Multiple Functions for Actin during Filamentous Growth of Saccharomyces cerevisiae

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Vol. 9, Issue 7, 1873-1889, July 1998

Multiple Functions for Actin during Filamentous Growth of Saccharomyces cerevisiae

Brian M. Cali,^* Timothy C. Doyle, David Botstein, and Gerald R. Fink^*^§

^*Whitehead Institute for Biomedical Research and ^§Department of Biology, Massachusetts Institute of Technology, Cambridge, Massachusetts 02142; and Department of Genetics, Stanford University Medical Center, Stanford, California 94305

Submitted January 16, 1998; Accepted March 13, 1998
Monitoring Editor: David Drubin

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Saccharomyces cerevisiae is dimorphic and switches from a yeast form to a pseudohyphal (PH) form when starved for nitrogen.PH cells are elongated, bud in a unipolar manner, and invade theagar substrate. We assessed the requirements for actin in mediatingthe dramatic morphogenetic events that accompany the transitionto PH growth. Twelve "alanine scan" alleles of the single yeastactin gene (ACT1) were tested for effects on filamentation, unipolarbudding, agar invasion, and cell elongation. Some act1 mutationsaffect all phenotypes, whereas others affect only one or two aspectsof PH growth. Tests of intragenic complementation among specificact1 mutations support the phenotypic evidence for multiple actinfunctions in filamentous growth. We present evidence that interactionbetween actin and the actin-binding protein fimbrin is importantfor PH growth and suggest that association of different actin-bindingproteins with actin mediates the multiple functions of actin infilamentous growth. Furthermore, characterization of cytoskeletalstructure in wild type and act1/act1 mutants indicates that PHcell morphogenesis requires the maintenance of a highly polarizedactin cytoskeleton. Collectively, this work demonstrates thatactin plays a central role in fungal dimorphism.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Genetic and biochemical studies in the budding yeast Saccharomyces cerevisiae have provided important insights into the cellularfunctions of actin and actin-binding proteins. More than 80 sequencedmutations affecting the single yeast actin gene (ACT1) have beenidentified (Ayscough and Drubin, 1996). Collectively, these mutationsaffect many aspects of cell growth, including secretion (Novickand Botstein, 1985), endocytosis (Riezman et al., 1996), bipolarbud site selection (Yang et al., 1997), and organellar trafficking(Drubin et al., 1993; Simon et al., 1995). Numerous yeast actin-bindingproteins have also been identified using genetic, biochemical,and two-hybrid approaches. Mutations in genes encoding many suchproteins perturb actin cytoskeletal structure and/or function(for examples and reviews, see Drubin et al., 1988, 1990; Adamsand Botstein, 1989; Adams et al., 1989; Liu and Bretscher, 1989;Amatruda et al., 1990; Welch et al., 1994; Amberg et al., 1995,1997; Brower et al., 1995; Ayscough and Drubin, 1996; Riezmanet al., 1996; Botstein et al., 1997).

Most observations regarding the yeast actin cytoskeleton have been made on yeast form (YF)¹ cells grown in the presence of ample nutrients. Under these conditions,diploid S. cerevisiae grow by budding to produce oval-shaped daughtersthat separate from the mother cell at cytokinesis and remain onthe surface of the agar substrate. However, S. cerevisiae is dimorphic.When starved for nitrogen in the presence of a fermentable carbonsource, S. cerevisiae switches to a pseudohyphal (PH), or filamentous,mode of growth (Gimeno et al., 1992). PH cells are much longerand thinner than YF cells, remain attached to mothers after cytokinesis,and invade the agar substrate. These growth characteristics, coupledwith a unipolar budding pattern, with daughters predominantlybudding away from mothers, lead to growth of filaments of longcells away from the body of the colony.

Differences in the polarity of the actin cytoskeleton between YF and PH cells suggest a specialized role for the actin cytoskeletonin PH growth. The yeast actin cytoskeleton comprises two majorstructures, patches and cables. Actin patches are punctate "dots"of filamentous actin present at the cell cortex, whereas cablesare oriented along the mother-bud axis and have been describedas cytoplasmic (Adams and Pringle, 1984). Patches are highly mobile(Doyle and Botstein, 1996; Waddle et al., 1996) and are localizedto areas of new cell growth throughout the cell cycle. In PH cells,actin patches are polarized to the distal tip of the daughtercell throughout bud growth and then repolarize to the site ofseptation shortly before cytokinesis (Kron et al., 1994). Thisbehavior contrasts with that of patches in YF cells, where thereis a distinct period between bud emergence and cytokinesis whenpatches are distributed around the entire cortex of the emergingbud (the isotropic growth phase) (Lew and Reed, 1993). These differencesindicate that actin cytoskeletal structure and dynamics are regulateddifferently in YF and PH cells.

Genetic analysis also indicates that the actin cytoskeleton has an important function in PH growth. In a general screen formutants defective for filamentation, Mösch and Fink (1997) identifiedmutations in several genes encoding cytoskeletal proteins. Theseinclude the genes encoding the actin-binding proteins Tpm1p (tropomyosin),Srv2p (cyclase-associated protein), and the formin homology domainprotein Bni1p. Deletion of SLA2, which encodes a protein withhomology to the focal adhesion protein talin, was also shown toblock filamentation (Yang et al., 1997).

Here we have investigated the functional requirements for actin in mediating the dramatic changes in agar invasion, bud siteselection pattern, and cell shape that accompany the transitionfrom growth in the YF to PH growth. This work indicates that actinhas multiple functions in filamentous growth and provides newinsight into actin structure-function relationships. In addition,image analysis of wild type and act1/act1 mutants suggests animportant role for cortical actin patch polarization in the morphogenesisof the PH cell.

	MATERIALS AND METHODS

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Yeast Strains, Plasmids, and Microbiological Methods

Yeast strains used in this study are isogenic and derived from the $Sigma$ 1278b strain background (Table 1). Standard media andmethods of sporulation, tetrad dissection, and scoring of matingtype were as previously described (Guthrie and Fink, 1991). Syntheticlow-ammonia dextrose (SLAD) medium has also been described (Gimenoet al., 1992). Plasmids used in this study have been previouslydescribed: pIL30 (Laloux et al., 1994), pRS314 and pRS316 (Sikorskiand Hieter, 1989), and AAB117 and AAB289 (Brower et al., 1995).Transformation was performed by the lithium acetate transformationmethod (Ito et al., 1983; Gietz et al., 1992).

