Functional Interaction between Ssu72 and the Rpb2 Subunit of RNA Polymerase II in Saccharomyces cerevisiae

doi:10.1128/MCB.20.22.8343-8351.2000

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Molecular and Cellular Biology, November 2000, p. 8343-8351, Vol. 20, No. 22
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Functional Interaction between Ssu72 and the Rpb2 Subunit of RNA Polymerase II in Saccharomyces cerevisiae

Donald L. Pappas Jr. and Michael Hampsey^*

Department of Biochemistry, Division of Nucleic Acids Enzymology, Robert Wood Johnson Medical School, Piscataway, New Jersey 08854

Received 18 July 2000/Returned for modification 9 August 2000/Accepted 15 August 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

SSU72 is an essential gene encoding a phylogenetically conserved protein of unknown function that interacts with the generaltranscription factor TFIIB. A recessive ssu72-1 allele was identifiedas a synthetic enhancer of a TFIIB (sua7-1) defect, resultingin a heat-sensitive (Ts) phenotype and a dramatic downstream shift in transcription startsite selection. Here we describe a new allele, ssu72-2, that confersa Ts phenotype in a SUA7 wild-type background. In an effort to furtherdefine Ssu72, we isolated suppressors of the ssu72-2 mutation.One suppressor is allelic to RPB2, the gene encoding the second-largestsubunit of RNA polymerase II (RNAP II). Sequence analysis of therpb2-100 suppressor defined a cysteine replacement of the phylogeneticallyinvariant arginine residue at position 512 (R512C), located withinhomology block D of Rpb2. The ssu72-2 and rpb2-100 mutations adverselyaffected noninduced gene expression, with no apparent effectson activated transcription in vivo. Although isolated as a suppressorof the ssu72-2 Ts defect, rpb2-100 enhanced the transcriptional defects associatedwith ssu72-2. The Ssu72 protein interacts directly with purifiedRNAP II in a coimmunoprecipitation assay, suggesting that thegenetic interactions between ssu72-2 and rpb2-100 are a consequenceof physical interactions. These results define Ssu72 as a highlyconserved factor that physically and functionally interacts withthe RNAP II core machinery during transcriptioninitiation.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Eukaryotic RNA polymerase II (RNAP II) is a multisubunit enzyme that is responsible for transcription of all protein-encodinggenes. Saccharomyces cerevisiae RNAP II is a 12-subunit complexencoded by the genes RPB1 to RPB12 (reviewed in references 2,53, and 55). The two largest subunits, Rpb1 and Rpb2, arehomologous to the $beta$ ' and $beta$ subunits of bacterial RNA polymerase(RNAP), respectively (23, 49). The yeast counterpart of thebacterial $alpha$ subunit appears to be shared between the Rpb3 andRpb11 subunits (26, 57). Accordingly, Rpb1, Rpb2, Rpb3, andRpb11 comprise the functional equivalent of the bacterial $alpha$ ₂ $beta$ $beta$ 'core RNAP. The functions of the remaining RNAP II subunits areless clear, although five subunits, Rpb5, Rpb6, Rpb8, Rpb10, andRpb12, are shared among all three forms of RNAP and thereforefunction in transcription of all genes. With the exception ofRpb4 and Rpb9, all subunits are essential for cell viability.Rpb4 forms a subcomplex with Rpb7 that is required for promoter-specificinitiation but is dispensable for elongation (13).

RNAP II is unable to initiate promoter-specific transcription on its own. Promoter recognition requires the general transcriptionfactors (GTFs), which include the TATA binding protein (TBP),TFIIB, TFIIE, TFIIF, and TFIIH (reviewed in references 17 and33). TBP nucleates assembly of a transcription preinitiationcomplex by binding the TATA element and inducing a sharp bendin the DNA template. TFIIB binds the TATA-TBP complex and is responsiblefor defining the polarity of transcription by binding asymmetricallyto the BRE element, located immediately upstream of the TATA box(28, 50). RNAP II, in association with TFIIF, binds the TATA-TBP-TFIIBternary complex, followed by TFIIE and TFIIH. TFIIH is a multisubunitcomplex with catalytic activities responsible for phosphorylationof the carboxy-terminal repeat domain of the Rpb1 subunit of RNAPII, promoter melting and promoter clearance (25).

The GTFs were discovered based on their requirement for accurate initiation in vitro (29, 52) and are highly conservedamong eukaryotic organisms (reviewed in references 17, 30,33, and 38). Furthermore, the TBP and TFIIB requirements fortranscription predate the divergence of Eukarya and Archaea (reviewedin reference 5). Nonetheless, the RNAP II requirement for GTFsis not universal but is instead dictated by promoter sequenceand architecture (16, 35, 51). Indeed, genome-wide expressionanalysis revealed that most components of the RNAP II transcriptionalmachinery are dispensable for expression of subsets of genes (21).Conversely, since only a limited number of promoters have beenanalyzed in vitro, it is conceivable that additional GTFs mightbe identified based on their requirement for accurate initiationfrom specific promoters. Other factors might be identified basedon their ability to stimulate activator-independent transcription.For example, the yeast Tsp1 (Sub1) protein was identified as apositive effector of in vitro transcription in the absence ofa sequence-specific activator (20). Tsp1 interacts physicallyand genetically with TFIIB and is homologous to the human transcriptionalcofactor PC4 (20, 27). Additional basal factors are likelyto be identified, either by their requirement for promoter-specificinitiation, by their ability to stimulate activator-independenttranscription, or by genetic interactions with GTFs or RNAP IIsubunits.

