Regulation of G2/M Progression by the STE Mitogen-activated Protein Kinase Pathway in Budding Yeast Filamentous Growth

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Vol. 10, Issue 10, 3301-3316, October 1999

Regulation of G2/M Progression by the STE Mitogen-activated Protein Kinase Pathway in Budding Yeast Filamentous Growth

Sung-Hee Ahn,^* Adriana Acurio,^* and Stephen J. Kron

Center for Molecular Oncology and Department of Molecular Genetics and Cell Biology, University of Chicago, Chicago, Illinois 60637

Submitted January 26, 1999; Accepted July 23, 1999
Monitoring Editor: Mark J. Solomon

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Inoculation of diploid budding yeast onto nitrogen-poor agar media stimulates a MAPK pathway to promote filamentous growth.Characteristics of filamentous cells include a specific patternof gene expression, elongated cell shape, polar budding pattern,persistent attachment to the mother cell, and a distinct cellcycle characterized by cell size control at G2/M. Although a requirementfor MAPK signaling in filamentous gene expression is well established,the role of this pathway in the regulation of morphogenesis andthe cell cycle remains obscure. We find that ectopic activationof the MAPK signal pathway induces a cell cycle shift to G2/Mcoordinately with other changes characteristic of filamentousgrowth. These effects are abrogated by overexpression of the yeastmitotic cyclins Clb1 and Clb2. In turn, yeast deficient for Clb2or carrying cdc28-1N, an allele of CDK defective for mitotic functions,display enhanced filamentous differentiation and supersensitivityto the MAPK signal. Importantly, activation of Swe1-mediated inhibitoryphosphorylation of Thr-18 and/or Tyr-19 of Cdc28 is not requiredfor the MAPK pathway to affect the G2/M delay. Mutants expressinga nonphosphorylatable mutant Cdc28 or deficient for Swe1 exhibitlow-nitrogen-dependent filamentous growth and are further inducedby an ectopic MAPK signal. We infer that the MAPK pathway promotesfilamentous growth by a novel mechanism that inhibits mitoticcyclin/CDK complexes and thereby modulates cell shape, buddingpattern, and cell-cellconnections.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

When diploid cells of dimorphic strains of the budding yeast Saccharomyces cerevisiae are inoculated onto agar media richin a fermentable carbon source but poor in nitrogen, they candifferentiate to enter filamentous growth. Previous studies (reviewedby Kron and Gow, 1995; Madhani and Fink, 1998a) have establishedthat the filamentous cell represents a distinct cell type characterizedby an elongated shape, a polar budding pattern, and persistentattachment of each daughter cell to the mother after septation.These features contribute to colony growth as branching filamentsthat invade the agar. Another characteristic of filamentous growthis that the cell division cycle is regulated by cell size controlat mitosis (Kron et al., 1994). Filamentous cells remain buddeduntil the cell doubles in size. Throughout most of this prolongedbudded period, the cell exhibits phenotypes suggestive of G2 arrest(Surana et al., 1991), such as a short mitotic spindle, a singlerounded nuclear mass, and an elongated, tubular bud. As a resultof the long G2/M growth period, daughter cells are born largerthan the critical size for progression to S phase at Start. Therefore,newly born daughter cells at the tip of filaments immediatelybud and reenter the cell cycle. Thus, the G2/M cell cycle controllikely contributes to the capacity of filamentous cells to continuemitotic growth even in the face of nitrogenlimitation.

A comparison of the shape and cell division pattern of filamentous cells with the results of Lew and Reed (1993) regardingthe effects of different cyclin/CDK complexes on cell morphogenesissuggests that the link between cell cycle and cell shape in filamentousgrowth may be direct. In the growth pattern of "well-fed" yeast(reviewed by Madden and Snyder, 1998), bud growth is initiallypolarized to the tip, leading to tube-like growth at S phase andinto G2. During mitosis, bud growth becomes isotropic, leadingto swelling growth. Finally, septation occurs upon completionof mitotic anaphase. Distinct cyclins combine with the Cdc28 CDKto mediate each of the nuclear transitions (reviewed by Mendenhalland Hodge, 1998). Altered expression of the cyclins or modulationof the activity of the cyclin/Cdc28 complexes has coordinate effectsof delaying or accelerating both the nuclear transition and therelated morphogenetic event (Lew and Reed, 1993). For example,increased expression of G1 cyclins or decreased expression ofmitotic cyclins each lead to a delay before the onset of mitosis.This prolongs the period of tubular bud growth, leading to a "filamentous"appearance. It is reasonable to hypothesize that the cell cyclemachinery may be a key target of the pathway regulating the morphogeneticevents characteristic of filamentous differentiation. Recent datahave shown that mutations in G1 cyclins can largely abrogate filamentousgrowth (Oehlen and Cross, 1998; Loeb et al., 1999), whereas deficiencyof the Clb2 mitotic cyclin or induction of inhibitory tyrosinephosphorylation of the principal CDK Cdc28 or a particular pointmutation of Cdc28 (Edgington et al., 1999) each significantlyinduces filamentous differentiation. What remains to be establishedis any specific link between the low-nitrogen signal and regulationof the cellcycle.

Previous studies of filamentous differentiation have established a branching signal transduction pathway involving elementsof the RAS GTPase/cAMP-dependent kinase cascade and the STE MAPKpathway (reviewed by Banuett, 1998). The STE MAPK cascade andgene expression pathway (reviewed by Leberer et al., 1997) isbest known for its role in mediating yeast mating response. Pheromonesinduce a sequence of phosphorylations in the STE MAPK cascade,consisting of a PAK kinase homolog Ste20, a MEK kinase Ste11,a MEK Ste7, and the MAPKs Fus3 and Kss1. The downstream targetis a transcriptional activator, Ste12, that binds to pheromoneresponse elements in promoters of effector genes such as Far1(Hagen et al., 1991). Far1 promotes G1 arrest in pheromone-stimulatedcells (Chang and Hersko-witz, 1990), acting as a stoichiometricinhibitor that sequesters Cln1,2 G1 cyclin/Cdc28 complexes (Peterand Herskowitz, 1994).

Filamentous differentiation requires only a subset of the STE pathway genes required for mating responses (Madhani and Fink,1998b). Mutations in the Ste20, Ste11, or Ste7 kinases or theSte12 transcription factor abrogate filamentous differentiation(Liu et al., 1993; Roberts and Fink, 1994). The MAPK Kss1 servesa dual role in filamentous differentiation as both inhibitor andactivator of Ste12-dependent gene expression (Cook et al., 1997;Madhani et al., 1997). Ectopic activation of the STE pathway bydominant active alleles of STE11 (Liu et al., 1993), STE7 (Madhaniet al., 1997), and KSS1 (Madhani et al., 1997) or by overexpressionof STE12 (Liu et al., 1993) all promote enhanced filamentous growthand can partially bypass upstream blockades in thepathway.

Ectopic activation of RAS/cAMP signaling can also promote filamentous growth. The dominant active allele RAS2-Val19 markedlyenhances filamentous growth in nitrogen-starved cells (Gimenoet al., 1992; Mosch et al., 1996) via activation of both cAMP-dependentand MAPK responses (Mosch et al., 1996, 1999). In turn, activationof the STE pathway alone by dominant active alleles such as STE11-4(Stevenson et al., 1992; Liu et al., 1993) apparently enhancesfilamentous growth by cAMP-independent mechanisms. Recent datasuggest that RAS signaling induces its cAMP-mediated effects andactivates the STE MAPK cascade independently (Mosch et al., 1999;Pan and Heitman, 1999) but that the signals transmitted via theseparallel pathways converge on similar targets (Robertson and Fink,1998; Pan and Heitman, 1999; Rupp et al., 1999).