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Table 1. Yeast strains

Genetic Manipulations and Strain Constructions

Actin mutant strains were constructed by single-step gene replacement using donor DNA fragments containing the desired act1allele with HIS3 integrated just downstream of the act1 codingsequence (act1-x::HIS3) and an act1 $Delta$ ::LEU2/ACT1 heterozygous diploidas recipient. To generate the act1 $Delta$ ::LEU2/ACT1 heterozygote foreventual gene replacement, an ACT1 disruption construct was madeby first subcloning the 3.8-kb EcoRI fragment containing ACT1from pKFW29 (Wertman et al., 1992) into the EcoRI site of pUC19to generate BCB109. BCB109 was digested with BclI and XhoI andligated in the presence of an XhoI-BglII fragment from YEp13 thatcontains LEU2. The resultant act1 $Delta$ ::LEU2 construct in pUC19 (BCB207)deletes all but the first three amino acids of the ACT1 codingregion and contains 1246 bp upstream and 1118 bp downstream ofACT1. BCY116 was transformed with the ApaI-SmaI fragment of BCB207,and Leu⁺ transformants were identified. Genomic DNA from 27 Leu⁺ transformants was tested by PCR for linkage of a LEU2-specificoligonucleotide (LEU2-P3: 5'-GATTTCTTGACCAACGTGGTC) with an oligonucleotide(ACT1-8: 5'-TTCAAACTGCTGTTGATCGG) specific to a genomic regionjust outside that contained in BCB207 and oriented toward LEU2-P3.Twelve transformants gave the 2.0-kb product expected for a disruptant.Three of these putative heterozygotes segregated two viable Leu:2 lethal spores, confirming heterozygosity for act1 $Delta$ ::LEU2. Onesuch heterozygote was kept as BCY144.

To introduce the act1 alleles by gene replacement, BCY144 was transformed independently with each of the EcoRI-digested plasmidderivatives of pKFW46 carrying the relevant act1 alleles withHIS3 integrated downstream (Wertman et al., 1992). His⁺ transformants were selected and screened for those that wereLeu. Two independent His⁺ Leu transformants were retained as candidate act1-x::HIS3/ACT1 heterozygotes,where x represents any given act1 allele. As HIS3 is tightly linkedto each of these alleles, they can be followed in crosses by monitoringhistidine prototrophy. Heterozygotes for each of the alleles weresporulated, and the tetrads were dissected. Nine alleles wereviable as haploids at 30°C. Strains heterozygous for three ofthe alleles (act1-109, act1-110, and act1-131) segregated twoviable His:2 lethal spores, indicating that these act1 alleles are recessivelethal in $Sigma$ 1278b, as they are in S288c (Wertman et al., 1992).Presence of the desired act1 mutation was confirmed by restrictionanalysis of an act1 PCR product amplified from the genome. Thisassignment was possible because each of the act1 alleles analyzedin this study creates or destroys a restriction site in ACT1 (Wertmanet al., 1992). To confirm the presence of the act1 mutation ineach of these strains, act1 was amplified by PCR with Taq polymeraseusing oligonucleotides act1-4 (5'-CTTTTCCTTAAAAATACTTTATTA) andACT1-10 (5'-GTACTAACATCGATTGCTTC) under standard conditions. Theexpected 1275-bp product was digested with enzymes diagnosticfor each mutation as previously described (Wertman et al., 1992).Restriction fragments of the size expected for the appropriateallele were seen in all cases. For all viable alleles, act1 wasamplified from two independent His⁺ haploids segregated from the original heterozygous diploids.For the recessive lethal alleles act1-109, act1-110, and act1-131,the ACT1 alleles were amplified from the heterozygous diploid,and both wild-type and mutant restriction patterns were observed.

act1/act1 homozygotes were constructed by first transforming act1-x::HIS3/ACT1 heterozygous diploids to Leu⁺ with the LEU2 CEN plasmid pIL30 (Laloux et al., 1994). Sporulation,dissection, and mating of appropriate haploids were then usedto generate prototrophic diploids homozygous for each of the viableact1 alleles (Table 1). For analysis of the recessive lethalalleles, the original act1-x::HIS3/ACT1 heterozygotes were transformedto Leu⁺ with pIL30 and used for subsequent analysis.

To generate a sac6 $Delta$ ::LEU2/sac6 $Delta$ ::LEU2 diploid, a 2.9-kb genomic fragment carrying the sac6 $Delta$ ::LEU2 allele of AAY1047 (Adamset al., 1995) was generated by PCR with oligonucleotides SAC6-1(5'-GCAGTTAAAGGTGCTTTGTC) and SAC6-2 (5'-AAAGTTCACAGGATATATGG)and used to transform BCY333 to Leu⁺. Candidate sac6 $Delta$ ::LEU2/SAC6 heterozygotes were tested by PCRto identify linkage of oligonucleotides LEU2-P3 and SAC6-3 (5'-GCTCAAGGACGCCCCATTTG);one transformant that gave the appropriate product was sporulatedand dissected; sac6 $Delta$ ::LEU2 was confirmed to segregate 2:2. Matingof appropriate haploids from this dissection and subsequent transformationwith pRS316 generated the sac6 $Delta$ ::LEU2/sac6 $Delta$ ::LEU2 homozygote BCY372.

Assessment of Filamentation, Cell Elongation, and Invasion Phenotypes

Strains to be analyzed were streaked for well-isolated single colonies on SLAD plates, with no more than four strains perplate. Plates were incubated for 4 d at 30°C, and well-isolatedcolonies were scored for filamentation. Strains with no filamentsextending beyond the perimeter of the colony were scored as ( $-$ )for filamentation; those with 1-10% of colonies showing some filamentswere scored as (+). (++) indicates that 80-100% of colonies hadfilaments, yet these filaments were disorganized relative to wildtype. (+++) = wild-type filamentation.