The yeast gene encoding TFIIB (SUA7) was identified as an effector of transcriptional accuracy (36). Replacements at eitherof two phylogenetically invariant residues, glutamate-62 (E62)or arginine-78 (R78), caused a marked start site shift downstreamof the normal site at the CYC1 and ADH1 promoters (37). Nearlyidentical effects on transcriptional accuracy are conferred bythe sua8 alleles of RPB1, suggesting a functional interactionbetween TFIIB and Rpb1 during start site selection (6). Inan effort to identify other factors that affect initiation, weisolated suppressors of the sua7-1 (E62K) mutation. The ssu71and ssu73 suppressors encode altered forms of the largest subunitof TFIIF (Tfg1) and the Rpb9 subunit of RNAPII, respectively (46,47). In contrast, ssu72 was identified as an enhancer of theTFIIB E62K defect: the ssu72-1 allele confers a heat-sensitive(Ts) growth defect and a dramatic downstream start site shift, withboth effects being dependent upon the sua7-1 allele (48).

The SSU72 gene is essential for cell viability and encodes a novel protein of undefined function (48). To further characterizeSsu72, we generated a new ssu72 allele that confers a tight Ts phenotype, independent of a TFIIB defect. We have taken advantageof the ssu72 Ts phenotype to isolate a new rpb2 mutation encoding an alteredfrom of the Rpb2 subunit of RNAP II. The results presented heredemonstrate that Ssu72 is a transcription factor that interactswith the core RNAP II machinery both in vivo and invitro.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Yeast strains. The yeast strains used in this study were derived from LRB535 (MATa his3 $Delta$ 200 leu2-3,112 ura3-52). YZS84 is isogenicto LRB535, except for the ssu72-2 allele, which was generatedby site-directed mutagenesis and subsequent allele replacement,as described below. YDP19 (ssu72-2 rpb2-100 shs2-1) is a spontaneousTs⁺ revertant of YZS84; YDP135 (ssu72-2 rpb2-100) is a segregantderived from a cross of YDP19 with YDP87 (ssu72-2 RPB2 SHS2).The plasmid-shuffle strain YZS89A (ssu72::LEU2 [SSU72-URA3]) wasdescribed previously (48).

Growth media, genetic methods, and phenotypes. All growth media were prepared according to standard recipes (43). $-$ Ino medium is synthetic complete medium lacking inositol;+Ino control medium contains 55 µM inositol. Standard yeast geneticmethods were used for making crosses, selecting diploids, inducingsporulation, and dissecting tetrads (44). The following designationsare used for phenotypes: Ts, temperature sensitivity, defined by impaired growth on YPD mediumat 37°C; Cs, cold sensitivity, defined by impaired growth on YPD medium at16°C; and Ino, impaired growth on $-$ Ino medium at 30°C relative to growth on+Ino control medium. Plasmids carrying the URA3 marker were counterselectedon synthetic medium containing 5-fluoro-orotic acid (8).

Construction of the ssu72-2 mutant. The ssu72-2 allele was constructed by site-directed mutagenesis as described previously (48) using synthetic oligonucleotideoZS-200 (5'-GAAGATTTGATGAATGCAGGTGGGAAATTAAAC-3'). The underlinedGC bases of the GCA triplet encode alanine at amino acid position129. The EcoRI-KpnI DNA fragment encompassing the ssu72-2 openreading frame (ORF) was cloned into the corresponding sites ofplasmid pRS314 (45), creating the ssu72-2 TRP1 CEN plasmid pM721.The phenotype of ssu72-2 was initially determined by plasmid shuffleusing host strainYZS89A.

Allele replacement of the normal SSU72 chromosomal locus was made by integration-excision (40). The EcoRI-KpnI fragmentencompassing ssu72-2 was cloned into the corresponding sites ofplasmid pRS306 (45), yielding the ssu72-2-integrating plasmidpM728. pM728 was linearized at the unique ClaI site located withthe SSU72 coding region and introduced into strain LRB535. Ura⁺ transformants were isolated and subsequently counterselectedon 5-fluoro-orotic acid medium. Strains retaining the ssu72-2allele were identified based on the Ts phenotype associated with this allele (see above) and confirmedby the ability of the Ts phenotype to be complemented by plasmid-borne SSU72. Southernblot analysis confirmed integration and excision at the SSU72locus (D. L. Pappas, Jr., unpublishedresults).

Isolation and sequence analysis of the rpb2-100 allele of RPB2. The rpb2-100 allele of RPB2 was recovered by gap repair (40). Plasmid RY2119 (RPB2 URA3 CEN) was digested to completionwith SnaBI, which removes most of the RPB2 ORF. Vector DNA flankedby RPB2 sequences was isolated by agarose gel electrophoresis,purified, and introduced into strain YDP135 (rpb2-100). Ura⁺ colonies were selected and subsequently screened for retentionof the Cs and Ino phenotypes conferred by the rpb2-100 allele of RPB2. PlasmidDNA was recovered, amplified in Escherichia coli, and analyzedby restriction digestion to confirm gap repair by the rpb2-100locus. This resulting plasmid, pDP73, failed to rescue the Cs and Ino phenotypes when introduced into strains YDP19 and YDP135, confirmingrecovery of rpb2-100. To facilitate sequence analysis, the 1.88-kbKpnI-EcoRI, 1.05-kb EcoRI-BglII, and 2.5-kb PstI-SalI rpb2-100fragments from pDP73 were cloned into the KpnI-EcoRI sites ofpRS316, EcoRI-BamHI sites of pRS316, and PstI-SalI sites of pRS424,respectively. Single-stranded DNA was generated using VCS-M13helper phage in the presence of kanamycin as described previously(41). The DNA sequence of the entire RPB2 ORF was determinedusing an ABI Prism automated DNA sequencer. DNA sequence comparisonswere performed using the BLAST algorithm accessed via the SaccharomycesGenome Database (http://genome-www.stanford.edu/Saccharomyces/).

