Global Roles of Ssn6 in Tup1- and Nrg1-dependent Gene Regulation in the Fungal Pathogen, Candida albicans

Susana García-Sánchez^*, Abigail L. Mavor, Claire L. Russell, Silvia Argimon, Paul Dennison, Brice Enjalbert, and Alistair J.P. Brown

Aberdeen Fungal Group, School of Medical Sciences, University of Aberdeen, Institute of Medical Sciences, Foresterhill, Aberdeen AB25 2ZD, United Kingdom

Submitted January 26, 2005; Revised March 25, 2005; Accepted March 30, 2005
Monitoring Editor: Thomas Fox

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

In budding yeast, Tup1 and Ssn6/Cyc8 form a corepressor thatregulates a large number of genes. This Tup1-Ssn6 corepressorappears to be conserved from yeast to man. In the pathogenicfungus Candida albicans, Tup1 regulates cellular morphogenesis,phenotypic switching, and metabolism, but the role of Ssn6 remainsunclear. We show that there are clear differences in the morphologicaland invasive phenotypes of C. albicans ssn6 and tup1 mutants.Unlike Tup1, Ssn6 depletion promoted morphological events reminiscentof phenotypic switching rather than filamentous growth. Transcriptprofiling revealed minimal overlap between the Ssn6 and Tup1regulons. Hypha-specific genes, which are repressed by Tup1and Nrg1, were not derepressed in ssn6 cells under the conditionsstudied. In contrast, the phase specific gene WH11 was derepressedin ssn6 cells, but not in tup1 or nrg1 cells. Hence Ssn6 andTup1 play distinct roles in C. albicans. Nevertheless, bothSsn6 and Tup1 were required for the Nrg1-mediated repressionof an artificial NRE promoter, and lexA-Nrg1 mediated repressionin the C. albicans one-hybrid system. These observations areexplained in models that are generally consistent with the Tup1-Ssn6paradigm in budding yeast.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Transcriptional repression plays a key role in controlling thegrowth and differentiation of eukaryotic cells. The fundamentalimportance of negative transcriptional regulators is reflectedin their conservation during eukaryotic evolution. For example,orthologues of the Ssn6 (Cyc8) and Tup1 proteins, which actas global repressors in Saccharomyces cerevisiae, have beenidentified in humans, flies, worms, slime molds, and fungi (reviewedby Smith and Johnson, 2000).

Our understanding of the mechanisms of action of Ssn6 and Tup1is based largely on studies in budding yeast. The S. cerevisiaeparadigm suggests that Ssn6 and Tup1 interact physically toform a corepressor complex that actively represses the transcriptionalmachinery (Williams et al., 1991; Redd et al., 1997; Gounalakiet al., 2000). The relevance of this paradigm to eukaryotesin general is emphasized by the observation that yeast Ssn6can interact with human Tup1-like proteins to mediate transcriptionalrepression in human cells (Grbavec et al., 1999).

The Ssn6-Tup1 corepressor is thought to repress transcriptionin yeast by two main mechanisms. First, the corepressor is thoughtto remodel chromatin on yeast promoters by recruiting histonedeacetylases to these promoters and by positioning nucleosomesvia direct interactions with histone tails (Edmondson et al.,1996; Davie et al., 2002, 2003; Zhang and Reese, 2004a). Second,Tup1 is thought to interact directly with the transcriptionalmachinery to attenuate its activity (Carlson, 1997; Redd etal., 1997; Gromoller and Lehming, 2000; Papamichos-Chronakiset al., 2000). Recent experiments suggest that both mechanismsoperate in yeast, but that they are utilized differentiallyto regulate distinct sets of yeast genes (Green and Johnson,2004). However, both mechanisms appear to operate in a redundantmanner to repress some yeast genes (Green and Johnson, 2004;Zhang and Reese, 2004b). In addition, Ssn6-Tup1 presumably regulatesthe expression of other genes indirectly by controlling thelevels of transcriptional activators or repressors that actdirectly on these genes.

The Ssn6-Tup1 corepressor complex does not interact with DNAdirectly. Instead the complex is targeted to specific promotersthrough interactions with sequence-specific DNA-binding proteins(Keleher et al., 1992; Smith and Johnson, 2000). For example,Mig1 and Nrg1 target Ssn6-Tup1 to glucose-repressed genes, whereasthe a1/ ${alpha}$ 2 heterodimer targets the corepressor complex to haploid-specificgenes in S. cerevisiae. In contrast, Rox1 and Crt1 target Ssn6-Tup1to hypoxia- and DNA damage-inducible genes in budding yeast.Therefore, Ssn6-Tup1 regulates the expression of functionallydiverse sets of yeast genes via interactions with differentDNA-binding proteins.

Ssn6-Tup1-mediated repression is generally controlled by regulatingthe levels or activities of these DNA-binding proteins (Smithand Johnson, 2000). For example, a1/ ${alpha}$ 2 levels are controlledprimarily at the transcriptional level in S. cerevisiae: a1and ${alpha}$ 2 are synthesized by the MATa and MAT ${alpha}$ loci, respectively,and hence the a1/ ${alpha}$ 2 heterodimer only forms in diploid cells.In contrast, the activity of Mig1 and Crt1 are regulated posttranscriptionally:the DNA-binding activity of Crt1 is inhibited by hyperphosphorylation,and the phosphorylation of Mig1 inhibits its interaction withSsn6-Tup1 and leads to its export from the nucleus (Huang etal., 1998; Ostling and Ronne, 1998; Papamichos-Chroakis et al.,2004).

