lrg-1(12-20)to 37°C, we observed a rapid cessation of tip extension.In contrast to the wild-type apex, which is a dome-shaped structure,the tips of lrg-1(12-20) generated a characteristic pointed,needle-like shape. This stop of tip extension was accompaniedby the appearance of numerous subapical needle-shaped branchesof $≤$ 10 µm in length that also stopped growth with a pointedtip. After prolonged incubation at restrictive temperature,the new branches as well as the primary hyphae began to swellup in a bulbous and apolar manner. Transfer of such a cultureback to permissive temperature resulted in growing tips havingnormal growth rates, diameter, and morphology within 30 min.Germination of lrg-1(12-20) at restrictive temperature resultedin the formation of compact colonies with multiple $≤$ 10-µm-longgerm tubes with pointed tips.

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Figure 1. LRG1 is essential for hyphal tip extension. (A) wild type was grown on minimal media plates at 25°C (left, DIC image; right, Calcofluor White staining). Bar, 40 µm. (B) lrg-1(12-20) was grown on minimal media plates at 25°C and shifted for the indicated times to restrictive temperature to illustrate the cessation of tip extension with pointed, needle-like tips and the progressive hyperbranching of the mutant (phase-contrast images, top panel). Increased septation and abnormal chitin distribution was monitored by labeling with Calcofluor White (bottom panel). Bar, 40 µm. (C) Growth of the heterokaryotic lrg-1 deletion strain lrg-1⁺ + ${Delta}$ lrg-1 on minimal medium, medium containing fpa and histidine and medium containing benomyl and pantothenic acid (which forces the knockout nucleus to predominate), resulting in morphological defects identical to lrg-1(12-20) germinated at restrictive temperature. Bar, 7.5 µm.

Chitin is the primary component of fungal septae and of theinner layers of the hyphal cell wall and is therefore accessibleto the Calcofluor White staining, primarily at the hyphal tipsand at septae. At permissive temperature, tips and septae oflrg-1(12-20) are strongly labeled in a manner identical to wildtype (Figure 1, A and B). Within 2 h at 37°C, lrg-1(12-20)showed extensive label in a patchy, subapical manner throughoutthe hyphae at positions of newly emerging branches, indicatingexcessive chitin deposition at sites of aberrant growth. Incontrast, the high Calcofluor White stain at the primary tipsobserved in hyphae grown at the permissive temperature is nearlyabsent when the strains are cultured at the restrictive temperature,indicating decreased chitin synthesis at these nonelongatingtips. Furthermore, we observed increased septation of lrg-1(12-20)compared with wild type grown at permissive temperature, whichis further increased after shifting cells to restrictive conditions.The length of hyphal compartments at 25°C were 53.7 ±21.0 and 148 ± 58.0 µm for lrg-1(12-20) and wildtype, respectively (n = 50). After the transfer of lrg-1(12-20)to 37°C for 2.5 h the compartment length was further reducedto 11.3 ± 4.3 µm (n = 50), whereas the compartmentlength of wild type remained unchanged. The hyphal diameterof wild type and lrg-1(12-20) were similar and did not changeduring the shift experiment (8.2 ± 0.8 and 8.4 ±1.6 µm, respectively, after 2.5 h at 37°C; n = 20).

To examine the phenotype of a lrg-1 deletion strain, we constructeda null mutant by using the sheltered disruption method (Narganget al., 1995), which takes advantage of the fact that N. crassais a multinucleated cell. The lrg-1 gene was deleted via homologousrecombination in the heterokaryotic strain HP1, thereby allowingthe generation of mutants in genes that are essential or importantfor growth. The resulting mutant harbors two kinds of nuclei,one with a null allele of lrg-1, and one with a wild-type copy.These nuclei contain selectable markers that allowed a shiftin the nuclear ratio within the heterokaryotic cells. Growthon media containing fpa and histidine favored the propagationof the wild-type nucleus. In contrast, growth of heterokaryoticcells on media containing benomyl and pantothenic acid forcedthe knockout nucleus to predominate and thus led to the depletionof LRG1 and morphological defects that were indistinguishablefrom lrg-1(12-20) germinated at restrictive temperatures (Figure 1C).These results characterize lrg-1(12-20) as a conditional loss-of-functionallele of lrg-1 and confirm an essential role of LRG1 duringthe apical extension of the hyphal tip and in controlling thenumber and position of subapical branches.

LRG1 Contains Three LIM Domains and a GAP Domain That Is Essential for Growth and Septation
Examination of the 1279 amino acid (aa) encoding LRG1 sequencerevealed two interesting features (Figure 2A). The N-terminalregion from aa 1–533 is cysteine- and histidine-rich andcan be arranged into three tandem zinc-finger–containingstructures called LIM domains that act as versatile protein–proteininteraction motifs (Schaller, 2001; Brown and Turner, 2004).Furthermore, a RHO-GAP domain was found in the C-terminal partof LRG1 (aa 791-1279). Sequence comparisons indicated that highlyhomologous proteins containing this domain architecture arepresent in all available fungal genomes. Apart from the fungalLRG1 relatives, the LIM domains of LRG1 are most closely relatedto the focal adhesion organizing protein paxillin (E-value of2e^–28 for Drosophila pseudoobscura paxillin vs. E = 1e^–17for mouse leupaxin, a more distantly related member of the paxillinsuperfamily, and E = 1e^–14 for human actin-binding LIMprotein 1 as the closest non-paxillin–related LIM domain-containinghit).

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Figure 2. The N-terminal region and the C-terminal Rho-GAP domain are both required for LRG1's cellular function. (A) Genomic organization of lrg-1 locus. The four exons are represented in white, the three introns in black. The lrg-1 gene encodes for a protein with three LIM domains (brown) in the N-terminal half and one Rho-GAP domain (blue) in the C-terminal part of the protein. Green arrows represent expression constructs under the control of the endogenous promoter. (B) Complementation experiments of lrg-1(12-20) transformed with the indicated constructs. Transformants were grown at 37°C to determine the complementation capability of the respective construct. Bar, 200 µm.