Thus, elements of the RAS/cAMP and STE MAPK pathways constitute a single "RAS/STE" filamentous response pathway. This compoundsignaling pathway mediates its effects predominantly via regulationof gene expression. RAS/STE signals induce cell type-specifictranscription (Mosch et al., 1996) via a distinct UAS, the filamentousresponse element (FRE) (Madhani and Fink, 1997), that consistsof adjacent Ste12 and Tec1 binding sites. Cells lacking eitherfactor lack FRE-dependent gene expression and are defective infilamentous differentiation (Gavrias et al., 1996; Lo et al.,1997; Madhani and Fink, 1997; Mosch and Fink, 1997). To date,only one effector essential for filamentous differentiation, theMUC1/FLO11 flocculin (Lambrechts et al., 1996; Lo and Dranginis,1998), has been shown to be expressed under RAS/STE control viaa FRE (Lo and Dranginis, 1998; Rupp et al., 1999). Cells deficientin Flo11 do not remain linked in chains and form only disorganizedcolonies that fail to invade the substratum. However, these cellsremain responsive to RAS/STE signals, retaining the elongatedcell shape, polar budding, and G2/M delay characteristic of filamentouscells (Kron and Dranginis, unpublished results). As yet, the genesthat mediate these aspects of filamentous development remain tobedescribed.

Potential links between the RAS/STE signal transduction pathway and the cell cycle machinery in the control of filamentousdifferentiation remain poorly defined. This is surprising, consideringthe well-established roles for cyclins and CDK in determiningyeast cell shape (Lew et al., 1997; Madden and Snyder, 1998; Mendenhalland Hodge, 1998). In pheromone response, ectopic activation ofthe Cln G1 cyclins can antagonize both gene expression (Oehlenand Cross, 1994) and cell cycle arrest (Edwards et al., 1997;Kron, unpublished results). Recent data have suggested that Cln2cyclin complexes with Cdc28 CDK mediate this effect by regulationof Ste20 (Oehlen and Cross, 1998; Wu et al., 1998; Leza and Elion,1999) and/or regulation of Ste11 (Wassmann and Ammerer, 1997).Importantly, Cln1,2/Cdc28 phosphorylation of Ste20 has been proposedto underlie the requirement for Cln G1 cyclins in filamentousdifferentiation (Oehlen and Cross, 1998). A pathway linking Clb1and Clb2 mitotic cyclins to morphogenesis via Cdc28 phosphorylationof a Ste20 homolog, Cla4, has been demonstrated (Tjandra et al.,1998), but any relationship to signal transduction remains uncharacterized.A broad interpretation of these studies would place the cell cyclemachinery as a regulator acting upstream in the RAS/STE signalingpathway.

An alternative hypothesis based on the role of the CDK inhibitor Far1 in pheromone-induced cell cycle arrest is that the cellcycle effect of RAS/STE signaling may be mediated by a FRE-regulatedeffector, such as a mitotic inhibitor. Such a factor might inhibitClb1- and Clb2-dependent forms of the Cdc28 CDK and function todelay both depolarization of the bud and completion of mitosis.To test this hypothesis, we set out to examine the relationshipbetween elements of the cell cycle machinery and the signalingpathways modulating filamentous growth. We observed that 1) ectopicactivation of the RAS/STE pathway slows mitotic progression, and2) modulation of mitotic cyclin expression dramatically affectsfilamentous differentiation. Cells deficient in mitotic cyclinsare activated for filamentous growth, whereas cells overexpressingmitotic cyclins cannot form filamentous colonies, even in thepresence of an inducing signal. Epistasis analysis places theactivity of the cyclins downstream of the RAS/STE signaling pathway.Our results establish a pathway for filamentous differentiationin which the cell cycle engine is a critical target of the RAS/STEpathway involved in promoting the elongated cell shape, polarizedcell division, and invasive growth characteristic of the differentiatedstate.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Yeast Media

Media were prepared as previously described (Kron et al., 1994) with yeast extract, peptone, and yeast nitrogen base fromUnited States Biochemical (Cleveland, OH). Other reagents wereobtained from Fisher Scientific (Pittsburgh, PA) and Sigma (St.Louis, MO). All low-nitrogen media contained 50 µM ammonium sulfateand 6.8 g/l yeast nitrogen base without amino acids or ammoniumsulfate and were filter sterilized through a 0.45-µm filter. Syntheticlow-ammonia dextrose (SLAD) medium also contained 2% dextrose.Agar (bacteriological, United States Biochemical) was preparedby autoclaving at 4% wt/vol in deionized water and diluting to2% final concentration with 2× liquid media. Low-ammonia agarmedia were made using agar washed four times in deionized waterbeforesterilization.

Yeast Strains and Plasmids

All yeast strains were derived in the $Sigma$ 1278b background (Grenson et al., 1966; Gimeno et al., 1992) using conventional geneticmethods. Marker segregation, PCR assay, and/or Southern blottingdetermined genotypes. Yeast strains are described in Table 1.Transformations were performed by a lithium acetate procedurebased on that of Schiestl and Gietz (1989). Plasmids are describedin Table 2.

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Table 1. Yeast strain list

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Table 2. Plasmid list

To derive strains that stably express STE11-4 from the STE11 chromosomal locus, a 3.6-kilobase XbaI fragment from pSL1509(yCP50-STE11-4) (Stevenson et al., 1992) was subcloned into pRS30(Sikorski and Hieter, 1989) to construct SKB4166, an integratingplasmid carrying the STE11-4 gene and a LEU2 marker. A diploidLEU strain, L5791, was transformed with SKB4166 guided to one STE11locus by digestion at a unique NcoI site in the STE11 ORF. Wechose a transformant, SKY2183, that exhibited slow growth in richmedia and striking filamentous growth on SLAD plus 1 mM uracil.When transformed with the Ty1-lacZ reporter pIL30 (Laloux et al.,1994; Mosch et al., 1996), a high constitutive level of expressionwas observed. Sporulation of SKY2183 yielded 2:0 LEU⁺ segregants that when crossed to wild-type haploids dominantlyconferred enhanced filamentous growth to the resultingdiploids.

A URA3-marked centromeric plasmid carrying the dominant CDC28-T18A, Y19F allele, SKB4167, was constructed by subcloning a2.3-kilobase XhoI/PvuII fragment from p3303 (Ycplac22 CDC28-T18A,Y19F) (Amon et al., 1992) into XhoI/SmaI-digested pRS316 (Sikorskiand Hieter, 1989). To construct a double mutant diploid carryingboth STE11-4 and CDC28-T18A, Y19F alleles on both pairs of chromosomes,SKY2183 and SKY1056 were sporulated and dissected. Segregantswere then mated and the heterozygous diploid was then sporulatedand dissected to yield double mutant STE11-4, CDC28-T18A, Y19Fhaploid segregants. These were then mated to each other to createthe STE11-4/STE11-4, CDC28-T18A, Y19F/CDC28-T18A, Y19F diploidstrain SKY2225. SKY2226 (STE11-4/STE11-4) was formed from LEU⁺ segregants ofSKY2183.