Ssn6 and Tup1 play different roles within the corepressor complex.Tzamarias and Struhl (1994) reported that the transcriptionalrepression mediated by a LexA-Ssn6 fusion in yeast was dependenton Tup1, whereas LexA-Tup1 repressed transcription even in theabsence of Ssn6. Furthermore, the mating defect of yeast tup1ssn6 cells can be suppressed by Tup1 overexpression, but notby Ssn6 overexpression (Komanchi et al., 1994). Hence, Tup1is thought to mediate the transcriptional repression, whereasSsn6 is thought to stabilize the interaction between Tup1 andthe DNA-binding protein. As described above, a diverse set ofSsn6-Tup1-targeting proteins have been identified in S. cerevisiae.These diverse proteins appear to interact with different regionsof the Ssn6-Tup1 corepressor complex (Komanchi et al., 1994;Tzamarias and Struhl, 1995; Smith and Johnson, 2000). For example,Rox1 and Mig1 contact different regions of the Ssn6 proteinwithin the Ssn6-Tup1 corepressor, whereas ${alpha}$ 2 is thought to contactTup1 directly (Komanchi et al., 1994; Tzamarias and Struhl,1995).

Candida albicans is the major systemic fungal pathogen of humans(Odds, 1988; Calderone, 2002). This fungus causes oral and vaginalcandidiasis and life-threatening blood-stream infections inimmunocompromised patients. Braun and Johnson (1997) were thefirst to reveal the importance of transcriptional repressionin the regulation of C. albicans virulence attributes by showingthat Tup1 represses hyphal development in this fungus. Tup1was subsequently shown to repress the transcription of hypha-specificgenes (i.e., genes that are expressed specifically during thehyphal growth phase of C. albicans; Sharkey et al., 1999; Braunand Johnson, 2000; Braun et al., 2000, 2001; Murad et al., 2001a;Zheng et al., 2004). This was confirmed by a transcript profilingstudy that examined the effects of inactivating Tup1 or theTup1-targeting protein, Nrg1, upon the expression of about one-thirdof C. albicans genes (Murad et al., 2001a, 2001b). This studyalso revealed that both Tup1 and Nrg1 play broader roles bycoordinating yeast-hypha morphogenesis with the expression ofother virulence attributes in this pathogen. Not surprisingly,a tup1 mutant displayed attenuated virulence in the mouse modelof systemic candidiasis (Murad et al., 2001a). Hence transcriptionalrepression, and Tup1 in particular, is an important regulatorof C. albicans virulence.

On the basis of the S. cerevisiae Ssn6-Tup1 paradigm, we andothers predicted that C. albicans Ssn6 would play an importantrole in Tup1-mediated transcriptional repression in this fungus(Smith and Johnson, 2000; Garcia and Brown, 2001). We have testedthis prediction by examining the cellular and molecular phenotypesof C. albicans ssn6 mutants. During the course of this studyHwang et al. (2003) reported in an elegant article that Ssn6regulates yeast-hypha morphogenesis and virulence in C. albicans.They suggested that complex relationships exist between Ssn6and the MAP kinase and cAMP-protein kinase A signaling pathwaysthat activate morphogenesis in C. albicans. They also reportedsubtle differences in the morphological phenotypes of ssn6 andtup1 mutants, suggesting that Ssn6 might play distinct rolesin C. albicans morphogenesis (Hwang et al., 2003). We show that,although ssn6 cells do display morphogenetic defects, thesedefects are distinct from those of tup1 or nrg1 cells and morereminiscent of phenotypic switching than yeast-hypha morphogenesis.We also show that although Ssn6 contributes to Tup1- and Nrg1-mediatedrepression at some promoters, Ssn6 is not essential for therepression of most Tup1- or Nrg1-regulated genes in C. albicans.The data suggest that Ssn6 executes roles that are independentof the Ssn6-Tup1 corepressor. These observations have importantimplications for the eukaryotic Ssn6-Tup1 paradigm.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Strains and Growth Conditions
C. albicans strains (Table 1) were grown in YPD, SD, SC (Sherman,1991, Kaiser et al., 1994), YPDA (YPD containing 0.01% adenine)or YPDAU (with 0.02% adenine and 0.008% uridine). Hyphal developmentwas stimulated using YPD containing 10% serum at 37°C. Celland colony morphology were analyzed using Olympus BX50 (LakeSuccess, NY) and Zeiss stereo microscopes (Thornwood, NY) asdescribed previously (Murad et al., 2001a).

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Table 1. C. albicans strains

Complementation tests were performed using the S. cerevisiaessn6 strains MAP6, which was a generous gift from Markus Proft,and PHFT5 (Tzamarias and Struhl, 1994; Loubradou et al., 2001).C. albicans SSN6 was cloned as a 6-kb EcoRI fragment into YCp50,and the phenotypes of YCp50-SSN6 and YCp50-containing S. cerevisiaePHFT5 cells were compared.

Both alleles of the SSN6 locus were sequentially disrupted inC. albicans CAI8 by Ura-blasting (Fonzi and Irwin, 1993) usinga ssn6::hisG-URA3-hisG cassette that deleted codons 385-955of the 1081 codon ORF (Table 1). To generate this cassette thehisG-URA3-hisG was cloned between the KpnI and HindIII sitesof a 6.2-kb PstI fragment from the SSN6 gene. The genotypesof homozygous ssn6/ssn6 mutants were confirmed by Southern blottingand PCR analysis (unpublished data). Eight independent ssn6/ssn6mutants were generated, all with similar phenotypes (unpublisheddata). Uridine auxotrophic mutants were generated by selectingura3 segregants on YPD containing 1 mg/ml 5-fluoroorotic acid(Fonzi and Irwin, 1993). SSN6 was also disrupted in C. albicansHLC54ura3 to generate the triple ssn6/ssn6 cph1/cph1 efg1/efg1mutant, SGC134 (Table 1). A conditional ssn6 mutant, SGC179,was generated by inactivating one SSN6 allele and placing theremaining SSN6 allele under the control of the C. albicans MET3promoter (Care et al., 1999). Again, the genotype of this ssn6/MET3-SSN6strain was confirmed by Southern blotting and PCR analysis (unpublisheddata). The expression of MET3-SSN6 allele was repressed using2.5 mM methionine and cysteine.