Cell elongation was quantified by growing colonies as above, scraping cells from the agar with a toothpick into 10 µl of water,and scoring morphology on a hemacytometer. Cells with length/widthratios $>=$ 2 were scored as long cells.

To score invasion, the same plates used to score filamentation and cell elongation were washed with a stream of water. Noninvasivecells were removed by gently rubbing the agar surface. Those strainswith <10% of washed colonies having residual cells in the agar,and only in the center of the colony, were scored as ( $-$ ). (+)denotes strains with 10-50% of washed colonies having residualcells. Typically, only cells in the center of the colony had invadedin this class. Mutants that showed 50-100% of colonies with invadedcells were scored either as (++) or (+++) depending on whetherpart (++) or all (+++) of the colony diameter contained invadedcells.

Preparation of PH Cells for Rhodamine-Phalloidin and Calcoflour Staining

Strains to be assayed were grown overnight at 30°C in 5 ml of YNB. Cells were washed once in 5 ml of water, spread on thesurface of a 10.5-cm SLAD plate, and incubated 24-48 h at 30°C.For rhodamine-phalloidin staining studies, prestarved cells werecollected in water and serially diluted in 1.25% alginate (wt/vol)(Sigma, St. Louis, MO; catalog number A-2158) in water. Suspensionsof cells (0.5 ml) were spread thinly over the surface of a SLADagar plate, alginate was allowed to solidify, and plates wereincubated 48 h at 30°C. For fixation, alginate was removed withforceps from plates with well-separated single colonies and placedin 6 ml of 0.8 M EGTA/3.7% formaldehyde in a 15-ml polypropylenetube (chelation of calcium by EGTA causes alginate to liquefy).After 1 h with intermittent shaking, cells were washed three timesin 1× PBS. Rhodamine-phalloidin staining was performed as describedpreviously (Kron et al., 1994). For calcoflour staining, prestarvedcells were grown in SLAD liquid overlay media, fixed, and stainedas previously described (Kron et al., 1994).

Microscopic Methods

Cells fixed and stained as above were mounted in 90% glycerol/1× PBS and viewed using epiflourescence on a Nikon (Garden City,NY) E6 inverted microscope, controlled by the Applied Precision(Issaquah, WA) DeltaVision wide-field microscope system. Fluorescentimages were obtained at 100× magnification (numerical aperture,1.4) and captured with a Princeton Instruments (Trenton, NJ) cooledcharged-couple device camera. Stacks of rhodamine and DAPI fluorescenceimages were captured at 0.2-µm intervals in the z-plane (1- to3-s image capture time), and out-of-focus fluorescence was removedby iterative deconvolution (Agard et al., 1989; Scalettar et al.,1996). Three-dimensional representations of these two-dimensionalstacks were then generated, and rotated views through the stackwere obtained and used to generate stereo images.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

To determine the functional requirements for actin during PH growth, we have taken advantage of an extant set of "charged-to-alaninescan" alleles of ACT1 (Wertman et al., 1992). These mutationsprovide a number of distinct advantages for dissecting the rolesof actin in PH growth. First, the residues affected by these mutationsare known and can be mapped to the crystal structure of actin.Collectively these mutations affect a large portion of the solvent-exposedsurface of the actin monomer. Second, the effects of these mutationson a number of actin-dependent processes have been well documented(for examples, see Read et al., 1992; Drubin et al., 1993; Smithet al., 1995). Third, the effects of these alanine scan alleleson the binding of many actin-interacting proteins have been determined(Holtzman et al., 1994; Honts et al., 1994; Amberg et al., 1995,1997). This detailed information on the functions affected bythese alleles provides an invaluable guide in assessing the possibleroles of actin and actin-binding proteins in PH growth.

Actin Mutants Exhibit Filamentation Defects

Twelve alanine scan act1 alleles were introduced into a strain (a $Sigma$ 1278b derivative) capable of PH growth (Gimeno et al.,1992) (see MATERIALS AND METHODS for details). These constructionswere necessary because the act1 alleles were originally studiedin S288c (Wertman et al., 1992), a background that does not exhibitPH growth (Liu et al., 1996). Nine of these alleles are viableas haploids at 30°C, whereas three alleles (act1-109, act1-110,and act1-131) are recessive lethal in $Sigma$ 1278b, as they are in S288c(Wertman et al., 1992).

As haploids do not make florid pseudohyphae (Gimeno, et al., 1992; Mösch and Fink, 1997), diploids homozygous for each ofthe viable alleles were constructed. Growth of all act1/ACT1 heterozygotesand viable act1/act1 homozygotes was assessed on YPD agar platesat 30 and 36°C to determine the recessive and dominant effectsof these mutations on YF growth and viability in the $Sigma$ 1278b strainbackground (Table 2). Strains homozygous for seven of the ninerecessive viable alleles (act1-111, act1-112, act1-113, act1-120,act1-124, act1-129, and act1-132) exhibit temperature-sensitivegrowth; only two of these alleles (act1-111 and act1-132) causeslow growth at 30°C. Diploids homozygous for the recessive viablealleles act1-104 and act1-117 grow as well as wild type at both30 and 36°C. All alleles show the same general trends of temperaturesensitivity and dominance as previously reported for these mutationsin S288c with the exception of act1-112, which has a dominanteffect on growth in $Sigma$ 1278b but was reported to be recessive inS288c (Wertman et al., 1992).

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Table 2. Summary of growth phenotypes of actin mutants on YPD

To determine the effects of actin mutations on PH growth, strains homozygous for the recessive viable act1 alleles and strainsheterozygous for act1 $Delta$ ::LEU2 or the recessive lethal act1 alleleswere streaked to SLAD media to induce PH growth, and the morphologyof the resulting colonies was examined after 4 d growth at 30°C(Figure 1, unwashed colonies). Of the nine viable alleles analyzed,all but act1-113 cause filamentation defects when homozygous.The severity of the filamentation phenotype is allele specific.For example, act1-112/act1-112 mutants make no filaments, whereasact1-117/act1-117 strains make many clumpy and disorganized filaments.Each of the recessive lethal alleles (act1-109, act1-110, andact1-131) has a dominant effect on PH growth, with act1-131 showingthe most severe phenotype. A decrease in actin dosage also hasa dominant effect on PH growth, as the act1 $Delta$ ::LEU2/ACT1 heterozygoteshows reduced filamentation. However, the phenotype of the act1 $Delta$ ::LEU2/ACT1 heterozygote is less severe than that of strains heterozygousfor act1-109, act1-110, and act1-131.

