Functional Dissection of Yeast Hir1p, a WD Repeat–Containing Transcriptional Corepressor

Functional Dissection of Yeast Hir1p, a WD Repeat–Containing Transcriptional Corepressor

Heshani DeSilva^a, Kenneth Lee^a, and Mary Ann Osley^a
^a Program in Molecular Biology, Sloan Kettering Cancer Center and Cornell University Graduate School of Medical Sciences, New York, New York 10021

Corresponding author: Mary Ann Osley, Box 554, Sloan Kettering Cancer Center, 1275 York Ave., New York, NY 10021, m-osley{at}ski.mskcc.org (E-mail).

Communicating editor: A. P. MITCHELL

ABSTRACT

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

The HIR1 gene product is required to repress transcription ofthree of the four histone gene loci in Saccharomyces cerevisiae,and like its counterpart, the HIR2 protein, it functions asa transcriptional corepressor. Although Hir1p and Hir2p arephysically associated in yeast, Hir1p is able to function independentlyof Hir2p when it is artificially recruited to the histone HTA1promoter. A deletion analysis of HIR1 has revealed two separaterepression domains: one in its N terminus, where seven copiesof the ß-transducin or WD40 motif reside, and the secondin the remaining C-terminal amino acids. Overexpression of theWD repeats in a hir1 ${Delta}$ strain complemented its Hir^- phenotype,while overexpression of the C terminus in a wild-type straincaused both Hir^- and Spt^- phenotypes. The Hir1p C terminus physicallyinteracted in vivo with Hir2p, and both Hir1p repression domainsinteracted with full-length Hir1p. It was additionally foundthat the Hir1p WD repeats functionally interacted with the SPT4,SPT5, and SPT6 gene products, suggesting that these repeatsmay direct Hir1p to different protein complexes.

TRANSCRIPTIONAL repression has emerged as an increasingly importantmechanism to control gene expression in eukaryotes. Althoughmany eukaryotic repressors are site-specific, DNA-binding proteins,a number of them have been classified as transcriptional corepressorsbecause they function without directly contacting DNA. In theabsence of DNA binding, transcriptional corepressors can betargeted to gene promoters in several ways. For example, theSaccharomyces cerevisiae Tup1p and Ssn6p corepressors (KELEHERet al. 1992 ; TZAMARIAS and STRUHL 1994 ) are recruited toa subset of yeast promoters by their association with site-specific,DNA-binding proteins such as ${alpha}$ 2 and Mig1p (KOMACHI et al. 1994; TREITEL and CARLSON 1995 ; TZAMARIAS and STRUHL 1995 ).Other transcriptional corepressors, such as yeast Sin4p ( JIANGand STILLMAN 1992 ), are recruited to promoters because theyare components of the RNA polymerase II mediator/holoenzymecomplex (LI et al. 1995 ). We have obtained evidence that Hir1pand Hir2p, two regulators of histone gene transcription (OSLEYand LYCAN 1987 ; SHERWOOD et al. 1993 ), are transcriptionalcorepressors of the class exemplified by the Tup1 and Ssn6 proteins.The two Hir proteins do not appear to bind to DNA, but can actas direct transcriptional repressors when artificially recruitedto yeast promoters (SPECTOR et al. 1997 ). We have speculatedthat they are targeted to specific histone gene promoters, includingthe promoter of the divergently transcribed HTA1-HTB1 locus,by their interactions with as yet unidentified DNA-binding proteinsthat act at defined upstream negative regulatory sites (OSLEYet al. 1986 ; LYCAN et al. 1987 ; OSLEY 1991 ; SHERWOOD 1993; FREEMAN et al. 1992 ). At these promoters, Hir1p and Hir2p,which appear to form a complex in vivo, function to keep thehistone HTA1, HTB1, HHT1, HHT2, HHF1, and HHF2 genes repressedfor most of the cell cycle (SPECTOR et al. 1997 ).

Hir1p and Hir2p may not act alone at histone gene promoters.Among the other proteins with which they are likely to act arethe products of the HIR3/HPC1, HPC2, HPC3, HPC4, and HPC5 genes,which were also identified in screens for histone gene regulators(XU et al. 1992 ), and the products of the SPT4, SPT5, and SPT6genes (CLARK-ADAMS and WINSTON 1987 ; NEIGEBORN et al. 1987; CLARK-ADAMS et al. 1988 ; SWANSON and WINSTON 1990 , SWANSONand WINSTON 1992 ; SWANSON et al. 1991 ; MALONE et al. 1993). The two HIR and three SPT gene products are functionallyrelated because mutations in both sets of genes suppress his4-912 ${delta}$ insertion mutations in the same way as mutations in the genesthat encode histones H2A and H2B (CLARK-ADAMS et al. 1988 ; SHERWOOD and OSLEY 1991 ). A further link between the two groupsof proteins was also shown by the observation that mutationsin the SPT4, SPT5, and SPT6 genes decrease the level of transcriptionfrom the histone HTA1- HTB1 locus, which is subject to Hir-mediatedrepression (COMPAGNONE-POST and OSLEY 1996 ). One possible explanationfor this effect is that the three SPT gene products affect HTA1and HTB1 transcription through Hir1p or Hir2p.

