The Skn7 Response Regulator of Saccharomyces cerevisiae Interacts with Hsf1 In Vivo and Is Required for the Induction of Heat Shock Genes by Oxidative Stress

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Vol. 11, Issue 7, 2335-2347, July 2000

The Skn7 Response Regulator of Saccharomyces cerevisiae Interacts with Hsf1 In Vivo and Is Required for the Induction of Heat Shock Genes by Oxidative Stress

Desmond C. Raitt,^* Anthony L. Johnson,^* Alexander M. Erkine, Kozo Makino,^§ Brian Morgan, David S. Gross, and Leland H. Johnston^*

^*Division of Yeast Genetics, National Institute for Medical Research, The Ridgeway, London NW7 1AA, United Kingdom; Department of Biochemistry and Molecular Biology, Louisiana State University Health Sciences Center, Shreveport, Louisiana 71130; ^§Department of Molecular Microbiology, Research Institute for Microbial Diseases, Osaka University, Osaka 565, Japan; and Department of Biochemistry and Genetics, Medical School, University of Newcastle, Newcastle-Upon-Tyne NE2 4HH, United Kingdom

Submitted January 21, 2000; Revised May 1, 2000; Accepted May 12, 2000
Monitoring Editor: Elizabeth Craig

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The Skn7 response regulator has previously been shown to play a role in the induction of stress-responsive genes in yeast,e.g., in the induction of the thioredoxin gene in response tohydrogen peroxide. The yeast Heat Shock Factor, Hsf1, is centralto the induction of another set of stress-inducible genes, namelythe heat shock genes. These two regulatory trans-activators, Hsf1and Skn7, share certain structural homologies, particularly intheir DNA-binding domains and the presence of adjacent regionsof coiled-coil structure, which are known to mediate protein-proteininteractions. Here, we provide evidence that Hsf1 and Skn7 interactin vitro and in vivo and we show that Skn7 can bind to the sameregulatory sequences as Hsf1, namely heat shock elements. Furthermore,we demonstrate that a strain deleted for the SKN7 gene and containinga temperature-sensitive mutation in Hsf1 is hypersensitive tooxidative stress. Our data suggest that Skn7 and Hsf1 cooperateto achieve maximal induction of heat shock genes in response specificallyto oxidative stress. We further show that, like Hsf1, Skn7 caninteract with itself and is localized to the nucleus under normalgrowth conditions as well as during oxidativestress.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Cells must survive challenges from the environment with regard to heat, UV radiation, and heavy metals as well as toleratethe endogenous generation of reactive oxygen intermediates duringrespiration. Oxygen, in the form of superoxide anion (O₂), hydroxyl ion (OH), and hydrogen peroxide (H₂O₂), causes damage to nucleic acids,cell membranes, and proteins (reviewed by Halliwell, 1994). Yeast,in common with all other organisms, has evolved protective mechanismsto survive in the presence of these by-products of aerobic metabolismand can mount distinct adaptive responses to different sourcesof oxidative stress (Jamieson, 1992; Ruis and Schüller, 1995).For example, the Cu,Zn-linked superoxide dismutase, encoded bythe SOD1 gene, detoxifies superoxide anion to hydrogen peroxide;catalase, encoded by the cytosolic CTT1 gene, can catalyze thebreakdown of hydrogen peroxide. Other free radical scavengersin the cell include glutathione, ascorbic acid, and thioredoxin.The SKN7 gene was initially isolated as a multicopy suppressorof a kre9 $Delta$ mutation, which results in defective cell wall biosynthesis(Brown et al., 1993). The SKN7 gene was also cloned as POS9 ina screen for mutants resulting in sensitivity to hydrogen peroxide(Krems et al., 1995), suggesting a role for SKN7 in the yeastoxidative stress response. The oxidative stress induction of thesmall antioxidant molecule thioredoxin, encoded by the TRX2 gene,was subsequently shown to be regulated by SKN7 and the yeast AP-1homologue YAP1, both of which bind to distinct sites within theTRX2 promoter (Kuge and Jones, 1994; Morgan et al., 1997).

Of the many proteins that are induced under adverse environmental conditions, perhaps the best understood are the heat shockproteins (Lindquist and Craig, 1988; Mager and De Kruijff, 1995).The major heat shock proteins have been classified according totheir molecular weight: Hsp104, the Hsp90 and Hsp70 families,Hsp60, Hsp26, and Hsp12 (Craig, 1992; Mager and Ferreira, 1993).The Hsp70 family of heat shock proteins act as molecular chaperones;this family contains at least five heat-inducible isoforms andothers that are expressed constitutively at high levels (Craig,1992; Rassow et al., 1997). Their principal role includes thetransport and folding of polypeptides and the solubilization ofdenatured proteins (Craig et al., 1994). Hsp104 is thought toprotect the cell during exposure to lethal heat shock and is requiredfor cross-protection against a variety of stress conditions (Sanchezet al., 1992), although its exact function remainsunclear.

The induction of these genes in response to heat shock is mediated by Heat Shock Factor, encoded by the essential HSF1 gene(Sorger and Pelham, 1988). The Hsf1 protein binds to heat shockelements (HSEs) consisting of tandem inverted repeats of the sequenceAGAAn (where n is any nucleotide) found in the promoters of manyheat shock genes (Fernandes et al., 1995). In Saccharomyces cerevisiae,Hsf1 binds HSEs as a trimeric complex: constitutively to high-affinitysites (Gross et al., 1990) and inducibly to low-affinity sites(Giardina and Lis, 1995; Erkine et al., 1999). The protein undergoesextensive phosphorylation on serine and threonine residues uponheat shock. This posttranslational modification has been correlatedwith its transcriptional activation (Sorger and Pelham, 1988;Sorger, 1990). However, evidence has also been presented to suggestthat hyperphosphorylation of serine residues located between thetrimerization and C-terminal activation domains is involved inthe deactivation of Hsf1 (H $phi$ j and Jakobsen, 1994). In additionto HSEs, a number of stress-responsive genes also contain stress-responsiveelements (STREs) within their promoters, through which the Zn-fingertranscription factors Msn2 and Msn4 can activate stress gene expressionin response to a variety of stress conditions independent of Hsf1(Schüller et al., 1994; Martínez-Pastor et al., 1996)

In addition to its role in the heat shock response, Hsf1 has also been shown to protect the cell against heavy metals, suchas copper and cadmium, through its activation of the copper metallothioneingene CUP1 (Silar et al., 1991; Sewell et al., 1995). Hsf1 becomesphosphorylated in response to the superoxide generator menadione.This modification correlates with transcriptional activation ofCUP1 by oxidative stress (Liu and Thiele, 1996). Hence, Hsf1 alsoplays a critical role in the cell's defense against oxidativestress. Because our previous work had established a role for theSkn7 response regulator in oxidative stress protection (Morganet al., 1997), it seemed possible that Skn7 and Hsf1 share overlappingfunctions.