Sequencing of lrg-1(12-20) revealed a single amino acid substitutionof the conserved tyrosine 926 (TAC) in the GAP domain by histidine(CAC), suggesting that the GAP domain is essential for the cellularfunction of LRG1. To analyze the function of the two LRG1 domains,we generated and expressed constructs lacking either the threeLIM (LRG^781–1279) or the GAP (LRG^1–847) motifs inlrg-1(12-20), and determined that the two individual domainswere unable to complement the tip extension defect of lrg-1(12-20)(Figure 2B). The importance of the GAP domain for hyphal growthwas further supported by a construct, in which the conservedlysine 910 in the full-length protein was substituted with alanine.This mutation has been shown to result in a nonfunctional GAPdue to loss of binding to the corresponding Rho (Li et al.,1997

). When we expressed this construct in lrg-1(12-20) or in ${Delta}$ lrg-1, no complementation of the mutants defects were detected(Figure 2B). To confirm that the GAP activity of LRG1 is essentialfor its function, we generated an allele, in which the conservedcatalytic arginine residue 847 of the GAP domain was substitutedby a lysine. This construct was expressed in lrg-1(12-20), butwas not sufficient for complementation (Figure 2B), thus providingstrong evidence for the importance of the enzymatic activityfor the function of LRG1.

An important function of the N-terminal part of LRG1 containingthe three LIM domains was indicated by the failure of LRG1^781–1279to complement lrg-1(12-20). Therefore, we generated a seriesof lrg-1 alleles, in which four of the eight metal ion–coordinatingcysteines or histidines of each of the three LIM domains weresubstituted with serines or alanines. These residues have beenshown to mimic the behavior of cysteines, but lack their zinc-coordinatingactivity, which has been shown to be essential for the functionof LIM domains (Schmeichel and Beckerle, 1997; Bombarda et al.,2002). Surprisingly, when we tested the three constructs thateach was defective in one of the three LIM domains, we foundthat they did lead to full phenotypic complementation of lrg-1(12-20).Also, when we combined the three mutated LIM domains by generatingLRG*, we did not observe abnormal growth of the lrg-1(12-20)(Figure 2B) or of homocaryotic ${Delta}$ lrg-1 transformants (data notshown) and measured overall radial growth rates on agar plates,which were comparable to wild type (LRG1: 1.1±0.1 mm/h;LRG1*: 1.0 ± 0.4 mm/h; n = 3). However, we noted a highervariability of extension rates of individual hyphal tips ofLRG1* grown on microscopic slides (7.2±6.2 µm/min;n = 50) in comparison to LRG1 (6.3±4.3 µm/min;n = 50), suggesting that the dysfunctional LIM domains impairproper tip extension. Nevertheless, the placement of septaewas not altered in LRG1*. The distance of the hyphal tip tothe first septum was 224.0 ± 41.9 µm in LRG1 and225.4±55.8 µm for LRG1* (n=30), whereas the distancebetween subapical septae was 84.9 ± 30.9 µm inLRG1 compared with 92.5 ± 32.4 µm in LRG1* (n =100).

The LIM Domains Are Required for Localizing LRG1 to Sites of Growth
To determine the cellular distribution of LRG1, we generatedan N-terminal myc⁹-tagged version of lrg-1, which complementedlrg-1(12-20). Immunolocalization experiments using anti-MYCantibodies revealed a punctate distribution throughout the cell,which was enriched at hyphal tips (Figure 3A). This localizationwas in line with a function of LRG1 at growing tips and wasalso observed, when we used antisera generated against LRG1(data not shown). Next, we characterized the localization patternof MYC⁹::LRG1^1–847 and LRG^781–1279::MYC⁹ in thewild-type background. Although LRG^781–1279::MYC⁹ aberrantlylocalized in a cortical manner throughout the whole hypha andalong septae, the MYC⁹::LRG1^1–847 distribution was similarto localization of LRG1, suggesting that the N-terminal partof LRG1 is involved in the localization of the GAP domain.

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Figure 3. LRG1 localization to sites of growth at the hyphal tip and the septum is dependent on functional LIM domains. (A) MYC::LRG1 and MYC::LRG1^1–847 immunolocalized in vesicular-reticulate structures that are enriched at hyphal tips, whereas LRG1^781–1279::MYC mis-localized to the hyphal cortex. Bar, 10 µm. (B) Localization data generated in the ApoTome modus indicate an apical vesicular–reticulate localization of GFP::LRG1 and a more diffuse localization of GFP::LRG1*. Bar, 5 µm. (C) GFP::LRG1 localized as a crescent at growing hyphal tips and at septae (left), whereas GFP::LRG1* containing the three mutated LIM domains did localize in a diffuse manner throughout the cell (right). Bar, 5 µm.

For a better resolution of the dynamics of LRG1, we generatedN-terminal GFP fusion constructs with LRG1 and with LRG1* (containingthe three mutated LIM domains). Both constructs were introducedinto homocaryotic ${Delta}$ lrg-1 and complemented the growth defect ofthe deletion strain. ApoTome-based fluorescence microscopy confirmedthe apical vesicular-reticulate localization of GFP::LRG1, butresulted in a more diffuse localization of GFP::LRG1* lackingthe prominent streaks (Figure 3B). In addition to this tip-enrichedvesicular–reticulate localization, we frequently observeda GFP::LRG1 cap along the apical cortex and strong stainingaround the septal pore (Figure 3C). In contrast, GFP::LRG1*was distributed in a more diffuse manner throughout the hyphawith only a weak accumulation at the hyphal apex and no localizationat septae. Thus, both the immunolocalization data and the GFP-fusionproteins indicated a function of the LIM domains in localizingthe GAP domain to sites of active growth in the apical regionand along septae.