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Figure 1. Filamentation and invasion phenotypes of actin mutants. Strains of indicated genotype were streaked for single colonies on SLAD agar and incubated for 4 d at 30°C. Complete genotypes of strains are listed in Table 1. Colonies were photographed before (unwashed column) and after (washed column) washing the surface of the agar to remove noninvaded cells. Bar, 500 µm.

Allele-specific Effects of Actin Mutations on Invasion, Cell Elongation, and Unipolar Bud Site Selection

The actin alleles were tested for their effects on other features of filamentous growth: 1) invasion $---$ PH cells can invade theagar substrate, whereas YF cells do not; 2) cell elongation $---$ PHcells are much longer and thinner than their YF counterparts;and 3) unipolar bud site selection $---$ PH daughters tend to bud primarilyfrom the pole opposite the birth end of the mother (the distalend). In contrast, YF diploids bud in a bipolar manner $---$ the firstand second daughters tend to bud from the distal end of the mothercell, and subsequent daughters bud with equal likelihood fromeither the proximal or distal poles. The subsequent section describesthe analysis, the results of which are summarized in Table 3.

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Table 3. Summary of effects of actin mutations on filamentous growth-specific properties.

Agar Invasion. Colonies grown on SLAD plates were compared before and after washing (Figure 1). Five alleles (act1-104, act1-109, act1-110,act1-113, and act1-117) have little or no effect on agar invasion.However, the remaining seven alleles show defects ranging froma slight reduction to virtually complete elimination of agar invasion.For example, act1-129/act1-129 homozygotes invade slightly lesswell than ACT1 strains, whereas act1-112/act1-112 homozygotesshow an extreme invasion defect.

Cell Elongation. The percentage of long cells made under conditions that induce PH growth was determined for both the wild type and mutantstrains harboring actin alanine scan alleles shown in Figure 1.The different alleles have distinct effects on elongation. Mostmutants make from 30 to 80% of wild-type numbers of long cells,but act1-112/act1-112 and act1-120/act1-120 strains make virtuallyno long cells (Figure 2A).

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Figure 2. Effect of act1 mutations on cell elongation. (A) Percentage of long cells in each of the actin mutants. Complete genotypes of strains are as indicated in Figure 1. Long cell counts were performed as described in MATERIALS AND METHODS. Bars show the SE of two independent experiments. (B) Examples of different cell elongation phenotypes. Images shown are differential interference contrast images of cells scraped from the agar as above. Bar, 10 µm.

Interestingly, the effect of a given mutation on cell elongation does not correlate with its effect on invasion. For example,both act1-111 and act1-112 block invasion (Figure 1), but act1-111/act1-111strains make substantial numbers of long cells, whereas act1-112/act1-112homozygotes do not (Figure 2, A and B). Thus, cell elongationand invasion appear to require different functions of actin thatare differentially affected by certain mutations.

Unipolar Budding Many mutations affecting actin (as well as mutations affecting other cytoskeletal proteins) cause random budding in YF diploidsbut have no effect on axial budding in haploids (Drubin et al.,1993; Sivadon et al., 1995; Haarer et al., 1996; Zahner et al.,1996; Yang et al., 1997). We examined whether this subset of actinmutations affects the unipolar budding pattern that diploids exhibitduring PH growth. The budding patterns of 10 of the 12 act1/act1mutants grown under PH growth-inducing conditions were assessed(act1-111/act1-111 and act1-132/act1-132 homozygotes could notbe scored because they exhibit abnormal chitin deposition andhigh background staining with calcoflour). Seven alleles causerandom budding under conditions that induce PH growth, whereasthree (act1-104, act1-113, and act1-117) do not (Table 3).

act1-113 and act1-117 are distinct because their effect on budding pattern is determined by nutritional conditions. act1-113/act1-113and act1-117/act1-117 YF diploids were shown to bud in a randompattern in the S288c strain background (Yang et al., 1997

). Thesame alleles do not cause random budding in the $Sigma$ 1278b strainbackground under conditions that induce PH growth. Quantitativeanalysis of bud site selection patterns of ACT1/ACT1, act1-113/act1-113,and act1-117/act1-117 strains grown under PH growth-inducing andnoninducing conditions shows that this difference reflects aneffect of growth condition, not strain background (Table 4).Whengrown in rich medium, act1-113/act1-113 and act1-117/act1-117diploids in the $Sigma$ 1278b strain background show a random buddingpattern similar to that seen for these alleles in S288c (Yanget al., 1997

). However, when grown under conditions that inducePH growth, act1-117/act1-117 diploids exhibit a budding patternthat most closely resembles the bipolar budding pattern of wild-typeYF cells. act1-113/act1-113 diploids bud in a unipolar mannersimilar to that of wild-type PH cells under such conditions.

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Table 4. Effect of growth condition on bud-site selection in ACT1/ACT1, act1-113/act1-113 and act1-117/act1-117 diploids

Intragenic Complementation between act1 Alleles

Different act1 alleles with similar PH phenotypes might disrupt filamentation by affecting either the same or different aspectsof actin function. If two mutations affect different functionsrequired for PH growth, then they might complement each otherfor filamentations defects. Mutations affecting the same functionswould not. To distinguish these possibilities, all heteroalleliccombinations of the nine viable act1 alleles were constructedand tested for ability to complement each other for filamentationdefects. The filamentation phenotypes of each of these strainswere compared with those of strains homozygous and heterozygousfor each allele (Table 5).

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Table 5. Filamentation phenotypes of act1 allelic combinations

Both positive and negative interactions were observed in our complementation analysis. act1-120, which completely eliminatesall aspects of PH growth as a homozygote, is able to complementthe filamentation defects of five other act1 alleles (act1-104,act1-111, act1-117, act1-124, and act1-129). An example of thiseffect is shown in Figure 3. Although both act1-111/act1-111 andact1-120/act1-120 homozygotes fail to make filaments, act1-111/act1-120heterozygotes exhibit filamentation indistinguishable from thatof wild type. One striking negative interaction was also observed.As shown in Figure 4, act1-111/act1-112 strains grow much morepoorly at 30°C than either act1-111/act1-111 or act1-112/act1-112homozygotes.