To create the NRE reporter, the sequence 5'-GTCGACGGATCCGCTAGCCCCCCTGACTGCTACCATCCCCCTAAATCGGATCCGCCCCCTTGCGAACAAGTCCCCCCTGCCTTGAACGAACTGCAG(SalI and PstI sites in italics; four C₅T NRE elements underlined)was cloned between the SalI and PstI sites upstream in plac-basal.This plasmid contains the basal ADH1 promoter region (Tripathiet al., 2002) cloned upstream of the Streptococcus thermophiluslacZ reporter (Uhl and Johnson, 2001) in CIp10 (Murad et al.,2000). A second NRE reporter was generated with two A₂C₃T andtwo C₅T elements. A single copy of each plasmid was integratedinto the XbaI-plus allele of RPS1 (Murad et al., 2000). (RPS1was previously known as RPS10 and RP10.)

To use the C. albicans one-hybrid system (Russell and Brown,2005), an expression vector encoding a Staphylococcus aureusLexA-C. albicans Nrg1 protein fusion was constructed by PCRamplification of the NRG1 ORF and inserting it into CIp-LexA,to create CIp-LexA-Nrg1. The 5' PCR primers used introduceda (Gly)₃-Pro-(Gly)₂ linker between the amino-terminal LexA domainand the carboxy terminal domains of Nrg1. CIp-LexA and CIp-LexA-Nrg1were introduced into C. albicans reporter strains that carriedpCR-lacZ (no lexA operator upstream of basic ADH1 promoter)or pCR-OplacZ (containing the lexA operator) integrated intothe ade2::hisG locus (Doedt et al., 2004). The one-hybrid systemrequires both URA3 and ADE2 markers for the CIp- and pCR-basedplasmids, respectively. Hence the analyses were performed inderivatives of CAI8 (Table 1). The nrg1 and ssn6 mutants wereMMC9 and SGC124. The tup1 mutant, CRC004, was created in CAI8by Ura-blasting (Fonzi and Irwin, 1993) using the same tup1::hisG-URA3-hisGcassette that was used to generate the original C. albicanstup1 mutants in CAI4 (Braun and Johnson, 1997).

DNA, RNA, and Protein Analyses
Southern, Northern (Murad et al., 2001a), and Western blotting(Cormack et al., 1997) were performed as described previously.RT-PCR was performed using standard methods using the intron-containingEFB1 product to control for loading and genomic DNA contamination(Schaller et al., 1998). To measure lacZ reporter activity,X-gal overlay assays and liquid ${beta}$ -galactosidase assays were performedas described previously and expressed in Miller units (Rupp,2002).

Transcript Profiling
Transcript profiling was performed using congenic C. albicansstrains: wild-type, CAI4 and CAI8; nrg1, MMC4; tup1, BCA2-9;ssn6, SGC124 (Table 1). For consistency, the nrg1, tup1, andssn6 strains were compared directly to CAI4. Then, to controlfor possible differences between CAI4 and CAI8, these strainswere compared directly. Cells were grown to midexponential phase(OD₆₀₀ = 0.6-0.8) in YPDAU at 30°C. The cells were thenharvested, frozen rapidly in liquid N₂, sheared mechanicallyusing a microdismembrator (Braun Melsungen, Germany) and RNAprepared by extraction with Trizol Reagent (Gibco-BRL), as describedpreviously (Hauser et al., 1998). Cy3- and Cy5-labeled cDNAswere prepared from total RNA, and the probes were hybridizedwith (nearly) whole genome C. albicans microarrays (Eurogentec,Seraing, Belgium). Slides were scanned using a ScanArray Litescanner (PerkinElmer Life Sciences, Beaconsfield, United Kingdom)and quantified using QuantArray software (version 2.0). Datanormalization and analysis were performed using GeneSpring (SiliconGenetics, Redwood City, CA), and statistical analysis was performedusing SAM (Significance Analysis of Microarrays: Tusher et al.,2001). Data from at least three independent biological replicateswere used for each analysis, and the SAM False Discovery Ratewas set at 10%. Expression ratios for each gene that displayeda reproducible and statistically significant change in expressionin mutant cells relative to the wild-type control are availablein the Supplementary Data and at the Galar Fungail website (http://www.pasteur.fr/recherche/unites/Galar_Fungail/;http://www.galarfungail.org/data.htm). C. albicans gene annotationswere obtained from CandidaDB (http://genolist.pasteur.fr/CandidaDB:d'Enfert et al., 2005). Functional categories for C. albicansgenes were assigned mainly on the basis of the MIPS functionalassignments for S. cerevisiae homologues (http://mips.gsf.de/proj/yeast/CYGD/db/index.html:Yin et al., 2004). Genes were assigned to a new virulence categorywas based on the functional analysis of putative virulence attributesin C. albicans.

Chromatin Immunoprecipitation Assays
Polyclonal rabbit anti-peptide antibodies were raised againstthe carboxy-terminal region of C. albicans Ssn6 using the peptideCMRKIEEDENYDDE (Diagnostics Scotland, Carluke, United Kingdom).The specificity of the anti-Ssn6 antiserum was confirmed byWestern blotting of protein extracts from C. albicans wild-typeand ssn6 cells (unpublished data). Chromatin immunoprecipitation(ChIPs) was performed in triplicate (Strahl-Bolsinger et al.,1997) comparing preimmune and anti-Ssn6 antisera and comparingC. albicans wild-type and ssn6 cells.

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

C. albicans Ssn6 Is Related to Ssn6-like Proteins in Other Eukaryotes
As reported by Hwang et al. (2003), C. albicans has a singlelocus with significant sequence similarity to S. cerevisiaeSSN6 (orf19.6798; IPF5957.1). This gene encodes a 1081 aminoacid protein, which contains nine tetratricopeptide (TPR) repeatsbetween amino acids 98 and 430. An additional degenerate TPR-likesequence lies between TPR repeats six and seven (Figure 1).This TPR region of the C. albicans Ssn6 protein is closely relatedto the corresponding regions of Ssn6-like proteins from otherfungi, slime molds, flies, worms, and mammals (Figure 1). However,the sequence similarity between these Ssn6-like proteins isrelatively low outside the TPR region. The TPR repeats in S.cerevisiae Ssn6 mediate protein-protein interactions with Tup1and with Ssn6-Tup1 targeting proteins (Tzamarias and Struhl,1995).