Confocal microscopy was used to characterize the dynamics ofGFP::LRG1 in more detail. We first asked, if the localizationof the apical cap is growth-dependent and analyzed 100 randomlychosen tips of the GFP::LRG1 expressing strain (Figure 4A).At a growth rate of $≥$ 0.2 µm/s, 70% displayed an apicalcap, whereas 2% did not. In contrast, only 10% of the hyphaegrowing at rates of <0.2 µm/s and displayed an apicalcap, whereas 18% did not. Thus, the localization of GFP::LRG1as a cap-like structure at the hyphal tip was dependent on activegrowth. When we quantified the localization of GFP::LRG1*, weobserved the opposite behavior. Only 13% fast-growing and 2%slow-growing tips displayed a cap, whereas 62 and 23%, respectively,did not show an apical cap of GFP::LRG1, confirming that theLIM domains are responsible for localizing LRG1 to the growinghyphal apex in addition to their importance in targeting LRG1to sites of septation.

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Figure 4. The localization of GFP::LRG1 is dependent on active growth. (A) One hundred randomly chosen hyphal tips were assayed for the presence of an apical GFP::LRG1 or GFP::LRG1* cap. In fast growing hyphae, an apical GFP::LRG1 cap was detected in 70% hyphal tips, whereas only 13% of GFP::LRG1* hyphae displayed a visible cap. (B) The size of the apical GFP::LRG1 cap correlated with the growth rate of the tip (determined by the distance between the tip in two images taken at 20-s intervals). Examples of slow, medium, and fast growing tips are shown in the top panel. Bar, 5 µm. (C) The GFP::LRG1 localization at the forming septum occurred in two phases. Approximately 1.5 min after the appearance of Calcofluor White–positive septae (a; white arrow) GFP::LRG1 began to localize along the septal plate initially as punctate specs (b; red arrow) that soon merged into a diffuse plate (c; red arrowheads). This septal GFP::LRG1 localization disappeared then for ca. 10 min (d; yellow arrow), before it strongly accumulated at the central part of the septum along the septal pore (e; white arrowheads). Bar, 5 µm. (D) Treatment of the GFP::LRG1 expressing strain with 1 µM latrunculin A affected the localization of GFP::LRG1 at the hyphal apex within 30 s (top left, and middle images) and before any morphological change, which occurred within 5 min (DIC image; top right image), but had no influence on the terminal localization of GFP::LRG1 along as bright spot at the septal pore (bottom images). Bar, 5 µm.

During this analysis, we noted that the size of the apical capvaried with the growth rate. GFP::LRG1 accumulated in slow growinghyphae primarily along the central apical cortex, whereas infast growing tips, an extended cap structure was visible, withthe highest GFP intensity frequently accumulating as a subapicalring $~$ 2 µm behind the apex (Figure 4B). When we quantifiedthe length of the GFP::LRG1 marked apical cortex relative tothe growth rate of the tip, we observed a positive correlation(R² = 0.6204) between growth rate and size of the apical cap.

Septum formation in filamentous fungi requires the formationof actin rings as an initial step before cross wall formation.The myosin-dependent constriction of these rings then servesas track for the delivery of glucan- and chitin-rich vesicles(visualized by Calcofluor White staining) that then form theseptal plate (Harris, 2001; Rasmussen and Glass, 2005, 2007).To investigate LRG1's function during septum formation, we analyzedthe dynamics of GFP::LRG1 in subapical regions (Figure 4C).Calcofluor White positive cross walls appeared before the accumulationof weak GFP::LRG1 dots along the cortical region of a formingseptum. These dots merged into a septal plate, resulting inweak labeling of the whole septum after $~$ 3 min. This diffuseseptal localization disappeared then for ca. 10 min, beforeGFP::LRG1 strongly accumulated in the central region aroundthe septal pore. This final localization remained permanentand was visible at most older septae. When we incubated growinghyphae with 1 µM latrunculin A, we found that the apicalcap was disappearing within 30 s (Figure 4D), before the cessationof growth. The actin-depolymerizing agent induced a morphologicalchange of the hyphal tip after $~$ 5 min. Nevertheless, the septalpore-associated localization of GFP::LRG1 remained unaffectedby this treatment, indicating that this terminal associationof LRG1 with the central region of the septum is independentof a functional actin cytoskeleton.

The Apical Localization of LRG1 Is Influenced by a Functional Microtubule System and Opposing Motor Proteins
We also tested the dependence of the localization of LRG1 ona functional microtubule cytoskeleton by growing GFP::LRG1 on4 µg/ml nocodazole or 5 µg/ml benomyl. For bothtreatments, the apical LRG1 cap persisted as long as growthwas observed, indicating that a functional microtubule cytoskeletonis dispensable for LRG1's localization (data not shown). However,the size of the apical GFP::LRG1 cap was reduced by ca. 50%in inhibitor-treated cells when compared with untreated wild-typetips growing at comparable rates (Figure 5, suggesting thata functional microtubule cytoskeleton is necessary for a stableaccumulation of LRG1 at the hyphal tip.

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Figure 5. The localization of GFP::LRG1 is influenced by opposing microtubule-dependent motor proteins. (A) Growth rate and size of the GFP::LRG1 cap was determined in hyphae treated with 4 µM nocodazole for 2 min and compared with untreated control cells. Because the inhibitor treatment resulted in reduced growth rates, only slow-growing control cells with growth rates of up to 0.15 µm/s were included in the comparison. (B) lrg-1(12-20), cot-1(1) and the respective double mutants with components defective in the dynein/dynactin subunits ro-1, ro-3, and ro-10 or in the phosphatase-associated factor gul-1 were cultivated for 3 d at 37°C. The increased colony diameter of lrg-1(12-20);ro-1/-3/-10 mutants compared with lrg-1(12-20) indicate suppression of the GAP defect by loss of dynein/dynactin function. (C) Apical GFP::LRG1 caps were detected in 78% of wild-type tips with growth rates of >0.05 µm/s. This rate of GFP::LRG1 caps increased in mutants defective in the anterograde directed motor protein nkin to 91% and decreased to 19% in the mutants defective in the retrograde directed motor protein ro-1. (D) GFP::LRG1* in a ro-1 background localized along the cortex and the hyphal morphology of the double mutant closely resembled the deletion phenotype.