To understand how Hir1p represses the transcription of selectedgenes, and to learn how the Hir2, Spt4, Spt5, and Spt6 proteinsfunction in this process, we identified the regions of Hir1pthat are responsible for repression in vivo. Hir1p was foundto have two separate repression domains. The first, which comprisesseven copies of a canonical ß-transducin (WD40) repeat(NEER et al. 1994 ), complemented the Hir^- defect of a hir1 ${Delta}$ strain when it was overexpressed. The second, which includesthe remaining Hir1p C-terminal amino acids, produced both Hir^-and Spt^- phenotypes when it was overexpressed in a wild-typestrain. These two regions of Hir1p also showed differentialin vivo interactions with Hir1p, Hir2p, and Spt4p/Spt5p/Spt6p:The C terminus of Hir1p could be coimmunoprecipitated from yeastcell extracts with Hir2p and Hir1p, while the WD40 repeats physicallyinteracted with Hir1p and functionally interacted with the threeSpt proteins. Together, the results suggest that the two repressiondomains promote the interaction of Hir1p with diverse proteinsand thus may contribute to the activity of Hir1p at selectedpromoters.

MATERIALS AND METHODS

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Strains, growth conditions, and RNA analysis:
The yeast strains used in this study are listed in Table 1.The lithium acetate method was used for plasmid transformations(ITO et al. 1983 ), with selection for the prototrophic markerpresent on each plasmid. Cells were grown in SD medium supplementedwith appropriate amino acids and bases or in YPD medium (KAISERet al. 1994 ). The latter medium was used for studies in whichDNA replication was blocked with 0.2 M hydroxy-urea for 30 minto measure the Hir phenotype of strains (OSLEY and LYCAN 1987). All strains were grown at 30°, except for FY546, whichwas grown at 24° and then shifted to 37° for 90 minto inactivate the SPT6 gene product. The Spt phenotype of HIRand hir1 ${Delta}$ strains was measured by spotting serial dilutions ofcells on SD medium with and without histidine, followed by incubationat 24° for 3–5 days.

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Table 1. Yeast strains

Total RNA was prepared from yeast strains and hybridized toend-labeled probes specific for lacZ and RP51A mRNA, as describedpreviously (OSLEY et al. 1986 ; MORAN et al. 1990 ). AfterS1 nuclease digestion, the protected fragments were separatedon 4% acrylamide–8-M urea gels, which were dried and exposedto film or quantitated by phosphoimager analysis on a phosphoimager(Fuji, Stamford, CT) using MACBAS software.

Plasmids:
HTA1-lacZ reporter plasmids with and without lexA operator sitesare derivatives of plasmid pCALA1 and have been described previously(RECHT et al. 1996 ; SPECTOR et al. 1997 ). Plasmid pCALA1is a LEU2 CEN4 plasmid in which the lacZ gene is under controlof the wild-type HTA1-HTB1 promoter (OSLEY et al. 1986 ).

Plasmid pBTM116 contains a full-length lexA gene under controlof the ADH1 promoter (S. FIELDS, personal communication). PlasmidspBTM-HIR1 and pBTM-HIR2, which contain fusions of the full-lengthHIR1 or HIR2 coding region to the C terminus of lexA, have beendescribed previously (SPECTOR et al. 1997 ). Truncated HIR1genes were fused to the C terminus of lexA on plasmid pBTM116using oligonucleotide-directed mutagenesis by PCR (AUSUBEL etal. 1989 ). For each fusion gene, a SmaI restriction site wascreated in frame with an ATG initiation codon, and SmaI-SalI restriction fragments that contained different segments ofHIR1 were ligated to SmaI-Sal I–digested pBTM116. In plasmidspBTM-HIR1^7WD, pBTM-HIR1^3WD, and pBTM-HIR1^1WD, a SmaI site andATG inition codon were placed at the beginning of the first(7WD), fifth (3WD), and seventh (1WD) WD repeat of HIR1 witholigonucleotides 5'-CCAAAGGTCTCTCCCGGGATGAAAGTG-3' (7WD), 5'-TATCACAACCCGGGGGATATGTCTTT-3'(3WD),and 5'-ACAAGTAGCCCGGGGCCAATGTTA-3'(1WD), and a translation terminationcodon and SalI site were placed immediately after the seventhWD40 repeat of HIR1 with the oligonucleotide 5'-AATTGGCTTGTCGACTTCATTATTTTC-3'.To create plasmid pBTM-HIR1^Cterm, a SmaI site and ATG codonwere placed at position +529 in the HIR1 ORF, immediately afterWD40 repeat 7, using the oligonucleotide 5'-AATAAT GACCCGGGCATGCCAATT-3'.A SmaI-Sal I fragment that contained the natural HIR1 translationtermination codon was then inserted into plasmid pBTM116.

Various segments of the HIR1 coding region were fused to thenative HIR1 promoter by their insertion into a promoter cassettein plasmid YEp352, a 2µ URA3 vector. To construct thiscassette, a SmaI site was created immediately before the HIR1ATG codon by PCR-directed mutagenesis, using the oligonucleotide5'TACCACTTTCATCCCGGGAGAGACCTT-3', and an EcoRI-SmaI fragmentthat contained the HIR1 promoter was subcloned into plasmidYEp352. The promoter cassette was digested with SmaI and SalIand was used as a recipient for SmaI-Sal I fragments isolatedfrom HIR1 inserts in plasmid pBTM116. Plasmid YEpHIR1 containsthe entire HIR1 ORF, YEpHIR1^1WD+Cterm contains the WD repeat7 and C terminus of HIR1, YEpHIR1^1WD contains WD repeat 7, YEpHIR1^3WDcontains WD repeats 5-7, YEpHIR1^7WD contains WD repeats 1–7,and YEpHIR1^Cterm contains amino acids 392–840) from theHIR1 C terminus. To construct YCpHIR1^7WD, an EcoR I-Sal I fragmentfrom YEpHIR1^7WD was subcloned into plasmid YCp50, a CEN-URA3vector.

