An Activator Binding Module of Yeast RNA Polymerase II Holoenzyme

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Lee, Y. C.
	Articles by Kim, Y.-J.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Lee, Y. C.
	Articles by Kim, Y.-J.

Previous Article | Next Article

Molecular and Cellular Biology, April 1999, p. 2967-2976, Vol. 19, No. 4
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

An Activator Binding Module of Yeast RNA Polymerase II Holoenzyme

Young Chul Lee, Jin Mo Park, Soyoung Min, Sang Jun Han, and Young-Joon Kim^*

Center for Molecular Medicine, Samsung Biomedical Research Institute, Sungkyunkwan University College of Medicine, Kangnam-ku, Seoul 135-230, Korea

Received 4 September 1998/Returned for modification 27 October 1998/Accepted 11 January 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The Mediator complex of Saccharomyces cerevisiae is required for both general and regulated transcription of RNA polymeraseII (PolII) and is composed of two stable subcomplexes (Srb4 andRgr1 subcomplexes). To decipher the function of each Mediatorsubcomplex and to delineate the functional relationship betweenthe subcomplexes, we characterized the compositions and biochemicalactivities of PolII-Mediator complexes (holoenzymes) preparedfrom several Mediator mutant strains of S. cerevisiae. We foundthat holoenzymes devoid of a functional Gal11 module were defectivefor activated but not basal transcription in a reconstituted invitro system. This activation-specific defect was correlated witha crippled physical interaction to transcriptional activator proteins,which could be bypassed by artificial recruitment of a mutantholoenzyme to a promoter. Consistent with this observation, adirect interaction between Gal11 and gene-specific transcriptionalactivator proteins was detected by far-Western analyses and columnbinding assays. In contrast, the srb5 deletion mutant holoenzymewas defective for both basal and activated transcription, despiteits capacity for activator binding that is comparable to thatof the wild-type holoenzyme. These results demonstrate that theGal11 module of the Rgr1 subcomplex is required for the efficientrecruitment of PolII holoenzyme to a promoter via activator-specificinteractions, while the Srb4 subcomplex functions in the modulationof general polymeraseactivity.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The activator-squelching assay, in which the addition of excess amounts of one activator interferes with transcriptional stimulationby another activator, suggests the existence of a common targetfor the two activators (20). The fact that a crude yeast fractiondevoid of all the basal transcription factors could relieve thesquelching effect demonstrated that a distinct intermediary moleculeis involved in the mediation of signal transfer between transcriptionalactivator proteins and basal transcription machinery (7, 20).Monitoring of this intermediary activity throughout the biochemicalfractionation of a yeast whole-cell extract led to the purificationof a multiprotein complex called Mediator (21). The Mediatorcomplex is tightly associated with RNA polymerase II (PolII) andenables PolII to respond to transcriptional activators in an invitro system reconstituted with pure general transcription factors.In addition, Mediator stimulates basal transcription, as wellas transcription factor IIH (TFIIH)-dependent, in vitro phosphorylationof the carboxy-terminal domain (CTD) of the largest subunit ofPolII, Rpb1 (21).

An independent genetic approach for identifying CTD-interacting proteins led to the discovery of the SRB gene family (31)and the identification of a PolII complex that contains all ofthe SRB gene products (16, 27, 40). Srb- and Mediator-containingPolII complexes contain Srb proteins (Srb2, Srb4, Srb5, Srb6,and Srb7) as well as the products of previously described transcriptionalregulatory genes (GAL11, SIN4, RGR1, ROX3, and HRS1/PGD1/MED3)(13, 21, 26, 30). In addition, several novel subunits(Med1, Med2, Med4, Med6, Med7, Med8, Med9, Med10, and Med11) wereidentified as components of both PolII complexes (12, 15,25, 30). However, some components differ between the two PolIIcomplexes; specifically, certain Srb proteins (Srb8, Srb9, Srb10,and Srb11) and the Swi-Snf complex are absent from the Mediator-PolIIcomplex (holoenzyme) (25, 30, 46).

Genetic studies revealed that some of the genes that encode Mediator subunits are required for the transcriptional regulationof specific genes, whereas others are necessary for general transcriptionin vivo (reviewed in reference 3). Differential dissociationof the Mediator components by high-urea treatment revealed thatfunctionally related Mediator subunits physically associate toform stable Srb4 and Rgr1 subcomplexes (24). The Gal11 moduleproteins (Gal11, Sin4, and Hrs1) are found in the Rgr1 subcomplextogether with several Med proteins (Med1, Med4, Med7, Med9, andMed10) and Srb7. We showed recently that newly identified Medproteins (Med9 and Med10) are required for the regulation of agroup of genes that are different from those regulated by theGal11 module (15). These results strongly suggest that otherMediator proteins in the Rgr1 subcomplex may also be involvedin the transcriptional regulation of distinct subsets ofgenes.

While the Rgr1 subcomplex is composed of Mediator subunits required for the transcriptional regulation of distinct subsetsof genes, the Srb4 subcomplex is composed of Mediator subunitsrequired for general transcription events (Srb2, Srb4, Srb5, Srb6,and Med6). The Srb4 subcomplex was successfully reconstitutedwith recombinant proteins in vitro (22), and the functionalinteractions between the components of this subcomplex were decipheredgenetically by determining the suppressor relationships amongSRB4, SRB6, and MED6 (23, 24). The general requirement forSrb4 in PolII transcription suggests that Srb4 and its associatedproteins function in the modulation of the basic activity of PolII,rather than in the reception of gene-specific activator signals.However, weak binding affinity between Srb4 and gene-specifictranscriptional activators was detected in an in vitro biochemicalassay (22).

Although Srb4 was suggested as an activator binding target on the basis of genetic and physical interactions (22), the generalrequirement of Srb4 for the expression of most PolII-transcribedgenes makes it difficult to explain how activator specificityis achieved. Therefore, in order to identify the activator bindingtargets of Mediator and to elucidate the mechanism by which Mediatorinteracts with specific transcriptional activator proteins, wesought to determine the distinct functions of the two Mediatorsubcomplexes, the Rgr1 and Srb4 subcomplexes. As a means of identifyingthe specific function of each Mediator module, we purified andanalyzed Mediator-PolII complexes (holoenzymes) from yeast strainsthat contained a mutation in one of the Mediator components. Ourdata reveal that activated transcription via the Gal11 moduleoccurs through a specific interaction of the Gal11 module witha gene-specific transcriptional activator in vitro. On the basisof these observations, we propose a transcriptional activationmechanism that involves (i) the recruitment of a holoenzyme byan activator through an interaction with a distinct Mediator moduleand (ii) the modulation of PolII activity by the Srb-containingMediator subcomplex upon activator-Mediatorinteraction.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Protein purification. The Mediator-PolII complex (holoenzyme) was purified from Saccharomyces cerevisiae wild-type cells (YCL10; MAT $alpha$ ade2 ura3lys2 trp1 his3 leu2 med6 $Delta$ ::LEU2 [MED6 on pRS313, HIS3]), rgr1 $Delta$ 2mutant cells (DY2010; MATa rgr1- $Delta$ 2::TRP1 can1 leu2 trp1ura3), srb5 $Delta$ mutant cells (CTY153; MATa ura3 his3 leu2lys2 srb5 $Delta$ ::URA3 hisG), gal11 $Delta$ mutant cells (HS301; MATa ura3trp1 leu2 prb1 pep4 prc1 gal2 gal11 $Delta$ ::LEU2), and hrs1 $Delta$ mutantcells (SSAB-2CF; MAT $alpha$ ade2 ura3 his3 leu2 hrs1 $Delta$ ::LEU2). The culturedcells were harvested, washed with cold water, and dissolved in0.5 ml of 3× lysis buffer (21) per g of wet cells. All subsequentsteps were carried out at 4°C. After freezing-thawing, the cellswere disrupted by 20 cycles of bead beating (one cycle: a 30-sburst followed by 90 s of chilling at 4°C) in a stainless steelchamber with an equal volume of 0.5-mm-diameter glass beads, andcell debris was removed from the lysate by centrifugation at 12,000× g for 20 min. To the supernatant, 0.1 volume of 4 M potassiumacetate (pH 7.6) and 0.01 volume of 10% (wt/vol) polyethyleneimine(pH 8.0) were added slowly, and the mixture was stirred gentlyfor 30 min. The resulting lysate was clarified by centrifugationin a Beckman Ti45 rotor at 42,000 rpm for 90 min and then subjectedto four consecutive chromatographic steps that included BioRex70 (Bio-Rad), DEAE-Sepharose FF (Pharmacia), Biogel-HTP hydroxyapatite(Bio-Rad), and MonoQ HR 5/5 (Pharmacia) as described previously(21). Holoenzyme activity was monitored with a specific transcriptionassay and immunoblot analysis. MonoQ column fractions that containedpeak holoenzyme activity (1 M potassium acetate eluate) were pooledand used in the in vitro transcription and CTD phosphorylationassays. The amount of each type of holoenzyme used in the assayswas normalized on the basis of its nonspecific transcription activityas described previously (21). Recombinant Gal4VP16, glutathioneS-transferase (GST)-VP16, GCN4, and GST-Gal11 were isolated frombacterial expression strains described previously (5, 28,32, 36).