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Figure 1. Ssn6-like proteins in eukaryotes. (A) S. cerevisiae paradigm of Ssn6-Tup1 function. (B) Arrangement of TPR repeats in Ssn6-like proteins from C. albicans, S. cerevisiae, Ustilago maydis, Schizosaccharomyces pombe, Dictyostelium discoideum, humans, Drosophila melanogaster, and Caenorhabditis elegans. Coordinates of TPR domains are shown, and percentage amino acid sequence similarities between the shaded regions of CaSsn6 and other Ssn6-like proteins are indicated.

We tested whether the C. albicans SSN6 gene encodes a functionalhomologue of S. cerevisiae Ssn6 (unpublished data). When transformedinto S. cerevisiae using the single-copy vector YCp50, C. albicansSSN6 suppressed the flocculation defects of the ssn6 cells aswell as their growth defects at 37°C and on glycerol. Thiswas consistent with the observations of Hwang et al. (2003

).We conclude that C. albicans Ssn6 is a functional homologueof S. cerevisiae Ssn6.

Phenotypes of C. albicans ssn6 Mutants
Tup1 inactivation derepresses morphogenesis in C. albicans,leading to the formation of characteristically wrinkly colonies(Braun and Johnson, 1997). If Ssn6 simply acts as a corepressorwith Tup1 in C. albicans, one might predict that the inactivationof Ssn6 would generate a similar phenotype. However, Hwang etal. (2003) described subtle morphological differences betweenC. albicans ssn6 and tup1 mutants. To examine these differencesin more detail, we generated independent homozygous ssn6/ssn6mutants in C. albicans CAI8 (ura3, ade2) and carefully examinedtheir morphologies.

As expected, wild-type SSN6/SSN6 cells and heterozygous ssn6/SSN6cells generated large smooth white colonies when streaked ontoYPDA plates (Figure 2). However, when freshly generated homozygousssn6/ssn6 mutants were restreaked onto fresh YPDA, dramaticcolony phenotypes were observed routinely. A range of colonyphenotypes arose from a single ssn6/ssn6 colony: small versuslarge, red versus white, and wrinkled versus smooth colonies(Figure 2). Cells from all of these colonies were ade2/ade2ssn6/ssn6 mutants as confirmed by diagnostic PCR. This colonyvariability was reproduced in eight independent mutants.

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Figure 2. Phenotypes of C. albicans ssn6 cells. (A) Mixed colony phenotypes of a freshly generated ssn6/ssn6 mutant (SGC123) restreaked on YPDA. (B) Characterization the various ssn6 colony types. Genotypes were rechecked by PCR diagnosis: +, wild-type allele; -, null allele (CAI8, SGC121 and SGC123: Table 1). For each colony type, cell morphology and growth in liquid medium in YPD at 30°C (length of lag phase, growth rate, and final OD₆₀₀) were determined. Growth on nonfermentable carbon sources as sole carbon source was examined on YNB plates at 30°C: +, robust growth; +/-, weak growth; -/+, very weak growth; -, no growth. (C) Morphogenetic responses of ssn6 (SGC123) and ssn6, cph1, efg1 cells (SGC133) after 3 h in YPD containing 10% serum.

In addition to displaying colony variability, most ssn6 colonytypes displayed phenotypic instability. For example, 5.9% ofcells from large pink wrinkly colonies switched to differentcolony morphologies when restreaked onto fresh YPDA (Figure 3).Ssn6 cells from large smooth white colonies were relativelystable, with only 0.1% of these cells switching colony morphologies.As a result, serial passaging of ssn6 strains generally ledto an accumulation of the large smooth white growth form. Largewrinkly white colonies also arose relatively frequently afterserial passaging.

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Figure 3. Phenotypic instability of C. albicans ssn6 cells. (A) The phenotypic stability of each colony type was assayed by replating cells on fresh YPD and measuring the proportion of colonies that had switched to an alternative form. (B) Phenotypic instability could be induced in a conditional ssn6/MET3-SSN6 strain following the addition of 2.5 mM methionine and cysteine to the medium: SSN6, CAI8; MET3-SSN6, SGC179 (Table 1).

A conditional ssn6/MET3-SSN6 mutant was constructed to confirmthat these dramatic phenotypic effects were caused by Ssn6 depletion.In the absence of methionine and cysteine, when the MET3-SSN6allele was expressed, this mutant displayed a poppy-like colonymorphology (Figure 3), presumably because of abnormal Ssn6 expressionpatterns from the MET3 promoter. This poppy-like phenotype wasstable. However, a range of different colony morphologies wasobserved when clonal ssn6/MET3-SSN6 cells were plated onto mediumcontaining methionine and cysteine, and these phenotypes wereunstable. Most cells in these colonies (73%) switched colonymorphologies when replated onto medium containing methionineand cysteine (Figure 3). In contrast they reverted to the poppy-likemorphology when replated onto medium lacking methionine andcysteine (unpublished data). These data confirmed that Ssn6depletion dramatically effects C. albicans colony morphologyand enhances switching between different colony phenotypes.

We examined the phenotypes of cells from the different colonytypes (Figure 2). During growth in liquid YPD, ssn6 cells fromsmaller colonies displayed longer lag periods and generatedless biomass than ssn6 cells from larger colonies. With theexception of the large smooth white colonies, all cell typesgrew on media containing ethanol, glycerol as the sole carbonsource.

Colonies formed by wild-type and SSN6/ssn6 strains on YPDA at30°C contained the ovoid budding cells typical of the yeastgrowth form of C. albicans (Sudbery et al., 2004). In contrast,homozygous ssn6/ssn6 cells from some colonies resembled pseudohyphaewith septa at mother-daughter junctions (Figure 2). However,there was significant population heterogeneity with respectto the morphology of these cells, and they did not divide synchronouslylike true C. albicans pseudohyphae. This suggested that thesecells were displaying a pathological morphological phenotypecaused by Ssn6 inactivation, rather than bone fide pseudohyphaldevelopment. Ssn6/ssn6 cells from other colonies were smalland stumpy, reminiscent of C. albicans efg1 cells (Lo et al.,1997). There was no clear correlation between the degree offilamentation and the wrinkliness of ssn6 colonies.