The 2µ URA3 plasmids that carry hemagglutinin (HA)-taggedHIR1 and HIR2 genes and untagged HIR1 and HIR2 genes have beendescribed previously (SPECTOR et al. 1997 ). Plasmid pBTM-SPT4(LexA-Spt4p) was constructed by oligonucleotide-directed mutagenesiswith the oligonucleotides 5'-GGTACAGTCCCGGGGATGTCTAGTGAAAGA-3'(SmaI at start codon) and 5'-GTGATATCAGAGTCGACGGTTTTACT CAAC-3'(Sal I at stop codon). Plasmid pBM65 (2µ URA3 HA-SPT4)was generously provided by FRED WINSTON.

All gene constructions were confirmed by DNA sequence analysisusing double-stranded DNA templates with dideoxy chain terminators(SANGER et al. 1977 ).

Immunological analysis:
Whole-cell extracts were prepared as described previously (SPECTORet al. 1997 ) from BJ5465 cells (Table 1) that had been cotransformedwith high copy number plasmids carrying various combinationsof epitope-tagged or untagged HIR1, HIR2, or SPT4 genes. Between150 and 600 µg of crude lysate were incubated with 2.5µl of monoclonal antibody 12C5A directed against the HAepitope or with 0.5 µl of rabbit polyclonal antibody againstLexA under conditions that have been described previously (SHERWOODet al. 1993 ; SPECTOR et al. 1997 ). After the last wash, theimmunoprecipitates were resuspended in 20 µl of SDS samplebuffer and heated at 100° for 5 min (AUSUBEL et al. 1989). The eluate (5 µl) was analyzed on 7.5 or 12.5% SDSpolyacrylamide gels for the presence of the tagged protein recognizedby the primary antibody, and 15 µl was analyzed by 7.5or 12.5% SDS-PAGE for the presence of coimmunoprecipitated proteins.After electrophoresis, the proteins were transferred to Immobilonfilters, and Western blot analysis was performed with eitheranti-HA antibody (1:1000 dilution) or anti-LexA antibody (1:2000dilution) using enhanced chemiluminescence for detection accordingto manufacturer's directions (Dupont-NEN, Wilmington, DE).

RESULTS

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Hir1p contains two repression domains:
The HIR1 gene product belongs to a diverse and expanding groupof proteins that contain multiple copies of the ß-transducinor WD40 motif, which has been been postulated to mediate protein–proteininteractions (FONG et al. 1986 ; HARTLEY et al. 1988 ; DALRYMPLEet al. 1989 ; WHITEWAY et al. 1989 ; KOMACHI et al. 1994 ; NEER et al. 1994 ; SATHE and HARTE 1995 ; KAUFMAN et al.1997 ). Seven copies of this motif are present at the N terminusof the Hir1 protein (LAMOUR et al. 1995 ). To investigate whetherthese repeats were required for Hir1p to function as a transcriptionalrepressor, we deleted the entire WD40 domain (amino acids 1–389)and fused the remaining C-terminal region (amino acids 392–840)to LexA (BRENT and PTASHNE 1984 ), and we then directed theLexA-Hir1(Cterm) fusion protein to lexA operator sites at thepromoter of an HTA1-lacZ reporter gene (Figure 1). We showedpreviously that a full-length LexA-Hir1 fusion protein actedas a direct transcriptional repressor in this context, and thatit responded appropriately to several cell-cycle regulatorysignals (SPECTOR et al. 1997 ). Thus, the LexA tethering assayprovided a convenient method by which to monitor the functionalstate of Hir1p. The results indicated that the seven WD repeatswere dispensable for repression by tethered Hir1p; in theirabsence, the 448 C-terminal amino acids (hereafter referredto as the Hir1p C terminus) repressed HTA1-lacZ transcriptionalmost as strongly as a full-length Hir1 fusion protein (Figure1A, Table 2). We next asked whether the seven WD repeats ontheir own (amino acids 1–389) repressed transcription whenthey were brought to the HTA1 promoter (Figure 1B). Althoughrepression was slightly weaker, it was still significant (Table2), indicating that Hir1p contains two separate repression domains—onethat includes the N-terminal seven WD repeats and another thatencompasses the remaining amino acids of the C terminus.

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Figure 1. The N and C terminus of Hir1p can repress transcription when tethered at the HTA1 promoter. A HIR strain (W303-1A, Table 1) that contained an HTA1-lacZ reporter gene with (+OP) or without (-OP) two lexA operator sites at the HTA1 promoter was transformed with LexA plasmids: (A) pBTM116 (LexA), pBTM-HIR1 (LexA-Hir1), and pBTM-HIR1^Cterm [(LexA-Hir1(Cterm)]; (B) pBTM116, pBTM- HIR1, pBTM-HIR1^7WD [LexA-Hir1(7WD)], pBTM-HIR1^3WD [LexA-Hir1(3WD)], and pBTM-HIR1^1WD [LexA-Hir1(1WD)]. The levels of lacZ mRNA were measured by an S1 nuclease protection assay and compared to the levels of RP51A mRNA, which served as an internal loading control.

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Table 2. Levels of HTA1-lacZ mRNA in HIR and hir1 ${Delta}$ strains transformed with lexA-HIR1 fusion genes

To determine how many WD repeats were required for transcriptionalrepression in this assay, we constructed two additional lexAfusion genes that contained either a single copy (WD repeat7, amino acids 448–389) or three copies (WD repeats 5–7,amino acids 213–389) of the Hir1p WD repeats, and we examinedtheir effects on HTA1-lacZ transcription (Figure 1B). Repressionwas observed in both cases, with the tethered protein that containedthree WD repeats conferring a slightly stronger effect (Table2). Nonetheless, because a single WD repeat caused significantrepression when it was brought to the HTA1 promoter, the datasuggest that a small number of these repeats might contributeto the repression function of the native Hir1 protein.