The Skn7 protein contains a region with a high degree of homology to the receiver domain of bacterial two-component systems,a class of proteins involved in signal transduction in bacteriaand lower eukaryotes (Stock et al., 1989; Parkinson, 1993). Thus,a membrane-bound sensor histidine kinase can phosphorylate a conservedaspartate residue within the receiver domain of its cognate responseregulator. This phospho-aspartate form of the response regulatorcan then carry out a function appropriate to the incoming signal,usually the transcriptional activation of a specific set of genes.A conserved aspartate, residue D427 in Skn7, has been shown tobe required for the function of the protein in cell wall biosynthesis(Brown et al., 1993) and the activation of G1 cyclin expression(Morgan et al., 1995). However, phosphorylation of this residuedoes not appear necessary for the role of SKN7 in the oxidativestress response (Morgan et al., 1997).

The Skn7 protein also contains a C-terminal glutamine-rich region consistent with a possible role in transcriptional activation(Brown et al., 1993; Morgan et al., 1995). Toward the N terminusthere is a region of extensive homology to the helix-turn-helixDNA-binding domain of Hsf1 (Figure 1). This domain is separatedfrom the receiver motif by a region of coiled-coil structure,again similar to the leucine zipper domain of the yeast Hsf1.Given the degree of conservation in the structures of both theDNA-binding domain and the leucine zipper region of the Skn7 andHsf1 proteins (Figure 1), it was of interest to determine whetherSkn7 interacted with Hsf1 and to establish the significance ofthese interactions in the yeast stress response.

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Figure 1. (A) Domain structures of Skn7 and Hsf1. (B) Homology between the DNA-binding domains of Skn7 and heat shock factor. The DNA-binding domain of Skn7p (amino acids 87-151) is aligned with the corresponding regions of S. cerevisiae Hsf1 (Hsf1sc), the fission yeast heat shock factor (Hsf1sp), and the human heat shock factor 2 (Hsf2hs). Highly conserved residues that may directly contact the DNA and may have diverged in Skn7 are indicated by asterisks.

We present evidence here for both genetic and direct biochemical interaction between Hsf1 and the Skn7 response regulator.Furthermore, we show that a protein other than Heat Shock Factor,Skn7, can bind to HSEs in vitro, is localized to the nucleus undernormal and oxidative stress growth conditions, and is requiredfor the full induction of heat shock genes in response to oxidativestress.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Yeast Strains and Growth Conditions

The yeast strains used were as follows: W303-1a (a ade2-1 trp1-1 can1-100 leu2-3112 his3-11 ura3); W303-1a skn7 $Delta$ (aade2-1 trp1-1 can1-100 leu2-3112 his3-11 ura3 skn7::HIS3);MYY290, a ura3 derivative of strain AH216 (a leu2 his3phoC phoE); MYY385 (a leu2 his3 ura3 phoC phoE hsf1-m3)(Smith and Yaffe, 1991); and DR20-2b, which was obtained as ahaploid HIS⁺ spore clone from a cross of MYY385 and W303 skn7 $Delta$ . Minimal andrich media for yeast propagation have been described previously(Sherman et al., 1996).

$beta$ -Galactosidase Assays

The vector pZJHSE2-137 (a gift from E. Craig, University of Wisconsin, Madison, WI) containing a region of the SSA1 promoterresponsible for heat shock activation of HSP70 cloned into the2µ-based lacZ fusion plasmid pLG660 was transformed into W303-1aand the isogenic skn7 $Delta$ strain. Transformants were grown to midlogphase in selective medium at 30°C and harvested before or afterthe addition of t-butyl hydrogen peroxide to 0.6 mM for 1 h. Forthe heat shock experiment, cells were initially grown in selectiveminimal medium at 25°C, and cells were harvested before and 1h after the culture was shifted to a 37°C water bath. Cell extractswere prepared as described previously (Guarente and Mason, 1983).Units of activity are given as the change in OD₄₂₀ per minuteper milligram of total protein. Values represent the average ofduplicate samples in two independentexperiments.

Hydrogen Peroxide Sensitivity Assays

Strains were tested for sensitivity to hydrogen peroxide by taking a suspension of cells in water and making a single streakof the suspension from the edge to the center of the plate, whichcontained a disk of 3MM paper onto which was placed 0.5-2 µl oft-butyl hydrogen peroxide (Sigma Chemical, St. Louis, MO). Thet-butyl hydrogen peroxide was allowed to diffuse freely throughoutthe agar, and the extent of growth inhibition from the centerpoint of the plate was taken as a measure of the sensitivity ofa given strain to oxidativestress.

Thermotolerance and Viability Assays

Midlog-phase cultures were grown in rich glucose medium (YPD) at 25°C, and an aliquot was shifted to a test tube placed ina 51°C water bath. Samples were taken at regular intervals, dilutedinto ice-cold YPD, and immediately plated onto YPD agar to assesscell viability. Survival was determined after 3 d of growth at30°C and expressed as percentage viability compared with cellsthat were maintained at 25°C throughout the experiment. Cell countswere performed in duplicate, and values correspond to the averageof twoexperiments.

Plasmid Constructions

CEN SKN7 and D427N-SKN7 plasmids were constructed by inserting a 3.8-kilobase (kb) XbaI-SacI fragment of pBAM1 or pBAM2 (Morganet al., 1997), which contains the entire SKN7 coding and promoterregions, into the multiple cloning site of YCplac111 (Gietz andSugino, 1988). YexH is a modified derivative of the 2µ-based galactose-inducibleexpression plasmid pEMBLYex4 (Murray, 1987) in which a six-histidinetag sequence was inserted upstream of the multiple cloning siteto allow the N-terminal tagging of inserted genes. YexH-SKN7 wasconstructed by inserting a 2-kb BamHI fragment containing theSKN7 coding region into the BamHI cloning site of the vector,which allows galactose-inducible expression of the 6His-taggedprotein. Plasmid p426GAG (P_GAL1-GST, URA3, 2µ) is based on thehigh-copy-number yeast vector pRS426 (Christianson et al., 1992)and was used to generate a GST-tagged Hsf1 as follows. A PCR strategywas used to generate a 2.5-kb XhoI-EcoRI fragment from plasmidpAKS80 (a gift from A. Sewell, University of Utah, Salt Lake City,UT) that contained the entire HSF1 genomic sequence. This fragmentwas inserted into XhoI-EcoRI-digested plasmid p426-GAG to producepGST-HSF1. The plasmid pGAL-HA-SKN7 was obtained by insertinga 2-kb BamHI fragment of the SKN7 gene from YexH-SKN7 into plasmidYCpIF16 (Foreman and Davis, 1994). The integrating epitope-taggedform of SKN7 was generated by inserting the 2-kb BamHI SKN7 fragmentinto the unique BamHI site of the integrating vector pRS306-Myc,which is based on the vector pRS306 (Christianson et al., 1992)into which has been inserted six copies of the Myc epitope tag(a gift from D. Fesquet, NIMR, London, UK). The SKN7-GFP plasmidwas made by inserting a PCR-generated XhoI-ended SKN7 fragmentinto the unique XhoI site of plasmid pRS416-sGFP-Nuf2t (a giftfrom the P. Silver laboratory, Harvard University, Boston,MA).