The cdc28-1N allele of K406 (Surana et al., 1991) was amplified by high-fidelity PCR and the XhoI/MunI fragment was subclonedinto pRS413 (Sikorski and Hieter, 1989) to make plasmid SKB4168.The complete ORF of this clone was sequenced and the mutationconfirmed. A URA3-marked integrating plasmid carrying the cdc28-1Nallele, SKB4169, was constructed by subcloning a 1.3-kilobaseBamHI/XhoI fragment from SKB4168 into pRS306 (Sikorski and Hieter,1989). To create a pair of haploid strains carrying only the cdc28-1Nallele, SKB4169 was digested with HindIII and transformed intoSKY754 and L5683 to integrate at the CDC28 locus. Transformantswere selected on synthetic media lacking uracil, colony purified,and grown nonselectively for several generations at 22°C. Clonesthat had evicted the URA3 plasmid, leaving behind the cdc28-1Nallele, were selected on media containing 1 mg/ml 5-fluoro-oroticacid and then screened for lack of growth at 36°C. A pair of cellsof opposite mating type were then mated to form a ts diploid,SKY2187, with the genotype cdc28-1N/cdc28-1N.

Strains overexpressing Clb1 and Clb2 were constructed by transforming L5791 with the plasmids YIpG2::CLB1 and YIpG2::CLB2(Stueland et al., 1993), respectively, each digested with BstEIIto direct integration to the LEU2locus.

Microscopy Methods

Microcolonies were imaged through the agar and plastic Petri dish with a Zeiss (Thornwood, NY) Axiovert 25 with bright-fieldillumination and a 32× LD Achroplan objective. Cells from suspensioncultures were spread gently onto agar plates and imaged similarly.Pixera VCS image-acquisition software and a Pixera charge-coupleddevice camera were used to capture images at 1280 ×1024 resolution.Images were converted to gray scale, filtered to remove noiseand enhance contrast, cropped, and assembled in Photoshop (Adobe,Mountain View,CA).

Staining of fixed cells with DAPI was carried out essentially as described (Pringle et al., 1991). DAPI-stained experimentaland control cells were placed on slides and imaged on a ZeissAxioskop by phase and epifluorescence microscopy using 365-nmexcitation and blue emission filters, a 40× Fluar oil-immersionobjective, and 16× eyepieces. The cell shapes and the positionsand forms of nuclei in each budded cell were determined. Eachcell was classified into groups by apparent bud size/mother cellsize ratio and into one of five nuclear morphology classes ofthe budding cycle: 1) central nucleus, S phase; 2) nucleus atneck in mother cell, S phase/G2; 3) nucleus distributed acrossneck, G2/metaphase; 4) nucleus stretched along mitotic spindle,anaphase; or 5) separate nuclear masses but no septum formed,telophase. Both as a control for staining and to evaluate nuclearphenotypes, propidium iodide-stained cells used for flow cytometrywere examined by epifluorescence microscopy as above but with546-nm excitation and orange-red emissionfilters.

Fixed cells grown on rich media were stained with rhodamine or fluorescein phalloidin (Molecular Probes, Eugene, OR) and DAPIas previously described (Pringle et al., 1991) to evaluate nuclearposition and reveal altered actin distribution patterns duringthe cell cycle. Cells from liquid cultures in rich media wereprepared for immunofluorescence microscopy and stained with YOL1/35 anti-tubulin antibody (Kilmartin et al., 1982) (AccurateChemical and Scientific) and Cy3 goat anti-rat immunoglobulinG polyclonal secondary antibody (Jackson Immunoresearch) and counterstainedwith DAPI to stain nuclear and mitochondrial DNA essentially asdescribed (Pringle et al., 1991), except that all steps were performedwith cells in suspension and gentle centrifugation was used toexchange solutions. Cells were imaged with 546-nm excitation andorange-red emission filters to evaluate tubulin, 365-nm excitationand blue emission filters for DNA, and Nomarski differential interferencecontrast optics for cell morphology. Calcofluor staining (Pringle,1991) was performed on exponentially growing cells. Samples werefixed in 3.7% formaldehyde at 25°C for 30 min. Aliquots of ~10⁷ cells were pelleted, resuspended in 1 ml of 0.1 µg/ml Calcofluorstaining solution, and incubated for 5 min. The cells were washedthree times with 1 ml of water and resuspended to a final volumeof 50 µl. Cells were examined to determine bud scar patterns using365-nm excitation and blue emission filters and Nomarski differentialinterference contrast optics. Images were recorded using epifluorescenceillumination on a Zeiss Axioskop using a 63× PlanApochromat objective,a Sensys 1600 charge-coupled device camera, and IPLab image-acquisitionsoftware.

Percentage Elongation on Agar

Yeast strains (SKY757, wild type, and L5535, ste7/ste7) were grown overnight to saturation at 30°C in 5 ml of synthetic minimalmedium. Cells were washed, diluted to 1000 cells/ml, and spreadonto plates of SLAD with uracil. Analysis of cell elongation wasperformed by microscopic examination using the Zeiss Axiovert25 and a 32× LD Achroplan objective to image cells through theagar and plastic Petri dish. Scoring was performed by visual estimationof the length-to-width ratios of at least 400 cells. For 6 h,cells were counted in three categories: unbudded, round buds (budlength $<=$ twofold bud width), and elongated buds (bud length $>=$ twofold budwidth).

Flow Cytometry

Cells from log-phase cultures were fixed and stained with propidium iodide to prepare samples for flow cytometry as described(Hutter and Eipel, 1978). To disrupt cell aggregates, sampleswere sonicated until judged well dispersed by phase microscopy.Staining was evaluated by epifluorescence imaging using 546-nmexcitation and orange emission filters. Samples were analyzedon a FacsScan (Becton-Dickinson, Franklin Lakes, NJ) flow cytometer,and 60,000 events were collected on each sample. The plots presentedhere represent the gated fluorescence area data. The gated datawere analyzed to determine relative DNAcontent.

Whole Cell Extracts and Protein Analysis

Whole cell extracts were obtained by a method based on that of Amon (1992). Strains were grown overnight to saturation inYPD rich liquid media, diluted 1:50, and regrown to a densityof ~10⁷ cells/ml in YPD at 30°C. Cells were chilled, collected by centrifugation,washed in 10 mM Tris-HCl (pH 8.0), and resuspended in 200 µl ofbuffer A (50 mM Tris-HCl, pH 7.5, 1 mM EDTA, 5 mM DTT, 1 mM PMSF,0.2 mM L-1-chloro-3-[4-tosylamido]-4-phenyl-2-butanone, 0.025mM L-1-chloro-3-[4-tosylamido]-7-amino-2-heptanone-HCl, 2 mg/mlpepstatin in DMSO). Approximately 0.2 ml of 0.2-mm-diameter acid-washedglass beads was added, cells were vortexed for 5 min, and theextract was cleared by a 5-min centrifugation at 16,000 × g at4°C. The supernatant was collected and stored at $-$ 80°C. Proteinconcentrations were determined by the Bradford protein assay (Bio-Rad,Richmond, CA) using BSA as astandard.