The Hir1 protein physically interacts with itself and with theHir2 protein in vivo (SPECTOR et al. 1997 ). Having identifiedtwo repression domains in Hir1p, we wished to determine whetherthese domains showed different physical interactions with Hir1por Hir2p. lexA-HIR1 fusion genes that contained the completeHIR1 ORF, the seven HIR1 WD repeats (lexA-HIR1^7WD), or the HIR1C terminus (lexA-HIR1^Cterm) were cotransformed with a HA-HIR1or HA-HIR2 gene into a protease-deficient strain to reduce nonspecificproteolysis during extract preparation. The HA-Hir1 or HA-Hir2proteins were precipitated from whole-cell extracts with anantibody against the HA epitope, and Western blot analysis withanti-LexA antibodies was used to follow the presence of thetwo LexA-Hir proteins both in the immune precipitates (P) andin the supernatant fractions (S) that remained after precipitation(Figure 2). The results showed that both the Hir1p WD repeatsand C terminus could be coprecipitated with full-length HA-Hir1p(Figure 2A, lanes 2 and 6), although only a fraction (~10%)of each LexA fusion protein was associated with HA-Hir1p. Thisassociation was specific, however, because it was not observedin strains in which an untagged HIR1 gene was substituted forthe HA-HIR1 gene (Figure 2A, lanes 4 and 8). In contrast, onlythe LexA-Hir1(Cterm) fusion protein was coprecipitated withHA-Hir2p (Figure 2B, lane 6), an association that was specificto the presence of the HA epitope in Hir2p (Figure 2B, lane8). It also appeared that a larger fraction of the LexA-Hir1(Cterm)protein was associated with HA-Hir2p (~20%) than with HA-Hir1p,perhaps reflecting stronger heterotypic interactions throughthis region of Hir1p. The small amount of LexA-Hir1(7WD) thatcoprecipitated with HA-Hir2p (Figure 2B, lane 2) appeared torepresent a nonspecific interaction because an equivalent amountof the fusion protein was present in the immuneprecipitate fromcells cotransformed with an untagged HIR2 gene and a lexA-HIR1^(7WD)gene (Figure 2B, lane 4).

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Figure 2. Differential immunoprecipitation of the Hir1p WD repeats and C terminus with Hir1p and Hir2p. Strain BJ5465 (Table 1) was transformed with high copy number plasmids: (A) YEpHIR1(HA) or YEpHIR1; (B) YEpHIR2(HA) or YEpHIR2. pBTM116 plasmids expressing the seven Hir1p WD repeats [LexA-Hir1p(7WD)] or Hir1p C terminus [LexA-Hir1p(Cterm)] were then introduced into each strain. Whole-cell extracts were prepared, and 150 µg of lysate was incubated with a monoclonal antibody against the HA epitope. After precipitation of the HA-tagged proteins, the presence of LexA-Hir1 proteins in the immuneprecipitates (P) and in 13 µg of the unbound supernatant fractions (S) was examined by Western blot analysis with a polyclonal antibody against LexA. (A) Lanes 1 and 2, HA-Hir1p and LexA-Hir1p (7WD); lanes 3 and 4, untagged Hir1p and LexA-Hir1p (7WD); lanes 5 and 6, HA-Hir1p and LexA-Hir1p(Cterm); lanes 7 and 8, untagged Hir1p and LexA-Hir1p(Cterm). (B) Lanes 1 and 2, HA-Hir2p and LexA-Hir1p(7WD); lanes 3 and 4, untagged Hir2p and LexA-Hir1p(7WD); lanes 5 and 6, HA-Hir2p and LexA-Hir1p(Cterm); lanes 7 and 8, untagged Hir2p and LexA-Hir1p(Cterm).

We addressed the functional significance of these physical interactionsby determining whether the HIR1 gene product was required forthe Hir1p WD repeats or C terminus to repress transcriptionwhen tethered at the HTA1 promoter (Table 2, Figure 3). Aswe observed previously (SPECTOR et al. 1997 ), the tethered,full-length Hir1 protein was not as strong a repressor whenHir1p was absent (Table 2). The tethered C terminus also showeda partial Hir1p dependence, while the tethered WD repeats (one,three, or seven copies) generally exhibited the strongest requirementfor Hir1p (Table 2). These dependencies represented true functionaldependencies because each LexA fusion protein was made at approximatelyequivalent levels in both HIR and hir1 ${Delta}$ backgrounds (H. DESILVA,unpublished data).

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Figure 3. Effect of hir1 ${Delta}$ on repression by the tethered WD repeats or C terminus of Hir1p. Strain W303 ${Delta}$ 1 (hir1::HIS3, Table 1), which contained an HTA1-lacZ reporter gene with (+OP) or without (-OP) lexA operator sites at the promoter, was transformed with LexA plasmids pBTM116, pBTM-HIR1, pBTM-HIR1^7WD, and pBTM-HIR1^Cterm. The levels of lacZ mRNA were measured by a quantitative S1 nuclease protection assay and were compared to the levels of RP51A mRNA.

The residual repression seen with all of the LexA fusion proteinswas unlikely to depend on the Hir2 protein because deletionof the HIR2 gene reduced repression by full-length Hir1p, theHir1p C terminus, or the seven Hir1p WD repeats less than 1.5-fold(M. A. OSLEY, unpublished data). Thus, one interpretation ofthese combined studies is that the physical association of theHir1p C terminus with Hir2p and the Hir1p WD–WD interactionsrepresent different functional states of Hir1p.