RNA analyses. CYC1 transcript levels were analyzed by S1 nuclease protection. Strains were grown at 30°C in synthetic complete medium containing2% glucose to mid-log phase (optical density at 600 nm [OD₆₀₀]= 0.6). Cells were collected, washed, and used to inoculate two50-ml cultures of synthetic complete medium containing either2% glucose or 3% glycerol plus 2% ethanol as the sole carbon sources.Cultures were incubated at 30°C for 8 h, and cells were harvested.Total RNA was isolated and S1 nuclease protection assays wereperformed as described previously (22), using synthetic oligonucleotides5'-GTGTAGCACCTTTCTTAGCAGAACCGGCCTTGAATTCAGTCGGACGG and 5'-GGAATTTCCAAGATTTAATTGGAGTCGAAAGCTCGCCTTAfor CYC1 and tRNA^W,respectively.

INO1 transcript levels were analyzed by Northern blotting. Cells were grown at 30°C in synthetic complete medium to mid-logphase, collected by centrifugation, washed, and used to inoculatetwo 50-ml cultures of synthetic complete medium either lackingor containing inositol (55 µM). Cultures were incubated at 30°Cfor 8 h, and cells were harvested. Total RNA was extracted andanalyzed as described previously (36). The INO1 probe was generatedby nick translation of a 1.0-kb INO1 EcoRI-HindIII fragment derivedfrom plasmid pJM310 in the presence of [ $alpha$ -³²P]dCTP. The U6 control probe was a nick-translated 450 bp fragmentencompassing the SNR6 gene. CYC1 and INO1 transcript levels werequantified using the National Institutes of Health Image program(http://rsb.info.nih.gov/nih-image/) and normalized to the tRNA^W and U6 RNA loading control signals,respectively.

$beta$ -Galactosidase assays. Strains harboring CYC1-lacZ (pLG265-UP1 [15]), INO1-lacZ (pJS325 [42]), or PGK1-lacZ (pN1086 [7]) reporter plasmidswere grown at 30°C in $-$ Ura medium to mid-log phase (OD₆₀₀ = 0.6).Cells were harvested and resuspended in $-$ Ura medium containingeither (i) 2% glucose or 3% glycerol plus 2% ethanol for CYC1-lacZstrains, (ii) synthetic complete medium either containing or lacking55 µM inositol for INO1-lacZ strains, or (iii) no addition forPGK1-lacZ strains. Cells were incubated for 8 h, harvested bycentrifugation, and resuspended in 500 µl of breaking buffer (100mM Tris-HCl [pH 8], 1 mM dithiothreitol, 20% glycerol; 2 mM phenylmethylsulfonylfluoride). Cell extracts were prepared by vortexing with 0.5-mm-diameterglass beads six times in 15-s bursts. $beta$ -Galactosidase assays weredone as described previously (24). Activities were determinedby duplicate assays of three independent transformants and areexpressed according to the following formula: (1.7 ml × OD₄₂₀units)/(0.0045 × cell extract volume [milliliters] × reactiontime [minutes] × protein concentration [milligrams per milliliter]).

In vitro transcription and translation reactions. Radiolabeled TBP, TFIIB, and Ssu72 were generated using the TNT kit (Promega) in the presence of [³⁵S]methionine according to vendor specifications. Template DNAswere purified using a Mini-Prep kit (Qiagen). Plasmids pT7-IID(9) and pET-SUA7 were used as templates for synthesis of TBPand TFIIB, respectively. SSU72 and ssu72 allelic DNAs were amplifiedby PCR using oligonucleotides 5'-GGAATTCCATATGCCTAGTCATCGC and5'-CGCGGATCCTTAGTGATGGTGATGGTGATGTTTGTAATATGAAGGAGCG. This amplifiesthe SSU72 ORF with sequences coding for a hexahistidine tag atthe C terminus and flanking NdeI and BamHI sites (underlined).The PCR products were digested and ligated into the NdeI and BamHIsites in pCITE-4a(+) (Novagen), generating the ssu72 templatespM1540 (SSU72), pM1541 (ssu72-1), pM1542 (ssu72-2), or pM1543(ssu72-4).

RNAP II immunoprecipitation. Immunoprecipitation assays were performed as described previously (34), with minor modifications. Highly purified yeastRNAP II (425 ng) and in vitro-transcribed and translated inputproteins (10 µl) were incubated in 250 µl of P100 buffer (50 mmTris-acetate [pH 7.9], 10% glycerol, 100 mM potassium acetate,14 mM magnesium acetate, 4 mM dithiothreitol, 1 mM EDTA, 50 µgof bovine serum albumin per ml, and protease inhibitors [0.5 µgof pepstatin A per ml, 0.5 µg of leupeptin per ml, 2 µg of chymostatinper ml, 2.5 µg of antipain per ml, 1 mM phenylmethylsulfonyl fluoride,2 mM benzamidine]) at 4°C for 18 h. Pansorbin (Calbiochem) washarvested by centrifugation and resuspended in blocking buffer(50 mM Tris-acetate [pH 7.9], 100 mM potassium acetate, 25 mgof PVP-40 [Sigma] per ml and 30 mg of bovine serum albumin perml [pH 7.9]). Following incubation for 20 min at room temperature,Pansorbin was centrifuged and resuspended to its original volumein P100 buffer. Twenty-five microliters of preblocked Pansorbinwas added to each reaction mixture. Samples were incubated at4°C for 30 min and centrifuged at 15,000 rpm for 2 min. Supernatantswere transferred to fresh tubes containing 5 µg of anti-RNAP IImonoclonal antibody (8WG16; Covance, Inc.) and incubated for 90min at 4°C. Preblocked Pansorbin (25 µl) was added, and the reactionmixtures were incubated for 60 min at 4°C. The samples were centrifugedat 16,000 × g for 2 min. The pellets were washed three times with250 µl of P100 buffer containing 0.1% NP-40 and once with 250µl of P100 buffer. Pellets were resuspended in 40 µl of samplebuffer, and 20 µl of each was resolved in a sodium dodecyl sulfate-12%polyacrylamide gel. Following electrophoresis, the gel was treatedwith En³Hance (Dupont NEN), dried, and exposed to a phosphor screen. Productswere visualized using a PhosphorImager and ImageQuant software(MolecularDynamics).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