For Western analysis, protein samples were solubilized with SDS/DTT sample buffer, boiled, and loaded onto 12% bis:acrylamidegels (1:19) with 50 µg of total yeast protein per lane. Sampleswere electrophoretically separated and transferred to nylon-supportednitrocellulose (Magna). Primary antibodies were, for Cdc28, amouse anti-PSTAIRE mAb (Calbiochem, La Jolla, CA), and for Clb2,a rabbit polyclonal antibody raised against a TrpE-Clb2 fusionprotein (Amon et al., 1994) and affinity purified using the antigen.Immunoreactivity was detected with ¹²⁵I-protein A (ICN, Costa Mesa, CA), and blots were scanned usinga phosphorimager (Molecular Dynamics, Sunnyvale, CA) and analyzedusing Imagequant and IPLab (Scanalytics). For analysis of expressionfrom the pIL30 (Laloux et al., 1994) Ty1::lacZ reporter, extractswere obtained, assayed for total $beta$ -galactosidase activity, andnormalized to total protein as described (Alfa et al., 1993).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Activation of the STE MAPK Signal for Filamentous Growth Induces a Delay in G2/M

Wild-type, prototrophic strains constructed in the $Sigma$ 1278b background exhibit filamentous development when subjected to low-nitrogenstress. When such cells are transferred to nitrogen starvationmedia (SLAD agar), many cells show a striking change in bud morphologywithin their first budding cycle, immediately adopting a filamentousgrowth pattern. In the first cell cycle under nitrogen starvationconditions, 91% of budded wild-type cells (n = 400) formed anelongated bud when examined 4 h after inoculation onto SLAD media.This phenotype is reminiscent of the arrest of cells carryingthe cdc28-1N mutation (Surana et al., 1991) overexpressing theSwe1 tyrosine kinase (Booher et al., 1993) or overexpressing aG1 cyclin (Lew and Reed, 1993), each of which blocks cell cycleprogression at the metaphase-to-anaphase transition by antagonizingClb1- and Clb2-dependent Cdc28 complexes. When cells lacking elementsof the RAS/STE filamentous development pathway are inoculatedonto SLAD, the proportion of elongated buds formed is significantlydecreased. Only 10% (n = 400) of cells lacking the STE7 MEK kinase,and thereby defective in RAS/STE signaling, formed elongated budsin their first cell cycles. Rather, most buds emerging from Ste7-deficientmother cells formed small ovoid shapes and soon detached fromthe mother cell (Figure 1A). This pattern is typical of yeastcell growth on YPD agar media (rich media containing yeast extract,peptone, and dextrose). Nonetheless, the rate of bud emergencein the RAS/STE-signaling mutant was indistinguishable from thatin the wild type (wild type, 78% budded at 4 h; ste7/ste7, 76%budded at 4 h). A simple inference is that the RAS/STE pathwaymay antagonize processes that are limiting for completion of mitosis(e.g., accumulation of Clb1,2/Cdc28 complexes) but has littleeffect on factors limiting Start (e.g., accumulation of Cln1,2/Cdc28complexes).

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Figure 1. Ectopic activation of the RAS/STE pathway via the STE11-4 mutation. (A) The dominant active STE11-4 mutation promotes enhanced filamentous differentiation. Microcolonies formed by the indicated strains (STE11-4 is the STE11:: STE11-4:: LEU2/STE11 strain SKY2183) on rich YPD media and low-nitrogen SLAD media reveal that the requirement for nutrient starvation is bypassed by activation of RAS/STE signaling. A cell deficient for STE7 (ste7/ste7, L5535), an element of the RAS/STE pathway, does not exhibit a filamentous phenotype on YPD or SLAD media. Photographs show representative colonies of each strain after 24 h at 22°C. (B) Diploid cell agar invasion assay. Strains were inoculated on YPD agar and grown for 72 h at 30°C. Photographs were taken after the nonadherent cells were washed away with water. The STE11-4 mutant is hyperinvasive even in the rich media. (C) Cell morphology of mutant cultured in liquid YPD nitrogen-rich media. The STE11-4 mutant exhibits highly elongated cells that grow as adherent cell aggregates reminiscent of filamentous colonies. This phenotype suggests that the agar signal requirement is also bypassed by ectopic RAS/STE signals. Bars, 50 µm. (D) Cell cycle kinetics of the STE11-4/STE11-4 homozygous diploid (SKY2226). Flow cytometry was performed on asynchronous cultures growing on YPD rich media to determine the distribution of nuclear DNA content. The STE11-4 mutant reveals a predominance of cells with G2/M DNA content, which correlates to a large G2/G1 ratio, reflecting the relative percentages of cells falling in the indicated gating intervals of fluorescence intensity.

To investigate this phenomenon further, we examined the behavior of cells in which the RAS/STE pathway was ectopically induced.We investigated the effect of the dominant activated STE11-4 mutantallele, T596I (Stevenson et al., 1992), on cell growth in richmedia. When introduced as a single copy into diploid cells viaintegration at the STE11 locus, STE11-4 confers enhanced filamentousgrowth on SLAD media, as previously reported by Liu et al. (1993)for the plasmid-borne allele (Figure 1A). We examined severalmarkers for filamentous development in these stable STE11-4 cells.When inoculated on YPD agar media, this strain (SKY2183) displayedphenotypes characteristic of nitrogen starvation and activationof the RAS/STE pathway, including striking filamentous colonymorphology (Figure 1A) and elevated expression of the pIL30 Ty1-lacZFRE reporter. After 2 d of growth on YPD agar, the STE11-4 cellsinvaded the agar surface to a greater degree than a wild-typediploid control (Figure 1B). Even in suspension culture in richmedia, the STE11-4 mutant grew as highly elongated cells thatremained attached in clusters, forming florets reminiscent offilamentous colonies (Figure 1C). As in bona fide filamentouscells (Kron et al., 1994), STE11-4 cells exhibited apical polarbudding. In the cell clusters and in colonies on agar, buds arosepreferentially from the apical end of the mother cell. However,when these cells were examined with the chitin stain Calcofluorto confirm bud-site selection pattern, rather than the usual chitinrings at bud scars, a delocalized distribution of stain was apparent(Figure 2), perhaps consistent with a loss of temporal and/orspatial restriction of chitin deposition. However, staining ofSTE11-4 cells with fluorescein phalloidin revealed persistenceof an apically polarized distribution of actin cortical patchesin large budded cells, as observed in wild-type cells respondingto nitrogen starvation (Kron et al., 1994; Cali et al., 1998).Thus, via ectopic activation of the RAS/STE pathway, many featuresof the filamentous cell phenotype can be dissociated from nitrogenstarvation.

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Figure 2. Fluorescence imaging of Calcofluor staining of chitin distribution. The STE11-4 mutant shows a delocalized distribution of chitin rather than the expected chitin rings that mark bud scars, as is seen in the wild type and the ste11/ste11 mutant.

Flow cytometry of a STE11-4/STE11-4 homozygous diploid (SKY2226) growing in rich media demonstrated a predominance of cellswith G2/M DNA content (Figure 1D). DAPI staining to determinethe distribution of nuclear DNA suggested that most cells withlarge buds do not have separated nuclear masses or an elongatedspindle (Figure 3). These data were confirmed by examination ofspindles by anti-tubulin immunofluorescence microscopy. Theseassays indicated that the STE11-4 cells do not have any increasein content of anaphase cells, despite their long budded periodand G2/M shift. From these data, we infer that the predominantcell type in STE11-4 cells grown on rich media is a cell carryingan elongated bud that has completed DNA synthesis but has yetto leave G2/metaphase, much like filamentous cells cultured onnitrogen starvation media.

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Figure 3. Distribution of nuclear DNA through the budding cycle. Cells were grown on YPD rich media and fixed, and nuclear DNA was stained with DAPI as described in MATERIALS AND METHODS. The cell shapes and the positions and forms of nuclei in 400 budded cells were determined. Each cell was scored individually and classified into groups by apparent bud size/mother cell size ratio and into nuclear morphology classes corresponding to stages in the budding cycle. The histograms plot the number of cells that fall in one morphology class, divided into six groups by their bud size/mother cell size ratio. The five morphology classes plotted are: central nucleus, S phase (A); nucleus at neck in mother cell, S phase/G2 (B); nucleus distributed across neck, G2/metaphase (C); nucleus stretched along mitotic spindle, anaphase (D); and separate nuclear masses but no septum formed, telophase (E). Representative cells are shown to the left of each histogram. These data show that mitotic progression correlates well with bud growth in wild-type cells. By contrast, STE11-4 and clb2/clb2 mutants display an overabundance of G2/metaphase nuclei throughout the budded period and a decreased proportion of anaphase and telophase morphologies. This phenotype is suggestive of a postreplication delay analogous to that of filamentous cells cultured on nitrogen starvation media. The ste7/ste7 clb2/clb2 mutant reveals a slight increase in the proportion of cells in anaphase compared with clb2/clb2 but still significantly fewer compared with the wild-type control or the ste7/ste7 mutant.