Effects of spt4, spt5, and spt6 mutations on transcriptional repression by tethered Hir1p:
One explanation for the residual repression conferred by tethered,full-length Hir1p in a hir1 ${Delta}$ or hir2 ${Delta}$ strain is that proteinsother than Hir1p or Hir2p assist Hir1p in this function. Candidatesfor such proteins are the products of the SPT4, SPT5, and SPT6genes, a group of functionally related transcriptional repressorsthat may also act without directly binding to DNA (CLARK-ADAMSet al. 1988 ; SWANSON and WINSTON 1992 ). We recently showedthat mutations in these three SPT genes decreased transcriptionof the HTA1-HTB1 locus, a target of repression by Hir1p (COMPAGNONE-POSTand OSLEY 1996 ). To test the idea that the Spt proteins mightalter HTA1-HTB1 transcription through Hir1p, we asked whethermutations in each of the three SPT genes affected transcriptionalrepression by tethered, full-length Hir1p (Figure 4, Table3). Repression by LexA-Hir1p was found to be reduced in allthree spt mutants. The loss of repression was modest in spt5and spt6 backgrounds, and the largest decrease was seen in thespt4 mutant (Table 3). These effects were specific to Hir1pbecause repression by a tethered, full-length Hir2p proteinwas unaffected by mutations in either the SPT4, SPT5, or SPT6genes (Figure 4).

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Figure 4. Effects of spt4, spt5, and spt6 mutations on repression by tethered Hir1p or Hir2p. Plasmids pBTM116, pBTM-HIR1, and pBTM-HIR2 were transformed into the following strains: (A) JR1-2B (SPT) and JR1-12D (spt4 ${Delta}$ 1); (B) FY429 (spt5-194) and FY776 (spt6-140), each of which carried an HTA1-lacZ reporter gene with (+OP) or without (-OP) lexA operator sites at the HTA1 promoter. The levels of lacZ mRNA were measured by a quantitative S1 nuclese protection assay and were compared to the levels of RP51A mRNA.

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Table 3. Levels of HTA1-lacZ mRNA in SPT, spt4, spt5, and spt6 strains transformed with lexA-HIR1 fusion genes

We next asked whether the requirement of tethered Hir1p forSPT4 depended on the presence of the seven Hir1p WD repeatsor the Hir1p C terminus. We found that an spt4 mutation significantlyreduced repression by the tethered WD repeats but had littleeffect on repression by the tethered C terminus (Figure 5 and Table 3). In addition, we observed that repression by the tetheredWD repeats also required Spt5p and Spt6p (Table 3). Becausethe LexA fusion proteins are stable (H. DESILVA, unpublisheddata), these results reflected true functional dependencies.Together, the results suggest that the products of all threeSPT genes play a role in the function of Hir1p as a transcriptionalrepressor, and that this role depends on the presence of theseven WD repeats.

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Figure 5. Effect of an spt4 mutation on repression by the tethered WD repeats and C terminus of Hir1p. Plasmids pBTM116, pBTM-HIR1^Cterm, and pBTM-HIR1^7WD were transformed into the following strains: (A) JR1-2B (SPT) or (B) JR1-12D (spt4 ${Delta}$ 1), each of which contained an HTA1-lacZ reporter gene with (+OP) or without (-OP) lexA operator sites at the promoter. The levels of lacZ mRNA were measured in an S1 nuclease protection assay and were compared to the levels of RP51A mRNA.

Physical association between Hir1p and Spt4p:
Because of the partial functional dependence of tethered, full-lengthHir1p on Spt4p, we asked whether Hir1p and Spt4p might be physicallyassociated in yeast cells. High copy number plasmids carryinga full-length HIR1 gene fused to lexA and an HA-SPT4 gene werecotransformed into a protease-deficient strain, and HA-Spt4pwas precipitated from cell extracts with anti-HA antibody. Thepresence of LexA-Hir1p in the immuneprecipitates was examinedby Western blot analysis, using an antibody directed againstLexA (Figure 6A). LexA-Hir1p was found in the HA-Spt4p immunoprecipitatesonly if the cell extract had first been incubated with anti-HAantibody (Figure 6A, lanes 3 and 5); incubation with a nonspecificantibody did not result in LexA-Hir1p precipitation (Figure6A, lanes 2 and 4). Using a second pair of epitope tagged genes,HA-HIR1 and lexA-SPT4, we next precipitated LexA-Spt4p fromcell extracts with an antibody against LexA, and we examinedwhether HA-Hir1p was present in the immune precipitates by Westernblot analysis with an anti-HA antibody (Figure 6B). Again, Hir1pwas found to be associated with Spt4p only when the extractwas incubated with an antibody against LexA (Figure 6B, lane3), not with a nonspecific antibody (Figure 6B, lane 2). Weestimated that only a low percentage (1–2%) of Hir1p coprecipitatedwith Spt4p. Thus, Hir1p–Spt4p interactions may be significantlyweaker than either Hir1p–Hir1p or Hir1p–Hir2p interactions,suggesting a dynamic or unstable association.