Fluorescence Microscopy

GFP was detected in unfixed cells with a Nikon (Garden City, NY) Optiphot-2 equipped with a MicroMax charge-coupled devicecamera (Princeton Instruments, Princeton, NJ). Images were takenat 100× magnification and converted to Photoshop version 4.0 format(Adobe Systems, Mountain View, CA). Nuclei were visualized byDAPIstaining.

RNA Analysis

Northern hybridization was performed as described previously (White et al., 1986). In all cases, probes for hybridizationto heat shock genes used in this study were derived from PCR amplificationof an internal fragment of the coding sequence of the gene, eitherfrom genomic DNA or from plasmids containing the gene of interest.The internal control used for mRNA quantitation in hydrogen peroxide-and heat shock-treated cells was ACT1, the abundance of whichwas found to be relatively insensitive to theseconditions.

Protein Extraction and Pull-Down Experiments

Yeast cell breakage was achieved through repeated vortexing with glass beads for 5 × 30 s with 30-s rests on ice in breakagebuffer (150 mM NaCl, 1% NP40, 50 mM Tris-HCl, pH 7.5, 1 mM EDTA,10 mM NaF, 50 mM $beta$ -glycerol phosphate). At time of use, a proteaseinhibitor mixture was added to a final concentration of 100 µg/mlPMSF, 2 µg/ml leupeptin, 2 µg/ml pepstatin A, 50 µg/ml N $alpha$ -p-tosyl-L-Lysinechloromethyl ketone, and 100 µg/ml L-1-tosylamide-2-phenylethylchloromethyl.Cleared lysates were prepared by centrifugation for 20 min at18,000 rpm (Beckman [Fullerton, CA] SS34 rotor), and 1 mg of wholecell extract was incubated at 4°C with 50 µl of a 50% suspensionof glutathione-Sepharose beads (Pharmacia, Piscataway, NJ) equilibratedin breakage buffer in a total volume of 250 µl. The beads werethen harvested and washed four times in breakage buffer containing200 mM NaCl, followed by one wash in the same buffer with 50 mMNaCl, and finally resuspended in an equal volume of 2× SDS samplebuffer. Coimmunoprecipitations with 9E10 mAb were performed byincubating 500 µg of cell extract with 2 µg of anti-myc mAb (BerkeleyAntibody, Berkeley, CA) for 1 h, and precipitates were recoveredby incubation with continuous mixing at 4°C with 50 µl of a 50%solution of protein G-Sepharose (Gammabind, Pharmacia) equilibratedin breakage buffer. Beads were washed six times in breakage buffercontaining 200 mM NaCl, and once in buffer containing 50 mM NaCl,before being resuspended in 2× SDS sample buffer. Proteins wereseparated by SDS-PAGE through 6% acrylamide gels and transferredto nitrocellulose membranes via semidry transfer before ECL (Amersham,Arlington Heights, IL). Western analysis was performed in accordancewith manufacturers' guidelines (Amersham), and membranes wereexposed to X-ograph XB-200 film (Eastman Kodak, Rochester, NY)for between 30 s and 5min.

For in vitro association assays, 1 mg of cell extract prepared as described above (with the omission of EDTA from the breakagebuffer) was added to 200 µl of Ni²⁺nitrilotriacetic acid (NTA) resin (50% slurry) equilibrated inbreakage buffer. After incubation with mixing at 4°C for 1 h,the resin was washed four times in wash buffer (200 mM NaCl, 50mM Tris-HCl, 1% NP40) and once in wash buffer containing 50 mMNaCl. Beads were then boiled for 2 min in 2× sample buffer, andthe supernatant was subjected to SDS-PAGE as describedabove.

Purification of 6His-Skn7 and Mobility Shift Assays

A 2-kb BamHI fragment of the original SKN7 genomic clone in YEp24, which contains the entire SKN7 ORF (Morgan et al., 1995),was inserted into plasmid pQE-30 (Qiagen, Chatsworth, CA). TransformedDH-5 $alpha$ (minimum 2 l) was grown to OD₆₀₀ = 0.5 at 37°C and thenbrought to 25°C by brief incubation on ice before induction byaddition of isopropyl-1-thio- $beta$ -D-galactoside to 1 mM for 5 h at25°C. Cells were harvested by centrifugation (5 min, 5000 rpm,GSA Sorval rotor, Kendro Laboratory Products, Newtown, CT), washedin cold distilled water, and resuspended in 2-5 ml of breakagebuffer (150 mM NaCl, 25 mM Tris, pH 7.5, 10% glycerol, 0.5% NP40).At the time of use, lysozyme was added at 1 mg/ml and PMSF at1 mM. The cell suspension was incubated on ice for 30 min andthen passed twice through a chilled French press chamber. Theclarified supernatant was then incubated with 5 ml of a 50% slurryof Ni²⁺-NTA resin, equilibrated in binding buffer (250 mM NaCl, 50 mMTris-HCl, pH 7.5, 15 mM imidazole), and allowed to mix at 4°Cfor 1 h before the material was packed into a 5-ml column. Afterwashing in binding buffer, tagged protein was eluted by a stepgradient of binding buffer containing 50, 100, and 250 mM imidazole.Bradford protein assays (Bio-Rad, Richmond, CA) were carried outon 0.5-ml fractions, and DNA-binding activity was assayed by gelmobility shiftassay.

Mobility shift assays have been described elsewhere (Lowndes et al., 1991). 6His-Skn7 protein was incubated with 0.5 ng (1× 10⁵ cpm) of ³²P 5'-end-labeled double-stranded oligonucleotides of the followingsequences: HSE2, 5' tcgaTTTTCCAGAACGTTCCATCGGC; MUT HSE, 5' tcgaTTTTCCAAAACGTTTCATCGGC.Binding reactions in 25 mM Tris-HCl, pH 7.5, 100 mM NaCl, 1 mMEDTA, 7 mM MgCl₂, 10% glycerol, protease mixture as describedabove, and 1 µg of poly(dI.dC) nonspecific competitor DNA wereincubated at room temperature for 15 min and on ice for another20 min. Protein-DNA complexes were resolved on a 4% nondenaturingpolyacrylamide gel (37.5:1) by electrophoresis at 200 V in 0.5×TBE buffer (89 mM tris base, 89 mM boric acid, 2 mM EDTA) for2 h. Gels were dried onto Whatman (Clifton, NJ) 3MM paper andexposed to Kodak (Rochester, NY) X-Omat AR film overnight at $-$ 20°C.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Skn7 $Delta$ Cells Are Sensitive to Acute Heat Stress

Deletion of the SKN7 gene does not confer a temperature-sensitive phenotype when cells are shifted from 25 to 37°C (Morganet al., 1995). However, given the high degree of homology betweenthe DNA-binding domains of Skn7 and Hsf1, we further investigatedthe effect of an skn7 $Delta$ mutation on cell viability under acuteheat shock at 51°C. Cells deleted for the SKN7 gene were foundto be some 10 times more sensitive to the lethal effects of acuteheat stress than the isogenic wild-type strain (Figure 2). Ithas been reported that the main cause of cell death under theseconditions is the generation of toxic intermediates of oxygenmetabolism (Davidson et al., 1996). Because SKN7 has been shownto be required for cell survival under conditions of oxidativestress (Krems et al., 1996; Morgan et al., 1997), it was of interestto determine whether SKN7 has a role, together with HSF1, in theinduction of heat shock gene expression in response to oxidativestress.