In order to tag the Gal4VP16 fusion protein with a site for phosphorylation, an adapter DNA molecule coding for a phosphorylationmotif sequence (Arg-Arg-Ala-Ser-Val) was prepared by annealingoligonucleotides AdapC (5'-CTAGTCGTCGTGCATCTGTTGGATCCCA-3') andAdapD (5'-TATGGGATCCAACAGATGCACGACGA-3'); the 28-bp adapter DNAfragment was flanked by SpeI and NdeI sites. This adapter DNAfragment and the NdeI-BamHI fragment of the Gal4VP16 gene obtainedfrom pET-Gal4VP16 were cloned together into the SpeI-BamHI sitesof pEHB1 (N-terminal six-histidine fusion system constructed bythe modification of pET-3a) to create pEh-KGVP. The recombinantGal4VP16 doubly tagged with a hexahistidine stretch and a phosphorylationmotif at its N terminus was purified from Escherichia coli BL21(DE3)carrying pEh-KGVP as described previously (5).

In vitro transcription and CTD phosphorylation. The reconstituted in vitro transcription assay was performed as described elsewhere (21). In order to examine the CTD phosphorylationevent during transcription initiation complex formation, transcriptionbuffer (25) supplemented with cold ATP (8 µM) and [ $gamma$ -³²P]ATP (3 µCi) was added to the DNA template JJ470, TFIIH, andother protein components. The mixture was incubated for 10 or40 min at 25°C. In order to examine CTD phosphorylation duringthe transcription reaction, CTP and UTP (0.8 mM each) were alsoadded to the above reaction mixture, which was incubated for 10min at 25°C. Except for the ribonucleotides, all the other componentswere as in the reconstituted transcription assay. Reactions werestopped by the addition of 4× sodium dodecyl sulfate (SDS) gelloading buffer (8 µl; 200 mM Tris-Cl [pH 6.8], 400 mM dithiothreitol,8% SDS, 40% glycerol, 0.4% bromophenol blue), and half of thereaction products were analyzed on an SDS-7.5% polyacrylamidegel. RNA transcripts and ³²P-labeled Rpb1 were quantitated with the use of a PhosphorImager(MolecularDynamics).

Immunoprecipitation and immunoblotting. Crude anti-Rgr1 antiserum (200 µl) (24) was conjugated with protein G-agarose beads (200 µl) (GIBCO BRL) as described previously(26), and each aliquot of antibody-beads (20 µl) was incubatedfor 6 to 12 h at 4°C with the holoenzyme fraction (MonoQ column).The beads were washed three times with IP buffer-100 (400 µl;20 mM Tris-HCl [pH 7.8], 0.1 mM EDTA, 0.2 mM Nonidet P-40, 1 mMdithiothreitol, 10% [vol/vol] glycerol, 100 mM potassium acetate),and the bound proteins were eluted twice with 100 mM glycine (pH2.5) (25 µl). The eluates were treated with 10% trichloroacetate,and the precipitated proteins were resolved on an SDS-polyacrylamidegel and analyzed by silver staining orimmunoblotting.

Immunoblot analysis was performed with monoclonal antibody 8WG16 (for Rpb1), rabbit antiserum directed against the Gal4 DNAbinding region (for Gal4VP16; Santa Cruz Biotechnology), and antiseradirected against various Mediator components. Anti-Sin4 antiserumwas generated in rats with a recombinant six-histidine-taggedSin4 protein fragment (N-terminal 430 amino acids) as anantigen.

SRP. Surface plasmon resonance (SPR) measurements for the detection of protein-protein interactions were taken with a BIAcore Biosensor(Biosensor). All measurements were taken at 25°C in running bufferHBP-150 (40 mM HEPES-KOH [pH 7.6], 7.5 mM MgCl₂, 150 mM potassiumacetate, 0.005% Surfactant P-20) at a flow rate of 5 µl/min. Purifiedproteins were immobilized on Sensor Chip CM-5 with the use ofan amine coupling kit (Biosensor) in accordance with the manufacturer'sinstructions at a flow rate of 5 µl/min. Gal4VP16 (100 ng/µl,50 µl) and GST-VP16 (50 ng/µl, 70 µl) were each coupled in 100mM sodium formate (pH 3.0). GCN4 protein (100 ng/µl, 50 µl) wascoupled in 100 mM sodium formate (pH 4.0), and TATA binding protein(TBP) (100 ng/µl, 50 µl) was immobilized in running buffer. Analyteproteins were diluted in running buffer to the appropriate concentrationsand were dialyzed against running buffer for 3 h. All injectedproteins were centrifuged for 5 min just prior to injection. Afterinjection, bound proteins were removed by injection of 30 µl of100 mM glycine (pH 3.0 or 4.0). The data were analyzed with theuse of BIAevaluation software (version 2.1;Biosensor).

Far-Western analysis and GST column binding assay. For far-Western blotting, ~2 µg of either wild-type or gal11 $Delta$ mutant holoenzyme (immunopurified from the active MonoQ fractionby use of anti-Rgr1 antibody-beads) was electrophoresed throughan SDS-10% polyacrylamide gel and transferred to a nitrocellulosemembrane. The proteins bound to the filter were denatured andrenatured as described previously (43) and were incubated for8 h at 4°C in binding buffer (5 ml) (17) containing ³²P-labeled Gal4VP16 protein (5 × 10³ to 1 × 10⁴ cpm/ng; total, 200 ng). The blot was washed three times withbinding buffer and twice with phosphate-buffered saline containing0.2% Triton X-100 and was subjected to autoradiography. Phosphorylationof Gal4VP16 was performed with 1 U of the catalytic subunit ofbovine heart kinase (Sigma) per µl and 1 µCi of [ $gamma$ -³²P]ATP per µl in 50 µl of HMK buffer as described previously (19).

For the GST column binding assay, purified recombinant GST-Gal11 protein or GST protein was bound to glutathione-agarose beads(Sigma) at a concentration of 1 µg of protein per 5 µl of beads.In vitro-translated (³⁵S-labeled) Gal4VP16, Gal4VP16^456FP442 (2), or GCN4 (32) (10 µl from each in vitro translationreaction) was incubated overnight at 4°C with 25 µl of GST- orGST-Gal11-conjugated agarose beads in IP buffer-100. After binding,the beads were washed three times with binding buffer (250 µl)and boiled in SDS sample buffer, and the bound proteins were analyzedby SDS-12.5% polyacrylamide gel electrophoresis (PAGE) andautoradiography.

Artificial recruitment assay. To generate a gal11 $Delta$ ::TRP1 strain (designated JMP1), the GAL11 targeting plasmid pRS304-GAL11KO was constructed by insertinga GAL11 gene fragment into the SpeI and EcoRI sites of pRS304.The GAL11 gene fragment was generated by PCR (the two oligonucleotidesused in the PCR were gal11-3spe [5'-TAACTAGTTGGAATAATTGGACAAGTGCTACTTGAACATTTGAAGTTAAC-3']and gal11-5ri [5'-TGGAATTCAGGAGCAGCAGACATAGCAGATTTAAAAGAAATAGCGTTAAC-3'])and digestion with SpeI and EcoRI. pRS304-GAL11KO was linearizedby digestion with HincII and transformed into S. cerevisiae YCL4(MAT $alpha$ ade2 ura3 lys2 trp1 his3 leu2 med6 $Delta$ ::LEU2 [MED6 on pRS316,URA3]). The URA3-based MED6 plasmid (pRS316-MED6) in YCL4 andJMP1 was replaced with pRS313-MED6 (strains YCL10 and JMP2) andpRS313-LexA-MED6 (strains JMP3 and JMP4), respectively, by theplasmid shuffling method as described previously (25).