The Ssu72 protein is phylogenetically conserved. Ssu72 was reported to be a novel protein with no apparent homologs in the databases (48). Genome sequencing projects havesince identified homologs of Ssu72 in Schizosaccharomyces pombe,human, Drosophila melanogaster, Arabidopsis thaliana, and Caenorhabditiselegans cells. Indeed, two distinct homologs of Ssu72 have beenfound in human cells. The yeast, human, fly, and plant proteinsare all approximately 200 residues in length and exhibit 46 to54% sequence identity (BLAST values of <e³⁹) to S. cerevisiae Ssu72 (Fig. 1). The C. elegans protein is muchlarger, comprising 1,357 residues, although the region of sequencesimilarity is confined to the N terminus, showing 43% identityto S. cerevisiae Ssu72 (data not shown). No proteins with structuralsimilarity to Ssu72 were found among the bacterial or archaealprotein sequence databases, suggesting that Ssu72 function iscommon to eukaryotes but is not conserved in either eubacteriaor archaea.

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FIG. 1. Sequence similarities among eukaryotic Ssu72 proteins. The Ssu72 proteins from S. cerevisiae (SC), S. pombe (SP), human (HS1 and HS2), fruit fly (DM), and A. thaliana (AT) were identified using the BLAST algorithm (1) and aligned using the University of Wisconsin Genetics Computer Group programs PILEUP and BOXSHADE. Identical and similar amino acid residues are highlighted in black and gray, respectively. The overbar encompassing residues 122 to 150 of S. cerevisiae Ssu72 indicates the region of sequence similarity to ATP-dependent RNA helicases noted previously (48). The asterisks indicate residues within this region that are phylogenetically invariant among the helicases. The ssu72-2 allele encodes an alanine replacement of the invariant arginine at position 129 (R129A).

Construction of the ssu72-2 mutant. The original ssu72 allele (ssu72-1) enhances the sua7-1 defect by conferring a Ts growth defect and by dramatically shifting transcription initiationdownstream of the normal site at the ADH1 gene (48). These arepronounced effects but are dependent upon the sua7-1 mutation.Indeed, the ssu72-1 mutation confers no apparent phenotype ina SUA7 wild-typebackground.

As part of our efforts to characterize SSU72, we sought an ssu72 mutant that exhibits phenotypes independent of sua7-1. TheSsu72 amino acid sequence includes a region, encompassing residues122 to 150, that is highly conserved among ATP-dependent RNA helicases(Fig. 1). Although other sequences common to this class of helicases,including the DEAD box and HRIGRXXR motif, are not found in Ssu72,all of the invariant residues within the conserved region arepresent in Ssu72 (Fig. 1). Since SSU72 is essential for cell viability,we reasoned that replacement of a conserved amino acid withinthis region might confer a growth phenotype. Accordingly, we constructedan allele, ssu72-2, that encodes an alanine replacement of theinvariant arginine at position 129 (R129A). Using a plasmid-shuffleassay, we found that the ssu72-2 mutant was viable but failedto grow at 37°C. The plasmid-borne ssu72-2 allele was then usedto replace the chromosomal copy of SSU72, yielding strain YZS84.Consistent with the phenotypes associated with the plasmid-bornessu72-2 mutation, YZS84 was viable but distinctly Ts (Fig. 2).

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FIG. 2. Growth defects associated with ssu72, rpb2-100, and shs2 mutations. Relevant genotypes are indicated for the wild-type strain LRB535 (SSU72 SHS1 SHS2), primary mutant YZS84 (ssu72-2 RPB2 SHS2), revertant YDP19 (ssu72-2 rpb2-100 shs2-1), a YDP19 derivative carrying a plasmid-borne copy of RPB2 (ssu72-2 RPB2 shs2-1), and the YDP135 segregant (ssu72-2 rpb2-100 SHS2). The complete genotypes of these strains and the growth media are defined in Materials and Methods.

Genetic suppression of ssu72-2. To identify factors that interact with Ssu72, we isolated suppressors of the ssu72-2 Ts defect. Forty spontaneous Ts⁺ revertants of strain YZS84 were isolated at 37°C. When scoredfor pleiotropic phenotypes, four revertants failed to grow inthe absence of inositol yet grew normally on synthetic completemedium. This phenotype is denoted Ino and is often associated with defects in components of the generaltranscriptional machinery (18). Two of the Ino revertants were also cold sensitive (Cs), growing poorly on YPD medium at 16°C. One of these strains,YDP19, exhibited distinct Ts⁺ Cs Ino phenotypes (Fig. 2) and was chosen for furthercharacterization.

Strain YDP19 (Ts⁺ Cs Ino) was backcrossed with strain YDP87 (Ts Cs⁺ Ino⁺), and the resulting diploid strain was phenotypically Ts Cs⁺ and Ino⁺, indicating that all YDP19 phenotypes are the result of a recessivemutation(s). When this strain was sporulated and dissected (11four-spore tetrads), the Ts⁺:Ts phenotypes segregated 0:4, 1:3, or 2:2, whereas the Cs⁺:Cs and Ino⁺:Ino phenotypes segregated 2:2. Furthermore, all Ts⁺ segregants were Cs and Ino. These data indicate that suppression of the ssu72-2 Ts phenotype is the result of mutations in two unlinked genes andthat mutation in one of these genes confers the Cs and Ino phenotypes. We tentatively designated these two suppressor genesshs1-1 (rpb2-100 [see below]) and shs2-1. The shs1-1 allele isresponsible for the Cs and Ino phenotypes, whereas shs2-1 confers no pronounced phenotype inthe absence of shs1-1.