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Figure 2. skn7 $Delta$ cells are sensitive to acute heat stress. Midlog-phase cultures of W303-1a and isogenic skn7 $Delta$ cells were grown in YPD at 25°C, and an aliquot was shifted to a test tube placed in a 51°C water bath. Samples were taken at the times indicated, diluted into ice-cold YPD, and immediately plated onto YPD agar to assess cell viability. Survival at 51°C was expressed as a percentage of viable cells relative to cells grown at 25°C. Because the vertical axis is logarithmic, only positive errors are included for clarity.

SSA1-LacZ Induction by Hydrogen Peroxide Requires SKN7

To investigate the potential role of the SKN7 gene in the induction of heat shock protein expression, we assessed the expressionof an Hsp70-LacZ reporter construct in wild-type and skn7 $Delta$ cells.The SSA1 gene encodes a major isoform of the yeast Hsp70 proteinthat is abundant under nonstressed conditions and is stronglyinduced by heat shock (Craig, 1992). The plasmid pZJHSE2-137 containsan HSE, HSE2, from the SSA1 promoter fused to the $beta$ -galactosidasecoding sequence (Slater and Craig, 1987; Park and Craig, 1989).The HSE2 sequence is responsible for the majority of both basaland heat shock-induced expression of SSA1 (Slater and Craig, 1987). $beta$ -Galactosidase assays were carried out on wild-type W303-1a andisogenic skn7 $Delta$ cells containing the reporter plasmid after treatmentfor 1 h with hydrogen peroxide. In wild-type cells, an eightfoldinduction of $beta$ -galactosidase activity was observed 1 h after theaddition of t-butyl hydrogen peroxide (Table 1). In the skn7 $Delta$ strain, basal expression of HSE2-LacZ activity was reduced andinduction in response to oxidative stress was abolished. However,induction of HSE2-LacZ activity in response to a temperature shiftfrom 25 to 37°C was unaffected in the skn7 $Delta$ strain, although theoverall level of expression in the skn7 $Delta$ cells was reduced. Thedecreased basal expression of HSE2-LacZ in the skn7 $Delta$ strain extendsprevious results that indicated a similar reduction in basal expressionlevels of an SSA1-LacZ reporter construct in response to an HSE2double point mutation (Park and Craig, 1989). Thus, HSE2 appearsto be critical for both basal and stress-induced expression ofthe SSA1 gene. It has been proposed that Yap1, which has beenshown to interact with Skn7 at the TRX2 promoter (Morgan et al.,1997), is also required for the induction of HSE2-LacZ activityin response to hydrogen peroxide (Stevens et al., 1995). However,in our genetic background, we found no evidence that yap1 $Delta$ affectsthe hydrogen peroxide induction of the SSA1 HSE2-LacZ reporterconstruct (D.C. Raitt, unpublished observations). Although dispensablefor heat shock induction, our data suggest that Skn7 may be requiredfor full induction of HSE-driven gene expression in response tofree radical stress.

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Table 1. Induction of SSA1-LacZ in response to t-butyl hydrogen peroxide requires Skn7

Skn7 Can Specifically Bind the HSE2 Element from the SSA1 Promoter

The DNA-binding domain of Skn7 is highly homologous to that of Hsf1 (Figure 1B). To determine whether Skn7 can recognize andbind specifically to the same recognition sequence as Hsf1, weperformed electrophoretic mobility shift assays (EMSA) with Escherichiacoli-expressed 6His-Skn7. The SKN7 gene was inserted into plasmidpQE-30, and the 6His-Skn7 fusion protein was subsequently purifiedon an Ni²⁺-NTA agarose affinity column (see MATERIALS AND METHODS). As demonstratedby EMSA, the 6His-Skn7 fusion protein binds specifically to the26-base pair sequence encompassing the HSE2 region of the SSA1promoter (Figure 3). To confirm the presence of the 6His-Skn7protein in the retarded complex, polyclonal antiserum to the proteinwas added to the band shift reaction mixture. The retarded complexformed with the HSE2 probe and the 6His-Skn7 protein was super-shiftedby the anti-Skn7 antibody, whereas no effect was observed withthe addition of preimmune serum at the same concentration.

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Figure 3. Purified 6His-Skn7p can specifically bind HSEs in vitro. EMSA was performed with the use of E. coli-expressed affinity-purified 6His-Skn7 protein and a probe comprising a double-stranded oligonucleotide corresponding to the 26-base pair HSE2 region of the SSA1 gene. The specificity of binding was assessed by the addition of cold HSE2 probe (HSE: tcgaTTTTCCAGAACGTTCCATCGGC) at 5-, 10-, and 50-fold molar excess, compared with the addition of a mutated HSE (MUT HSE: tcgaTTTTCCAAAACGTTTCATCGGC) at 10-, 50-, and 100-fold molar excess. Mutation of the underlined nucleotides in the consensus HSE abolishes Hsf1 binding to the sequence. Polyclonal anti-Skn7 antibody ( $alpha$ -Skn7) at a 1:100 dilution or preimmune serum at the same concentration (Pre Imm) was added to the binding reaction 15 min before the addition of labeled probe. Free probe without the addition of protein migrated off the gel and is indicated (Free).

To determine the specificity of this binding, competitive binding assays were performed with the native HSE2 oligonucleotideand a mutated probe, MUT-HSE2, in which the G and C positionsof the consensus HSE sequence AGAAnnTTCn were changed to A andT, respectively. These mutations within the consensus have previouslybeen shown to abolish binding of Hsf1 (Park and Craig, 1989).The native 26-mer HSE competes efficiently for the binding ofSkn7 at a 10-fold molar excess (Figure 3). However, the mutatedversion of the HSE, MUT-HSE2, does not compete for binding ofthe 6His-Skn7 protein at up to 100-fold molar excess. Similarresults have been seen with an E. coli-expressed Skn7 derivativeconsisting of the DNA-binding domain alone fused in frame to GSTand also with full-length 6His-Skn7 protein purified from yeast(our unpublished results). These results demonstrate that Skn7binds to HSEs with a specificity similar to that ofHsf1.