The high rate of fungal tip extension requires efficient microtubule-basedand motor protein-dependent transport systems for supplyingthe growing tip with all necessary growth supplies and regulatoryfactors (Steinberg, 2007

). This transport toward the growingtip could be the reason for the observed microtubule-dependenceof apical LRG1 localization. Thus we analyzed the impact ofmutants defective in anterograde- (kinesin-1) and retrograde-directed(dynein) on apical GFP::LRG1 localization (Seiler et al., 1999

;Zhang et al., 2003

). We compared the growth rates of variousropy (= dynein/dynactin) strains in single as well as doublemutants in combination with lrg-1(12-20) and found that ropymutations partially suppressed lrg-1(12-20) (Figure 5B). Incontrast to this common phenotype of lrg-1(12-20) and the Ndrpathway mutants cot-1(1) and pod-6(31–21), gul-1 thathad been implicated in phosphatase-associated, COT1/POD6-antagonizingfunctions (Terenzi and Reissig, 1967

; Seiler et al., 2006

),only suppressed the growth defects of cot-1(1) and pod-6(31–21),but not those of lrg-1(12-20). Next, we tested for a geneticconnection between lrg-1(12-20) and nkin, which had been shownto counteract dynein's retrograde transport activity (Seileret al., 1999

; Zhang et al., 2003

; Seiler et al., 2006

). Thegrowth rate of a lrg-1(12-20);nkin double mutant at semirestrictivetemperature was reduced by 42% when compared with lrg-1(12-20)as the slower growing of the two parental strains, indicatinga synthetic interaction between lrg-1(12-20) and nkin.

These data suggested that both opposing microtubule-dependentmotor proteins are involved in localizing LRG1. Therefore, wedetermined the localization of GFP-tagged LRG1 in these motormutants. As determined previously (Figure 4A), the majorityof slow-growing hyphal tips of wild type displayed no GFP::LRG1cap. The growth rates of the two motor mutants is ca. 20% ofwild type (Seiler et al., 1997, 1999), and thus, a visible capshould be rarely visible, if the GFP::LRG1 localization is independentof the two motors. We observed apical caps in only 22% of wild-typetips at growth rates <0.05 µm/s (Figure 5C). This contrastedsharply with 81% of ro-1 tips growing at rates of <0.05 µm/sthat displayed an apical GFP::LRG1 cap, while the number ofGFP::LRG1 caps at growth rates >0.05 µm/s was reducedto 8% in the nkin background (Figure 5C). Thus the apical localizationof LRG is influenced by opposing microtubule-dependent motorproteins. This localization dependence of LRG1 on both motorproteins and functional LIM domains was further supported whenwe introduced GFP::LRG1* in the ro-1 background. The resultingprogeny closely resembled the lrg-1 deletion phenotype, withpoorly growing and highly hyperbranched cells (Figure 5D). Interestingly,GFP::LRG1* localized in an aberrant cortical manner similarto what we have determined for the GAP domain alone (Figure 3A), suggesting that either of the two localization mechanismalone is sufficient for apical localization of LRG1, but disturbingof both targeting mechanisms results in abnormal localizationof LRG1.

LRG1 Is a RHO1-specific GAP Affecting Several Output Pathways of RHO1
Given LRG1's homology with Rho-GAP proteins, we determined,which of the six Rho-GTPases present in the N. crassa genomeare regulated by LRG1. When we overexpressed the wild-type formsof all RHO proteins in lrg-1(12-20), only RHO1 was capable ofpartially complementing the lrg-1(12-20) growth defect. Alsodominant active (Rho1^G15V) as well as dominant negative (Rho1^E41I)RHO1 alleles were able to overcome the lrg-1(12-20) dependentgrowth defect initially and generated hyphal tips that are capableof apical extension (Figure 6A). Nevertheless, all growing transformantsdied within 2 d with swollen and lysed hyphae (data not shown).This death phenotype was also observed when we overexpressedthe three RHO1 alleles in wild type and is thus likely the resultof interfering with endogenous RHO1 function (Figure 6B). Adeletion strain of rho-1 was available through the NeurosporaGenome Project (Dunlap et al., 2007). Its heterocaryotic naturealready suggested the essentiality of RHO1. When we plated asexuallyderived conidiospores on hygromcyin-containing media, we detecteda mixture of germinating and isotropically growing spores, indicatingthat RHO1 is essential for establishing polarity (Figure 6C).Similarly, we were unable to obtain viable hygromycin-resistantascospores from wild type x ${Delta}$ rho-1::hph + rho-1⁺ crosses (Figure 6C).The majority of the hyg^R ascospores did germinate apolarly,indicating that RHO1 is required for polarity establishmentin both types spores. Rarely, we observed the formation of hyg^Rcolonies, which then showed a high rate of cell lysis, suggestingthat suppressor mutation can overcome the rho-1 deletion, butcell wall integrity remains affected.