To construct strains JMP5, JMP6, and JMP7, wild-type cells (YPH499; MATa ade2 ura3 lys2 trp1 his3 leu2 GAL⁺), gal11 $Delta$ mutant cells (HS16; MAT $alpha$ ade2 his3 ura3 trp1 leu2 can1gal11 $Delta$ ::LEU2), and srb5 $Delta$ mutant cells (CTY153) were transformedwith pRS313-LexA-MED6, respectively. The srb5 null strain CTY153was transformed with pRS313-MED6 to make JMP8. In order to constructpRS313-LexA-MED6, the 1.6-kb ScaI-EcoRI fragment from pEG202 (14)and the 1.3-kb EcoRI-NaeI fragment from pGBT-MED6 were insertedsequentially between the EcoRV-EcoRI and EcoRI-SmaI sites inpRS313.

An episomal lacZ reporter plasmid (pLGSD5 [11] for control experiments, pSH18-34T [6] for strains JMP2 to JMP6, or pSH18-34TLeufor strains JMP7 and JMP8) with an appropriate selective markerwas also introduced into the resulting strains. In order to constructpSH18-34TLeu, the SmaI fragment containing the lacZ gene was insertedinto the SmaI site of pRS425. Transformant cells were grown inselective synthetic complete medium containing 2% glucose untilthe mid-log phase. At an optical density at 600 nm of 1.0, thecells were harvested by centrifugation, resuspended in yeast extract-peptonemedium containing 2% glucose, and further shaken for 3 h. $beta$ -Galactosidaseactivity was measured from permeabilized cells as described previously(10).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Subunit compositions of mutant holoenzymes. In order to identify a distinct function for each Mediator subunit, we purified holoenzymes from wild-type and mutant yeaststrains carrying either an Rgr1 C-terminal truncation (rgr1 $Delta$ 2),a gal11 deletion (gal11 $Delta$ ), or an srb5 deletion (srb5 $Delta$ ). Despitethe expected differences in subunit composition, the chromatographicproperties of the mutant holoenzymes were identical to those ofthe wild-type holoenzyme. In order to determine more preciselythe composition of each variation of holoenzyme, the holoenzymefractions (MonoQ) were immunoprecipitated with anti-Rgr1 antibodies.Silver staining and immunoblot analyses of the immunoprecipitatedholoenzymes revealed mutant-specific deficiencies in Mediatorsubunits. For example, the rgr1 $Delta$ 2 holoenzyme was deficient inthe Sin4, Gal11, and Hrs1 polypeptides (Fig. 1A and B, lanes R)and had substoichiometric amounts of Med7 to Med11, while theimmunopurified gal11 $Delta$ holoenzyme (lanes G) was completely deficientin Gal11 and devoid of most of Hrs1 but retained all of the otherMediator components in stoichiometric amounts (lanes W). Althougha reduced amount of Sin4 was associated with the immunoprecipitatedgal11 $Delta$ holoenzyme, immunoblot analysis of the gal11 $Delta$ holoenzymefraction (MonoQ) revealed that a wild-type amount of Sin4 copurifiedwith other Mediator components (Fig. 1B, lane G). This resultindicates that Sin4 does associate with the gal11 $Delta$ holoenzymein vivo but that their interaction is weakened when Gal11 andHrs1 are absent; this weakening may cause a partial dissociationof Sin4 during immunoprecipitation.

View larger version (103K):
[in this window]
[in a new window]

FIG. 1. Subunit compositions of mutant holoenzymes. (A) Immunoprecipitation analysis. Holoenzymes (MonoQ fractions) were prepared from wild-type (YCL10; W), rgr1 $Delta$ 2 (DY2010; R), gal11 $Delta$ (HS301; G), hrs1 $Delta$ (SSAB-2CF; H), and srb5 $Delta$ (CTY153; S) strains and immunoprecipitated with anti-Rgr1 antibody-beads as described in Materials and Methods. Proteins were resolved on an SDS-10% polyacrylamide gel and visualized by silver staining. The positions of core polymerase subunits (Rpb) and Mediator components are indicated at the left and right, respectively. (B) Immunoblot analysis. Wild-type (W) and mutant (R, rgr1 $Delta$ 2; S, srb5 $Delta$ ; G, gal11 $Delta$ ; H, hrs1 $Delta$ ) holoenzymes (MonoQ fractions) were subjected to immunoblot analysis with antisera specific for the PolII and Mediator components indicated between the panels.

Although HRS1 was isolated originally as an extragenic suppressor of the hyperdeletion phenotype of hpr1 $Delta$ cells (37), ithas been reported that hrs1 $Delta$ mutant strains have transcriptionaldefects similar to those of gal11 and sin4 null mutant strains(33). Therefore, the loss of Hrs1 from the gal11 $Delta$ holoenzymeprompted us to examine whether the hrs1 $Delta$ holoenzyme has similardefects. To this end, we purified the hrs1 $Delta$ holoenzyme and examinedits subunit composition (Fig. 1A and B, lanes H). Interestingly,Gal11 is the only other Mediator component deficient in the hrs1 $Delta$ holoenzyme besides Hrs1 (Fig. 1B, lanes G and H) (immunoblot analysisalso revealed that Sin4 was associated with the hrs1 $Delta$ holoenzymein vivo). These results strongly suggest that the similar mutantphenotypes exhibited by rgr1 $Delta$ 2, sin4 $Delta$ , gal11 $Delta$ , and hrs1 $Delta$ mutantstrains resulted mainly from the common loss of Gal11 and Hrs1in thesestrains.

The subunit composition of the srb5 $Delta$ holoenzyme was quite different from that of the rgr1 $Delta$ 2 holoenzyme (Fig. 1A and B, lanesS). The srb5 $Delta$ holoenzyme was completely devoid of Srb2 and Srb5but retained all of the other Mediator subunits, although certainsubunits were present in substoichiometric amounts (Hrs1, Med7to Med9, and Med11). In addition, the loss of the Srb2 and Srb5proteins from the holoenzyme appeared to have a secondary effecton the overall integrity of the holoenzyme. The absolute amountof each Mediator subunit was one-fifth the wild-type level, asjudged from immunoblot analyses of both purified holoenzymes (MonoQfraction; Fig. 1B) and crude chromatographic fractions (BioRex70and DEAE-Sepharose fractions; data not shown). Therefore, thephenotype of the srb5 $Delta$ mutant strain may result from the combinedeffects of the loss of Srb2- and Srb5-specific functions, as wellas the reduced amount of the holoenzymeitself.

Transcriptional activities of mutant holoenzymes in vitro. In order to determine which of the compositional defects of the mutant holoenzymes are directly responsible for each of thetranscriptional defects, we examined the transcriptional activitiesof the mutant holoenzymes by using a reconstituted in vitro system.When equivalent amounts of each holoenzyme (based on nonspecifictranscription activity) were used to assess basal transcription,the rgr1 $Delta$ 2 holoenzyme displayed basal transcription activity comparableto that of the wild-type holoenzyme (Fig. 2A, lanes 1 and 2).The gal11 $Delta$ and hrs1 $Delta$ holoenzymes also displayed basal transcriptionlevels similar to those of the wild-type holoenzymes (Fig. 2B,lanes 1, 4, and 7). However, the srb5 $Delta$ holoenzyme consistentlyshowed basal transcription activity three- to fourfold weakerthan those of the other enzymes (Fig. 2A, lane 3). These resultsindicate that Srb5 and Srb2 are required for basal transcription,whereas the Gal11 module proteins are dispensable for basal transcriptionin vitro.

View larger version (45K):
[in this window]
[in a new window]

FIG. 2. In vitro transcription of mutant holoenzymes. Wild-type and mutant holoenzymes (700 ng each) containing the same levels of nonspecific transcriptional elongation activities were analyzed for their promoter-specific transcriptional activities in the presence of the indicated activators in an in vitro transcription system reconstituted with pure general transcription factors and other supplements as described previously (21). RNA transcripts from templates containing either the Gal4 binding site (GAL4:G) or the GCN4 binding site (GCN4:G) are indicated. (A) Transcriptional defects of rgr1 $Delta$ 2 and srb5 $Delta$ holoenzymes. The specifically initiated transcripts from reactions that contained wild-type (W), rgr1 $Delta$ 2 (R), and srb5 $Delta$ (S) holoenzymes in the absence (none) or presence of activator protein (Gal4VP16 or GCN4; 30 ng each) are shown. (B) Transcriptional defects of gal11 $Delta$ and hrs1 $Delta$ holoenzymes. The specifically initiated transcripts from reactions that contained wild-type, gal11 $Delta$ , and hrs1 $Delta$ holoenzymes in the absence ( $-$ ) or presence of activator protein (Gal4VP16 [V] or GCN4 [N]; 30 ng each) are shown.