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Figure 6. Coprecipitation of Spt4p and Hir1p from yeast cell extracts. Strain BJ5465 (Table 1) was cotransformed with plasmids expressing full-length, epitope-tagged SPT4 and HIR1 genes: (A) pBM65 (HA-Spt4p) and pBTM-HIR1 (LexA-Hir1p); (B) pBTM-SPT4 (LexA-Spt4p) and YEpHIR1-HA (HA-Hir1p). Whole-cell extracts were prepared, and the lysates were incubated with (A) monoclonal antibody against the HA epitope or (B) polyclonal antibody against the LexA epitope. After precipitation of the tagged Spt4 proteins, the presence of LexA-Hir1p or HA-Hir1p in the immuneprecipitates was measured by Western blot analysis, using antibodies against (A) LexA or (B) the HA epitope. The arrowheads indicate the position of the two epitope-tagged Hir1 proteins. (A) Lane 1, 27 µg of crude lysate; lane 2, 270 µg of lysate incubated with nonspecific primary antibody (rabbit ${alpha}$ -mouse); lane 3, 270 µg lysate incubated with ${alpha}$ -HA antibody; lane 4, 270 µg lysate incubated with nonspecific primary antibody (rabbit ${alpha}$ -mouse); lane 5, 270 µg lysate incubated with ${alpha}$ -HA antibody. Lanes 4 and 5 are the results of immuneprecipitation from a second crude lysate (not shown). (B) Lane 1, 60 µg of crude lysate; lane 2, 600 µg of lysate incubated with nonspecific primary antibody (rabbit ${alpha}$ -mouse); lane 3, 600 µg of lysate incubated with ${alpha}$ -LexA antibody.

We performed a similar analysis with HA-Spt6p (F. WINSTON, unpublisheddata) and LexA-Hir1p, but we were unable to detect reproduciblecoprecipitation of LexA-Hir1p with this Spt protein (K. L. LEE,unpublished data). Hir1p, then, may preferentially interactin vivo with Spt4p, which also interacts with Spt5p and Spt6p(F. WINSTON, personal communication). Because of the strongfunctional interactions between the seven Hir1p WD repeats andboth Spt4p (Figure 5) and Spt6p (Table 3), we also asked whetherLexA-Hir1p (7WD) could be coprecipitated with either HA-taggedSpt protein; again, we were unable to obtain reproducible coprecipitation(K. L. LEE, unpublished data). These interactions will be reinvestigatedwith untagged Hir1 proteins when antibodies against native Hir1pbecome available.

Effects of overexpression of the Hir1p WD repeats and C terminus:
Having identified two repression domains in Hir1p by the LexAtethering assay, we asked whether these domains functioned independentlyin the context of the native Hir1 protein. The seven Hir1p WDrepeats or the Hir1p C terminus were expressed under controlof the HIR1 promoter on a high copy number plasmid in a hir1 ${Delta}$ strain. The overexpressed WD repeats fully complemented theHir^- phenotype of this mutant (OSLEY and LYCAN 1987 ), restoringits ability to repress HTA1 transcription when DNA replicationwas inhibited (Figure 7A). The presence of the same repeatson a CEN plasmid failed to complement the Hir^- phenotype ofthe hir1 ${Delta}$ strain (Figure 7B), indicating that complementationrequired the overexpression of the Hir1p N terminus. To determinehow many WD repeats were required for complementation, we alsoexamined the effects of overexpression of three WD repeats (repeats5–7; Figure 7B) because these same three repeats wereable to repress transcription when tethered at the HTA1 promoter(Figure 1B). This construct was unable to complement the Hir^-phenotype of the hir1 ${Delta}$ mutant. These results suggest that morethan three WD repeats are required to substitute for the absenceof native Hir1p at the histone gene promoter. Alternatively,the presence of specific WD repeats might be required to conferthis regulatory effect.

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Figure 7. Effects of overexpression of the Hir1p WD repeats and C terminus on the Hir phenotype of HIR and hir1 ${Delta}$ strains. (A) Strain W303 ${Delta}$ 1 (hir1::HIS3, Table 1) carrying an HTA1-lacZ reporter gene under control of the wild-type HTA1 promoter was transformed with high copy number plasmids YEp352, YEpHIR1, YEpHIR1^1WD+Cterm, YepHIR1^Cterm, and YEpHIR1^7WD. (B) Strain W301 ${Delta}$ 1 carrying an HTA1-lacZ reporter gene was transformed with high copy number plasmids YEp352, YEpHIR1, YEpHIR1^7WD, YEpHIR1^3WD, and a centromeric plasmid, YCpHIR1^7WD. (C) Strain W303 (HIR) carrying an HTA1-lacZ reporter gene was transformed with high copy number plasmids YEp352, YEpHIR1, YEpHIR1^Cterm, and YEpHIR1^7WD. The strains were incubated in the absence (-) or presence (+) of hydroxyurea (HU) for 30 min to block DNA replication, and the levels of HTA1-lacZ mRNA were measured by a quantitative S1 nuclease protection assay and compared to the levels of RP51A mRNA. A Hir^- phenotype is represented by continued transcription of lacZ in the presence of HU.

Unlike the Hir1p WD repeats, the overexpressed Hir1p C terminuswas unable to complement the Hir^- phenotype of the hir1 ${Delta}$ mutant(Figure 7A). Instead, when this region of Hir1p was overexpressedin a HIR strain, it caused a Hir^- phenotype, an effect not observedwhen the Hir1p WD repeats or full-length Hir1p were overproducedin the same wild-type background (Figure 7C). A surprising resultwas observed when a single copy of the Hir1p WD40 motif (repeat7) was added back to the C terminus. This construct now complementedthe Hir^- phenotype of the hir1 ${Delta}$ strain (Figure 7A), and it suppressedthe Hir^- phenotype caused by overexpression of the C terminusin a wild-type strain (H. DESILVA, unpublished data).