These ssn6 phenotypes were significantly different from thoseof tup1 and nrg1 cells, which display stable cellular and colonialphenotypes (Braun and Johnson, 1997; Braun et al., 2001; Muradet al., 2001a). A direct comparison of cells growing on YPDAat 30°C confirmed the contrasting cellular and colonialmorphologies of wild-type, nrg1, tup1, and ssn6 cells (Figure 4).The ssn6 cells were more similar to the budding wild-typeparent than the pseudohyphal nrg1 and tup1 cells. Furthermore,the wrinkly ssn6 colonies were not invasive, unlike the nrg1and tup1 colonies (Figure 4).

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Figure 4. Phenotypic differences between wild-type, nrg1, tup1, and ssn6 cells. (A) Morphology of cells growing exponentially in YPD at 30°C: wild-type, CAI8 containing CIp10; nrg1, MMC3; tup1, BCA2-9; ssn6, SGC123 (Table 1). (B) Colony morphology (prewash) and invasiveness (postwash) of the same strains growing on YPD at 30°C. To measure invasiveness, cells were washed off the surface of the plate into H₂O with a glass spreader.

Hwang et al. (2003) examined the role of Ssn6 in morphogenesisby examining the epistatic relationships between Ssn6, Tup1,Cph1, and Efg1. Cph1 and Efg1 define the MAP kinase and cAMP-proteinkinase A pathways, respectively, that activate hyphal developmentin C. albicans (Liu et al., 1994; Bockmuhl and Ernst, 2001).Based on the complex phenotypes of the various mutants theyexamined, Hwang et al. (2003) suggested that Ssn6 inactivationinduces pseudohyphal growth and that both Cph1 and Efg1 mightactivate this pseudohyphal growth. In our hands, Ssn6 inactivationdid not lead to the formation of true pseudohyphae (Figures2 and 4). We examined the effects of serum on ssn6 mutants becauseserum is a strong inducer of hyphal development in C. albicans.In response to serum stimulation, ssn6 cells appeared to retainthe ability to form germ tubes, the progenitors of true hyphae(Figure 2C). Furthermore, unlike tup1 cells (Braun and Johnson,1997; Murad et al., 2001), ssn6 cells were still able to respondto serum after Cph1 and Efg1 inactivation, although the filamentsformed by the ssn6, efg1, cph1 triple mutants were not truehyphae. We suggest that although Cph1 and Efg1 can influencethe morphology of ssn6 cells, the morphological phenotypes causedby Ssn6 inactivation are not related to bone fide morphogeneticdevelopmental programs.

Global Molecular Phenotypes of Wrinkly and Smooth C. albicans ssn6 Cells
The global molecular phenotypes of C. albicans ssn6 cells fromlarge white wrinkly and smooth colonies were compared by transcriptprofiling. The analysis of other growth forms was precludedby their phenotypic instability. About 1.5% of the $~$ 6000 C. albicansgenes displayed reproducible and statistically significant increasesin expression of twofold or more in the wrinkly or smooth growthforms relative to wild-type cells (Figure 5A). Similar numbersof C. albicans genes displayed decreased expression. A directcomparison of the transcript profiles of C. albicans CAI4 andCAI8 (Supplementary Data) confirmed that these differences werenot due to differences between the parental strains use in thisstudy (Table 1). The Ssn6 repressor might regulate these genesindirectly. Alternatively, Ssn6 might also be able to act asa transcriptional activator (Conlan et al., 1999).

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Figure 5. (A) Numbers of C. albicans genes that were up- or down-regulated twofold or more in smooth and wrinkly ssn6 cells (SGC123), relative to the wild-type control (CAF2-1). (B) Numbers of C. albicans genes that were significantly up- or down-regulated in wrinkly ssn6 (SGC123), tup1 (BCA2-9), and nrg1 cells (MMC3), relative to the wild-type control (CAF2-1). Significant changes of twofold or more were identified using SAM (FDR set at 10%) using data from three independent replicates for each cell type.

There was limited overlap between the transcript profiles ofthe wrinkly and smooth growth forms (Figure 5A), which mightaccount for at least some of the phenotypic differences betweenthese cells. A significant proportion (31%) of the genes thatwere up-regulated only in the wrinkly form encode functionsinvolved in carbon metabolism (Table 2). In contrast, glycolyticgenes were down-regulated in the smooth form. Ribosomal proteingenes represented 28% of those that were up-regulated only insmooth cells. Iron assimilatory functions (FTR1, HEM1, RBT2)represented 9% of the genes that were up-regulated in both celltypes. These observations were consistent with the differencesin growth rates and carbon assimilation patterns of the variousssn6 growth forms (Figure 2).

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Table 2. C. albicans genes that are up-regulated in smooth and/or wrinkly ssn6 cells

Global Comparison of the Ssn6, Tup1, and Nrg1 Regulons in C. albicans
Transcript profiling was also performed to compare the globalroles of Ssn6, Tup1, and Nrg1 in C. albicans. Ssn6, Tup1, andNrg1 regulons were defined operationally as those subsets ofC. albicans genes whose expression was altered twofold or morein ssn6, tup1, and nrg1 cells, respectively. If Ssn6 acts simplyas a corepressor with Tup1, one might expect their regulonsto overlap. Nrg1 is thought to be one of a number of proteinsthat targets the Tup1-Ssn6 complex to specific C. albicans promoters.On this basis one might predict that the Nrg1 regulon wouldbe a subset within the Ssn6-Tup1 regulon. However, neither ofthese simplistic predictions was supported by our data (Figure 5B),indicating that the roles of these factors are more complex.

C. albicans genes that are repressed by Tup1 or Ssn6 are expectedto be overexpressed in tup1 and ssn6 cells, respectively. However,there was limited overlap between the Ssn6 and Tup1 regulons(Figure 5B). Most genes that were up-regulated in tup1 cellswere not significantly up-regulated in ssn6 cells (186 of 224genes). This suggests that Tup1 represses the expression ofthese genes, but that Ssn6 is not essential for their repression.