When the transcriptional activator protein Gal4VP16 was added to basal transcription reaction mixtures containing the wild-typeholoenzyme under permissive conditions, transcription from theactivator-specific template was increased more than 20-fold (Fig.2A, lane 4, and 2B, lane 2). However, all of the other mutantholoenzymes that we tested were completely defective for transcriptionalactivation by Gal4VP16, even under permissive conditions (Fig.2A, lanes 5 and 6, and 2B, lanes 5 and 8) (1.1- to 2-fold activation).Even when five times more srb5 $Delta$ holoenzyme fraction was used tomake the amounts of other Mediator proteins in that fraction equivalentto those in the other holoenzyme fractions, the srb5 $Delta$ holoenzymewas not able to mediate transcriptional activation (data not shown).Only when recombinant Srb2 and Srb5 proteins were added to thetranscription reaction mixture was the srb5 mutant holoenzymeable to respond to the activator (data not shown). These resultsshow that Rgr1, Sin4, Gal11, and Hrs1 are required mainly foractivated transcription, while Srb5 and Srb2 are required forboth activated transcription and basal transcription invitro.

Transcriptional activation by GCN4 was affected similarly in that the rgr1 $Delta$ 2 and srb5 $Delta$ holoenzymes were nearly incapable ofresponding to the activator (Fig. 2A, lanes 8 and 9) (one- andtwofold activation, respectively). However, the gal11 $Delta$ and hrs1 $Delta$ holoenzymes retained some level of activation by GCN4 comparedto the rgr1 $Delta$ 2 and srb5 $Delta$ holoenzymes (Fig. 2B, lanes 5 to 9) (three-and fivefold activation for the gal11 $Delta$ and hrs1 $Delta$ holoenzymes,respectively). Whether this small but activator-specific differencein transcriptional activation between the mutant holoenzymes reflectsan activator-specific requirement for certain Mediator subunitsis currently under investigation (seeDiscussion).

CTD phosphorylation of mutant holoenzymes. The unphosphorylated form of PolII is recruited to the transcriptional preinitiation complex (PIC) and then phosphorylatedat the CTD by TFIIH during the transition from transcriptionalinitiation to elongation (reviewed in reference 35). TFIIH-dependentCTD phosphorylation of both the core polymerase and the holoenzymewas stimulated by conditions that promote PIC formation (Fig.3A, lanes 1 to 4). However, due to the presence of Mediator activity,phosphorylation of the holoenzyme was more than 15-fold higherthan that of the core polymerase under each of the conditionstested (Fig. 3A, lanes 1 to 4). Furthermore, the addition of Gal4VP16increased the efficiency of phosphorylation of the holoenzymethreefold but had no effect on the phosphorylation of the corepolymerase (Fig. 3A, lanes 4 and 5). The various conditions thatprevent activated transcription (such as the omission of a generaltranscription factor or DNA template) all yielded a complete lossof activator-dependent stimulation of CTD phosphorylation (datanot shown).

View larger version (42K):
[in this window]
[in a new window]

FIG. 3. TFIIH-dependent CTD phosphorylation of mutant holoenzymes. (A) Core polymerase (core-polII, 0.3 µg) and holoenzyme (Holo-polII, 0.9 µg) were incubated with [ $gamma$ -³²P]ATP and without ( $-$ ) or with (+) the indicated supplements (Gal4VP16 [Gal4VP, 30 ng], TBP [50 ng], TFIIB [50 ng], TFIIE [60 ng], TFIIH [60 ng], TFIIF [F, 20 ng], and DNA [pJJ470, 200 ng]) in transcription buffer for 10 min (holoenzyme) or 40 min (core polymerase) at 25°C. Phosphorylated Rpb1 was analyzed by SDS-PAGE (7.5% gel) and visualized by autoradiography. (B) CTD phosphorylation of mutant holoenzymes during Gal4VP16-mediated transcriptional activation. The degrees of CTD phosphorylation of the indicated holoenzymes (900 ng) under various transcription reaction conditions are shown. CTD phosphorylation by TFIIH (60 ng) only in the presence of the DNA template (pJJ470, 200 ng; lane H) and under basal (lane B) or activated (Gal4VP16 mediated, lane A) transcription conditions is shown. (C) CTD phosphorylation of mutant holoenzymes during GCN4-mediated transcriptional activation. CTD of wild-type (W), rgr1 $Delta$ 2 (R), srb5 $Delta$ (S), gal11 $Delta$ (G), and hrs1 $Delta$ (H) holoenzymes was phosphorylated by TFIIH under basal or activated (GCN4-mediated) transcription conditions.

In order to investigate whether the mutant holoenzymes were defective in any aspect of CTD phosphorylation, we examined theirphosphorylation efficiencies under conditions that support basaland activated transcription. Under basal transcription conditions,the levels of CTD phosphorylation displayed by the rgr1 $Delta$ , gal11 $Delta$ ,and hrs1 $Delta$ holoenzymes were equal to that of the wild-type holoenzyme;however, the srb5 $Delta$ holoenzyme consistently exhibited only one-thirdthe level of CTD phosphorylation exhibited by the wild-type holoenzyme(Fig. 3B, lane B, and 3C, lane S). Under conditions that supportactivated transcription, all of the mutant holoenzymes lost theirability to respond to Gal4VP16, in that no activator-dependentstimulation of CTD phosphorylation was observed (Fig. 3B, laneA). These results reveal a positive correlation between the rateof in vitro transcription and the level of TFIIH-dependent CTDphosphorylation and confirm the specific requirements for eachMediator subunit in transcriptional activation that were suggestedby the in vitro transcription assays (Fig. 2).

We also tested whether this simple correlation between transcriptional activation and CTD phosphorylation efficiency holdstrue for GCN4-mediated reactions. The mutant holoenzymes werealso defective for the stimulation of CTD phosphorylation in responseto GCN4 (Fig. 3C). Although we detected a small increase in theCTD phosphorylation efficiencies of the gal11 $Delta$ and hrs1 $Delta$ holoenzymes(Fig. 3C, lanes G and H) (1.3- to 1.5-fold stimulation) in responseto GCN4-mediated transcriptional activation (Fig. 2B) (3- to 5-foldactivation), the effect was not significant. Therefore, for unknownreasons there appears to be no simple correlation between activationand CTD phosphorylation under the conditions that weused.

Direct interactions between transcriptional activators and holoenzymes. Although the VP16 activation domain has been shown to interact physically with a number of general transcription factors (18,34, 39, 47), this type of interaction (that is, in the absenceof the Mediator complex) does not elicit an activator responsein a reconstituted in vitro transcription system. In order toexplore the possibility of an activator-Mediator interaction andits relevance in transcriptional activation, we examined the activatorbinding strengths of wild-type and mutant holoenzymes by usinga conventional immunoprecipitation analysis (Fig. 4C). The wild-typeholoenzyme was coimmunoprecipitated with a stoichiometric amountof Gal4VP16 (Fig. 4C, lane W), while the amount of the activatorthat was coimmunoprecipitated with the rgr1 $Delta$ 2 holoenzyme was lessthan 15% that immunoprecipitated with the wild-type holoenzyme(lane R). This result showed that the activator binds to at leastone of the Mediator subunits associated with the C-terminal regionof Rgr1. In order to quantitate the activator binding strengthsof wild-type and mutant holoenzymes in equilibrium, we used theSPR assay (performed with a BIAcore instrument; see Materialsand Methods). When a saturating amount of the wild-type holoenzymewas passed over a surface-immobilized Gal4VP16 chip (applicationwas followed by extensive washing), the refractory index was increasedmore than 5,500 $Delta$ RU (change in the refractory index units), indicatinga very strong interaction between the activator and the holoenzyme(Fig. 4A). This interaction was specific for a functional activationdomain, as the holoenzyme bound efficiently to the VP16 activationdomain alone (GST-VP16) but not to a mutated, nonfunctional activationdomain (GST-VP16^456FP442) (Fig. 4B and data not shown). The holoenzyme also bound efficientlyto GCN4 (4,000 $Delta$ RU), indicating the activator-holoenzyme interactionto be a general phenomenon (Fig. 4B).