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Figure 6. LRG1 is a RHO1–specific GTPase activating protein. (A) Overexpression of wild type as well as dominant-active (rho-1^G15V) and dominant-negative (rho-1^E41I) rho-1 alleles, but not of any of the other Rho proteins was sufficient to overcome the morphological defect of lrg-1(12-20) at restrictive temperature. Bar, 50 µm. (B) Death phenotypes of wild-type cells transformed with the overexpression constructs of the indicated RHO1 alleles. (C) Conidia (left side) of a heterocaryotic ${Delta}$ rho-1::hph^R + rho-1⁺ strain were germinated on minimal media supplemented with hygromycin. Spores harboring only the deletion nucleus germinated isotropically (red arrows), whereas heterokaryotic cells were able to produce polar germ tubes (blue arrowheads). Bar, 20 µm. Ascospore progeny (right side) of ${Delta}$ rho-1::hph^R + rho-1⁺x wild-type crosses predominatly germinated apolarly on medium supplemented with hygromycin (top image). Bar, 20 µm. Rarely (<1 of 1000 ascospores) we observed growing hyg^R colonies, which then displayed a high rate of cell lysis (bottom image). Bar, 200 µm. (D) Intrinsic and LRG1^650–1035 stimulated GTPase activities of the six Rho proteins. Bacterially expressed and affinity-purified Rho proteins were preloaded with [ ${gamma}$ -32-P]GTP, and the reactions started by the addition of LRG1^650–1035 or buffer. GTPase activities were determined by measuring remaining RHO-bound [ ${gamma}$ -³²P]GTP after 8 min at 25°C (see Materials and Methods). (E) Kinetics of in vitro RHO1 GTPase activity in the presence and absence on LRG1^650–1035.

Next, we performed in vitro GTPase assays with the six bacteriallyexpressed and affinity-purified His6::GST::Rho fusion proteins(Figure 6, D and E). All G-proteins had significant intrinsicGTP-GDP turnover rates, indicating that the purified enzymeswere active. The addition of the GST::GAP domain of LRG1 stimulatedonly the GTPase activity of RHO1 (ca. 10-fold). None of theother GTPases exhibited any significant change in activity.Thus, both the genetic and the in vitro experiments identifyLRG1 as a RHO1–specific GAP.

RHO1 is a bona fide regulatory subunit of the cell wall enzymeβ1,3-glucan synthase in yeasts and filamentous fungi. Furthermore,it is activating the cell wall integrity MAP kinase pathway(Beauvais et al., 2001; Levin, 2005). Therefore, we tested theimpact of defective LRG1 function on these signaling routes.We have recently described conditional mutants in gs-1, a regulatorof β1,3-glucan synthase (Seiler and Plamann, 2003), andwhen we generated a lrg-1(12-20);gs-1(8-6) double mutant, itdid display strong synthetic defects (Figure 7A). Its growthrate at permissive or semirestrictive temperature was reducedby 25 and 41%, respectively, when compared with lrg-1(12-20)as the slower growing of the two parental strains. At restrictiveconditions, gs-1(8-6) generated growth-inhibited hyperbranchedhyphae that were still capable of slow apical growth. In contrast,lrg-1(12-20);gs-1(8-6) formed apolarly growing spheres whengerminated at 37°C. When germinated hyphae were transferredto restrictive conditions, chains of spherical-growing cellswere generated within 8 h. Furthermore, these strains were lesssensitive against caspofungin at semipermissive conditions (Figure 7B),a specific inhibitor of fungal β1,3-glucan synthesis (Denning,2003), indicating hyperactive β1,3-glucan synthase in lrg-1(12-20)and gs-1(8-6). Although the growth rate of lrg-1(12-20) increasedin the presence of caspofungin, hyphal morphology, and branchingfrequency was not different in treated versus untreated cells(Supplementary Figure S1).

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Figure 7. LRG1 is affecting several RHO1-dependent effector pathways. (A) The indicated strains were grown at permissive temperature and shifted to 37°C for 10 h (top) or germinated at restrictive temperature for 15 h (bottom) to illustrate the synthetic nature of the two mutations. Bar, 40 µm. (B) lrg-1(12-20), gs-1(8-6), and lrg-1(12-20);gs-1(8-6) grown at permissive temperature are hyposensitive against the β1,3-glucan synthase inhibitor caspofungin. (C) Growth of the indicated strains for 48 h at 32°C on plates supplemented with the kinase inhibitors staurosporine, KT5720, or cercosporamide. The growth defects of lrg-1(12-20) were suppressed by staurosporine and cercosporamide, but not by KT5720. The growth of wild-type cells was not affected by the mentioned conditions. One example of three consistent experiments is shown. (D) Total soluble protein was extracted from wild type and lrg-1(12-20) shifted to 37°C for the indicated times. The blot was probed with anti-phospho-ERK ( ${alpha}$ -P-ERK) antibody to detect activated MAK1 (top panel) induced by the temperature stress. A replicate was probed with anti-ERK to confirm equal loading (bottom panel). Wild type but not lrg-1(12-20) showed stress-induced MAK1 activation after 20 min at 37°C. (E) MAK1 phosphorylation induced by the addition of 7 mM H₂O₂ for 30 min to wild type and lrg-1(12-20) indicate that the response capacity of the MAK1 pathway is not affected in lrg-1 mutants. One example of five consistent experiments is shown in D and E (originating from individually treated biological cultures and independent protein preparations). (F) lrg-1(12-20) grown at permissive conditions is hypersensitive against the actin-depolymerizing drug latrunculin A.

The abnormal chitin distribution observed in lrg-1(12-20) (Figure 1A)could be a result of increased activity of the N. crassa PKC/MAK1cell integrity pathway and subsequently the altered expressionof additional cell wall enzymes. Therefore, we tested for alteredactivity levels of PKC in the GAP mutant. We observed a partialsuppression of the lrg-1(12-20) growth defect on media supplementedwith 1 µM staurosporine, a protein kinase inhibitor withhighest specificity toward PKC (Figure 7C). Nevertheless, staurosporineis also inhibiting PKA (although with a ca. 10-fold lower affinity).Therefore, we tested the impact of 50 µM KT5720, a PKA-specificinhibitor, on the growth behavior of lrg-1(12-20), but observedno morphological changes (Figure 7C), indicating that PKC ishyperactive in lrg-1(12-20). This was further supported by growthtests on media supplemented with 60 nM cercosporamide, a highlyspecific inhibitor for PKC (Sussman et al., 2004