Identification of the shs1-1 suppressor. We exploited the Cs and Ino phenotypes of shs1-1 to clone the wild-type gene from a YCp50 genomic library (39). From approximately90,000 Ura⁺ transformants of YDP135 (ssu72-2 shs1-1), 25 Cs⁺ strains were isolated, 4 of which were restored to Ino⁺. Plasmid DNAs were isolated from each of these four transformantsand were found to include overlapping DNA inserts within the YCp50vector. One plasmid, pDP99, was reintroduced into YDP135, andall of the scored transformants were Cs⁺ and Ino⁺, indicating that complementation of the Cs and Ino phenotypes was a consequence of plasmid DNA rather than strainreversion.

Restriction analysis of plasmid pDP99 defined an insert of approximately 8.0 kb in the YCp50 vector. Partial DNA sequenceanalysis identified a segment of the yeast genome from chromosomeXV encompassing RPB2, the gene encoding the second-largest subunitof RNAP II. To further define the relationship between shs1-1and RPB2, plasmid RY2119, which includes the entire RPB2 codingregion but neither of the flanking ORFs of the original clone,was introduced into YDP135. The resulting transformants were phenotypicallyTs, Cs⁺, and Ino⁺, confirming that RPB2, rather than a flanking gene, complementsthe suppressor mutation. To confirm that the suppressor is allelicto RPB2, the URA3 gene was integrated by homologous recombinationadjacent to the RPB2 locus of strain YDP87. The resulting strain(ssu72-2 ura3 RPB2-URA3) was crossed with YDP19 (ssu72-2 ura3shs1-1 shs2-1), and a diploid strain was sporulated and dissected.A total of 44 segregants were obtained and scored. All Ura⁺ progeny were phenotypically Cs⁺ and Ino⁺, and all Ura progeny were Cs and Ino. Thus, the suppressor segregates opposite to RPB2, thereby confirmingthat shs1-1 is allelic to RPB2. Accordingly, we have renamed theshs1-1 suppressor rbp2-100.

The rpb2-100 mutation. The rpb2-100 allele was cloned by gap repair, and the entire ORF was sequenced using a collection of primers that span theRPB2 ORF. A single-base-pair substitution at position 1534 (C1534T)was identified, encoding replacement of arginine-512 by cysteine(R512C). The Rpb2 subunit of RNAP II is structurally conservedamong eukaryotic, archaeal, and bacterial RNAPs, including eukaryoticRNAPs I, II, and III. Sequence comparisons identified nine blocks,designated A to I, which are highly conserved among all RNAPs(49). R512 is the first amino acid within homology block D andis phylogenetically invariant (Fig. 3). The results presentedhere indicate that R512, despite its phylogenetic invariance,is not essential for cell viability. Indeed an rpb2-100 allelein an otherwise normal (SSU72⁺) genetic background displays only weak growth impairment at 30°Cbut is severely Cs and Ino (data not shown).

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FIG. 3. The rpb2-100 mutation. The rpb2-100 allele of RPB2 encodes an R512C replacement at a phylogenetically invariant position within homology block D of Rpb2. The alignment of homology block D (30 residues) is shown for S. cerevisiae (Sc), S. pombe (Sp), A. thaliana (At), Plasmodium falciparum (Pf), C. elegans (Ce), Homo sapiens (Hs), Drosophila melanogaster (Dm), Pyrococcus horikoshii (Ph), the second-largest subunits (Rpa135 and Rpc128) of RNAP I and RNAP III of S. cerevisiae [Sc (I) and Sc (III), respectively], and the $beta$ subunits of E. coli (Ec) and T. aquaticus (Ta) RNAPs. Amino acids are indicated by the single-residue code; the numbers at the right indicate the position of the C-terminal residue of block D.

The ssu72-2 and rpb2-100 alleles affect noninduced transcription in vivo. The effects of ssu72-2 and rpb2-100 mutations on transcription from specific promoters were determined in vivo using the wild-typestrain (LRB535), an ssu72-2 primary mutant (YZS84), an ssu72-2rpb2-100 shs2-1 suppressor strain (YDP19), and an ssu72-2 rpb2-100segregant (YDP135). Effects on CYC1 expression are presented inFig. 4A. Under repressing conditions (2% glucose), the CYC1 transcriptlevel was reduced in the ssu72-2 mutant to 42% of normal (comparelanes 1 and 3). Expression was further diminished in the ssu72-2rpb2-100 shs2-1 revertant to 17% of normal (lane 5), an effectthat could be attributed to rpb2-100 rather than shs2-1, sincethe same level of expression was observed in the ssu72-2 rpb2-100mutant (lane 7). These effects occur at the level of noninducedtranscription, since all strains retained the ability to respondto derepressing conditions.

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FIG. 4. Effects of ssu72 and shs mutations on CYC1 expression. (A) The top panel indicates CYC1 transcript levels, determined by S1 nuclease protection, for strains grown under repressing (2% glucose) (lanes R) and derepressing (3% glycerol and 2% ethanol) (lanes D) conditions. Strains are LRB535 (wild type [WT]), YZS84 (ssu72-2), YPD19 (ssu72-2 rpb2-100 shs2-1), and YDP135 (ssu72-2 rpb2-100). Transcript levels under repressing conditions are presented as percentages, normalized to the level for the wild-type strain. The bottom panel is a loading control and indicates tRNA^W levels. (B) $beta$ -Galactosidase activities expressed from the CYC1-lacZ plasmid pLG265-UP1. Activity units under repressing and derepressing conditions, respectively, are 1,300 ± 66 and 4,900 ± 1030 (WT), 140 ± 13 and 310 ± 40 (YZS84), 4.8 ± 1.2 and 19 ± 3.5 (YDP19), and 3.3 ± 0.54 and 97 ± 14 (YDP135). The indicated units of $beta$ -galactosidase activity represent the means for three independent transformants assayed in duplicate; standard deviations are indicated by error bars.