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Figure 3. act1-111 and act1-120 exhibit intragenic complementation for filamentation defects. Shown is the growth on SLAD agar after four days at 30°C. (A) BCY209 (ACT1/ACT1); (B) BCY204 (act1-111/act1-111); (C) BCY210 (act1-120/act1-120); (D) BCY310 (act1-111/act1-120). Bar, 500 µm.

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Figure 4. act1-111 and act1-112 exhibit a negative growth interaction. Shown are colonies after growth for 3 d at 30°C on YNB. (A) BCY209 (ACT1/ACT1); (B) BCY204 (act1-111/act1-111); (C) BCY202 (act1-112/act1-112); (D) BCY302 (act1-111/act1-112). Bar, 1 mm.

Dominant Effects on PH Growth

The complementation analysis also revealed that some act1 alleles that are recessive with regard to YF growth and viability(Table 2) have dominant effects on PH growth (Table 5). Fouralleles that reduce filamentation as homozygotes (act1-112, act1-124,act1-129, and act1-132) also reduce filamentation in act1/ACT1heterozygotes, whereas another set (act1-104, act1-111, act1-117,and act1-120) are completely recessive. We considered the possibilitythat the dominance of these alleles is due to a reduction in actindosage, as act1 $Delta$ /ACT1 heterozygotes show a reduction in filamentation(Figure 1 and Table 5). However, strains heterozygous for act1-112,act1-129, and act1-132 show stronger filamentation defects thanthe act1 $Delta$ /ACT1 control (Table 5). This result shows that thephenotype of these heterozygotes is due to a dominant effect ofthe mutant actin encoded by these alleles, rather than a simplereduction in actin levels.

The Role of the Fimbrin-Actin Interaction in PH Growth

Although act1-120/act1-120 homozygotes are defective for all aspects of PH growth investigated, this allele complements thePH growth defects of many other actin mutants (Table 5). Thus,act1-120 appears to encode a mutant actin that retains substantialfunction. Genetic and biochemical studies in yeast have establishedthat act1-120 perturbs binding of the actin filament-bundlingprotein fimbrin (Sac6p) both in vitro and in vivo (Holtzman etal., 1994; Honts et al., 1994, Sandrock et al., 1997, Doyle andBotstein, unpublished observations). This is consistent with structuraldata showing that the residues affected by act1-120 (E99 and E100)are in a region of subdomain 1 of actin that forms extensive contactswith the amino-terminal domain of fimbrin (Hanein et al., 1997).Specific mutations affecting either of the two actin-binding domainsof fimbrin can suppress the temperature-sensitive lethal phenotypeof act1-120 (Brower et al., 1995; Sandrock et al., 1997).

We propose that the major effect of act1-120 on PH growth is through its effect on fimbrin binding. This model can be directlytested by evaluating two important predictions: 1) sac6/sac6 andact1-120/act1-120 mutants will show similar PH growth defects;and 2) sac6 alleles that restore the interaction between fimbrinand the mutant actin encoded by act1-120 will suppress some orall of the PH growth defects of act1-120/act1-120 mutants. Bothof these predictions are borne out. As shown in Figure 5, sac6 $Delta$ ::LEU2/sac6 $Delta$ ::LEU2 diploids, like act1-120/act1-120 mutants, make nofilaments, are invasion defective, and are severely reduced forcell elongation at 30°C. Expression of a mutant fimbrin encodedby sac6-10 rescues both the cell elongation and invasion phenotypesof these mutants. sac6-10 alters a conserved tryptophan in thefirst actin binding domain of fimbrin (W252C) and was shown tosuppress the temperature-sensitive phenotype of act1-120, presumablyby restoring the fimbrin-actin interaction (Brower et al., 1995;Sandrock et al., 1997). Importantly, sac6-10 does not suppressthe PH growth defects of two actin mutations (act1-111 and act1-124)that affect residues in subdomains 4 and 2, respectively, andare not predicted to interfere with fimbrin binding to actin.These data indicate that the invasion and cell elongation phenotypesof act1-120/act1-120 mutants are due primarily to a defect infimbrin binding.

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Figure 5. Expression of a mutant fimbrin (Sac6p) with an altered actin-binding domain suppresses the invasion and cell elongation defects of an act1-120/act1-120 diploid. Strains BCY209 (ACT1/ACT1), BCY210 (act1-120/act1-120), BCY372 (sac6/sac6), BCY412 (act1-120/act1-120 $<$ SAC6+ $>$ ), BCY411 (act1-120/act1-120 $<$ sac6-10 $>$ ), BCY432 (act1-111/act1-111 $<$ sac6-10 $>$ ), and BCY433 (act1-124/act1-124 $<$ sac6-10 $>$ ), where genotypes in angle brackets refer to relevant genotypes of plasmids AAB117 (SAC6 URA3 CEN) and AAB289 (sac6-10 URA3 CEN) (Brower et al., 1995

), were streaked to SLAD agar and incubated at 30°C for 4 d. The resultant colonies were photographed before and after washing the agar surface. Long cells were quantified as described in MATERIALS AND METHODS and are reported with SE. Bar, 500 µm.

Characterization of the Actin Cytoskeleton in PH Cells in Wild Type and act1 Mutants

As a basis for understanding the similarities and differences in the YF and PH actin cytoskeletons and how this may accountfor the differences in cell shape and other growth propertiesin these distinct cell types, the actin cytoskeleton was imagedin both YF and PH cells at various stages of the cell cycle (Figure6). The major structural features of the PH and YF actin cytoskeletonsare similar in that a prominent ring of filamentous actin is seenat the site of bud emergence, cortical patches are found almostexclusively in the emerging bud, and cables are oriented towardthe site of bud emergence in both mother and daughter cells. However,there are notable differences in cytoskeletal structure betweenthese cell types that bear mention. As observed previously (Kronet al., 1994), we find that the polarity of patch localizationis enhanced in PH cells relative to YF cells, as patches tendto remain at the distal pole throughout bud emergence in PH cellsuntil a new ring of filamentous actin is formed at the eventualsite of cytokinesis. In addition, actin cables are more pronouncedin PH cells than in YF cells.