A second phenotype associated with the absence of HIR1 is thesuppression of the his4-912 ${delta}$ allele, or an Spt^- (His⁺) phenotype(SHERWOOD and OSLEY 1991 ; SHERWOOD et al. 1993 ). We thereforeasked whether overexpression of either the seven Hir1p WD repeatsor Hir1p C terminus complemented the Spt^- phenotype of a hir1 ${Delta}$ his4-912 ${delta}$ strain (Figure 8A). Neither construct was able to correctthe Spt^- defect of this strain (Figure 8A). Next, we asked whetheroverexpression of either Hir1p domain produced a Spt^- phenotypein a HIR his4-912 ${delta}$ background (Figure 8B). A strong Spt^- phenotypewas found to be associated with overexpression of the Hir1pC terminus, but not with overexpression of full-length Hir1por the seven Hir1p WD repeats. The addition of a single WD40repeat (repeat 7) to the Hir1p C terminus reversed its abilityto cause an Spt^- phenotype in the wild-type strain (Figure 8B),but this same construct could not complement the Spt^- phenotypeof a hir1 ${Delta}$ mutant (Figure 8A).

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Figure 8. Effects of overexpression of the Hir1p WD repeats and C terminus on the Spt phenotype of HIR and hir1 ${Delta}$ strains. High copy number plasmids YEp352, YEpHIR1, YEpHIR1^1WD+Cterm, YEpHIR1^Cterm, and YEpHIR1^7WD were transformed into strains (A) W303 ${Delta}$ 1 (hir1 ${Delta}$ ) and (B) W303 (HIR), each of which carrried the his4-912 ${delta}$ allele. Transformants were spotted onto SD-URA and SD-URA-HIS plates and grown for 3–5 days at 24°. An Spt^- phenotype is manifest as growth on SD-Ura-His plates, and an Spt⁺ phenotype is represented by failure to grow in the absence of histidine.

These phenotypic studies support the notion that the WD repeatsand C terminus make different contributions to the functionof Hir1p as a transcriptional corepressor. The WD repeats appearto be responsible for the specificity of Hir1p interactions,while the C terminus may contribute to the stoichiometry ofHir1p associations. Moreover, because overexpression of theHir1p WD repeats could correct the Hir^- but not the Spt^- phenotypeof a hir1 ${Delta}$ mutant, these data provide the first evidence thatdifferent requirements must be met for Hir1p to function atthe HTA1 and his4-912 ${delta}$ promoters.

DISCUSSION

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Our previous studies led us to propose that the Hir1 corepressoris targeted to histone gene promoters by its association witha factor that binds at promoter-specific negative regulatoryelements or with another protein that directly contacts thisfactor, and that once at a promoter, it contacts a downstreamtarget to bring about repression (SHERWOOD 1993 ; SPECTOR etal. 1997 ). Hir1p is associated in vivo with a second corepressor,Hir2p, but when Hir1p is artificially recruited to the histoneHTA1 promoter, it can repress transcription in the absence ofHir2p (SPECTOR et al. 1997 ). This result helped support thenotion that the role of Hir2p is to bring Hir1p to relevantpromoters, where it then acts as a direct transcriptional repressor.Hir1p also acts directly or indirectly at other genes besidesthose encoding core histones, notably alleles of HIS4 and LYS2that contain ${delta}$ insertion mutations, although it is not knownhow it is targeted to these loci (SHERWOOD and OSLEY 1991 ).In this study, we performed a functional analysis of Hir1p tounderstand its role in the transcription of the genes it controls.The results showed that the Hir1 protein contains two separaterepression domains. The first domain encompasses seven copiesof the ß-transducin or WD40 repeat at the Hir1p N terminus(amino acids 1–390), and the second includes the remaining448 C-terminal amino acids. In native Hir1p, these domains mostlikely mediate the interactions of Hir1p with different proteinsto bring about its transcriptional effects.

The N-terminal domain is both necessary and sufficient for thefunction of Hir1p at histone gene promoters because overexpressionof the seven WD repeats allowed repression of the histone HTA1gene in a strain lacking Hir1p (Figure 7). Thus, the notionthat the primary function of Hir2p is to recruit Hir1p to thesepromoters is probably not the case because it was the Hir1pC terminus, not the WD repeats, that physically interacted invivo with Hir2p (Figure 2). The WD repeats, therefore, mightinteract directly with a DNA-binding factor at the HTA1 promoter,bringing Hir1p to this promoter without the mediation of Hir2p.It is unlikely that these repeats directly contact downstreamtargets of repression as well, because when they were tetheredat the HTA1 promoter, either Hir1p (Figure 3) or Spt4p/Spt5p/Spt6p(Figure 5, Table 3) had to be present for repression to occur.

The Hir1p C terminus, while unable to correct the Hir^- phenotypeof a hir1 ${Delta}$ mutant, was identified as a separate repression domainbecause it repressed HTA1 transcription when tethered at thepromoter (Figure 1). Unlike the WD repeats, however, the tetheredC terminus repressed transcription independently of both Hir1p(Figure 1) and the three Spt proteins (Table 3). This suggeststhat the Hir1p C terminus might contact downstream repressiontargets directly without the intervention of other proteins.

Based on the assumption that the two repression domains havespecialized roles, we propose the following model for how nativeHir1p inhibits HTA1 transcription: the WD domain is postulatedto contact the factor that binds at the HTA1-negative site,bringing Hir1p to the promoter, while the C-terminal domainis presumed to have direct contact with a downstream target,causing repression. We also suggest that when the WD repeatsare overexpressed in a hir1 ${Delta}$ mutant, truncated Hir1p is stillbrought to the HTA1 promoter, but the interaction of the WDrepeats with Spt4p/Spt5p/Spt6p now allows Hir1p to contact thisdownstream target. Thus, the Hir1p C terminus and Spt4p/Spt5p/Spt6pmight be functionally equivalent. Although this predicts thatoverexpression of the WD repeats would be unable to represstranscription in a strain that is deleted for both HIR1 andSPT4, this cannot be tested directly because a hir1 ${Delta}$ spt4 ${Delta}$ double-mutantis inviable (F. WINSTON, personal communication).