The effects on CYC1 transcription were confirmed using a CYC1-lacZ reporter. In the wild-type strain 1,300 U of activity wasmeasured under repressing conditions, and this activity was enhanced3.5-fold under derepressing conditions (Fig. 4B). Noninduced expressionwas diminished 9-fold in the ssu72-2 primary mutant (140 U) andwas reduced an additional 30-fold in the ssu72-2 rpb2-100 shs2-1suppressor strain (4.8 U). The shs2-1 allele did not contributeto this effect, since activity was equally low in an ssu72-2 rpb2-100strain (3.3 U). Each mutant responded to derepressing conditions,although the absolute activities were diminished in parallel witheffects on basal activity. These results are consistent with theRNA analyses (Fig. 4A), confirming that ssu72-2 and rpb2-100 diminishnoninduced transcription from the CYC1promoter.

INO1 expression was determined by Northern blot analysis (Fig. 5A). Strong induction of INO1 mRNA was observed in the wild-typestrain (compare lanes 1 and 2). Induced levels were diminishedto approximately 70% of normal in the ssu72-2 mutant (lane 4)and were further reduced to 43% of normal in the ssu72-2 rpb2-100shs2-1 suppressor strain (lane 6). Interestingly, rpb2-100 hada more dramatic effect in the absence of shs2-1, nearly eliminatingINO1 expression (lane 8). These results are consistent with theeffects of ssu72-2 and rpb2-100 on INO1-lacZ reporter gene expressionunder repressing conditions (Fig. 5B). Although the Northern analysisdoes not distinguish between effects on noninduced versus activatedexpression, the measurable levels of $beta$ -galactosidase activityfrom the INO1-lacZ reporter under repressing conditions demonstratethat the effects of ssu72-2 and rpb2-100 on INO1 expression canbe accounted for by effects on noninduced transcription.

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FIG. 5. Effects of ssu72 and shs mutations on INO1 expression. (A) The top panel indicates INO1 transcript levels, determined by Northern blot analysis, for strains grown under repressing (+Ino medium) (lanes R) and derepressing ( $-$ Ino medium) (lanes D) conditions. Strains are identical to those in Fig. 4. The bottom panel is a loading control showing U6 RNA levels. (B) $beta$ -Galactosidase activities expressed from the INO1-lacZ plasmid pJS325 under repressing conditions. Activity units are 310 ± 39 (wild type [WT]), 210 ± 36 (YZS84), 86 ± 12 (YDP19), and 17 ± 4.1 (YDP135). Error bars indicate standard deviations. (C) Same as panel B, except the host strain in each case is YDP135 (ssu72-2 rpb2-100) carrying the INO1-lacZ reporter and plasmid-borne copies of wild-type SSU72, RPB2, or vectors alone, as indicated by the genotypes. Activity units are 56 ± 2.8 (WT), 47 ± 4.7 (ssu72-2), 1.9 ± 0.07 (rpb2-100), and 5.3 ± 0.63 (ssu72-2 rpb2-100).

The INO1-lacZ reporter assays were repeated using strain YDP135 that had been complemented with plasmid-borne copies of SSU72and/or RPB2, allowing the effects of ssu72-2 and rpb2-100 to beassessed in an isogenic background independent of shs2-1. Consistentwith the previous results, ssu72-2 alone had only a minor effecton INO1-lacZ expression, whereas the effects of the rpb2-100 singleand ssu72-2 rpb2-100 double mutations were more dramatic, yieldingless than 10% of normal activity (Fig. 5C). Thus, ssu72-2 exertsadverse effects on gene expression that are markedly enhancedby the rpb2-100 allele, and these effects are manifest at thelevel of noninducedtranscription.

The effects of ssu72-2 and rpb2-100 were also assessed using the PGK1 promoter, which is expressed at a high constitutivelevel. A PGK1-lacZ reporter plasmid was introduced into each strain,and $beta$ -galactosidase activities were measured (Fig. 6). Expressionfrom the PGK1 promoter was diminished to 60% of normal in thessu72-2 mutant and to 40% of normal in the ssu72-2 rpb2-100 shs2-1triple mutant. Expression was markedly diminished in the ssu72-2rpb2-100 double mutant, to 3% of normal. Although these experimentsdo not distinguish noninduced from activated expression, the dramaticeffect of the double mutant indicates that ssu72-2 and rpb2-100can exert synergistic effects on gene expression. The more adverseeffect of rpb2-100 in the SHS2⁺ background is consistent with its effect on INO1 expression (Fig.5). These results demonstrate that shs2-1, which is required inaddition to rpb2-100 for suppression of the ssu72-2 Ts phenotype (Fig. 2), also suppresses the adverse effects of rpb2-100on noninduced transcription.

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FIG. 6. $beta$ -Galactosidase activities expressed from a PGK1-lacZ plasmid. Strains are identical to those in Fig. 4 and in Fig. 5A and B, except that each was transformed with the PGK1-lacZ reporter plasmid pN1086. Activity units are 2,500 ± 88 (wild type [WT]), 1,500 ± 160 (YZS84), 1,000 ± 52 (YDP19), and 86 ± 3.6 (YDP135).

Physical interaction between Ssu72 and RNAP II. The genetic interactions among ssu72, sua7, and rpb2 suggest that Ssu72 interacts directly with the core transcriptional machinery.Indeed, Ssu72 directly binds TFIIB, consistent with allele-specificinteractions between ssu72 and sua7 (54). Physical interactionbetween Ssu72 and RNAP II was investigated by a coimmunoprecipitationassay using purified yeast RNAP II and a monoclonal antibody directedagainst the Rpb1 subunit of RNAP II. Input proteins were ³⁵S-labeled Ssu72, with labeled TBP and TFIIB as controls. RNAPII is known to bind TFIIB, but not TBP, whose interaction withRNAP II requires TFIIB as a bridging factor. The Ssu72 input includedtwo forms of the protein, corresponding to full-length Ssu72 andN-terminally truncated Ssu72 resulting from initiation at AUGcodon 23. The results demonstrate that RNAP II binds stably toTFIIB and Ssu72 but not to the TBP control (Fig. 7A). Thus, thegenetic interaction between ssu72-2 and rpb2-100 is likely toreflect a physical interaction between Ssu72 and RNAP II.