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Figure 6. Comparison of the YF and PH actin cytoskeletons. Stereo images of the filamentous actin cytoskeleton (stained with rhodamine-phalloidin) in strain BCY209 grown either in YPD (A) or in SLAD alginate (B-D). (A) YF cells: all stages of cell cycle. (B) PH cell, early bud emergence; note prominent ring of actin in mother cell at site of bud emergence and at the neck of the very small emerging bud. (C) PH cell, midbud emergence; image shows the pronounced actin cables and patch polarization to the distal end of the emerging bud. (D) PH cell shortly before cytokinesis; a ring of actin has formed at the septation site between mother and daughter, whereas some patches remain near the distal end of the daughter cell. Bar, 10 µm.

As was recently shown for YF cells in the S288c background (Botstein et al., 1997), we find that actin cables are corticalin both YF and PH cells in the $Sigma$ 1278b genetic background. Cablesappear to run just under the plane in which patches reside andto follow the overall contour of the cell. Thus, it appears generallytrue that actin cables do not run directly through the cytoplasmas has long been thought. It seems likely that the cortical natureof actin cables was not noticed previously because the generationand manipulation of high resolution stereo images of the yeastactin cytoskeleton has only recently become possible.

Actin patch dynamics were also examined in wild-type PH cells using a previously described GFP-SAC6 fusion (Doyle and Botstein,1996). Expression of this fusion protein rescues all PH growthdefects associated with deletion of SAC6, providing additionalevidence to that previously presented that this fusion proteinis fully functional (Doyle and Botstein, 1996). Analysis of actinpatch dynamics showed that actin patches are mobile in PH cells,as they are in YF cells (Doyle and Botstein, 1996; Waddle et al.,1996). Patch dynamics did not appear to differ significantly betweenYF and PH cells.

Rhodamine-phalloidin staining of all act1/act1 mutants (with the exception of act1-129, which encodes an actin that does notbind phalloidin; Drubin et al., 1993) grown under PH growth-inducingconditions revealed numerous defects in actin cytoskeletal structure.Cytoskeletal structure in a sample of mutants is shown in Figure7. (Rotations of these mutants and of the wild-type PH cells inFigure 6 further illustrate many of the features of the actincytoskeleton discussed here and are available on the internetversion of this manuscript.) In all mutants with effects on PHgrowth, actin cables are either absent or thin and disorganized.Perturbation of actin patch polarization and morphology was alsoobserved, with the most pronounced effects in those mutants displayingthe most severe cell elongation defects. For example, in act1-120/act1-120homozygotes and act1-131/ACT1 heterozygotes, which both show strongdefects in cell elongation (Figure 2), actin patches are depolarizedand located in both mother and daughter cells. act1-112/act1-112homozygotes, which are also severely affected in cell elongation,show defects in patch polarization, an overall reduction in patchnumber and staining intensity, and a large proportion of cellswith thick or clumpy patches (Figure 7). Multibudded and multinucleatecells were also apparent in many mutants under PH growth-inducingconditions (e.g., -act1-120/act1-120 and act1-112/act1-112 inFigure 7). The abnormal patch structures and nuclear segregationand budding defects we observed under these conditions closelyresemble those previously described for these and other act1 mutantsin YF cells (Drubin et al., 1993).

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Figure 7. The actin cytoskeleton in actin mutants grown under conditions that induce PH growth. Shown are wild-type and actin mutant strains grown in SLAD alginate and stained with rhodamine-phalloidin (to detect F-actin) and DAPI (to detect DNA) as described in MATERIALS AND METHODS. F-actin images are in stereo. Strains shown are BCY209 (ACT1/ACT1), BCY157 (act1-110/ACT1), BCY204 (act1-111/act1-111), BCY202 (act1-112/act1-112), BCY210 (act1-120/act1-120), and BCY168 (act1-131/ACT1). Bar, 10 µm.

For those mutants capable of making long cells, actin patch polarization is more normal under PH growth-inducing conditionsthan for those mutants with the most severe cell elongation defects.For example, act1-111/act1-111 homozygotes and act1-110/ACT1 heterozygotesboth show relatively normal patch morphology and polarizationin long cells (Figure 7), whereas actin cables are rarely seenin these mutants. These data underscore the importance of patchpolarization to the distal end of the emerging bud for cell elongationduring PH growth (see DISCUSSION).

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Actin Has Multiple Functions in Filamentous Growth

We have shown that act1 mutations disrupt the PH growth-specific properties of agar invasion, cell elongation, and unipolarbud site selection. Some act1 mutations show allele-specific effectson invasion, cell elongation, and unipolar budding (Table 3).In addition, certain act1 mutations exhibit specific intrageniccomplementation with respect to PH growth defects (Table 5).These data suggest that there are multiple requirements for actinfunction in PH growth.

Several observations indicate that the effects of these mutations on PH growth are due to specific effects on functions ofactin required for PH growth and not general effects on cell growthand physiology. First, two alleles that have no effect on viabilityat any temperature (act1-104 and act1-117) both exhibit pronouncedeffects on filamentation. Second, filamentation defects are seenat the "permissive" temperature (30°C) for the temperature-sensitiveact1 alleles and the sac6 mutant analyzed in this study. Third,only two alleles analyzed in this study (act1-111 and act1-132)show obvious growth defects at the temperature at which thesestudies were conducted (30°C) (Table 2), and these mutationshave less severe effects on PH growth than other alleles withno overt growth phenotypes at this temperature (e.g., -act1-112and act1-120) (Table 3).

The Utility of Filamentous Growth for Studying Actin Function

Filamentous growth provides a uniquely sensitive assay for actin cytoskeletal function during a developmental switch. Thesensitivity of this system allowed us to identify new phenotypicconsequences for mutations affecting actin. We found dominanteffects on filamentation for several actin mutations previouslyclassified as recessive based on their effects on YF growth. Effectson PH growth were also found for certain act1 alleles that haveno (or subtle) effects on YF growth and viability. In addition,using the filamentation phenotype, we have been able to identifygenetic interactions between actin alleles. Similar efforts todefine act1 intragenic complementation by assessing growth atrestrictive temperature have led to ambiguous results.