A significant number of C. albicans genes were down-regulatedin tup1 cells (Figure 5B). Tup1 might regulate these genes indirectly.Significantly, most genes that were down-regulated in tup1 cellswere not down-regulated in ssn6 cells (112 of 117 genes). Againthis suggests that Ssn6 is not essential for the Tup1-mediatedregulation of these genes.

Of the 85 C. albicans genes that were up-regulated in nrg1 cells,32 were not up-regulated in tup1 cells, and most were not up-regulatedin ssn6 cells (Figure 5B). This suggested that Tup1 is not essentialfor the repression of some genes by Nrg1 and that Ssn6 is notessential for the repression of most Nrg1-repressed genes. HenceNrg1 appears to act independently of Tup1 and Ssn6 to represssome C. albicans genes.

We examined the functions of the genes in the Nrg1, Tup1, andSsn6 regulons in C. albicans. These genes and their functionsare listed in the Supplementary Data. Previously, we reportedthat hypha-specific genes are regulated both by Nrg1 and Tup1(Murad et al., 2001a). This observation, which was made usingmacroarrays containing about one-third of C. albicans genes,was confirmed in this study, which used (nearly) whole genomeC. albicans microarrays. The hypha-specific genes HWP1, ECE1,RBT1, and RBT5 were among the most strongly regulated genesin the subset of genes regulated by Tup1 and Nrg1 (Table 3).These data are consistent with those of Kadosh and Johnson (2005)in the accompanying paper. The hypha-specific genes, ALS3 andALS8, were absent from the subset of Tup1- and Nrg1-regulatedgenes because they were not on the microarray. However, we haveshown previously that ALS3 is regulated both by Nrg1 and Tup1(Murad et al., 2001a). (ALS8 is now known to be an allele ofALS3: Zhao et al., 2004.) The expression of HYR1, which encodesa hypha-specific cell wall glycoprotein (Bailey et al., 1996),was elevated 2.3-fold in tup1 cells, but was not elevated innrg1 or ssn6 cells. The expression of HGC1/CLN21, which encodesa hypha-specific cyclin (Zheng et al., 2004), was elevated 4.0-foldin tup1 cells, 1.6-fold in nrg1 cells, and 1.0-fold in ssn6cells. Therefore, whereas HGC1/CLN21 formally lies outside theNrg1-Tup1 regulon, it does appear to be regulated by both ofthese factors.

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Table 3. C. albicans genes that are up-regulated in nrg1 and tup1 cells, but not in ssn6 cells

Interestingly, our transcript profiling indicated that hypha-specificgenes were not derepressed in ssn6 cells grown at 30°C andwas confirmed by northern blotting (Figure 6A). The HWP1 mRNAwas derepressed in nrg1 and tup1 cells, but not in the ssn6mutant. Hwang et al. (2003) reported that HWP1 and ECE1 werederepressed in ssn6 cells. However, this derepression was partial,only being observed at 37°C and not at 30°C. We concludethat Nrg1-Tup1 mediates the repression of most hypha-specificgenes in C. albicans, but that Ssn6 is not essential for thisrepression, at least under the conditions examined in this study.

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Figure 6. (A) Northern analysis of C. albicans mRNAs in wild-type (CAI8), tup1 (BCA2-9), ssn6 (SGC123), and nrg1 cells (MMC3). (B) Chromatin immunoprecipitation revealing association of Ssn6 with the WH11 promoter: wild-type cells (CAI8), ssn6 cells (SGC123); PCR with genomic DNA template, Total DNA; reaction with preimmune serum, PREI; reactions with anti-Ssn6 serum.

A comparison of the global cellular roles of Ssn6 and Tup1 wasperformed by examining whether specific functional categorieswere enriched in the subsets of genes whose expression levelswere altered in ssn6 and tup1 cells (Table 4). This analysisreinforced the view that Ssn6 does not contribute to the regulationof hypha-specific genes under these growth conditions. The analysisalso highlighted the important roles of Tup1 and Ssn6 in repressinggenes involved in carbon metabolism. Most notably, the gluconeogenicgenes PCK1 and FBP1 and the glyoxylate cycle gene MLS1 werederepressed in both ssn6 and tup1 cells (Table 4; Figure 6A).We note that phenotypic switching is associated with changesin the expression of genes involved in central carbon metabolism(Lan et al., 2002

). Tup1 and Ssn6 also appear to play rolesin the regulation of genes involved in amino acid metabolism.Further details are provided in the Supplementary Data.

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Table 4. Enrichment of functional categories in subsets of genes whose expression was significantly altered in ssn6 or tup1 cells

Relative enrichment of functional category^a

Role of Tup1 and Ssn6 in NRE-mediated Repression
Nrg1 represses the hypha-specific gene expression via Nrg1 ResponseElements (NREs: Murad et al., 2001a). Therefore, we tested whetherSsn6 and Tup1 are required for NRE-mediated repression in C.albicans. An oligonucleotide containing four NRE elements ofthe type C₅T was cloned upstream of a basal lacZ reporter andtransformed into C. albicans. The expression levels of the NRE-lacZand basal-lacZ reporters were then compared in wild-type, nrg1,tup1, and ssn6 cells (Figure 7A). The introduction of the NREelements repressed expression in wild-type cells, and this repressionwas released in nrg1 cells. This confirmed that Nrg1 was requiredfor the repression imposed by the NRE element. Repression wasalso released in tup1 and ssn6 cells. This indicated that bothSsn6 and Tup1 were required for Nrg1-NRE-mediated repressionin C. albicans. Similar findings were made using a second NREreporter containing the A₂C₃T and C₅T elements seen in the ALS3promoter (unpublished data).