Induction of Heat Shock Gene Expression by Hydrogen Peroxide Requires Skn7

We have previously shown that Skn7 cooperates with the yeast AP-1 homologue Yap1 in the oxidative stress induction of theTRX2 gene (Morgan et al., 1997). Given the defect in hydrogenperoxide-mediated induction of HSE-LacZ expression in skn7 $Delta$ cellsrelative to isogenic wild-type cells described above, we exploredthe possibility that Skn7 could have a role in the induction ofheat shock genes in response to oxidative stress. Therefore, Northernanalysis was carried out on a number of heat shock genes in W303-1aand W303-1a skn7 $Delta$ . In wild-type cells, the genes encoding HSP12,HSP26, and HSP104 were found to be strongly induced by t-butylhydrogen peroxide (Figure 4A). However, the 5-fold induction ofHSP12 in response to hydrogen peroxide was practically abolishedby the skn7 $Delta$ deletion. Similarly, the 18-fold induction of HSP26was reduced significantly in skn7 $Delta$ cells, and the 9-fold inductionof HSP104 was again reduced by the skn7 $Delta$ mutation. These heatshock genes, therefore, appear to be dependent on the Skn7 responseregulator for their full induction in response to hydrogen peroxide-mediatedoxidative stress. Furthermore, evidence for a role of Skn7 inthe oxidative stress induction of other heat shock proteins (SSA1and HSP82) has recently been presented (Lee et al., 1999); however,in the W303-1a genetic background, we found no significant inductionof any Hsp70 gene (SSA1, SSA2, SSA3, or SSA4) or of HSP82 in responseto 0.6 mM t-butyl hydrogen peroxide (our unpublished results).

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Figure 4. Skn7 is required for the induction of heat shock gene expression specifically in response to hydrogen peroxide. (A) Northern blot analysis of the effect of skn7 $Delta$ mutations on heat shock gene induction by oxidative stress. Total RNA was prepared from midlog-phase cultures of W303-1a and W303-1a skn7 $Delta$ grown at 30°C in YPD. Samples for RNA extraction were taken before (time 0) and at the times indicated after the addition of 0.6 mM t-butyl hydrogen peroxide. Northern blots were prepared as described (see MATERIALS AND METHODS) and hybridized to probes specific for HSP12, HSP26, and HSP104. (B) Skn7 is not required for the heat shock induction of heat shock gene expression. W303-1a and skn7 $Delta$ cells were grown to midlog phase at 25°C, and a portion of the culture was transferred to a 39°C water bath. Cells were harvested at the times indicated, and RNA was extracted for Northern hybridization with the probes specified in A. Quantitation of mRNA was by PhosphorImager analysis (Molecular Dynamics, Sunnyvale, CA) and was expressed relative to the ACT1 transcript, the abundance of which appeared to be unaffected by oxidative stress.

To determine whether Skn7 also contributed to heat shock-induced expression, we performed Northern analysis of heat-shockedW303-1a and isogenic skn7 $Delta$ cells. The kinetics of induction ofseven genes (HSP12, HSP26, SSA1, SSA3, SSA4, HSP82, and HSP104)were found to be virtually indistinguishable between wild-typeand skn7 $Delta$ cells (Figure 4B; our unpublished results). SKN7, therefore,is specifically required for the oxidative stress induction ofheat shock genes. This is in accord with our observations thatskn7 $Delta$ cells show no increased sensitivity upon a temperature shiftfrom 25 to 37°C compared with the isogenic wild-type strain (D.C.Raitt, unpublishedobservations).

Genetic Interactions between SKN7 and HSF1

To explore the possibility that SKN7 and HSF1 may interact in vivo, we took a genetic approach and determined whether deletionof the SKN7 gene combined with a conditional mutation in HSF1would result in a synthetic phenotype. Although the gene encodingyeast heat shock factor is essential, an hsf1 temperature-sensitiveallele, hsf1-m3, has been isolated (Smith and Yaffe, 1991). Thus,an skn7 $Delta$ derivative of W303-1a was crossed with the hsf1^ts strain MYY385, and an hsf1^ts spore clone containing the HIS3⁺-marked skn7 $Delta$ deletion, strain DR20-2b, was selected for furtherstudy. Both the hsf1^ts strain and strain DR20-2b were then tested for growth at varioustemperatures. As expected, both strains grew at the permissivetemperature of 25°C and neither grew at the restrictive temperatureof 37°C (our unpublished results). However, at an intermediatetemperature of 33°C, the hsf1^ts strain formed colonies but the double mutant, DR20-2b, failedto grow (Figure 5A). Because these strains were not isogenic,strain DR20-2b was transformed with a CEN version of the SKN7gene. This restored growth at 33°C (Figure 5A), indicating thatthe increased temperature sensitivity of DR20-2b is due specificallyto the deletion of the SKN7 gene rather than to genetic backgroundeffects. Thus, deletion of SKN7 exacerbates the growth defectof the hsf1^ts strain.

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Figure 5. Genetic interactions between SKN7 and HSF1. (A) Single-copy expression of SKN7 rescues the growth defect of DR20-2b (hsf1^ts skn7 $Delta$ ) at 33°C. DR20-2b (hsf1^ts skn7 $Delta$ ) was transformed with the CEN vector YCplac111 (vector) or with this vector containing the SKN7 gene (+ SKN7) and was incubated at permissive (25°C) and intermediate (33°C) temperatures on rich medium. (B) High-copy expression of SKN7 rescues the growth defect of the hsf1^ts strain, MYY385, at 35°C. The hsf1^ts strain MYY385 was transformed with the 2µ-based plasmid YEp24 containing the SKN7 gene or with the vector alone (vector) and was streaked onto selective medium and incubated at 35°C for 4 d. The wild-type strain MYY290 (HSF1⁺) was included as a positive growth control.

We then assessed whether overexpression of the SKN7 gene could suppress the growth defect associated with the hsf1^ts allele at higher temperatures. The hsf1^ts strain was transformed with the high-copy vector Yep24-SKN7 orthe empty vector alone. The hsf1^ts cells expressing high levels of Skn7 displayed strong growthat a temperature of 35°C, whereas the hsf1^ts strain containing the empty vector alone could not form coloniesat this temperature (Figure 5B). However, the high-copy expressionof SKN7 failed to rescue the hsf1^ts strain at 37°C (our unpublished results). Given the pleiotropicnature of the hsf1-m3 allele, which causes defects in mitochondrialprotein import, reduces heat shock gene induction in responseto increased temperatures, and leads to specific defects in cellcycle progression (Smith and Yaffe, 1991), the absence of suppressionat 37°C is perhaps not surprising. Although there is clearly someoverlap between the functions of SKN7 and HSF1 in the cell, theSkn7 response regulator cannot completely substitute for Hsf1and thus fails to rescue the hsf1-m3 mutation at 37°C.