These data are consistent with a mechanism by which the RAS/STE pathway negatively regulates the onset of mitotic anaphase,independent of any direct effects of nitrogen starvation. A reasonabletarget is the abundance or activity of mitosis-promoting factor(MPF), the mitotic form of CDK. We asked whether yeast mitoticcyclins Clb1 and Clb2 and/or the CDK Cdc28 might be regulatedby RAS/STEsignals.

STE MAPK Signaling Can Promote Filamentous Growth in the Absence of Cdc28 Tyrosine Phosphorylation

Mitotic onset in most eukaryotes is controlled by the reversible inhibitory phosphorylation of a conserved tyrosine and threonineadjacent to the active site in CDKs (Feilotter et al., 1992).Phosphorylation sequesters preformed CDK/cyclin complexes as preMPFand delays anaphase. Our previous studies showed that cells carryingthe constitutively active CDC28-T18A, Y19F (AF) mutant allelein which the Thr and Tyr residues are substituted with Ala andPhe still form filamentous colonies when inoculated onto low-nitrogenagar, although they are attenuated in their development. Thisresult does not eliminate a pathway whereby the RAS/STE signalfor filamentous differentiation promotes phosphorylation of thistyrosine.

We reexamined the behavior of mutants with altered Cdc28 tyrosine phosphorylation and/or altered RAS/STE function exposedto low-nitrogen agar media. We found that cells in which tyrosinephosphorylation is decreased (CDC28-T18A, Y19F/CDC28-T18A, Y19F,swe1/swe1, [2 µm MIH1]) are impaired in filamentous developmentand yield colonies on SLAD media in which cells at the colonyperiphery lack the degree of cell elongation observed in wild-typestrains (data not shown). On the other hand, mutants with constitutivelyincreased tyrosine phosphorylation (mih1/mih1, [2 µm SWE1]) aremoderately enhanced in filamentous growth and produce markedlyelongated cells at the colony periphery (data not shown). We confirmedpublished results that cells lacking certain elements of the RAS/STEpathway (ste7/ste7, ste12/ste12 [see Figure 8A], or ste11/ste11[data not shown]) display markedly reduced filamentous developmentand cells carrying mutations that increase RAS/STE signaling ([CENRAS2-Val19], [CEN STE11-4], [2 µm STE12] [data not shown]) displaydramatically enhanced filamentousgrowth.

One model consistent with these data, as suggested by Edgington et al. (1999), is that inhibition of anaphase by the RAS/STEpathway is mediated by hyperphosphorylation of Thr-18 and/or Tyr-19of the Cdc28 CDK, affected by activation of the Swe1 kinase orinhibition of the Mih1 phosphatase. Alternatively, the RAS/STEpathway and Cdc28 tyrosine phosphorylation may contribute independentlyto differentiation. In support of the latter possibility, we observedthat ectopic activation of the RAS/STE pathway via plasmids containingthe STE11-4 or RAS2-Val19 mutations or overexpressing STE12 suppressedboth the impaired filamentation and the decreased cell elongationof swe1/swe1 and CDC28-T18A, Y19F mutants (Figure 4A). Finally,the double-mutant diploid carrying CDC28-T18A, Y19F and STE11-4showed enhanced filamentous growth (Figure 4B). Like the STE11-4strain, it showed enhanced agar invasion, highly elongated cellsthat remain attached in clusters, and a G2/M cell cycle shift(Figure 4, C-E). Furthermore, we confirmed our previous observations(Kron et al., 1994) that CDC28-T18A, Y19F is dominant with respectto SWE1. Overexpression of SWE1 via an integrated copy of a fusionbetween the inducible GAL1,10 promoter and SWE1 (Booher et al.,1993) did not significantly delay cell division or alter filamentousgrowth in the CDC28-T18A, Y19F mutant. These data suggest thatthe RAS/STE pathway and Cdc28 tyrosine phosphorylation are independentpathways modulating filamentous growth.

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Figure 4. The RAS/STE pathway and Cdc28 tyrosine phosphorylation independently modulate filamentous growth. (A) Filament formation of Cdc28 tyrosine phosphorylation mutants with altered RAS/STE function on synthetic nitrogen (SC) or nitrogen starvation (SLAD) agar. Mutants with decreased tyrosine phosphorylation lacking the inhibitory Swe1 kinase or its phosphorylation site on Cdc28 (swe1/swe1 and CDC28-T18A, Y19F [AF]) show impaired filamentous development on SC and SLAD media compared with the wild-type strain. On the other hand, lack of the reactivating phosphatase Mih1 (mih1/mih1) confers constitutively increased Cdc28 tyrosine phosphorylation and a moderately enhanced filamentous phenotype. Plasmids expressing the STE11-4 or RAS2-Val19 allele suppress the impaired filamentation of both the swe1/swe1 and CDC28-T18A, Y19F strains and further enhance the filamentous phenotype of mih1/mih1 strains. (B) STE11-4/STE11-4 CDC28-AF/CDC28-AF double mutants on YPD or SLAD agar. The nonphosphorylatable CDK mutant CDC28-T18A, Y19F does not block an ectopic RAS/STE signal. (C) Agar invasion assay. Cells were treated as described in Figure 1B. Like the STE11-4 mutant, the double mutant is hyperinvasive in YPD agar. (D) Cell morphology in liquid YPD media. Highly elongated cells that grow as adherent cell aggregates reminiscent of the STE11-4 florets are apparent in STE11-4/STE11-4 CDC28-AF/CDC28-AF double mutant cultures. Bars, 50 µm. (E) Flow cytometry. Cells were prepared as described in MATERIALS AND METHODS. The STE11--4/STE11-4 CDC28-AF/CDC28-AF double mutant reveals a marked shift to 4N DNA content relative to the CDC28-AF/CDC28-AF control and comparable to that of the STE11-4/STE11-4 mutant alone.

Altered Cyclin Expression Modulates Filamentous Growth

Although control of mitotic anaphase by the RAS/STE pathway may not involve regulation at the level of tyrosine phosphorylation,other modes of regulation of MPF cannot be eliminated. One limitingfactor for completion of mitosis is the accumulation of the functionallyredundant mitotic cyclins Clb1 and Clb2. We examined whether alteringthe activity of mitotic kinase by changing the expression of mitoticcyclins might have a significant effect on filamentousdevelopment.

Previous studies have shown that deletion or moderate overexpression of either CLB1 or CLB2 has only subtle effects on cellgrowth on rich media (but see Stueland et al., 1993). To testwhether altered mitotic cyclin expression might differentiallyaffect filamentous development, we constructed diploid cells deficientfor either the CLB1 or CLB2 gene. In contrast to other geneticbackgrounds, diploid $Sigma$ 1278b cells carrying a homozygous deletionof CLB2 exhibited several characteristics of filamentous developmenteven when grown on rich complete media. When inoculated on YPDagar, clb2/clb2 cells initially formed microcolonies consistingof mostly filamentous cells (Figure 5A). When patches of Clb2-deficientcells were inoculated on YPD agar and allowed to grow for severaldays, they displayed increased cell adhesion (rough surface andgranular consistency) and enhanced agar invasion (Figure 5B) comparableto that displayed by the STE11-4 strain.