New Insights into Actin Structure and Function Revealed by Analysis of PH Growth Phenotypes

Many actin mutations are likely to cause defects in PH growth by blocking the interaction between actin and other proteins.Indeed, we have shown that act1-120, which is known to disruptbinding of fimbrin to actin, can be suppressed for its invasionand cell elongation defects by a compensatory mutation in theactin-binding domain of fimbrin (Figure 5). Other act1 alleleswith effects on PH growth are known or presumed to affect thebinding of proteins required for filamentation, suggesting thatthe phenotypes of these act1 mutants may be also be due, in part,to an effect on the binding of these proteins. For example, act1-110alters residues (E237 and K238) that are part of the binding sitefor the actin filament-stabilizing protein tropomyosin (Milliganet al., 1990; Saeki et al., 1996), which is encoded by TPM1 andTPM2 in yeast (Drees et al., 1995). tpm1/tpm1 mutants, like act1-110/ACT1heterozygotes, are defective for filamentation (Mösch and Fink,1997). act1-104 is particularly interesting, in that this allelehas no known YF phenotype and is not known to affect the bindingof any actin-binding protein, yet it has an obvious effect onfilamentation. act1-104 alters residues (K315 and E316) predictedto lie on the surface of both the actin monomer (Figure 8) andthe actin filament. Thus, these amino acids are well positionedto be a binding site for an as yet unidentified protein with aspecific role in PH growth.

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Figure 8. Modeling of the mutations analyzed in this study onto the solvent-exposed surface of an actin monomer. Shown is the calculated surface of the actin monomer based on the coordinates of the rabbit muscle actin filament structure (Lorenz et al., 1993

). Actin subdomains are indicated. Red, locations of residues altered by viable, temperature-sensitive alleles with recessive effects on PH growth; yellow, location of residues altered by viable, temperature-sensitive alleles with dominant effects on PH growth; blue, positions of residues affected by recessive lethal alleles with dominant effects on PH growth; green, locations of residues affected by mutations that have no effect on viability but disrupt PH growth; magenta, positions of residues altered by mutations with no effect on PH growth. Surfaces were generated using GRASP (Nicholls et al., 1991

) on a Silicon Graphics Iris computer.

Several mutations may act by altering the interaction of actin with itself. Four alleles that show effects on PH growth (act1-111,act1-112, act1-129, and act1-132) disrupt actin-actin interactionsin the two-hybrid assay (Amberg et al., 1995) and alter residuespredicted to stabilize actin-actin contacts (Holmes et al. 1990;Lorenz et al., 1993). Actin monomers defective for one such interactioncould disrupt filament assembly in a dominant manner by theirincorporation into a growing filament and blocking additionalcontacts necessary for filament stability and/or elongation. Interestingly,three alleles that affect actin-actin contacts (act1-112, act1-129,and act1-132) do indeed show dominant effects on PH growth.

The synthetic growth defect of act1-111/act1-112 (Figure 4) may also be explained by effects on actin filament assembly andstability. Insertion of a hydrophobic loop from one actin monomerinto a hydrophobic hole defined in part by the cleft between subdomains2 and 4 in an adjacent actin monomer has been suggested to stabilizeinteractions within the actin filament (Chen et al., 1993; Lorenzet al., 1993; Kuang and Rubenstein, 1997). act1-111 affects aminoacids (D222, E224, and E226) that form a pocket in which the hydrophobicloop resides in monomeric actin and may perturb the ability ofthe hydrophobic loop to swing out of the pocket to interact withthe hydrophobic cleft (Amberg et al., 1995). act1-112 alters residues(K213, E214, and K215) that form one-half of the cleft into whichthe hydrophobic loop is inserted. Thus, the negative interactionbetween these alleles could reflect a synergistic effect of perturbingboth structural features required for filament stability.

The demonstration that some act1 mutations exert their effects by altering the binding of specific actin-binding proteinssuggests a mechanism for the intragenic complementation we haveobserved. Such alleles might allow formation of heteropolymericactin filaments that can bind ligands that neither homopolymercan bind. For example, as shown in Figure 9, two actin alleles(X and Y) might affect binding of distinct proteins (A and B)that are both required for filamentation. If allele X blocks bindingof A, and allele Y blocks binding of B, act1-x/act1-x and act1-y/act1-yhomozygotes would be defective for PH growth, but because of distinctmolecular effects. However, actin filaments comprising X and Ymonomers would be competent to bind both A and B, and so act1-x/act1-ystrains would exhibit filamentation. Intragenic complementationbetween act1 alleles based on such a mechanism has been predicted(Ayscough and Drubin, 1996). However, to our knowledge the datapresented here represent the first experimental demonstrationof this effect.

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Figure 9. Model for mechanism of intragenic complementation between act1 alleles (after Ayscough and Drubin, 1996

). Actin monomers encoded by ACT1, act1-x, and act1-y are represented by white, black, and gray circles, respectively. The ability of hypothetical actin-binding proteins A and B to interact with actin filaments comprising wild-type actin, each mutant actin singly, or a combination of mutant actins is schematized. The PH growth phenotype of strains containing such actin filaments is also indicated.

This model predicts that mutations exhibiting intragenic complementation should affect binding of distinct subsets of ligandsand will likely reside in different regions of the actin monomerand/or filament. Indeed, act1-120 is the only mutant analyzedin this study localized to subdomain 1 of actin (Figure 8), andit is able to complement mutations in subdomains 2, 3, and 4 thatare quite distant (in both the monomer and filament) from thosemutations it complements for PH growth defects (act1-104 [subdomain3], act1-111 [subdomain 4], act1-117 [subdomain 4], act1-124 [subdomain2], and act1-129 [subdomain 3]). In addition, in the two-hybridassay, the actin encoded by act1-120 binds many ligands whosebinding was disrupted by act1 mutations that act1-120 can complement(Amberg et al., 1995).