View larger version (40K):
[in this window]
[in a new window]

FIG. 4. Interactions of transcriptional activators with wild-type and mutant holoenzymes. (A, B, and D) Plotted is the change in the refractory index units (RU) versus time after injection of the indicated holoenzymes onto an activator-immobilized Biosensor chip. (A) SPR analysis of the interactions between Gal4VP16 and wild-type and rgr1 $Delta$ 2 holoenzymes (70 µl of a MonoQ fraction at a concentration of 200 µg/ml). (B) SPR analysis of the interactions between wild-type (W) and hrs1 $Delta$ (H) holoenzymes (50 µl of a MonoQ fraction at a concentration of 250 µg/ml) and GST-VP16 or GCN4. (C) Coimmunoprecipitation (I.P.) of Gal4VP16 with wild-type (W) and mutant (R, rgr1 $Delta$ 2) holoenzymes followed by Western blotting. Each holoenzyme (MonoQ fraction, 10 µg) was mixed with Gal4VP16 (300 ng) and immunoprecipitated with anti-Rgr1 antibody-beads (see Materials and Methods). In order to measure the amounts of precipitated Gal4VP16 and holoenzymes, we included equimolar amounts of recombinant Gal4VP16 and Med6 proteins (r-P; Med6, 80 ng; Gal4VP16, 60 ng) as quantitative standards. Immunoblot analyses with antisera specific for the proteins indicated to the right of the panel are shown. (D) SPR analysis of the interactions between wild-type (W, 150 µg/ml) and srb5 $Delta$ (S, 450 µg/ml) holoenzymes and an activator (GST-VP16). Due to the low specific concentration of the srb5 $Delta$ holoenzyme in the MonoQ fraction (one-fifth the wild-type level), a threefold-larger amount of srb5 $Delta$ MonoQ fraction was injected to supply an amount of the srb5 $Delta$ holoenzyme comparable to that of the wild-type enzyme.

In contrast to the strong interaction between the activator and the wild-type holoenzyme, the rgr1 $Delta$ 2 holoenzyme caused onlya minor increase in the refractory index under identical conditions( $Delta$ RU, 880; corresponding to ~15% of the $Delta$ RU observed with thewild-type holoenzyme), indicating that the mutant holoenzyme boundpoorly to Gal4VP16. The gal11 $Delta$ and hrs1 $Delta$ holoenzymes were alsodefective in activator interaction, according to the SPR analysis(Fig. 4B and data not shown). The fact that these three mutantholoenzymes all lacked Gal11 and Hrs1 suggests that Gal11 andHrs1 are required for activator binding and may serve as the majorbinding targets for transcriptionalactivators.

In order to test whether the transcriptional defect of the srb5 $Delta$ holoenzyme resulted from a defect in activator binding, wemeasured the interaction between the activator (Gal4VP16) andthe srb5 $Delta$ holoenzyme by using SPR analysis. As shown in Fig. 4D,the srb5 $Delta$ holoenzyme displayed activator binding activity comparableto that of the wild-type holoenzyme. This result implies thatthe crippled transcriptional activation observed with the srb5 $Delta$ holoenzyme did not result from a defective activator interaction.Rather, this result and the CTD phosphorylation data (Fig. 3B)suggest that Srb2 and Srb5 function at a later step to modulatePolII activity through an interaction with theCTD.

Identification of Gal11 as a target for activator binding. In order to determine which Mediator subunit(s) interacts directly with the activator, we probed an immunoaffinity-purifiedholoenzyme with radioactive Gal4VP16 by using far-Western analysis(see Materials and Methods). Two polypeptides with an apparentmolecular size equivalent to that of Gal11 interacted stronglywith the Gal4VP16 probe (Fig. 5A, lane W). These polypeptidescross-reacted with an anti-Gal11 antibody and were absent in thegal11 $Delta$ holoenzyme (Fig. 5A, lane G). These results demonstratethat two polypeptides are encoded by GAL11 (the faster-migratingband might be a breakdown product of Gal11) and that Gal11 aloneis sufficient for activator binding. In order to examine whetherthis interaction requires a functional activator, we analyzedthe interactions between GST-Gal11 and ³⁵S-labeled Gal4VP16 mutant derivatives (Fig. 5B). A substantialamount of wild-type Gal4VP16 (10% of the amount in the loadedcolumn fraction) bound specifically to the GST-Gal11 column butnot to the GST column. However, nonfunctional mutant Gal4VP16^456FP442 did not bind at all to the GST-Gal11 column. These results clearlyshow a specific and direct interaction between Gal11 and a functionalVP16 activation domain. Furthermore, we obtained similar resultswhen GCN4 was used as the activator in the GST-Gal11 column bindingassay. Therefore, Gal11 appears to constitute a general bindingsite for acidic transcriptional activation domains.

View larger version (27K):
[in this window]
[in a new window]

FIG. 5. Direct interaction of Gal11 with acidic activators. (A) Far-Western analysis of holoenzymes with Gal4VP16. Wild-type (W) and gal11 $Delta$ (G) holoenzymes (immunopurified from a MonoQ fraction with an anti-Rgr1 antibody column, ~2 µg each) were resolved on an SDS-10% polyacrylamide gel and transferred to a nitrocellulose membrane. The proteins were renatured and allowed to bind to ³²P-labeled Gal4VP16 as described in Materials and Methods. The position of the Gal11 protein was revealed by Western analysis of the same blot with the use of anti-Gal11 antiserum ( $alpha$ Gal11). (B) Column binding assay for interactions between Gal11 and acidic activators. Agarose beads conjugated with purified GST or GST-Gal11 (5 µg each) were incubated overnight at 4°C with 10 µl of in vitro-translated, ³⁵S-labeled Gal4VP16, Gal4VP16^456FP442, or GCN4. After extensive washing, the beads were boiled in SDS sample buffer, and the proteins were resolved by SDS-12.5% PAGE and subjected to autoradiography. Load represents 10% of the amount of in vitro-translated products loaded on the beads.

Artificial recruitment of the gal11 mutant holoenzyme. The fact that the Rgr1 subcomplex, in particular, the Gal11 module interacts directly with acidic transcriptional activatorssuggests that the Gal11 module functions in the recruitment ofthe holoenzyme to the promoter via a specific interaction withactivator proteins. Therefore, it is conceivable that transcriptionaldefects in gal11 mutant cells would originate mainly from theinefficient recruitment of PolII to the promoter. In order totest this hypothesis, we examined whether artificial recruitmentof the gal11 mutant holoenzyme to the promoter could bypass therequirement for the Gal11 module in transcriptionalactivation.

Transformation of a LexA-Med6 fusion construct on a CEN-ARS plasmid into a wild-type strain as an extragenic copy caused 300-foldtranscriptional activation of the reporter gene containing LexAbinding sites at the promoter. The addition of the LexA-Med6 fusionconstruct to the gal11 null strain also induced more than 90-foldtranscriptional activation of the reporter gene (Table 1). Interestingly,the substitution of wild-type Med6 with a LexA-Med6 fusion proteinin the above strains clearly demonstrated that the artificialrecruitment of the holoenzyme could bypass the requirement forthe Gal11 module in transcriptional activation. The artificialrecruitment of the holoenzyme via LexA-Med6 to the LexA bindingsites of the reporter gene caused almost 2,000-fold transcriptionalactivation in both the wild-type and the gal11 null mutant strains(Table 1). When similar experiments were performed with the srb5null mutant strain, artificial recruitment of the srb5 holoenzymevia LexA-Med6 to LexA binding sites did not rescue the transcriptionaldefect of the srb5 $Delta$ holoenzyme (Table 1). These results suggestthat Gal11 functions mainly in the holoenzyme recruitment stepand may be dispensable for subsequent steps in the transcriptionprocess once the holoenzyme is brought to a promoter through specificinteractions with an enhancer-bound activator. In contrast, Srb5appears to be required for the postrecruitment steps of transcriptionalactivation.

View this table:
[in this window]
[in a new window]

TABLE 1. Artificial recruitment of the RNA PolII holoenzyme restores the transcriptional defects in a gal11 null strain but not in an srb5 null strain

Activator-mediated interactions between holoenzymes and TBP. The physical interaction between the activator and Gal11, which can be functionally replaced by the artificial recruitmentof the mutant holoenzyme to the promoter, suggests that transcriptionalactivators facilitate PIC formation chiefly by recruiting a holoenzymeto the promoter. TBP binding to the TATA promoter element is alsoa rate-limiting step of PIC formation, and it has been suggestedthat transcriptional activators promote TBP binding by interactingwith basal transcriptional factors. Therefore, the concurrentrecruitment of the holoenzyme and TBP to a promoter should greatlyenhance transcriptional efficiency. In order to test whether anactivator could bind to Mediator and TBP simultaneously, the interactionsbetween TBP, Mediator, and a transcriptional activator were examined.When the holoenzyme was passed over a TBP-immobilized Biosensorchip for SPR analysis, we did not observe any specific interactions(data not shown), whereas Gal4VP16 bound efficiently to immobilizedTBP (Fig. 6). However, when the holoenzyme was injected afterthe activator was allowed to bind to immobilized TBP, a significantincrease in the refractory index was observed (Fig. 6). Threeindependent experiments performed with various concentrationsof protein gave rise to similar results (data not shown). Theseresults suggest that there is no direct physical interaction betweenTBP and the holoenzyme; however, the two could associate witheach other indirectly through their simultaneous interactionswith a transcriptional activator.