Next, we tested the activity of the cell integrity MAP kinaseMAK1 by the use of phospho-specific antibodies against activatedERK-type MAPKs. No obvious differences were found in MAK1 phosphorylationpattern in wild-type extracts from cultures grown at 25 and37°C. Stressing these cells by a temperature shift from25 to 37°C for 20 min resulted in activation of cell integritysignaling and increased MAK1 activity (Figure 7D). In contrast,the MAK1 phosphorylation pattern in lrg-1(12-20) shifted torestrictive temperature for 20 min did not result in heat stress-inducedphosphorylation of MAK1, suggesting that MAK1 regulation maybe affected in lrg-1(12-20). However, we did not detect increasedMAK1 activity levels in lrg-1(12-20) after prolonged temperatureshift (Figure 7D) or in ${Delta}$ lrg-1 germinated on benomyl and panthotenicacid (data not shown) as one would predict for increased RHO1–MAK1signaling. To test, whether the capacity of the MAK1 pathwayto respond to stress signals is affected in lrg-1(12-20) ina general manner, wild type and lrg-1(12-20) were grown at 37°Cand stressed by the addition of 7 mM H₂O₂ for 20 min (Figure 7E).Both strains displayed identical activation patterns as detectedby MAK1 phosphorylation, indicating that the response capacityof the MAK1 pathway is not affected in lrg-1(12-20). Taken together,these data indicate that RHO1–PKC signaling is increasedin lrg-1(12-20), but also suggest that the downstream MAK1 MAPkinase pathway is only affected to a minor extent.

Furthermore, we determined that lrg-1(12-20) was hypersensitiveagainst the actin depolymerizing drug latrunculin A, suggestingan altered actin cytoskeleton in the GAP mutant (Figure 7F).In summary, we suggest that LRG1 acts as a general GAP for RHO1and regulates several RHO1-dependent signaling pathways in N.crassa.

Genetic Interactions of lrg-1 with the Ndr Kinase Mutant cot-1 Indicate Two Parallel Pathways for Polar Tip Growth
The morphological defects of lrg-1(12-20) and of ${Delta}$ lrg-1 werestrikingly similar to those of the Ndr kinase mutant cot-1 andits upstream regulating kinase pod-6 (Yarden et al., 1992; Seileret al., 2006). The common defects of these mutants are a blockin apical tip extension and the generation pointed, needle-liketips, the induction of multiple subapical branches, excessiveand mislocalized chitin distribution, and a highly thickenedcell wall. Furthermore, several recessive alleles of cot-1,pod-6, and lrg-1 showed unlinked noncomplementation (Seilerand Plamann, 2003) and suggest LRG1 and COT1/POD6 either ascomponents of two independent pathways that act in parallelto support apical tip growth or hint for a physical interactionof the three proteins. In contrast to a cot-1(1);pod-6(31–21)double mutant, which displayed defects identical to the twoparental strains (Seiler et al., 2006), cot-1(1);lrg-1(12-20)or pod-6(31–21);lrg-1(12-20) double mutants were syntheticallylethal (Figure 8A). Double mutant ascospores germinated at permissiveconditions generated polar germ tubes, but grew in a compactand highly vacuolated manner with very slow tip extension ratesand frequent lysis of hyphal tips or subapical regions. Germinationat 37°C resulted in apolar germination and death of thedouble mutants. In combination with the observation that lrg-1and cot-1/pod-6 share the same suppressors (Figure 5B), thesegenetic data indicate two parallel, COT1/POD6- and LRG1-dependent,pathways for apical tip extension.

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Figure 8. LRG1 acts in a pathway parallel to the Ndr kinase COT1 (A) lrg-1(12-20) and cot-1(1) displayed nearly identical defects with tip extension terminating with 2–10- and 10–30-µm-long pointed tips, respectively, when shifted from permissive to restrictive conditions for 12 h (top panel) or when germinated at 37°C for 15 h (middle panel). Double mutant ascospores germinated at 25°C produced compact, highly vacuolated and slow growing hyphae. Germination at 37°C resulted in apolar germination and death of lrg-1(12-20);cot-1(1) ascospores. (bottom panel). Bars, 40 µm. (B) Double mutants of cot-1(1) and gs-1(8-6) did not display synthetic defects after shift to restrictive temperatures (left image) or when germinated under restrictive conditions (right image). Bar, 40 µm. (C) The growth behavior of cot-1(1) is identical to wild type on medium supplemented with 0.5 µM caspofungin. (D) cot-1(1) is not hypersensitive to the addition of 0.5 µM latrunculin A. (E) Total soluble protein of the indicated strains grown at 25 or shifted to 37°C for 10 h was extracted. The Blot was probed with an anti-phospho-ERK antibody to detect increased MAK1 activity levels in cot-1(1) grown at restrictive conditions (top panel). To confirm equal loading the blot was reprobed with anti-tubulin antibody (bottom panel). One example of five consistent experiments is shown. (F) The PKC-specific inhibitors staurosporine and cercosporamide partially suppressed the tip extension defects of lrg-1(12-20), but not those of cot-1(1). The growth of wild-type cells was not affected by the mentioned conditions. One example of three consistent experiments is shown.

Intrigued by these results, we tested for a potential connectionbetween COT1 and RHO1 signaling and analyzed the RHO1 effectorpathways that are affected by lrg-1. A highly thickened cellwall of cot-1(1) grown at 37°C described in electron microscopicsections (Gorovits et al., 2000

) and the excessive chitin distributionat sites of aberrant growth (Seiler et al., 2006

) already indicateda defect in cell wall organization. However, we did not observeany synthetic interaction in a cot-1(1);gs-1(8-6) double mutant(Figure 8B) and detected growth characteristics of cot-1(1)identical to wild type on media supplemented with caspofungin(Figure 8C), indicating no direct regulation of β1,3 glucansynthase by COT1. Furthermore, in contrast to the hypersensitivityof lrg-1(12-20) to latrunculin A, we did not observe any differenceof cot-1(1) compared with wild type when the strains were grownon media supplemented with 0.5 µM latrunculin A (Figure 8D).However, when we analyzed the activity of the cell wall integritypathway in cot-1(1), we observed increased MAK1 activity levelsin cot-1(1) cultures grown at restrictive temperature (Figure 8E),implying COT1 as a potential negative regulator of the MAK1pathway. Interestingly, the cot-1(1) defect was not suppressedby the PKC inhibitors straurosporine and cercosporamide (Figure 8F),indicating that MAK1 MAP kinase activation is not induced viaRHO1–PKC signaling. Taken together, these results establishdistinct effects of LRG1 and of COT1 on the analyzed RHO1-dependenteffector pathways.