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FIG. 7. Physical interaction between Ssu72 and RNAP II. (A) Equal amounts of highly purified yeast RNAP II were incubated with ³⁵S-labeled mock, TBP, TFIIB, and Ssu72 input proteins. Samples were immunoprecipitated (IP) using a monoclonal antibody directed against the C-terminal repeat domain of Rpb1. Following centrifugation, samples were washed three times with buffer containing 100 mM potassium acetate plus 0.1% NP-40 and once with buffer containing 100 mM potassium acetate and then resuspended in sample buffer. Input proteins (5% of the total; lanes 1, 3, 5, and 7, respectively) and the precipitates (50% of the total; lanes 2, 4, 6, and 8, respectively) were fractionated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and analyzed by autoradiography. WT, wild type. (B) Same as panel A, except that different forms of Ssu72 were used as input proteins. The ssu72-1 allele encodes a duplication of amino acid residues 9 to 18, ssu72-2 encodes the R129A replacement, and ssu72-4 encodes an inviable C15S replacement. The upper and lower bands of Ssu72 input proteins correspond, respectively, to the full-length protein and a truncated protein whose N terminus corresponds to methionine at position 23. In the case of Ssu72-1, RNAP II interacts with both the full-length and truncated forms of the protein. Control reactions lacking RNAP II failed to coimmunoprecipitate Ssu72 (data not shown).

The N terminus of Ssu72 is essential for Ssu72 function and cell viability, yet RNAP II binds the smaller form of Ssu72, lackingthe N-terminal 22 residues. This was further investigated by askingwhether specific mutations in the Ssu72 N terminus affect RNAPII binding. The ssu72-1 allele, which enhances the sua7-1 mutation,encodes a 10-amino-acid duplication in the N terminus of Ssu72(residues 9 to 18), and ssu72-4 encodes a serine replacement ofcysteine 15 that abolishes cell viability (48). The interactionbetween Ssu72 and RNAP II appeared to be unaffected by the ssu72-2(R129A) and ssu72-4 (C15S) mutations (Fig. 7B, lanes 5 to 8).Interestingly, however, the 10-amino-acid duplication resultedin preferential binding of RNAP II to the longer form of Ssu72(Fig. 7B, lanes 1 to 4). These results confirm that Ssu72 bindsdirectly to RNAP II and imply that the Ssu72 N terminus affectsthisinteraction.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The results in this paper define genetic and physical interactions between Ssu72 and RNAP II and support a role for Ssu72in basal (noninduced) transcription by RNAP II. Ssu72 was initiallyidentified based on a genetic interaction with TFIIB. The ssu72-1allele confers a synthetic Ts growth defect that is dependent upon the sua7-1 mutation (48).The interaction of ssu72-1 with sua7 is specific, resulting insynthetic phenotypes only in combination with sua7 alleles thataffect transcription start site selection (54). Ssu72 is alsogenetically linked to Sub1 (Tsp1), a homolog of the human generaltranscriptional cofactor PC4, in that a sub1 deletion also enhancessua7 mutations and does so in an allele-specific manner that isidentical to the specificity of the ssu72-1 sua7 interactions(54). Consistent with the genetic data, TFIIB directly interactswith the Ssu72 and Sub1 proteins (27, 54). Here we demonstratethat Ssu72 binds stably to RNAP II and that the ssu72-2 and rpb2-100alleles affect basal transcription. Taken together, these datademonstrate functional interactions of Ssu72 with TFIIB, Sub1,and Rpb2 and provide strong support for Ssu72 as an RNAP II transcriptionfactor.

We do not know the specific function of Ssu72. Our efforts to characterize Ssu72 have been hampered because sequence tagsadded to the N terminus appear to expose a cryptic proteolyticsite just within the Ssu72 N terminus, thereby removing the tag,whereas sequences added to the C terminus render Ssu72 nonfunctionalin vivo, perhaps due to the conserved, tandem aromatic residuesat the C terminus (Fig. 1). Interestingly, there are no apparentSsu72 homologs in bacterial or archaeal genomes, implying thatSsu72 function is specific to eukaryotes. In yeast, depletionof Ssu72 causes growth arrest and diminishes total poly(A) RNAlevels by about 20 to 40% but is without effect on RNAP I andRNAP III transcription (Pappas, unpublished results). These resultssuggest that Ssu72 is critical for transcription of many, butnot all, RNAP II genes yet plays no role in RNAP I or RNAP IIItranscription.

All evidence points to a role for Ssu72 in core promoter function. The original ssu72-1 allele, which encodes a 10-amino-acidduplication near the N terminus, affects transcription start siteselection (48). This effect is dramatic, but it is dependentupon a sua7 allele (TFIIB) that also affects initiation. Herewe demonstrate that the ssu72-2 allele adversely affects noninducedtranscription. The rpb2-100 suppressor of ssu72-2 also diminishesnoninduced transcription, and this effect can be synergistic withssu72-2. The magnitude of the ssu72-2 effect on transcriptionappears to be promoter specific: whereas CYC1 transcription isdiminished nearly 10-fold, less than 2-fold effects are observedfor INO1 and PGK1 expression. The promoter elements responsiblefor these effects are unknown but can readily be addressed bywhole-genome microarray analysis using wild-type and ssu72-2strains.

It is noteworthy that rpb2-100 was isolated as a suppressor of the ssu72-2 Ts growth defect, yet rpb2-100 and ssu72-2 exert similar effectson transcription. This anomaly can be explained by the resultsfrom genetic analysis of the YDP19 revertant, revealing that mutationsin two genes, rpb2-100 and shs2-1, are required for suppressionof the ssu72-2 Ts phenotype. Indeed, the effect of either allele in the absenceof the other is to enhance the ssu72-2 phenotype, essentiallyeliminating growth at 37°C (Fig. 2). This result not only accountsfor the similar effects of ssu72-2 and rpb2-100 on transcriptionbut also is consistent with their synergistic effects on transcriptionfrom the PGK1 promoter (Fig. 6). Although isolated as a suppressor,the rpb2-100 allele is an enhancer of ssu72-2 in the absence ofshs2-1.