View larger version (12K):
[in this window]
[in a new window]

FIG. 6. Simultaneous interactions of an activator with a holoenzyme and TBP. The $Delta$ RU during the time course of the SPR analysis with a TBP-immobilized Biosensor chip is shown. Gal4VP16 (30 µg/ml, 30 µl) and wild-type holoenzyme (Holo-polII; 300 µg/ml, 50 µl) were injected sequentially after washing of the chip with binding buffer. The $Delta$ RU for activator binding to TBP and that for holoenzyme binding to activator bound to TBP are shown.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Extensive biochemical studies have demonstrated the essential role of TBP-associated factors in transcriptional activationand selective activator interactions (8, 9, 42). However,in vivo analyses with yeasts have revealed that TBP-associatedfactors are dispensable for general transcription (29, 44)but are required for the transcription of a subset of essentialgenes (1, 38, 45). On the other hand, Mediator has beenshown to be required for the general regulation of PolII transcriptionin vivo (41), but the mechanism by which Mediator enables thebasal transcription machinery to respond to gene-specific transcriptionalregulatory proteins is not known. From the biochemical analysesof various mutant holoenzymes, we have identified the Gal11 moduleas a specific and direct target for activator binding and havecharacterized the functional relevance of this interaction witha reconstituted in vitro transcription system. Our results clearlyshow that Mediator is involved in transcriptional regulation throughits direct and specific interactions withactivators.

The major activator binding module of Mediator. Analyses of physical interactions within the Mediator complex have revealed that about two-thirds of the Mediator subunitsare tightly bound to Rgr1 (the so-called Rgr1 subcomplex [24]).Within the Rgr1 subcomplex, a group of genetically characterizedtranscriptional regulators (Sin4, Gal11, and Hrs1) appears toform a separate functional module (Gal11 module). The direct bindingof activator proteins to Gal11 supports the idea that the Gal11module may participate in the regulation of transcription by itsinteraction with activator and repressor (or corepressor) proteins.The severe reduction in the activator binding efficiency of thegal11 $Delta$ holoenzyme and its accompanying inability to respond tothe activator in a reconstituted transcription system argue stronglyfor the physiological significance of the activator-Gal11 interaction.Furthermore, the fact that the artificial tethering of the gal11mutant holoenzyme to promoters can bypass the requirement forGal11 in transcriptional activation also supports that notion.Once enhancer-bound activators contact a holoenzyme, they mayhold the enzyme in the appropriate conformation for stable PICformation. Although free activator domains that do not associatewith an enhancer may still interact with Gal11, the low specificconcentration of activator proteins probably limits this interactionto only the relevant promoters invivo.

Activator-specific transcriptional activation of Mediator. Although the gal11 $Delta$ and hrs1 $Delta$ holoenzymes were defective in their interaction with GCN4 and Gal4VP16, both of the mutant holoenzymessupported some transcriptional activation by GCN4 but not by Gal4VP16(Table 2). This result suggests that GCN4 has additional targetseither in the holoenzyme complex or among the other general transcriptionfactors, whereas Gal4VP16 utilizes the Gal11 module as its majortarget during the transcription initiation step (4). We recentlyobtained a result that supports this notion. During the analysisof novel Mediator subunits, we found that a newly identified Mediatorcomponent, Med10, is absolutely required for GCN4-mediated transcriptionalactivation in vivo, whereas the loss of the Gal11 module has arelatively minor effect on GCN4-mediated transcriptional activation(15). Therefore, the Med10-mediated GCN4 response may be morecrucial to the activation process than activator binding by theGal11 module.

View this table:
[in this window]
[in a new window]

TABLE 2. Quantitation of functional activities of wild-type and mutant holoenzymes in vitro^a

Although the mechanism by which Med10 mediates GCN4-induced transcriptional activation is not yet known, the presence of stoichiometricamounts of the Med10 subunit in the gal11 $Delta$ and hrs1 $Delta$ holoenzymesmay enable the mutant holoenzymes to respond to GCN4 to some degree.This idea is further supported by the fact that the rgr1 $Delta$ 2 holoenzymecontains substoichiometric amounts of Rgr1-associated Mediatorsubunits, including Med10 (Fig. 1B and data not shown). Therefore,the loss of the major activator binding module (Gal11 module)and GCN4-specific Mediator subunit Med10 in the rgr1 $Delta$ 2 holoenzymemay result in an additive (or synergistic) defect in GCN4-mediatedtranscriptionalactivation.

Although our immunoblot analyses of the gal11 $Delta$ and hrs1 $Delta$ holoenzymes revealed no difference in their subunit compositions,the hrs1 $Delta$ holoenzyme showed a higher response to the activatorthan did the gal11 $Delta$ holoenzyme (Table 2). One possible explanationfor this observation is that small amounts of Hrs1 and Gal11 mayremain associated with the gal11 $Delta$ and hrs1 $Delta$ holoenzymes, respectively.A residual amount of Gal11 in the hrs1 $Delta$ holoenzyme may be responsiblefor the slightly higher activator response observed with the hrs1 $Delta$ holoenzyme.

Mediator subunits involved in the postrecruitment process of transcriptional activation. Our previous studies revealed the absolute and specific requirement for Med6 in transcriptional activation (25). However,the Mediator-activator interaction was not affected by a deficiencyin Med6, indicating that Med6 has no apparent binding affinityfor activators in vitro (data not shown). It was also shown thatMed6 associates with Srb proteins rather than with the componentsof the Rgr1 subcomplex (24). In addition, while analyses ofthe srb5 $Delta$ holoenzyme revealed a requirement for Srb2 and Srb5in both basal and activated transcription in vitro, mutant holoenzymesthat lacked these subunits showed a capacity for activator bindingthat was comparable to that of the wild-type holoenzyme (Fig.4D). Taken together with the results of an artificial recruitmentexperiment with the srb5 $Delta$ holoenzyme (Table 1), these findingssuggest that facilitated recruitment of a holoenzyme to a promoteris necessary but not sufficient for transcriptional activationand that an unknown biochemical activity other than physical recruitmentto the promoter is required for transcriptional activation. Asmentioned previously, the genetic interaction between the SRBgenes and the CTD of PolII indicates that SRB gene products (theSrb4 subcomplex) may function in the modulation or isomerizationof holoenzyme activity, possibly subsequent to activator binding.The identification of the mechanism of SRB function is essentialfor the elucidation of the transcriptional activationmechanism.

Despite the requirement for an activator-Gal11 interaction in transcriptional activation in a defined system, all of the componentsof the Gal11 module (Sin4, Gal11, and Hrs1) are dispensable forcell viability (30 and references therein). Both SPR and coimmunoprecipitationanalyses of mutant holoenzymes that lack Gal11 have shown thatthese holoenzymes retain a weak ability to interact with activators.Thus, the Gal11 module may constitute the major activator bindingsite, but secondary activator interaction sites may provide enoughbinding to sustain cell viability in vivo. Srb4, which was shownto have a low binding affinity for transcriptional activators(22), and other members of the Rgr1 subcomplex may be good candidatesfor secondary Mediator subunits that interact withactivators.

TBP-activator-Mediator interactions. It is interesting that an activator can bind to TBP and Mediator simultaneously. This result indicates that the activatoraccelerates and stabilizes PIC formation by interacting with bothTBP and a holoenzyme at the same time. Although the TFIIB-PolIIinteraction helps to stabilize the PIC (reviewed in reference35), the affinity of the TFIIB-PolII interaction alone may notbe high enough to sustain stable PIC formation. The strong connectionbetween TBP and PolII established by the interactions of an activatorand Mediator may provide an important contribution to stable PICformation during transcriptional activation. Therefore, recruitmentof TBP and a holoenzyme to the promoter, the stabilization ofPIC formation, and isomerization (modulation) of holoenzyme activityappear to constitute the major mechanisms of transcriptional activationby the holoenzyme invitro.

	ACKNOWLEDGMENTS

We thank Jeong Kon Seo and Juri Kim for technical help, Kelly LaMarco for careful reading of the manuscript, and other membersof Young-Joon Kim's laboratory for helpful comments. We also thankRoger Kornberg, Richard Young, Toshio Fukasawa, David Stillman,and Andres Aguilera for providing Mediator mutant strains, antibodies,and related plasmids. We are grateful to Michael Green for GST-VP16fusion plasmids and Steve Hanes for reporterplasmids.

This work was supported by grants from SBRI (B-96-004) and the Ministry of Health and Welfare, Republic of Korea (HMP-97-B-3-0030of the 1997 Good Health R&D Project), to Y.-J.K.