Both HSF1 and SKN7 have been shown to play a role in the activation of stress-responsive gene expression under conditionsof free radical stress (Krems et al., 1996; Liu and Thiele, 1996;Morgan et al., 1997). Therefore, we wished to establish whetherthey might somehow cooperate in the yeast oxidative stress response.We assessed the sensitivity to oxidative stress of the hsf1^ts, skn7 $Delta$ , and skn7 $Delta$ hsf1^ts strains by means of a standard plate assay (see MATERIALS ANDMETHODS). The hsf1^ts mutation alone caused a modest increase in hydrogen peroxidesensitivity relative to the wild-type strain MYY385 (Figure 6),and a more pronounced effect was observed with the skn7 $Delta$ mutationcompared with its wild-type parent, W303-1a. However, the skn7 $Delta$ hsf1^ts strain showed an enhanced hypersensitivity to hydrogen peroxidestress relative to either the skn7 $Delta$ or the hsf1^ts strain alone (Figure 6). Introduction of SKN7 on a CEN plasmidreversed this increased sensitivity, restoring it to that of thehsf1^ts strain, indicating that the phenotype was not due to geneticbackground effects. Confirming this result, an isogenic straincontaining the skn7 $Delta$ deletion in an hsf1^ts background was also found to be hypersensitive to oxidative stressrelative to either single mutant alone (A.L. Johnson, unpublishedresults). The additive effect of these mutations on stress sensitivitysuggests that Skn7 and Hsf1 might in some way cooperate in theresponse to free radical stress.

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Figure 6. The double mutant hsf1^ts skn7 $Delta$ is hypersensitive to hydrogen peroxide. Sensitivity to hydrogen peroxide was assayed for W303-1a and isogenic skn7 $Delta$ , for MYY290 (HSF1⁺) and the hsf1^ts derivative MYY385, and for an hsf1^ts skn7 $Delta$ spore clone (DR20-2b) derived from a cross between skn7 $Delta$ and MYY385. Cell suspensions were streaked on a YPD plate (Control) and a YPD plate onto which 1 µl of 7.7 M t-butyl hydrogen peroxide was spotted on a disk of Whatman 3MM paper positioned in the center of the plate (+ hydroperoxide). Suppression of hypersensitivity was judged by the ability to grow in the presence of hydrogen peroxide of a YCplac111 (Gietz and Sugino, 1988

) plasmid expressing the SKN7 gene (+SKN7) or an SKN7^D427N mutant (+ SKN7-DN) in which the conserved aspartate residue (D427) was mutated to asparagine. The hsf1^ts skn7 $Delta$ strain was also transformed with the YCplac111 vector alone (+ vector); plates were incubated for 2 d at 30°C.

In a complementary approach, we found that the W303-1a skn7 $Delta$ cells containing a high-copy plasmid with multiple HSE insertsexhibited significantly enhanced hydrogen peroxide sensitivity(D.C. Raitt, unpublished results). By presenting the cell withmultiple copies of the binding site for Hsf1, the protein mayhave been competed away from its native binding sites, therebydecreasing its overall activity in the cell. Thus, when Hsf1 activityis depleted, either through competition for binding sites or bymutation, the survival of skn7 $Delta$ cells under stress is furthercompromised. This observation further supports the proposal thatboth Skn7 and Hsf1 contribute to cell survival during oxidativestress, perhaps through a related or sharedpathway.

Previous data concerning the function of Skn7 indicated that phosphorylation of the conserved aspartate (D427) within thereceiver domain was not required for survival under conditionsof oxidative stress (Morgan et al., 1997). Significantly, an episomalD427N version of SKN7 was also found to reverse the hypersensitivityof DR20-2b to hydrogen peroxide (Figure 6). Furthermore, the Skn7^D427N mutant also restored HSE2-LacZ expression in skn7 $Delta$ cells (ourunpublished results), suggesting that phosphorylation of D427is not required for Skn7p function through binding HSEs. In contrast,Skn7^D427N fails to activate CLN1 and CLN2 expression in a swi4^ts swi6 $Delta$ background (Morgan et al., 1995) or to rescue the cellwall assembly defect of the kre9 $Delta$ mutant (Brown et al., 1994).Hence, phosphorylation of the receiver domain, presumably by theSLN1-YPD1 phosphohistidine relay (Li et al., 1998; Posas et al.,1996), can direct the activation of Skn7 function to differenttargetgenes.

Skn7 and Hsf1 Interact Physically

To extend these data suggesting a genetic interaction between Skn7 and Hsf1, we undertook copurification analysis to determineif these proteins interact physically. Thus, the SKN7 gene wasplaced under the control of the GAL1 promoter in plasmid YCpIF16(Foreman and Davis, 1994) and fused in frame to the hemagglutinin(HA) epitope, and the HSF1 gene was fused in frame to the GSTepitope in the high-copy expression plasmid p426-GAG. Cell extractswere prepared from galactose-induced cultures and incubated withGST-Sepharose beads (see MATERIALS AND METHODS). Immunoblot analysisindicated that Skn7-HA copurified with GST-Hsf1 on the GST-Sepharosebeads (Figure 7A, lane 4). When the extracts were prepared froma strain containing the empty vector, p426-GAG, Skn7-HA was notdetected in association with the beads (Figure 7A, lane 2). Toconfirm this result, we used extracts prepared from the same straincontaining p426-GAG-HSF1 grown on glucose to repress synthesisof Skn7-HA from the GAL promoter. Skn7 was found not to associatewith the GST-Sepharose beads (Figure 7B, lane 3; compare withlane 4, in which galactose-grown cells were used).

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Figure 7. Hsf1 and Skn7 copurify. (A) Western blot analysis with 12CA5 mAb reveals that pGAL-Skn7-HA copurifies with GST-Hsf1. Lane 1, crude extract containing GST vector alone and pGAL-Skn7-HA; lane 2, GST pull-down from extract containing pGAL-Skn7-HA and GST vector alone; lane 3, crude extract containing pGAL-Skn7-HA and GST-Hsf1; lane 4, GST pull-down from cells containing pGAL-Skn7-HA and GST-Hsf1. (B) Lane 1, 20 µg of input protein (HA-Skn7); lane 2, GST pull-down of extract from cells containing empty GST vector and pGAL-Skn7-HA; lane 3, GST pull-down of extract from cells containing GST-Hsf1 vector and pGAL-Skn7-HA and grown in glucose; lane 4, GST pull-down of extract from galactose-grown cells containing pGAL-Skn7-HA and pGST-Hsf1. (C) Nickel-affinity copurification of Hsf1 with 6His-tagged Skn7. Lane 1, immunoprecipitate with anti-Hsf1 antibody from 1 mg of whole cell extract of galactose-grown cells expressing pGAL-SKN7-6His; lane 2, Ni²⁺-NTA agarose beads plus 1 mg of cell extract that does not contain the 6His-Skn7 protein; lane 3, Ni²⁺-NTA agarose beads plus 1 mg of galactose-induced extract from cells expressing pGAL-SKN7-6His; lane 4, 20 µg of input galactose-induced extract. (D) Skn7p can interact with itself. Coimmunoprecipitations from cell extracts containing galactose-induced pGAL-Skn7-HA and 6Myc-Skn7 were performed with the use of 9E10 mAb followed by 12CA5 Western blot analysis. HA-Skn7p expression was under the control of the GAL promoter, and integrated 6Myc-Skn7 was under the control of its own promoter. Immunoprecipitations with 1.5 µg of 9E10 were as follows: lane 1, 20 µg of extract from galactose-grown cells; lane 2, immunoprecipitation of extract from glucose-grown cells; lane 3, immunoprecipitation of extract from galactose-grown cells that did not contain the Myc-tagged SKN7; lane 4; immunoprecipitation of extract from galactose-grown cells containing 6Myc-Skn7 and pGAL-Skn7-HA. Western blot analysis was carried out with 12CA5 mAb.