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Figure 5. Mutations in mitotic control genes modulate filamentous differentiation. The clb2/clb2 mutant exhibits exaggerated filamentous development and a growth pattern similar to that of the STE11-4 mutant. (A) Both the strain carrying the ts mitotic arrest allele cdc28-1N and the strain deficient in CLB2 exhibit filamentous growth on YPD media and are further induced by nitrogen starvation. Photographs show representative colonies of each strain after 24 h at 22°C. (B) Agar invasion assay. Cells lacking CLB2 have enhanced YPD agar invasion comparable to that displayed by the STE11-4 mutant. (C) Cell morphology in liquid YPD media. The clb2/clb2 strain grows as highly elongated cells that remain attached in clusters, reminiscent of the STE11-4 mutant. Bars, 50 µm. (D) Cell cycle kinetics. Like STE11-4 cells, CLB2-deficient cells demonstrate a predominance of cells with G2/M DNA content. (E) Deficiency in mitotic Cdc28 activity conferred by deficiency in the Clb2 mitotic cyclin dramatically enhances filamentous growth on both synthetic nitrogen (SC) and nitrogen starvation (SLAD) media. Activation of the RAS/STE pathway via plasmids containing STE11-4 or RAS2-Val19 augments the striking cell elongation phenotype of these strains. Bars, 50 µm.

In liquid YPD media, the clb2/clb2 mutant cells were heterogeneous, with an unusual number of elongated cells that grew asadherent cell aggregates reminiscent of the STE11-4 florets (Figure5C). Flow cytometry revealed a marked shift to cells with 4N DNAcontent (Figure 5D). When inoculated onto SLAD, the clb2/clb2mutant exhibited remarkable filamentous growth characterized byhighly elongated cells and very few rounded cells in the colonies(Figure 5A), a growth pattern similar to that of the STE11-4mutant.

Cells lacking Clb2 are specifically sensitized to the RAS/STE signal. When [CEN RAS2-Val19] or [CEN STE11-4] was introducedinto the clb2/clb2 mutant cells, a compound effect of dramaticcell elongation and striking filamentation was observed on SLADmedia (Figure 5E). Further supporting the hypothesis that diploidcells lacking Clb2 are sensitized to the filamentous growth-inducingsignal, we observed that when this mutant is grown in the presenceof high-ammonia-containing synthetic media, the cells adopt arounded shape like that of a wild-type control strain. This suggeststhat 1) the elongated phenotype on YPD media, a nitrogen sourcerelatively low in ammonia but rich in short peptides and othercomplex forms of nitrogen, may be due to low but significant basalactivity of the signaling pathway, and 2) the presence of ammonianitrogen might actively repress the signaling pathway, ratherthan starvation for ammonia nitrogen inducing itsfunction.

Using the same logic that prompted examination of the Clb2 mutant, we tested whether a strain lacking the Clb1 cyclin mightalso demonstrate induced filamentous growth. A diploid Clb1 mutantconstructed by deletion of both CLB1 alleles showed few or norich media phenotypes and less cell cycle shift but a moderateinduction of filamentous growth on SLAD. This induction was furtherincreased by transformation with the [CEN RAS2-Val19] or [CENSTE11-4]inducer.

To confirm that the effects of the CLB1 and CLB2 deletions were mediated via reduced activation of the Cdc28 CDK, we examinedthe effect of substituting the temperature-sensitive G2 arrestallele, cdc28-1N, for wild-type CDC28 in an otherwise wild-typestrain. Like the Clb2-deficient strain, when grown at a permissivetemperature the cdc28-1N/cdc28-1N strain exhibited significantcell elongation on YPD media and dramatic filamentous growth onSLAD low-nitrogen media (Figure 5A). The [CEN STE11-4]- and [CENRAS2-Val19]-inducing plasmids further enhanced this filamentousphenotype (Figure 5E).

To study the effect of overexpression of mitotic cyclins, we constructed strains carrying integrated copies of fusions betweenthe inducible GAL1,10 promoter and the CLB1 and CLB2 cyclin genes.Although diploid cells carrying an integrated GAL1::CLB2 constructexhibited normal filamentous growth on repressing SLAD agar media,induction of Clb2 overexpression by inoculating cells onto syntheticlow-ammonia galactose agar media abrogated filamentous growth.Rather than forming the chains of elongated cells characteristicof filamentous growth, these cells formed piles of rounded cells(Figure 6). Diminution of filamentous growth was also observedin cells overexpressing the Clb1 cyclin, whereas overexpressionof the Clb3, Clb4, or Clb5 cyclin had only modest effects on PHgrowth. Finally, overexpression of Clb1 and Clb2 suppressed thefilamentous phenotype of cdc28-1N cells (data not shown).

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Figure 6. Overexpression of the Clb1 and Clb2 mitotic cyclins abrogates filamentous development and antagonizes RAS/STE signaling. Strains containing integrated copies of the CLB1 and CLB2 genes under an inducible GAL1,10 promoter and a control plasmid or the STE11-4 or RAS2-Val19 allele were grown on nitrogen starvation (SLAD) or synthetic low-ammonia galactose (SLARG) media for 24 h. Both basal and enhanced filamentous growth are abolished by Clb1 or Clb2 overexpression on SLARG media, indicating that the RAS/STE pathway may function upstream of Clb1 and Clb2. Representative colonies of each strain were photographed after 24 h at 22°C. Bars, 50 µm.

These data suggest that the mitotic cyclin Clb2 performs a function in direct antagonism to the RAS/STE pathway. However,although mitotic cyclins may be negatively regulated at some levelby the RAS/STE pathway, these results do not indicate that eitherClb1 or Clb2 is the sole target of the RAS/STE pathway in thecontrol ofanaphase.

One biochemical mechanism consistent with the genetic results described above is that the cell cycle shift observed upon ectopicactivation of the RAS/STE pathway, as in the STE11-4 mutant, mightbe due to down-regulation of the Clb2 cyclin. A lower cellularcontent of Clb2 would result in a proportional decrease in Clb2-dependentCdc28 kinase and thereby slow mitotic entry. Furthermore, lowcellular Clb2 content would predict the observed similarity inphenotypes between STE11-4-expressing cells and Clb2-deficientcells. Protein extracts were prepared from asynchronous culturesof cells grown on rich YPD media. When we compared levels of Clb2protein in extracts derived from the wild-type, Ste11-deficient,Clb2-deficient, and STE11-4-expressing strains, we observed theexpected absence of Clb2 protein from the Clb2-deficient strain.However, the other strains showed equal levels of expression ofClb2 irrespective of genotype (Figure 7), suggesting that theRAS/STE pathway might have little or no effect on Clb2 cyclinexpression or stability.

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Figure 7. Modulating RAS/STE signaling regulates filamentous growth without altering Clb2 abundance. The anti-PSTAIRE mAb recognizing Cdc28 was used as a loading control. Western analysis of Clb2 and Cdc28 reveals that Clb2 levels are relatively unaffected by RAS/STE signals. WT, wild type.