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cellular polarity is a fundamental property of every cell, andfungal hyphae are among the most highly polarized cells knownin nature. In a visual screen designed to identify factors criticalfor hyphal morphogenesis, we isolated lrg-1 as a component thatis essential for apical tip extension and to restrict excessivebranch formation in subapical regions of the hypha (Seiler andPlamann, 2003). The data presented here characterize LRG1 asa RHO1–specific GAP. In vitro, only the GTPase rate ofRHO1 is stimulated significantly by LRG1, and the in vivo resultsindicate several misregulated RHO1 effector pathways in mutantslacking a functional GAP. Interesting, but difficult to explainis that overexpression of wild type and of both dominant rho-1versions is partially compensating the lrg-1 growth defects.Similar results were obtained for mammalian Cdc42 during cellproliferation, where the stable overexpression of the constitutivelyactive G12V mutant did result in a dominant negative phenotypeafter prolonged growth (Vanni et al., 2005). Furthermore, thefact that lrg-1(12-20) cells, which are deficient for Rho-GAPactivity, are defective in polarized growth, suggests that cyclingof RHO1, rather than its GTP-bound form alone is important forits function. Thus, our results indicate that polar tip extensionand the regulation of branch formation may involve cycling ofN. crassa RHO1 to gain full activation, rather than its functioningas simple on/off switch.

Rho1 is a key regulator of hyphal growth and polarity and hasbeen described as integral part of the β1,3-glucan synthasecomplex in yeasts and A. fumigatus (Arellano et al., 1996; Beauvaiset al., 2001; Levin, 2005). The observed caspofungin hyposensitivityand the genetic interaction of lrg-1(12-20) with gs-1(8-6) areconsistent with increased β1,3-glucan synthase activityin lrg-1(12-20) and gs-1(8-6). Furthermore, the latrunculinA sensitivity suggest altered RHO1–actin signaling inlrg-1(12-20). Difficult to interpret are the data presentedfor the PKC/MAK1 pathway. The suppression of lrg-1(12-20) bythe PKC specific inhibitors staurosporine and cercosporamideindicate hyperactivity of PKC in the GAP mutant. Nevertheless,downstream MAK1 activity is not enhanced, suggesting that theMAP kinase cascade is not regulated by LRG1. However, the MAK1activation pattern in heat-stressed lrg-1(12-20) is differentfrom wild type, supporting a regulatory function of the cellintegrity pathway by LRG1. Thus, additional feedback mechanismsmay regulate the activation of the PKC–MAK1 part of thecell integrity pathway in N. crassa.

Which of these RHO1 effector pathways may be responsible forthe block in tip extension and the subapical hyperbranchingobserved in lrg-1? On the basis of data presented here, we donot believe that the altered activities of the PKC–MAK1pathway are the primary defect. Nevertheless, the unregulateddeposition of excessive chitin with in the cell wall of lrg-1may be a result transmitted through PKC. As demonstrated inbudding yeast, cell wall stress can result in up to a 10-foldincrease of the cell wall's chitin content by stress-inducedmobilization of Chs3p from chitosome vesicles to the plasmamembrane. This stress signal is transmitted via Rho1p and Pkc1p,involving components of the cell integrity pathway, but doesnot include the downstream MAP kinase components (Valdivia andSchekman, 2003).

Loss of LRG1 results in increased glucan formation, which mayinterfere with the plasticity of the hyphal cell wall and couldthus lead to the cessation of tip extension and the inductionof branch formation in subapical regions of the hypha. Thishypothesis is supported by a common hyperbranching phenotypeof lrg-1(12–10) and gs-1(8-6) as a result of increasedglucan deposition in the cell walls of both strains as monitoredby the hyposensitivity to the glucan synthase inhibitor caspofungin.Interesting is that the lrg-1(12–10);gs-1(8-6) doublemutant loose cellular polarity when hyphae are shifted to restrictiveconditions and are unable to establish polarity when conidiaare germinated at high temperature. This phenotype is reminiscentto conditional mutants of key regulators of the actin cytoskeletonsuch as bem-1 and cdc-24 (Seiler and Plamann, 2003) and suggestsa tight connection between cell wall function and the actincytoskeleton for apical tip extension and regulation of branchformation. Thus, we speculate that increased GS1 activity andaltered actin organization are the major cause for the observedlrg-1 defects.

A clear homolog of LRG1 is also found in S. cerevisiae (E =1e^–111), but conflicting evidence about the Rho protein(s)and the Rho effector pathway(s) that are regulated by Lrg1pwas reported. In vitro and yeast two hybrid analyses identifiedLrg1p as a GAP for Rho1p, Rho2p, or Cdc42p or for combinationsof these GTPases (Lorberg et al., 2001; Roumanie et al., 2001;Watanabe et al., 2001; Fitch et al., 2004). However, most geneticdata link Lrg1p with Rho1p functions (Lorberg et al., 2001;Watanabe et al., 2001; Fitch et al., 2004; Varelas et al., 2006;Stewart et al., 2007), suggesting that Lrg1p is a Rho1p specificGAP in budding yeast. Furthermore, the effector pathways thatare regulated by Lrg1p are discussed in a controversial manner.Two studies report enhanced MAP kinase activity (Lorberg etal., 2001; Stewart et al., 2007) in contrast to a report describingno effect on the MAP kinase (Watanabe et al., 2001). In addition,increased glucan synthase activity was reported for ${Delta}$ lrg-1 (Lorberget al., 2001; Watanabe et al., 2001; Fitch et al., 2004), butno effect of Lrg1p on the Bni1p/actin branch of Rho1p signalingcould be identified in any of these studies. In contrast, Nakanoet al. (2001) reported delocalized actin patches in a mutantdefective in rga-1, the fission yeast homolog of LRG1.