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Figure 7. (A) An NRE imposes repression on a lacZ reporter in C. albicans in an Nrg1-, Ssn6-, and Tup1-dependent manner: wild-type, CAI4; nrg1, MMC4; tup1, BCA2-9; ssn6, SGC124 (Table 1); basal reporter lacking NRE, basal; NRE [(C₅T)₄] containing reporter. (B) In a C. albicans one-hybrid assay, a lexA-Nrg1 fusion imposes repression on a Lex Operator-lacZ reporter in an Ssn6- and Tup1-dependent manner: wild-type, CAI8; nrg1, MMC9; tup1, CRC004; ssn6, SGC124. Fold repression was measured by comparing ${beta}$ -galactosidase levels (Miller Units) for C. albicans cells expressing LexA with those expressing the LexA-Nrg1 fusion. Means and standard deviations from triplicate assays on three independent transformants are shown.

The roles of Ssn6 and Tup1 in Nrg1-mediated repression wereanalyzed further using the C. albicans one-hybrid system (Doedtet al., 2004; Russell and Brown, 2005). Briefly, we tested theability of a lexA-Nrg1 fusion to impose repression on a lacZreporter that carries a lexA operator. The expression levelsof the LexOP-lacZ reporter were analyzed in wild-type, nrg1,tup1, and ssn6 cells expressing either the lexA-Nrg1 fusionor the lexA protein alone (Figure 7B). The presence of Nrg1in the lexA-fusion caused nearly threefold repression in wild-typeand nrg1 cells. This repression was significantly attenuatedin ssn6 and tup1 cells, indicating that both Ssn6 and Tup1 wererequired for repression by the lexA-Nrg1 fusion in C. albicans.

Regulation of WH11 by Ssn6
The phenotypic instability induced by Ssn6 depletion (Figure 3)was reminiscent of the phenotypic switching described bySoll and colleagues (Slutsky et al., 1985; Soll, 2002). Theyhave reported that misexpression of TUP1 or the white-phase-specificgene WH11 can induce phenotypic switching in the C. albicansstrain WO1 (Kvaal et al., 1997; Zhao et al., 2002). Therefore,we examined whether WH11 expression was affected in C. albicansssn6 cells. WH11 mRNA levels were significantly elevated inssn6 cells, but not in tup1 or nrg1 cells (Figure 6A). Thenwe tested whether Ssn6 is associated with the WH11 promoterby chromatin immunoprecipitation. WH11 promoter sequences weresignificantly enriched in wild-type cells, but not in ssn6 cellsafter chromatin immunoprecipitation with an anti-Ssn6 antibody(Figure 6B). This enrichment was not observed with preimmunesera. Therefore, Ssn6 appears to associate with the WH11 promoterin vivo.

These observations lend weight to the idea that Ssn6 can actindependently of Tup1 and Nrg1 to regulate the expression ofsome C. albicans genes (Figure 5B). Furthermore, they providea possible mechanism by which Ssn6 depletion can promote phenotypicinstability. Ssn6 depletion appears to cause WH11 misexpression,which is known to promote phenotypic switching in C. albicans(Kvaal et al., 1997).

DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

The prevailing view is that Ssn6 interacts with Tup1 to forma corepressor complex that regulates a large number of genesin budding yeast and that this corepressor complex is conservedfrom yeast to humans (reviewed by Smith and Johnson, 2000).Based on this S. cerevisiae paradigm, it was predicted thatSsn6 and Tup1 might execute equivalent functions in C. albicans.Consistent with this, Johnson and coworkers have shown thatTup1 plays a critical role in the repression of filamentousgrowth and the expression of hypha-specific genes in C. albicans(Braun and Johnson, 1997, 2000; Braun et al., 2000, 2001; Kadoshand Johnson, 2005). Others have added to this by confirmingthat Tup1 regulates hypha-specific genes and by identifyingother putative Tup1 gene targets in C. albicans (Sharkey etal., 1999; Murad et al., 2001b).

The role of Ssn6 in C. albicans remained less clear. In theirelegant article, Hwang et al. (2003) showed that C. albicansSSN6 is a functional homologue of S. cerevisiae SSN6. They alsoexamined the morphological phenotypes of C. albicans ssn6 mutantsand the epistatic relationships between Ssn6, Tup1, Cph1, andEfg1, which were complex. They suggested that Ssn6 plays animportant role in regulating yeast-(pseudo)hypha morphogenesis,pointing out that Ssn6 might play some distinct roles in thisprocess. However, the relationship between Ssn6 and Tup1 inC. albicans remained obscure. Hence we have examined this issuein some detail. As a result we are able to draw a number ofimportant conclusions.

First, C. albicans Ssn6 is member of a conserved family of eukaryoticSsn6-like proteins that display a relatively high level of sequencesimilarity in their TPR domains (Figure 1). This is significantbecause these domains mediate interactions with Tup1-like proteins(Tzamarias and Struhl, 1995). On this basis, C. albicans Ssn6would be expected to form a corepressor complex with Tup1.

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Figure 8. Models illustrating Ssn6 function in C. albicans. (A) Ssn6 is not required for Tup1-mediated repression at some promoters, suggesting that Tup1 might interact directly with the DNA-binding protein (DBP). (B) Ssn6 is partially required for Tup1-mediated repression at some C. albicans promoters, suggesting that Ssn6 stabilizes Tup1 interactions with the DNA-binding protein. (C) Ssn6 is essential for Tup1-mediated repression at other promoters, suggesting that Tup1 depends on Ssn6 for its interaction with the DNA-binding protein. The DNA-binding protein might differ between these promoters, or alternatively differences in the sequence context of the Response Element (RE) might affect the Ssn6 dependency. (D) The repression of some C. albicans promoters by Ssn6 is not dependent on Tup1 (see text).