To determine whether Hsf1 also copurifies with Skn7, the complementary experiment was undertaken with an Ni²⁺-NTA affinity matrix to purify 6His-tagged Skn7p from a galactose-inducedcell extract. Subsequent Western analysis of the proteins associatedwith the nickel-bound Skn7 indicated that Hsf1 copurified withthe 6His-tagged Skn7 protein (Figure 7C, lane 3). No Hsf1 waspulled down in an extract without 6His-Skn7 (Figure 7C, lane 2).These results are consistent with the copurification of Skn7 withHsf1 and strongly suggest that they interact physically invivo.

Skn7 Can Interact with Itself In Vivo

Because Hsf1 is known to form homotrimers through its leucine zipper, we determined whether Skn7 could also interact withitself, given that Skn7 contains a similar coiled-coil region(Figure 1). To address this question, coimmunoprecipitations werecarried out with extracts from cells containing integrated 6Myc-taggedSkn7 under control of its own promoter and with high-copy HA-taggedSKN7 under galactose-inducible expression. Western analysis with12CA5 antibody revealed that precipitation with monoclonal 9E10anti-myc antibody specifically coprecipitates HA-Skn7 (Figure7D, lane 4) from a galactose-induced extract containing 6Myc-Skn7.In the absence of a Myc-tagged SKN7 gene, or with the use of acell extract derived from glucose-grown cells expressing GAL-HA-SKN7,no such coprecipitation was apparent (Figure 7D, lanes 2 and 3).These data suggest that Skn7 can oligomerize in vivo and thatthis may be central to its function, because disruption of theleucine zipper motif in Skn7 significantly compromises its function(Alberts et al., 1998).

Skn7p Is Localized to the Nucleus

To determine whether regulated nuclear import and export is an important mechanism by which the activity of the Skn7 responseregulator may be controlled, we constructed an SKN7-GFP fusionprotein in the CEN plasmid pRS416-sGFP (a gift from P. Silver)and examined the localization of Skn7. Figure 8 (C) shows thatSkn7-GFP colocalizes with the DAPI-stained nucleus (B) under nonstressedgrowth conditions. This localization was unaffected by the additionof t-butyl hydrogen peroxide (our unpublished results). The nuclearlocalization of Skn7 is consistent with its role as a transcriptionalregulator.

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Figure 8. The Skn7 response regulator is localized in the nucleus. An SKN7-GFP fusion protein expressed from a CEN plasmid was visualized in cells from a midlog-phase culture (A; Nomarski image). The Skn7p-GFP fusion protein visualized by fluorescence (C) colocalizes with the DAPI signal of nuclear DNA (B).

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Both Skn7 and Hsf1 have previously been shown to play important roles in the cellular response to oxidative stress. In thecase of the response regulator Skn7, it has been shown to cooperatewith the yeast AP-1 homologue Yap1 at the TRX2 promoter and tospecifically activate transcription of the thioredoxin and thioredoxinreductase genes in the presence of hydrogen peroxide (Morgan etal., 1997). Similarly, Hsf1-dependent activation of the CUP1 metallothioneingene was observed in yeast cells treated with the superoxide generatormenadione (Liu and Thiele, 1996). Here, we provide evidence thatSkn7 is required for efficient heat shock gene activation in responseto hydrogen peroxide. We also show that Skn7 and Hsf1 interactphysically and genetically and have identified target genes knownto be regulated by Hsf1 that are also regulated by Skn7 in responseto free radicalstress.

Physical and Genetic Interactions between Hsf1 and Skn7

A genetic interaction between Hsf1 and Skn7 is indicated by several observations. First, the restrictive temperature of anhsf1^ts skn7 $Delta$ strain is decreased relative to that of the parental hsf1^ts strain. Second, the growth defect of the hsf1^ts strain is partially suppressed by high-copy expression of theSKN7 gene. That this suppression is partial indicates that Skn7can fulfill some but not all of the functions of Hsf1 in the cell.This observation is not surprising given the pleiotropic natureof the hsf1-m3 mutation (Smith and Yaffe, 1991). Third, by reducingthe activity of Hsf1 in skn7 $Delta$ cells through construction of thedouble mutant strain hsf1^ts skn7 $Delta$ , the sensitivity of skn7 $Delta$ cells to hydrogen peroxide isgreatly enhanced. This hypersensitivity could be suppressed byectopic expression of either SKN7 or SKN7^D427N. These observations indicate that Skn7 and Hsf1 have overlappingfunctions in the stress response, presumably in the activationof particular stress-responsivegenes.

Consistent with these observations, we have obtained several lines of evidence suggesting that Skn7 and Hsf1 interact physically.First, in extracts prepared from strains coexpressing Skn7-HAand GST-Hsf1, HA-tagged Skn7 copurified with GST-Hsf1 on glutathione-Sepharosebeads. Physical interaction between these proteins was also shownwith the use of a complementary pull-down assay; Hsf1 associatedwith 6His-tagged Skn7 on nickel-agarose beads. Previous work hadsuggested that Skn7 interacts with a number of proteins, includingYap1 (Morgan et al., 1997), Rho1 (Alberts et al., 1998), Sln1-Ypd1(Li et al., 1998), and Mbp1 (Bouquin et al., 1999). In no casehas coimmunoprecipitation been demonstrated with any of theseproteins. Only a small proportion of total cellular Skn7 may associatewith any of these proteins at one time, rendering coimmunoprecipitationstudies difficult. Nonetheless, the copurification of Skn7 withHsf1 described here argues strongly for a physicalinteraction.