	FOOTNOTES

^* Corresponding author. Mailing address: Center for Molecular Medicine, Samsung Biomedical Research Institute, SungkyunkwanUniversity College of Medicine, 50 Ilwong-dong, Kangnam-ku, Seoul135-230, Korea. Phone: 82-2-3410-3638. Fax: 82-2-3410-3649. E-mail:yjkim{at}smc.samsung.co.kr.

Present address: Center for Ligand and Transcription, Chonnam National University, 300 Yongbong-dong, Puk-ku, Kwangju 500-757,Korea.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Apone, L. M., C. M. Virbasius, J. C. Reese, and M. R. Green. 1996. Yeast TAF(II)90 is required for cell-cycle progression through G2/M but not for general transcription activation. Genes Dev. 10:2368-2380[Abstract/Free Full Text].

2. Berger, S. L., W. D. Cress, A. Cress, S. J. Triezenberg, and L. Guarente. 1990. Selective inhibition of activated but not basal transcription by the acidic activation domain of VP16: evidence for transcriptional adaptors. Cell 61:1199-1208[Medline].

3. Bjorklund, S., and Y. J. Kim. 1996. Mediator of transcriptional regulation. Trends Biochem. Sci. 21:335-337[Medline].

4. Brown, S. A., C. S. Weirich, E. M. Newton, and R. E. Kingston. 1998. Transcriptional activation domains stimulate initiation and elongation at different times and via different residues. EMBO J. 17:3146-3154[Medline].

5. Chasman, D. I., J. Leatherwood, M. Carey, M. Ptashne, and R. D. Kornberg. 1989. Activation of yeast polymerase II transcription by herpesvirus VP16 and GAL4 derivatives in vitro. Mol. Cell. Biol. 9:4746-4749[Abstract/Free Full Text].

6. Estojak, J., R. Brent, and E. A. Golemis. 1995. Correlation of two-hybrid affinity data with in vitro measurements. Mol. Cell. Biol. 15:5820-5829[Abstract].

7. Flanagan, P. M., R. J. Kelleher III, M. H. Sayre, H. Tschochner, and R. D. Kornberg. 1991. A mediator required for activation of RNA polymerase II transcription in vitro. Nature 350:436-438[Medline].

8. Goodrich, J. A., G. Cutler, and R. Tjian. 1996. Contacts in context: promoter specificity and macromolecular interactions in transcription. Cell 84:825-830[Medline].

9. Goodrich, J. A., and R. Tjian. 1994. TBP-TAF complexes: selectivity factors for eukaryotic transcription. Curr. Opin. Cell Biol. 6:403-409[Medline].

10. Guarente, L. 1983. Yeast promoters and lacZ fusions designed to study expression of cloned genes in yeast. Methods Enzymol. 101:181-191[Medline].

11. Guarente, L., R. R. Yocum, and P. Gifford. 1982. A GAL10-CYC1 hybrid yeast promoter identifies the GAL4 regulatory region as an upstream site. Proc. Natl. Acad. Sci. USA 79:7410-7414[Abstract/Free Full Text].

12. Gustafsson, C. M., L. C. Myers, J. Beve, H. Spahr, M. Lui, H. Erdjument-Bromage, P. Tempst, and R. D. Kornberg. 1998. Identification of new mediator subunits in the RNA polymerase II holoenzyme from Saccharomyces cerevisiae. J. Biol. Chem. 273:30851-30854[Abstract/Free Full Text].

13. Gustafsson, C. M., L. C. Myers, Y. Li, M. J. Redd, M. Lui, H. Erdjument-Bromage, P. Tempst, and R. D. Kornberg. 1997. Identification of Rox3 as a component of mediator and RNA polymerase II holoenzyme. J. Biol. Chem. 272:48-50[Abstract/Free Full Text].

14. Gyuris, J., E. Golemis, H. Chertkov, and R. Brent. 1993. Cdi1, a human G1 and S phase protein phosphatase that associates with Cdk2. Cell 75:791-803[Medline].

15. Han, S. J., Y. C. Lee, B. S. Gim, G.-H. Ryu, S. J. Park, W. S. Lane, and Y.-J. Kim. 1999. Activator-specific requirement of yeast Mediator proteins for RNA polymerase II transcriptional activation. Mol. Cell. Biol. 19:979-988[Abstract/Free Full Text].

16. Hengartner, C. J., C. M. Thompson, J. Zhang, D. M. Chao, S. M. Liao, A. J. Koleske, S. Okamura, and R. A. Young. 1995. Association of an activator with an RNA polymerase II holoenzyme. Genes Dev. 9:897-910[Abstract/Free Full Text].

17. Henry, N. L., A. M. Campbell, W. J. Feaver, D. Poon, P. A. Weil, and R. D. Kornberg. 1994. TFIIF-TAF-RNA polymerase II connection. Genes Dev. 8:2868-2878[Abstract/Free Full Text].

18. Ingles, C. J., M. Shales, W. D. Cress, S. J. Triezenberg, and J. Greenblatt. 1991. Reduced binding of TFIID to transcriptionally compromised mutants of VP16. Nature 351:588-590[Medline].

19. Kaelin, W. G., Jr., W. Krek, W. R. Sellers, J. A. DeCaprio, F. Ajchenbaum, C. S. Fuchs, T. Chittenden, Y. Li, P. J. Farnham, M. A. Blanar, D. M. Livingston, and E. K. Flemington. 1992. Expression cloning of a cDNA encoding a retinoblastoma-binding protein with E2F-like properties. Cell 70:351-364[Medline].

20. Kelleher, R. J., III, P. M. Flanagan, and R. D. Kornberg. 1990. A novel mediator between activator proteins and the RNA polymerase II transcription apparatus. Cell 61:1209-1215[Medline].

21. Kim, Y. J., S. Bjorklund, Y. Li, M. H. Sayre, and R. D. Kornberg. 1994. A multiprotein mediator of transcriptional activation and its interaction with the C-terminal repeat domain of RNA polymerase II. Cell 77:599-608[Medline].

22. Koh, S. S., A. Z. Ansari, M. Ptashne, and R. A. Young. 1998. An activator target in the RNA polymerase II holoenzyme. Mol. Cell 1:895-904[Medline].

23. Lee, T. I., J. J. Wyrick, S. S. Koh, E. G. Jennings, E. L. Gadbois, and R. A. Young. 1998. Interplay of positive and negative regulators in transcription initiation by RNA polymerase II holoenzyme. Mol. Cell. Biol. 18:4455-4462[Abstract/Free Full Text].

24. Lee, Y. C., and Y.-J. Kim. 1998. Requirement for a functional interaction between mediator components Med6 and Srb4 in RNA polymerase II transcription. Mol. Cell. Biol. 18:5364-5370[Abstract/Free Full Text].

25. Lee, Y. C., S. Min, B. S. Gim, and Y. J. Kim. 1997. A transcriptional mediator protein that is required for activation of many RNA polymerase II promoters and is conserved from yeast to humans. Mol. Cell. Biol. 17:4622-4632[Abstract].

26. Li, Y., S. Bjorklund, Y. W. Jiang, Y. J. Kim, W. S. Lane, D. J. Stillman, and R. D. Kornberg. 1995. Yeast global transcriptional regulators Sin4 and Rgr1 are components of mediator complex/RNA polymerase II holoenzyme. Proc. Natl. Acad. Sci. USA 92:10864-10868[Abstract/Free Full Text].

27. Liao, S. M., J. Zhang, D. A. Jeffery, A. J. Koleske, C. M. Thompson, D. M. Chao, M. Viljoen, H. J. van Vuuren, and R. A. Young. 1995. A kinase-cyclin pair in the RNA polymerase II holoenzyme. Nature 374:193-196[Medline].

28. Lin, Y. S., and M. R. Green. 1991. Mechanism of action of an acidic transcriptional activator in vitro. Cell 64:971-981[Medline].

29. Moqtaderi, Z., Y. Bai, D. Poon, P. A. Weil, and K. Struhl. 1996. TBP-associated factors are not generally required for transcriptional activation in yeast. Nature 383:188-191[Medline].

30. Myers, L. C., C. M. Gustafsson, D. A. Bushnell, M. Lui, H. Erdjument-Bromage, P. Tempst, and R. D. Kornberg. 1998. The Med proteins of yeast and their function through the RNA polymerase II carboxy-terminal domain. Genes Dev. 12:45-54[Abstract/Free Full Text].

31. Nonet, M. L., and R. A. Young. 1989. Intragenic and extragenic suppressors of mutations in the heptapeptide repeat domain of Saccharomyces cerevisiae RNA polymerase II. Genetics 123:715-724[Abstract/Free Full Text].