Second, Ssn6 and Tup1 do not execute equivalent cellular rolesin C. albicans. This conclusion is based on several complementaryobservations. C. albicans ssn6 and tup1 mutants display dramaticallydifferent phenotypes. C. albicans tup1 cells display stablephenotypes, growing constitutively as pseudohyphae that formhighly wrinkled and invasive colonies (Braun and Johnson, 1997

).In contrast, independent C. albicans ssn6 mutants and conditionalMET3-ssn6 mutants displayed unstable phenotypes, switching athigh frequencies between different growth forms (strains SGC123and SGC179: Table 1, Figures 2 and 3). Some ssn6 growth formsgenerated pseudohyphal-like cells. However, these cells didnot divide synchronously, they showed a high degree of populationheterogeneity, and they were not invasive (Figure 4). We alsoobserved that ssn6 cells were able to form filaments in responseto serum, even in the absence of Cph1 and Efg1 (Figure 2C).This indicated that the filamentous structures generated byssn6 cells were not dependent on the MAP kinase and cAMP-proteinkinase A signaling pathways that trigger hyphal developmentin response to serum (Lo et al., 1997

; Ernst, 2000

; Brown 2002

).Furthermore, the inactivation of Ssn6 led to the derepressionof the phase-specific gene WH11, but did not affect the expressionof hypha-specific genes (Figures 5 and 6). These data are consistentwith the idea that Ssn6 depletion does affect cell morphology(Hwang et al., 2003

). However, we conclude that, under the conditionsanalyzed in this study, Ssn6 depletion promotes phenotypic switchingrather than morphogenesis.

Third, Ssn6 is not essential for Tup1-mediated repression ofmany genes in C. albicans. If Ssn6 were essential for Tup1-mediatedrepression, transcript profiling would have revealed a highdegree of concordance between the Ssn6 and Tup1 regulons, aswas the case in S. cerevisiae (Hughes et al., 2000). In general,S. cerevisiae ssn6 and tup1 cells display only quantitativedifferences in expression levels. However, this was not thecase in C. albicans. The repression of most Tup1-regulated geneswas not dependent on Ssn6 (Figure 5). Hence Ssn6 does not simplyact as a corepressor with Tup1 in C. albicans.

Fourth, Ssn6 can act independently of Tup1 to repress some C.albicans genes. The repression of a significant number of Ssn6-regulatedgenes was not dependent on Tup1 (Figure 5). Furthermore, althoughthe repression of the HWP1 gene was dependent on Tup1 but notSsn6, the repression of WH11 was dependent on Ssn6 but not Tup1(Figure 6).

Fifth, Ssn6 and Tup1 are required to differing extents for Nrg1-mediatedrepression at specific C. albicans promoters. Nrg1 repressesthe transcription of some C. albicans promoters in a Tup1-dependentmanner via the NRE element (Braun et al., 2001; Murad et al.,2001a). This knowledge facilitated the functional analysis ofSsn6 in C. albicans by allowing us to investigate the role ofthis protein at specific promoters. Under the conditions analyzedin this study, it is clear that Ssn6 is not essential for theNrg1-mediated repression of C. albicans genes, including hypha-specificgenes (Figures 5 and 6). However, both Ssn6 and Tup1 are essentialfor Nrg1-mediated repression at two artificial promoters (Figure 7).

Many of these observations can be explained in the context ofthe S. cerevisiae Ssn6-Tup1 paradigm (Tzamarias and Struhl,1995; Smith and Johnson, 2000). According to this paradigm,Ssn6 stabilizes the interaction between Tup1 and the Tup1 targetingprotein. We suggest that the extent to which Ssn6 is requiredto stabilize this interaction depends on the C. albicans promoter(Figure 8). Ssn6 might essentially be redundant at some C. albicanspromoters, but this does not exclude the possibility that Ssn6remains bound to Tup1 at these promoters (Figure 8A). At otherpromoters, Ssn6 might promote the interaction between Tup1 andthe Tup1-targeting protein. Under some conditions the role ofSsn6 might be minimal, but this does not exclude the possibilitythat under other conditions, Ssn6 might become more importantto maintain the stability of the complex (Figure 8B). Finallyat other promoters, Ssn6 might be essential for the integrityof the complex (Figure 8C). In reality, Tup1-regulated C. albicanspromoters probably represent a continuum between the extremesshown in Figure 8.

These models predict that different Tup1 targeting proteinswill depend to differing extents on Ssn6 for their interactionwith Tup1 (Tzamarias and Struhl, 1995; Smith and Johnson, 2000).However, if one assumes that the sequence context of the NREcan influence Nrg1 conformation, then these models can alsoexplain why the Nrg1-mediated repression of some promoters,but not others, depends on Ssn6 (Figures 5 and 7). Furthermore,these models also account for the observation that Ssn6 is notrequired for the repression of hypha-specific promoters at 30°C(Figures 5 and 6), but is apparently essential at 37°C (Hwanget al., 2003). However, an additional model is required to accountfor the observation that the repression of some promoters, suchas WH11, is dependent on Ssn6, but not Tup1 (Figures 5 and 6).Clearly, Ssn6 can repress some C. albicans genes independentlyof Tup1 (Figure 8D). It remains to be established whether Ssn6can act in concert with an alternative corepressor at some C.albicans promoters.

ACKNOWLEDGMENTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

We are grateful to David Kadosh and Sandy Johnson for communicatingdata before publication. We also thank Sandy Johnson for helpfuldiscussions and providing strains. We thank Markus Proft forproviding strains and Susan Budge for excellent technical assistance.S.G. and S.A. were supported by fellowships from the BasqueGovernment and the Argentinean Antorchas Foundation, respectively.A.M. and B.E. were supported by the European Commission (QLRT-1999-30795;MRTN-CT-2003-504148). P.D. and C.R. were supported by the BBSRC.A.B. is supported by the BBSRC (1/P17124, BBS/B06679) and theWellcome Trust (063204, 068143).

Footnotes

This article was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E05-01-0071)on April 6, 2005.

The online version of this article contains supplemental materialat MBC Online (http://www.molbiolcell.org).

^* Present address: Department of Biotechnology, Basque Institutefor Agricultural Research and Development, PO Box 46, 01080Vitoria-Gasteiz, Spain

Present address: Robert Koch-Institut, Nordufer 20, D-13353Berlin, Germany

Present address: Centre for Biomolecular Sciences, Universityof St. Andrews, St. Andrews KY16 9ST, United Kingdom

Address correspondence to: Alistair J.P. Brown (Al.Brown{at}abdn.ac.uk).

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