Epistasis Experiments Place Clb2 Downstream of the RAS/STE Pathway

Were the RAS/STE pathway genetically upstream of Cdc28 and Clb2, one inference would be that loss of function in Clb2, whichconfers enhanced filamentous growth, might suppress the decreasedfilamentous growth observed in mutants lacking components of theRAS/STE pathway. We examined mutants lacking the STE20 MEK kinasekinase, the STE11 MEK kinase, and the STE7 MEK. As previouslyreported (Liu et al., 1993), ste7/ste7 and ste12/ste12 mutantseach confer decreased filamentous development, and ste20/ste20mutants display complete loss of filamentous growth (Figure 8A).Furthermore, all of these mutants were readily washed off theagar with flowing water (Figure 8B) and failed to grow in suspensionculture as adherent cell aggregates (Figure 8C). We constructedmutant strains that combined each of the STE kinase mutationswith deletion of the CLB2 cyclin gene and examined their filamentousphenotypes. We found that the ste20/ste20 clb2/clb2, ste7/ste7clb2/clb2, and ste12/ste12 clb2/clb2 double mutants all exhibiteda limited form of filamentous differentiation when placed underinducing conditions of low-nitrogen agar (Figure 8A). All of thesemutants showed partial agar invasion (Figure 8B) and an elongatedcell phenotype (Figure 8C), even in liquid media. By comparison,the ste20/ste20 clb2/clb2 double mutant showed only a very subtlesuppression. The flow cytometry profiles for each double mutantshowed a significant shift toward the 4N DNA content (Figure 8D),and we observed a decrease in the population of anaphase cells(Figure 3). Thus, the bypass of the STE pathway blockade effectedby a deletion of CLB2 was partial but nonetheless significant.

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Figure 8. Bypass of mutations in the RAS/STE pathway by Clb2 deficiency. (A) STE20-, STE7-, and STE12-deficient mutants have a decreased filamentous development phenotype. Cells lacking both the Ste20 PAK kinase and the Clb2 mitotic cyclin show only a very subtle suppression, whereas double mutants lacking Ste20 and Clb2, Ste12 and Clb2, or Ste7 and Clb2 exhibit limited filamentous growth on both rich YPD media and low-nitrogen SLAD media. These phenotypes suggest partial bypass of the RAS/STE pathway. Photographs show representative colonies of each strain after 24 h at 22°C. (B) Agar invasion assay. Double mutants lacking both Clb2 and components of the RAS/STE pathway exhibit partial invasion, but ste7/ste7, ste12/ste12, and ste20/ste20 mutants confer decreased agar invasion. (C) Cell morphology in liquid YPD media. ste7/ste7 clb2/clb2, ste12/ste12 clb2/clb2, and ste20/ste20 clb2/clb2 double mutants display limited cell elongation, but to a greater degree than ste7/ste7, ste12/ste12, and ste20/ste20 mutants. Bars, 50 µm. (D) Cell cycle kinetics. A shift toward G2/M DNA content is apparent in cells deficient in both Clb2 mitotic cyclin and elements of the RAS/STE pathway.

A complementary test to reveal order of function was to examine whether the induction of filamentous growth by a dominantactive allele of a component of the RAS/STE pathway could overridethe inhibitory effect of Clb1 or Clb2 overexpression. We foundthat cells carrying the integrated GAL1::CLB1 and GAL1::CLB2 constructsfailed to form filaments on low-nitrogen galactose-containingmedia, even if they also carried a [CEN RAS2-Val19] or [CEN STE11-4]plasmid (Figure 6). These data suggest that the RAS/STE pathwayindeed acts upstream of mitotic cyclins as part of the filamentousdifferentiationresponse.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Physiological study of filamentous growth has suggested that a change in cell cycle control is critical to the differentiationof rounded yeast cells into elongated filamentous cells. We setout to examine whether modulation of the cell cycle machinerymight be both necessary and sufficient for proper morphogenesisin filamentous growth. In particular, we asked whether other cell-autonomousfeatures of filamentous differentiation, such as elongated cellmorphology, polar budding, persistent cell connections, and agarinvasion, might be downstream of the cell cycleswitch.

The STE MAPK Pathway Regulates the G2/M Transition in Diploid Yeast Cells

Previous studies have shown that the low-nitrogen signal for filamentous growth is transduced via a dual signaling pathwayinvolving elements of the STE MAPK- and RAS GTPase/cAMP-dependentkinase cascades. A critical question is whether the cell cycleshift to G2/M in filamentous cells is downstream of the RAS/STE-signalingpathway or is an independent response to nitrogen starvation.The results described here establish a pathway linking the MAPK-signalingcascade directly to the cell cyclemachinery.

Our logic is based on the following argument. We have used a dominant activated mutant, STE11-4, to produce an ectopic, constitutivesignal that stimulates the filamentous development pathway, evenin the absence of nitrogen starvation or an agar substrate. Previousstudies (Liu et al., 1993) found that the STE11-4 mutation confersenhanced filamentous growth and promotes expression of the filamentoussignaling reporter, Ty1-lacZ (Mosch et al., 1996), via its FREelement in a low-nitrogen-independentmanner.

We extended these observations by creating diploid yeast strains in which the STE11-4 mutation is stably expressed from itsgenomic locus. As expected, these strains exhibit enhanced filamentousgrowth on low-nitrogen media and display high constitutive expressionof the Ty1-lacZ reporter. However, we found that such STE11-4strains express an ectopic filamentous growth phenotype, evenin rich liquid media. Because of persistent attachment to themother cell after septation, they grow as florets that may containdozens of cells. STE11-4 florets formed in rich liquid media areindistinguishable from microcolonies of wild-type cells growingon the surface of low-nitrogen agar. Thus, STE11-4 is sufficientto replace at least the nitrogen starvation and agar componentsof the conditions conducive to filamentous growth and to providea model system that reveals the RAS/STE pathway-specific aspectsof filamentousgrowth.

We examined these STE11-4 cells for markers of cell cycle progression known to be altered during filamentous differentiation.STE11-4 filamentous cells grown on rich liquid media are shiftedinto G2/M. Most cells were budded, many with a single nucleuslodged in the bud neck and a short mitotic spindle spanning thenucleus. Even though many cells had buds nearly equal in sizeto the mother cell, very few STE11-4 cells were observed withthe elongated mitotic spindle or separated nuclear masses suggestiveof anaphase. This finding suggests that a RAS/STE signal aloneis sufficient to produce the characteristic cell cycle of filamentousgrowth.

The RAS/STE-dependent Mitotic Delay Is Not Mediated by Cdc28 Tyr-19 Phosphorylation

A simple model, as suggested by Edgington et al. (1999), might explain the link between signal and cell cycle: the physiologicalpathway from nitrogen starvation to cell cycle may be via a MAPKcascade that promotes increased Tyr-19 phosphorylation of Cdc28.In fact, many observations are consistent with this model. Ectopicactivation of the Swe1 kinase by mutation of an inhibitory kinase(Edgington et al., 1999) or overexpression of the Swe1 kinaseor lack of the Mih1 phosphatase, as shown here, promote hyperphosphorylationof Cdc28 Tyr-19, delay mitotic onset, and enhance filamentousgrowth. Mutation of the Cdc28 Tyr-19 residue to Phe or deficiencyof the Swe1 kinase each promote mitosis and, as shown here, attenuatefilamentous growth. Nonetheless, we observed that the RAS/STEsignal can still induce ectopic filamentous development, evenin cells lacking the Swe1 kinase or expressing the dominant activeCDC28-T18A, Y19F mutant lacking the site for inhibitory tyrosinephosphorylation. Although our data and those of Edgington et al.(1999) demonstrate that regulation of Cdc28 tyrosine phosphorylationmodulates filamentous development, we find that this regulationis neither necessary nor sufficient to confer the mitotic delayor other effects induced by RAS/STE pathway activation. Furthermore,although nitrogen starvation may promote Cdc28 tyrosine phosphorylationand thereby contribute to differentiation, this regulation isnot essential for most aspects of filamentous differentiation,including the G2/M cell cycleshift.