The domain analysis of LRG1 revealed that both parts of theprotein are essential for its cellular function. Whereas deletionof the GAP domain and point mutations in residues that are requiredfor either the interaction of LRG1 with RHO1 or for the GAPactivity of LRG1 strongly support the importance of the enzymaticfunction of LRG1, several lines of evidence indicate that theN-terminal part of the protein is required for the localizationof the GAP domain to sites of active growth. A construct lackingthe first 780 aa (LRG^781–1279) is not capable of complementingthe mutant defects, but this N-terminal domain (LRG^1–847)is sufficient for correct localization. The morphological defectsobserved in the mutant and the localization pattern of LRG1indicate a function of the GAP at sites of active growth atthe hyphal tip and during septation. This is further supportedby its growth-dependent localization of LRG1 at the hyphal apexand along septae and by the correlation between the growth rateand size of the GFP::LRG1 cap at the hyphal tip. A clear indicationfor the involvement of the three LIM domains within the N-terminusof LRG1 in the localization process is the altered localizationpattern in GFP::LRG1*, in which the three LIM domains have beenmutated. However, despite its localization defect, GFP::LRG1*was capable of rescuing the growth defect of ${Delta}$ lrg-1, indicatingadditional functional motifs within the N-terminus. Interestingin this respect is the high sequence similarity of these domainswith paxillin (E = 1e^–28, whereas other LIM domain proteinsaside from LRG1 homologues have much weaker similarities ofE = 1e^–14), suggesting that LRG1 might act as a cytoskeletalorganizer similar to paxillin in focal adhesion complexes (Schaller,2001; Brown and Turner, 2004). Another possibility could bethe interaction of microtubule-dependent motor proteins withadditional sites within the N-terminus of LRG1. We showed thattreatment of cells with anti-microtubule drugs reduced the apicalLRG1 localization and that motor-driven transport affected thelocalization of LRG1. The reduced retrograde transport of dynein/dynactinmutations resulted in enriched apical localization of LRG1,whereas its abundance is reduced in nkin, which is defectivefor apical-directed transport. Thus we suggest that the opposingtransport rates of NKIN and dynein result in a balanced distributionof LRG1 and thus allow growth that is independent of the functionalityof the LIM domains. The abolishment of both—the microtubule-and LIM domain-dependent—localization mechanisms by deletingthe whole N-terminus is resulting in the loss of function ofLRG1 as observed in LRG1^781–1279 and by the introductionof LRG1* into the ro-1 background. Both conditions resultedcells resembling the lrg-1 loss-of-function phenotype and inan aberrant cortical localization of the GAP. A similar dependencefor correct localization on opposing motor proteins was alsoobserved for cot-1 and pod-6 and suggest a general mechanismto supply all regions of fast growing, highly polar cells withthe necessary components. In contrast to this microtubule-dependentdistribution of LRG1 throughout the hypha, its localizationas an apical cap during active growth is clearly F-actin–dependent,as determined in the latrunculin A inhibitor experiments.

In addition to this motor-dependent localization of LRG1 andCOT1/POD6, mutants defective in the two kinases of the Ndr signalingnetwork and in lrg-1 displayed nearly identical phenotypes.The major difference of the kinase mutants versus lrg-1 is thereduced length of the subapical branches that are induced bythe temperature shift in lrg-1. Our double mutant analysis,nonalleleic noncomplementing alleles and common suppressorsprovide strong evidence that the COT1/POD6 complex is actingin parallel to LRG1/RHO1 signaling. Genetic data in S. cerevisiaesuggest that the COT1 homolog Cbk1p may negatively regulatethe small GTPase Rho1p, although the mechanism of interactionremained open (Jorgensen et al., 2002; Schneper et al., 2004).A similar negative effect of COT1 on RHO1 signaling in N. crassawould explain the observed synthetic lethality of the lrg-1(12-20);cot-1(1)double mutant. However, loss of COT1 function did not affectGS1 activity or the actin cytoskeleton, and the only RHO1 effectorpathway that is altered in cot-1(1) is the MAK1 MAP kinase pathway(but not the upstream acting PKC). Thus, the molecular basisfor the observed genetic interactions remains open. Interestingin this context is that a physical interaction between the Ndrkinase ORB6 and a different Rho-GAP has been proposed to existin fission yeast based on two hybrid studies (Das et al., 2007).An indication that the connection between Rho GTPases and Ndrsignaling is conserved between fungi and animals has been providedby studies in D. melanogaster and Caenorhabditis elegans (Zallenet al., 2000; Emoto et al., 2004). Thus, the genetic connectionestablished, but also the distinctions between COT1/POD6 andLRG1/RHO1 signaling during hyphal growth, and the similaritiesof LRG1 to the focal adhesion organizer paxillin may provideinsights in the regulation of morphogenesis in other highlypolar cells such as neurons.

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Figure 9. Model summarizing components and potential connections between the LRG1/RHO1 and COT1/POD6 pathways in the regulation of hyphal tip extension in N. crassa. Details are discussed in the text.

ACKNOWLEDGMENTS

The authors acknowledge the help of Inga von Behrens and SeemaSingh in the initial phase of this work and thank Angela Hoffman(University of Portland, Portland, OR) for a gift of cercosporamide.Caspofungin was kindly provided by MSD Sharp & Dohme, GMBH.This research project was financially supported by the DeutscheForschungsgemeinschaft through the DFG Schwerpunkt Zellpolarität(SPP1111) and the DFG Research Center of Molecular Physiologyof the Brain (CMPB).

Footnotes

This was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E07-12-1266)on August 20, 2008.

Address correspondence to: Stephan Seiler (sseiler{at}gwdg.de)

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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