What, then, is the role of Hir2p in the function of Hir1p asa repressor of HTA1 transcription? Based on the results of thisand a previous study (SPECTOR et al. 1997 ), we postulate thatwhile both Hir1p and Hir2p are required for repression at theHTA1 promoter (SHERWOOD et al. 1993 ), and while a fractionof Hir1p and Hir2p are physically associated in vivo (Figure2), Hir1p and Hir2p may in fact function independently. Thisconclusion is based on the observation that Hir2p is dispensablefor repression by tethered full-length Hir1p (SPECTOR et al.1997 ), the tethered Hir1p WD repeats, and the tethered Hir1pC terminus (M. A. OSLEY, unpublished data). Hir1p and the Spt4/Spt5/Spt6proteins, on the other hand, may function together at the HTA1promoter because all three Spt proteins are required for thetethered Hir1p WD repeats to repress transcription. We haveobserved previously, however, that in spt4, spt5, and spt6 mutants,the HTA1 promoter is partially repressed rather than derepressed,as the tethering studies would have predicted (COMPAGNONE-POSTand OSLEY 1996 ). These conflicting data can be reconciled ifthe absence of the Spt proteins frees Hir1p to enter into alternativeprotein interactions to repress HTA1 transcription.

Different requirements must be met for Hir1p to function atthe his4-912 ${delta}$ promoter. Overexpression of the Hir1p WD repeatswas unable to correct the Spt^- phenotype of a hir1 ${Delta}$ strain, indicatingthat the Hir1p C terminus has an essential function in thiseffect. We had previously suggested that the Spt^- phenotypeof hir mutants could be an indirect effect of the unbalancedproduction of histones in these strains, a physiological situationthat results in suppression of the ${delta}$ insertion (CLARK-ADAMS etal. 1988 ; SHERWOOD and OSLEY 1991 ). The results of the presentstudy, however, provide the first evidence that Hir1p acts directlyat both the HTA1 and his4-912 ${delta}$ promoters because the restorationof histone stoichiometry by WD overexpression did not concomitantlyproduce an Spt⁺ phenotype. Despite this conclusion, we stilldo not know whether Hir1p acts independently or with the Spt4/Spt5/Spt6proteins to affect his4-912 ${delta}$ transcription.

The effects of overexpression of the Hir1p C terminus provideadditional support for the notion that this region of Hir1pforms different protein associations from those of the WD repeats.Hence, the dominant Hir^-Spt^- phenotype produced by the overexpressedC terminus could have resulted from the disruption of specificprotein–protein interactions at both the HTA1 and his4-912 ${delta}$ promoters. For example, because the Hir1p C terminus could becoprecipitated with Hir2p in vivo (Figure 2), the overexpressedC terminus might bind to Hir2p and prevent it from interactingwith other proteins required for HTA1 repression, leading toa Hir^- phenotype. The Spt^- phenotype could also have resultedfrom the disruption of protein complexes that act at the his4-912 ${delta}$ promoter. As discussed above, our data suggest that the Hir1pC terminus must be present for Hir1p to function at this promoter.Overexpression of the C terminus, which interacts in vivo withHir1p and Hir2p (Figure 2), might favor Hir1p–Hir1p interactionsand thus prevent the association of Hir1p with Spt4p or otherproteins at the his4-912 ${delta}$ locus.

The observation that the mutant phenotypes produced by overexpressionof the Hir1p C terminus in a wild-type strain were reversedby the addition of a single WD repeat suggests that the interactionsof the WD repeats are dominant to those of the C terminus innative Hir1p. This supports the notion that WD-protein interactionstarget the C-terminal repression domain to appropriate locations.For example, the WD repeats could promote Hir1p interactionswith a DNA-binding factor at the HTA1 promoter, thereby targetingthe Hir1p C terminus to this promoter, where it could now engagein appropriate contacts with downstream targets to inhibit transcription.

The presence of WD repeats in a protein is postulated to providemultiple interfaces for interactions with other proteins, althoughthe broad sprectrum of proteins that contain these repeats suggeststhat the range of targets is also broad (NEER et al. 1994 ).The Tup1p transcriptional corepressor contains WD repeats withsome structural and functional similarity to those of Hir1p(KOMACHI et al. 1994 ; TZAMARIAS and STRUHL 1995 ). A singleTup1p WD repeat contacts the ${alpha}$ 2 repressor at a cell-specificgenes (KOMACHI et al. 1994 ), raising the issue of the specificityof WD associations: If the Hir1p WD repeats also contact a site-specific,DNA-binding protein, how do Hir1p and Tup1p recognize theircorrect DNA-binding targets? Perhaps the structure of the twoWD repeats is sufficiently different, or association with otherproteins, e.g., Ssn6p with Tup1p (WILLIAMS et al. 1991 ), confersan additional level of specificity.

ACKNOWLEDGMENTS

We thank DESSISLAVA DIMOVA and JUDITH RECHT for their criticalreading of the manuscript, MARK TREITEL for construction ofthe lexA-SPT4 fusion gene, ROGER BRENT for the gift of anti-LexAantibodies, and FRED WINSTON and STAN FIELDS for strains orplasmids. This work was supported by National Institutes ofHealth grant GM40118 to M.A.O.

Manuscript received August 5, 1997; Accepted for publication November 17, 1997.

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