The rpb2-100 allele encodes a single amino acid replacement, R512C, located at the first position within homology block Dof Rpb2 (Fig. 3). The viability of the R512C mutant indicatesthat R512, despite its phylogenetic invariance, is not functionallyinvariant. Not only does the rpb2-100 allele (in combination withshs2-1) suppress the ssu72-2 Ts phenotype, but the ssu72-2 rpb2-100 shs2-1 strain (YDP19) exhibitsonly marginally impaired growth on rich (YPD) medium at 30°C.The viability of rpb2-100 mutants cannot be attributed to a suppressiveeffect of ssu72-2 on rpb2-100, because an rpb2-100 mutant is alsoviable in an SSU72⁺ background, with a growth rate comparable to that of YDP19 (Pappas,unpublished results). Furthermore, the rpb2-100 SSU72⁺ strain exhibits the same severe Cs and Ino phenotypes as YDP19, thereby confirming that these phenotypesare due to the R512Creplacement.

Other rpb2 alleles have been isolated in genetic selections for mutations that affect core promoter function (3, 4,14, 19). The spt alleles of RPB2 were identified as suppressorsof $delta$ -element insertions at the HIS4 and LYS2 promoters (19).These alleles encode amino acid replacements in the region betweenhomology blocks B and C of Rpb2 and underscore a role for theRpb2 subunit in core promoter recognition. The sit1 and sit2 allelesof RPB1 and RPB2, respectively, were isolated as enhancers ofHIS4 transcription in the absence of the trans activators Gcn4,Bas1, and Bas2 (4). These mutations are comparable to rpb2-100in that they also affect noninduced transcription, albeit withopposite effects. Furthermore, the sit1 and sit2 mutants, likethe rpb2-100 mutant, are inositol auxotrophs. The sit1 allelesencode Rpb1 amino acid replacements in either region D or regionF, both of which are within or near the active center of RNAP(3). In the Thermus aquaticus RNAP structure, the sit1 regionF replacements are adjacent to R428, the counterpart of R512 inRpb2. The opposite effects of the sit1 and rpb2-100 mutationson transcription might be accounted for by their proximity tothe secondary channel, where the distinction between the stimulatoryor inhibitory effects might be accounted for by structural changesthat affect substrate access to the active site and, consequently,the efficiency of promoterclearance.

A crystal structure of yeast RNAP II was recently solved at a resolution of 3 Å (10). Unfortunately, R512 is located withinan approximately 13-residue gap that precludes interpretationof the R512C replacement in the context of the RNAP II three-dimensionalstructure. However, a crystallographic structure of RNAP fromE. coli has been determined at a 12-Å resolution (11, 12),and, more recently, that of RNAP from T. aquaticus has been determinedat a 3.3-Å resolution (56). R512 is highly conserved, correspondingto R548 and R428 of the $beta$ subunits of RNAPs from E. coli and T.aquaticus, respectively (Fig. 3). The sequence conservation amongall forms of RNAP and the nearly superimposable structures ofE. coli and T. aquaticus RNAPs (32) allow for the R512C replacementto be interpreted in the context of the T. aquaticus crystal structure.Moreover, a comprehensive description of site-specific interactionsbetween catalytically competent RNAP and promoter open DNA wasrecently defined by protein-DNA photo-cross-linking (31). Accordingly,R428 forms part of the binding site for double-stranded DNA downstreamof position +1 and is positioned to make direct contact with thephosphate 5' to position +6 of the nontemplate strand. The positionof this residue suggests possible roles for R428 in stabilizingRNAP-DNA interaction, in facilitating clamping of RNAP on duplexDNA, in facilitating RNAP translocation, and/or in defining thedownstream boundary of the transcription bubble. Furthermore,the catabolite gene activator protein has no effect on cross-linkingbetween RNAP and the core promoter region (31). These resultsreadily account for the effects of rpb2-100 on noninduced transcriptionand underscore our premise that Ssu72 is a core RNAP II transcriptionfactor.

	ACKNOWLEDGMENTS

We are especially grateful to Zu-Wen Sun for constructing the ssu72-2 mutant and to Sung-Joon Kim and Danny Reinberg for theirgenerous gift of purified yeast RNAP II. We are also gratefulto Richard Ebright, Danny Reinberg and David Gross for valuablediscussions and comments on the manuscript and to Steve Buratowski,Bryan Cullen, Leonard Guarente, Lucy Robinson, Hans-Joachim Schüller,and Nancy Woychik for strains andplasmids.

This work was supported by NIH grantGM39484.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biochemistry, Robert Wood Johnson Medical School, 675 Hoes Lane, Piscataway,NJ 08854. Phone: (732) 235-5888. Fax: (732) 235-5889. E-mail:hampsemi{at}umdnj.edu.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
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Meinhart, A., Silberzahn, T., Cramer, P. (2003). The mRNA Transcription/Processing Factor Ssu72 Is a Potential Tyrosine Phosphatase. J. Biol. Chem. 278: 15917-15921 [Abstract] [Full Text]
He, X., Khan, A. U., Cheng, H., Pappas, D. L. Jr., Hampsey, M., Moore, C. L. (2003). Functional interactions between the transcription and mRNA 3' end processing machineries mediated by Ssu72 and Sub1. Genes Dev. 17: 1030-1042 [Abstract] [Full Text]
Chen, B.-S., Sun, Z.-W., Hampsey, M. (2001). A Gal4-sigma 54 Hybrid Protein That Functions as a Potent Activator of RNA Polymerase II Transcription in Yeast. J. Biol. Chem. 276: 23881-23887 [Abstract] [Full Text]

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