Skn7 Is Required to Activate Heat Shock Gene Expression Specifically in Response to Hydrogen Peroxide

An implication of the interaction between Hsf1 and Skn7 is a role for Skn7 in regulating heat shock gene expression. Preliminarystudies with the use of an SSA1-LacZ fusion construct indicatedthat Skn7 was required for HSE-mediated LacZ induction in responseto hydrogen peroxide but was not required for the heat shock inductionof the reporter (Table 1). Northern analysis of heat shock geneexpression in wild-type and skn7 $Delta$ cells confirmed that SKN7 wasnot required for induction of these genes in response to heatshock. For example, when cells are shifted from 25 to 39°C, theheat shock induction of HSP12 in skn7 $Delta$ cells was identical tothat in the isogenic wild-type strain. In contrast, the 5-foldinduction of this gene by hydrogen peroxide in the wild type waslargely abolished in the isogenic skn7 $Delta$ strain. The skn7 $Delta$ mutationalso significantly reduced the 20-fold induction of HSP26 andthe 9-fold induction of HSP104 by hydrogen peroxide without affectingtheir responses to heat shock activation (Figure 4). The residualinduction of these genes in response to oxidative stress couldbe dependent on the other known activators of these genes, suchas Hsf1 and the Msn2/Msn4 transcription factor. The latter canactivate expression through upstream activation sequence elementsunrelated to HSEs (Martínez-Pastor et al., 1996; Schmitt andMcEntee, 1996).

The requirement for Skn7 in hydrogen peroxide induction of HSP12 is intriguing given that induction of this gene by a varietyof other stresses has been shown to be mediated through STRE sequencesby Msn2/Msn4 (Martínez-Pastor et al., 1996) and, in responseto osmotic shock, by the high osmolarity glycerol (HOG) MAPK pathway(Varela et al., 1995). We note, however, that hydrogen peroxideinduction of this and other STRE-regulated genes does not appearto be affected significantly by mutations in Msn2 or Msn4 (Schülleret al., 1994). It appears likely, therefore, that regulation ofHSP12 (and perhaps other STRE-regulated genes such as HSP26 andHSP104) in response to hydrogen peroxide-generated oxidative stressis mediated principally by Skn7 and Hsf1, whereas activation inresponse to other stress conditions is regulated through the STREelements and downstream effectors of the HOG pathway. In thiscontext, it is interesting that the HOG1 pathway is itself regulatedby the SLN1 histidine kinase, which also seems to regulate theactivity of the Skn7 response regulator (Li et al., 1998).

Structural Homology between Skn7 and Hsf1

With regard to the Skn7-Hsf1 interaction in the oxidative stress response, the structural similarities of the two proteinsare of particular interest. We have shown through EMSA that Skn7purified from yeast or E. coli can bind to a 26-base pair probederived from the HSE2 regulatory region of the SSA1 promoter.This binding is of a similar specificity to that of Hsf1, insofaras mutation of the GAAnnTTC sequence to AAAnnTTT ablates bindingof both Hsf1 and Skn7. Previously, we identified a regulatorysite within the TRX2 promoter through which Skn7 can act (Morganet al., 1997). The site contains the sequence CCGAAA in whichmutation of the CG nucleotides to AT was found to reduce the bindingof Skn7 by 20-fold. The common motif between this regulatory sequenceand HSEs is the GAA triplet, three inverted repeats of which inthe sequence AGAAn constitute a consensus HSE. Although the exactconsensus binding site for Skn7 has not been established, thetriplet GAA evidently represents a potential core recognitionsequence.

In terms of sequence specificity of Skn7 recognition of HSEs versus that of Hsf1, there is one notable divergence betweentheir otherwise highly conserved DNA-binding domains. This occursat the last residue of the $alpha$ 3 sequence recognition helix of Hsf1(Harrison et al., 1994), where the invariant M58 and G60 residuesare replaced by K58 and D60, respectively, in the Skn7 protein(with residues numbered according to Figure 1). These substitutionsmay have a significant effect on DNA-binding specificity or thestability of Skn7 relative to Hsf1 because G60 of Hsf1 has beenproposed to contact the DNA (Damberger et al., 1994). All otherresidues proposed to contact the DNA, however, are conserved betweenSkn7 andHsf1.

The other region of structural homology between these two proteins lies between residues 222 and 303 of the Skn7 protein.This stretch contains five heptad repeats, with hydrophobic residuesat positions 1 and 4 and polar residues elsewhere in the repeatunits, characteristic of regions that form coiled-coil structures(Lupas, 1996). Hsf1 contains six heptad repeats that have beenshown to mediate trimerization of the protein through the formationof triple-stranded $alpha$ -helical coiled coils (Sorger and Nelson,1989; Peteranderl and Nelson, 1992; Rabindran et al., 1993). Thesecoiled coils are also known to mediate heterodimerization andhomodimerization, e.g., of the yeast GCN4 member of the bZIP transcriptionfactor family (Harbury et al., 1993). We have demonstrated thatSkn7, in common with Hsf1, can interact with itself in vivo andthat these proteins can interact with each other. We have alsoshown that the Skn7 response regulator is constitutively localizedto the nucleus and can bind to HSEs with a similar specificityto that of Hsf1. We are currently exploring the possibility thatit is through the formation of heterodimers and/or heterotrimersthat Skn7 and Hsf1 can mediate the activation of heat shock genes,and possibly other sets of genes, in response to oxidative stress.The markedly increased sensitivity to oxidative stress of an hsf1^ts skn7 $Delta$ strain relative to either single mutant (Figure 6) supportssuch a cooperativeassociation.

In summary, we have shown that Skn7 interacts with Hsf1 and can bind to the same consensus sequence as Hsf1. We have furthershown that SKN7 is required for the induction of heat shock genesin response to t-butyl hydrogen peroxide, although it is not requiredfor their heat shock induction. In addition, we have demonstratedfor the first time the nuclear localization of a response regulatorin yeast, which was found to be independent of the presence orabsence of oxidative stress. In the light of these data, we proposea model whereby Skn7 becomes activated in response to hydrogenperoxide stress and either by dimerization or through the formationof a heterotrimeric Skn7-Hsf1 complex binds to the promoters ofstress-responsive genes. The actual mechanism by which eitherSkn7 or Hsf1 activates gene expression in response to stress remainsunclear, although recent evidence suggests that Hsf1 can interactwith TATA-binding protein (Mason and Lis, 1997) and with a phosphatasethat may modulate the transcriptional activity of a subset ofpromoters, including CUP1, through interaction with the repressorregion of Hsf1 (Lin and Lis, 1999). Hsf1 can also antagonize nucleasomalrepression (Erkine et al., 1996). It is possible, therefore, thatthe transcription activation function of Hsf1 is enhanced by itsinteraction with Skn7 or that Skn7 itself potentiates the interactionswith components of the basal transcription apparatus at heat shockcore promoters in response to oxidativestress.

	ACKNOWLEDGMENTS

We gratefully acknowledge the kind gifts of plasmid pZJHSE2-137 and anti-GST HSF antibodies from E. Craig and the gifts ofstrains, plasmids, and antibody reagents used in the initial stagesof this work from S. Lindquist. We also thank A. Sewell for plasmidpAKS80. We thank A. Spanos, D. Fesquet, and W. Morgan for helpfuladvice and discussion. D.C.R. was supported by a European CommunityNetwork fellowship (contract number ERBCHRXCT930248). Work performedin the laboratory of D.S.G. was supported by a grant from theNational Institute of General Medical Sciences(GM45842).

	FOOTNOTES

Corresponding author. E-mail address: desmond_raitt{at}dfci.harvard.edu.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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