Altered Cyclin Expression, Mitotic Cdc28 Activity, and Filamentous Development

Perhaps the most remarkable findings reported here and by Edgington et al. (1999) are that simple genetic manipulations tocreate strains deficient in or overexpressing a single mitoticcyclin are so altered in their developmental responses. Cellslacking the mitotic cyclin Clb2 are highly induced for filamentousgrowth. When inoculated onto low-nitrogen agar, Clb2-deficientcells form colonies of almost exclusively filamentous cells. Inturn, when inoculated onto rich complex agar media (YPD) or evenwhen grown on rich complex liquid media, Clb2 mutants remain highlyelongated, bud in a polar pattern, remain attached to their mothercells, and show a dramatic cell cycle shift to G2/M when assayedby flow cytometry. We find that these phenotypes derive in partfrom supersensitivity to the low-nitrogen signal. Activation ofthe RAS/STE pathway, as by the STE11-4 mutation, or expressionof RAS2-Val19 exacerbates the Clb2 mutant phenotype on low-nitrogenmedia.

That these effects are due to decreased activation of the mitotic forms of Cdc28 is indicated by the phenotypes conferredby the cdc28-1N ts mutation at a permissive temperature. At thenonpermissive temperature (37°C), cells carrying only cdc28-1Narrest before mitotic anaphase but with completed DNA synthesisand an assembled mitotic spindle (Surana et al., 1991). Overexpressionof mitotic cyclins suppresses this ts arrest. In turn, cells carryingboth cdc28-1N and a deficiency for CLB1 or CLB2 are nonviableeven at 22°C. This synthetic lethality demonstrates a criticaldefect in mitotic kinase activity in cdc28-1N mutants even atthe permissive temperature. When yeast cells carrying the cdc28-1Nmutation were inoculated onto low-nitrogen media and culturedat a permissive temperature, like the Clb2-deficient cells, theywere hyperfilamentous. Furthermore, when superstimulated by expressionof the STE11-4- or RAS2-Val19-inducing mutations, like the Clb2-deficientcells, the cdc28-1N mutants displayed a dramatically enhancedfilamentousphenotype.

As noted above, Myers and colleagues (Edgington et al., 1999) have shown that filamentous growth is modulated by Cdc28 function,but they focus on mitotic functions. They isolated a Cdc28 mutant,cdc28-127 C127Y, that causes constitutive expression of most filamentousgrowth characteristics, such as enhanced cell polarity, elongatedshape, and G2/M cell cycle delay. Like cdc28-1N, cdc28-127 isdefective in mitotic progression. Their data confirm our observationsthat altered Clb1,2/Cdc28 activity can modulate filamentous growthindependent of signal transduction. In contrast to the resultsreported here, their data indicate a significant role for Cdc28Tyr-19 phosphorylation by Swe1 kinase in filamentous differentiation.However, as cdc28-127 remains subject to regulation by Tyr-19phosphorylation, their data also suggest that there may be multiplemeans of regulating CDK activity to promote filamentousdifferentiation.

In reciprocal experiments, we determined that hyperactivity of mitotic cyclins and, by inference, high activity of mitotickinase can abrogate filamentous development directed by RAS/STEsignaling. Cells overexpressing Clb1 or Clb2 maintain a roundcell shape and a nonfilamentous growth pattern even in the faceof maximal stimulation provided by the nutritional signal of low-nitrogenmedia combined with dominant active mutations in the RAS/STE signalingpathway. In turn, overexpression of the Clb1 or Clb2 cyclin doesnot repress the low-nitrogen-induced expression of a FRE reporter(our unpublished results). These data suggest that 1) mitoticfunctions of the Cdc28 CDK are a critical target of the RAS/STEsignal, and 2) repression of mitotic kinase is both necessaryand sufficient to induce a coordinated developmental switch characterizedby elongated cell shape, polar budding, persistent cell attachment,and G2/M cell cycle delay. This pattern recapitulates key featuresof filamentous differentiation as stimulated by the physiologicalsignal.

Rather than proving a direct pathway that links RAS/STE to mitotic cyclins, we cannot eliminate the possibility that the effectsof altered cyclin activity on filamentous growth, like the effectsof modulating Cdc28 Tyr-19 phosphorylation, are simply evidencefor a parallel pathway regulating morphogenesis. Other data linkingthe Cln1 and Cln2 G1 cyclins to filamentous differentiation suggestthat their effects may be quite direct, serving as modulatorsof the RAS/STE response in the signaling pathway (Oehlen and Cross,1998) and/or as pathway-independent activators of gene expression(Loeb et al., 1999). Nonetheless, neither mechanism adequatelyaddresses the origin of the mitotic delay or its regulation byRAS/STE signals. We propose an alternative model whereby the RAS/STEpathway directly effects repression of mitotic kinase activityin diploid cells. Our hypothesis is based on the paradigm of pheromoneresponse, in which distinct gene products induced by the STE MAPKpathway mediate cell surface (Fus1) and cell cycle (Far1) aspectsof differentiation. Far1 serves as an inhibitor of Cln1,Cln2-dependentCdc28 activity and thereby enforces the G1 arrest of conjugatinghaploid cells. We imagine a functional equivalent for Far1 actingdownstream of the RAS/STE pathway to enforce its cell cycle effects.Coordinately with expression of the cell surface flocculin Flo11that is required for the increased cell adhesion in filamentousgrowth, this hypothesized gene product would be under FRE controlso that it would be induced in diploid cells upon activation ofthe RAS/STE pathway to mediate the mitotic delay. As we did notobserve any decrease in the steady-state abundance of Clb2 proteinin our STE11-4 cells, we suppose that activation of the RAS/STEpathway neither decreases expression nor increases destructionof mitotic cyclins. An alternative biochemical activity of thisfactor might be direct, stoichiometric inhibition of Clb1- andClb2-dependent Cdc28 mitotic kinase activity. As a preliminaryexperiment to detect regulation at the level of Cdc28 activity,we assayed precipitates of extracts derived from asynchronouscultures of wild-type and RAS/STE pathway mutant yeast strainsfor histone H1 phosphorylation to quantitate CDK activity. Initialresults suggest that although total, p13^suc1-associated CDK activity may be unaltered, Clb2-associated Cdc28activity in STE11-4 cells appears relatively depressed (our unpublishedresults). Confirmation and characterization of this apparent mitoticinhibition remain to be pursued. In turn, genetic studies mayreveal mutations that do not block Flo11 expression but preventdown-regulation of the mitotic activity of Cdc28. Such studieswould provide the critical evidence for the hypothesized factorcoupling the gene expression program induced by the RAS/STE filamentoussignaling pathway to its effects on cell cycleprogression.

	ACKNOWLEDGMENTS

We thank Ankit Desai for technical assistance. Preliminary studies leading to the results reported here were completed byS.J.K. while a postdoctoral fellow with Gerald R. Fink at theWhitehead Institute (Cambridge, MA). S.J.K. gratefully acknowledgesDr. Fink for his generous support, guidance, and scientific insightsand Cora Styles for help with strain constructions and valuablesuggestions. We thank A. Amon, R. Booher, B. Errede, D. Lew, H.Liu, H.-U. Mosch, S. Reed, and P. Russel for reagents and helpfulcomments. This work was supported by grants to S.J.K. from theArnold and Mabel Beckman Foundation, the Horace W. Goldsmith Foundation,the Cancer Research Foundation, and funds from a Howard HughesMedical Institute Research Resources for Medical Schools grantto the University ofChicago.

	FOOTNOTES

^* These two authors contributed equally to thismanuscript.

Corresponding author. E-mail address: skron{at}midway.uchicago.edu.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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