Actin Function in Cell Elongation, Unipolar Budding, and Agar Invasion

Our results suggest that cytoskeletal integrity is essential for filamentation. What might be the specific requirements foractin in each of the PH growth-specific traits we analyzed?

Cell Elongation. The PH and YF actin cytoskeletons are different in structure. In YF cells, there is a distinct period during bud emergencein which actin patches are distributed over the cortex of theemerging bud. In PH cells, actin patches remain polarized at thetip of the cell throughout bud emergence (Kron et al., 1994).Our imaging of the PH actin cytoskeleton in wild type and act1mutants confirms and extends this observation to suggest thatactin patch polarization plays an important role in the elongationof the PH cell. In act1/act1 mutants with the most pronouncedeffects on cell elongation (act1-112/act1-112 and act1-120/act1-120homozygotes and act1-131/ACT1 heterozygotes), substantial perturbationof actin patch polarization during bud emergence is observed (Figure7). In contrast, actin patches are polarized to the distal endof many emerging buds in those actin mutants capable of makingsubstantial numbers of long cells. These results are consistentwith the proposal that actin patches play an important role indirecting secretion of new membrane and cell wall material inthe emerging bud (Novick and Botstein, 1985; Mulholland et al.,1994). Thus, the extended polarization of actin patches to thedistal end of PH cells throughout bud emergence would promoteelongation of the PH cell.

Unipolar Budding. The demonstration that actin cytoskeletal mutants are unable to exhibit bipolar budding in YF cells led to the suggestionthat the actin cytoskeleton is required to maintain, and perhapsdirect, the placement of bipolar bud site selection cues (Zahneret al., 1996; Yang et al., 1997). These presently unidentifiedsignals, present at both the proximal and distal ends of the cell,would then serve to direct new bud formation at either end ofthe mother cell. The fact that nearly all actin mutants we characterizedexhibit random budding under conditions that induce PH growthdemonstrates that, like bipolar bud site selection in YF diploids,unipolar bud site selection in PH cells requires actin cytoskeletalfunction. However, act1-113/act1-113 and act1-117/act1-117 strainsare suppressed for their YF random budding phenotype when grownunder conditions that induce PH growth (Table 4). Thus, despitetheir similar dependency for actin function, these results demonstratethat the YF and PH bud site selection programs are regulated somewhatdistinctly in response to nutrient conditions.

Invasion. The mechanism by which PH cells invade agar is not known. However, it has been suggested that these cells might secrete enzymesthat hydrolyze agar and thus facilitate growth through the substrate(Gimeno et al., 1992). Indeed, many invasive fungi, includingCandida albicans, have been shown to secrete proteases and otherenzymes believed to facilitate their invasion (Macdonald and Odds,1983). Given the well-established role for actin in secretion,it is tempting to speculate that actin is required for the secretionof such enzymes.

	ACKNOWLEDGMENTS

We thank Alison Adams for plasmids used in this work, Ken Holmes for the actin filament coordinates, and James Berger forassistance using GRASP. We are grateful to members of the Finkand Botstein laboratories for helpful discussions and Todd Milnefor critical reading of the manuscript. Many thanks to Katja Schwartzfor providing help with some of the microscopy in Figure 6. B.M.C.is a Chiron Fellow of the Life Sciences Research Foundation. G.R.F.is an American Cancer Society Professor of Genetics. The DeltaVisionmicroscope system is supported by National Institutes of HealthResearch Resources grant RR11939-01. This work was supported bygrants from the National Institutes of Health (GM46406-07 to D.B.and GM35010 to G.R.F.).

	FOOTNOTES

Corresponding author. E-mail address: fink{at}wi.mit.edu.

Present address: Molecular Biology Institute, Department of Chemistry and Biochemistry, UCLA, Los Angeles CA 90095.

Online version of this article contains video material for Figures 6 and 7. Online version available at www.molbiolcell.org.

¹ Abbreviations used: GFP, green fluorescent protein; PH, pseudohyphal; SLAD, synthetic low-ammonia dextrose; YF, yeast form.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
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Enhanced Cell Polarity in Mutants of the Budding Yeast Cyclin-dependent Kinase Cdc28p
Mol. Biol. Cell, November 1, 2001; 12(11): 3589 - 3600.
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C. M. Asleson, E. S. Bensen, C. A. Gale, A.-S. Melms, C. Kurischko, and J. Berman
Candida albicans INT1-Induced Filamentation in Saccharomyces cerevisiae Depends on Sla2p
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Different Domains of the Essential GTPase Cdc42p Required for Growth and Development of Saccharomyces cerevisiae
Mol. Cell. Biol., January 1, 2001; 21(1): 235 - 248.
[Abstract] [Full Text]

T. Freedman, A. Porter, and B. Haarer
Mutational and hyperexpression-induced disruption of bipolar budding in yeast
Microbiology, November 1, 2000; 146(11): 2833 - 2843.
[Abstract] [Full Text]

K. L. Richards, K. R. Anders, E. Nogales, K. Schwartz, K. H. Downing, and D. Botstein
Structure-Function Relationships in Yeast Tubulins
Mol. Biol. Cell, May 1, 2000; 11(5): 1887 - 1903.
[Abstract] [Full Text]

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The Secretory Pathway Mediates Localization of the Cell Polarity Regulator Aip3p/Bud6p
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Type 1 protein phosphatase is required for maintenance of cell wall integrity, morphogenesis and cell cycle progression in Saccharomyces cerevisiae
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[Abstract] [PDF]

S.-H. Ahn, A. Acurio, and S. J. Kron
Regulation of G2/M Progression by the STE Mitogen-activated Protein Kinase Pathway in Budding Yeast Filamentous Growth
Mol. Biol. Cell, October 1, 1999; 10(10): 3301 - 3316.
[Abstract] [Full Text]

D. I. Johnson
Cdc42: An Essential Rho-Type GTPase Controlling Eukaryotic Cell Polarity
Microbiol. Mol. Biol. Rev., March 1, 1999; 63(1): 54 - 105.
[Abstract] [Full Text] [PDF]

D. C. Amberg
Three-dimensional Imaging of the Yeast Actin Cytoskeleton through the Budding Cell Cycle
Mol. Biol. Cell, December 1, 1998; 9(12): 3259 - 3262.
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