32. O'Neil, K., J. D. Shuman, C. Ampe, and W. F. DeGrado. 1991. DNA-induced increase in the alpha-helical content of C/EBP and GCN4. Biochemistry 30:9030-9034[Medline].

33. Piruat, J. I., S. Chavez, and A. Aguilera. 1997. The yeast HRS1 gene is involved in positive and negative regulation of transcription and shows genetic characteristics similar to SIN4 and GAL11. Genetics 147:1585-1594[Abstract].

34. Roberts, S. G., I. Ha, E. Maldonado, D. Reinberg, and M. R. Green. 1993. Interaction between an acidic activator and transcription factor TFIIB is required for transcriptional activation. Nature 363:741-744[Medline].

35. Roeder, R. G. 1996. The role of general initiation factors in transcription by RNA polymerase II. Trends Biochem. Sci. 21:327-335[Medline].

36. Sakurai, H., Y. Hiraoka, and T. Fukasawa. 1993. Yeast GAL11 protein is a distinctive type transcription factor that enhances basal transcription in vitro. Proc. Natl. Acad. Sci. USA 90:8382-8386[Abstract/Free Full Text].

37. Santos-Rosa, H., B. Clever, W. D. Heyer, and A. Aguilera. 1996. The yeast HRS1 gene encodes a polyglutamine-rich nuclear protein required for spontaneous and hpr1-induced deletions between direct repeats. Genetics 142:705-716[Abstract].

38. Shen, W. C., and M. R. Green. 1997. Yeast TAF(II)145 functions as a core promoter selectivity factor, not a general coactivator. Cell 90:615-624[Medline].

39. Stringer, K. F., C. J. Ingles, and J. Greenblatt. 1990. Direct and selective binding of an acidic transcriptional activation domain to the TATA-box factor TFIID. Nature 345:783-786[Medline].

40. Thompson, C. M., A. J. Koleske, D. M. Chao, and R. A. Young. 1993. A multisubunit complex associated with the RNA polymerase II CTD and TATA-binding protein in yeast. Cell 73:1361-1375[Medline].

41. Thompson, C. M., and R. A. Young. 1995. General requirement for RNA polymerase II holoenzymes in vivo. Proc. Natl. Acad. Sci. USA 92:4587-4590[Abstract/Free Full Text].

42. Verrijzer, C. P., and R. Tjian. 1996. TAFs mediate transcriptional activation and promoter selectivity. Trends Biochem. Sci. 21:338-342[Medline].

43. Vinson, C. R., K. L. LaMarco, P. F. Johnson, W. H. Landschulz, and S. L. McKnight. 1988. In situ detection of sequence-specific DNA binding activity specified by a recombinant bacteriophage. Genes Dev. 2:801-806[Abstract/Free Full Text].

44. Walker, S. S., J. C. Reese, L. M. Apone, and M. R. Green. 1996. Transcription activation in cells lacking TAF(II)s. Nature 383:185-188[Medline].

45. Walker, S. S., W. C. Shen, J. C. Reese, L. M. Apone, and M. R. Green. 1997. Yeast TAF(II)145 required for transcription of G1/S cyclin genes and regulated by the cellular growth state. Cell 90:607-614[Medline].

46. Wilson, C. J., D. M. Chao, A. N. Imbalzano, G. R. Schnitzler, R. E. Kingston, and R. A. Young. 1996. RNA polymerase II holoenzyme contains SWI/SNF regulators involved in chromatin remodeling. Cell 84:235-244[Medline].

47. Xiao, H., A. Pearson, B. Coulombe, R. Truant, S. Zhang, J. L. Regier, S. J. Triezenberg, D. Reinberg, O. Flores, C. J. Ingles, and J. Greenblatt. 1994. Binding of basal transcription factor TFIIH to the acidic activation domains of VP16 and p53. Mol. Cell. Biol. 14:7013-7024[Abstract/Free Full Text].

This article has been cited by other articles:

Thakur, J. K., Arthanari, H., Yang, F., Chau, K. H., Wagner, G., Naar, A. M. (2009). Mediator Subunit Gal11p/MED15 Is Required for Fatty Acid-dependent Gene Activation by Yeast Transcription Factor Oaf1p. J. Biol. Chem. 284: 4422-4428 [Abstract] [Full Text]
Takahashi, H., Kasahara, K., Kokubo, T. (2009). Saccharomyces cerevisiae Med9 comprises two functionally distinct domains that play different roles in transcriptional regulation. GENES CELLS 14: 53-67 [Abstract] [Full Text]
Bourbon, H.-M. (2008). Comparative genomics supports a deep evolutionary origin for the large, four-module transcriptional mediator complex. Nucleic Acids Res 36: 3993-4008 [Abstract] [Full Text]
Linder, T., Rasmussen, N. N., Samuelsen, C. O., Chatzidaki, E., Baraznenok, V., Beve, J., Henriksen, P., Gustafsson, C. M., Holmberg, S. (2008). Two conserved modules of Schizosaccharomyces pombe Mediator regulate distinct cellular pathways. Nucleic Acids Res 36: 2489-2504 [Abstract] [Full Text]
Lariviere, L., Seizl, M., van Wageningen, S., Rother, S., van de Pasch, L., Feldmann, H., Strasser, K., Hahn, S., Holstege, F. C.P., Cramer, P. (2008). Structure-system correlation identifies a gene regulatory Mediator submodule. Genes Dev. 22: 872-877 [Abstract] [Full Text]
Kim, D.-H., Kim, G. S., Yun, C. H., Lee, Y. C. (2008). Functional Conservation of the Glutamine-Rich Domains of Yeast Gal11 and Human SRC-1 in the Transactivation of Glucocorticoid Receptor Tau 1 in Saccharomyces cerevisiae. Mol. Cell. Biol. 28: 913-925 [Abstract] [Full Text]
Guglielmi, B., Soutourina, J., Esnault, C., Werner, M. (2007). TFIIS elongation factor and Mediator act in conjunction during transcription initiation in vivo. Proc. Natl. Acad. Sci. USA 104: 16062-16067 [Abstract] [Full Text]
Baidoobonso, S. M., Guidi, B. W., Myers, L. C. (2007). Med19(Rox3) Regulates Intermodule Interactions in the Saccharomyces cerevisiae Mediator Complex. J. Biol. Chem. 282: 5551-5559 [Abstract] [Full Text]
Leroy, C., Cormier, L., Kuras, L. (2006). Independent Recruitment of Mediator and SAGA by the Activator Met4. Mol. Cell. Biol. 26: 3149-3163 [Abstract] [Full Text]
Sulahian, R., Johnston, S. A., Kodadek, T. (2006). The proteasomal ATPase complex is required for stress-induced transcription in yeast. Nucleic Acids Res 34: 1351-1357 [Abstract] [Full Text]
Li, L., Quinton, T., Miles, S., Breeden, L. L. (2005). Genetic Interactions Between Mediator and the Late G1-Specific Transcription Factor Swi6 in Saccharomyces cerevisiae. Genetics 171: 477-488 [Abstract] [Full Text]
Takagi, Y., Chadick, J. Z., Davis, J. A., Asturias, F. J. (2005). Preponderance of Free Mediator in the Yeast Saccharomyces cerevisiae. J. Biol. Chem. 280: 31200-31207 [Abstract] [Full Text]
Lu, Z., Rowe, S. P., Brennan, B. B., Davis, S. E., Metzler, R. E., Nau, J. J., Majmudar, C. Y., Mapp, A. K., Ansari, A. Z. (2005). Unraveling the Mechanism of a Potent Transcriptional Activator. J. Biol. Chem. 280: 29689-29698 [Abstract] [Full Text]
Govind, C. K., Yoon, S., Qiu, H., Govind, S., Hinnebusch, A. G. (2005). Simultaneous Recruitment of Coactivators by Gcn4p Stimulates Multiple Steps of Transcription In Vivo. Mol. Cell. Biol. 25: 5626-5638 [Abstract] [Full Text]
Malik, S., Baek, H. J., Wu, W., Roeder, R. G. (2005). Structural and Functional Characterization of PC2 and RNA Polymerase II-Associated Subpopulations of Metazoan Mediator. Mol. Cell. Biol. 25: 2117-2129 [Abstract] [Full Text]
Larschan, E., Winston, F. (2005). The Saccharomyces cerevisiae Srb8-Srb11 Complex Functions with the SAGA Complex during Gal4-Activated Transcription. Mol. Cell. Biol. 25: 114-123 [Abstract] [Full Text]
Wang, X., Michels, C. A. (2004). Mutations in SIN4 and RGR1 Cause Constitutive Expression of MAL Structural Genes in Saccharomyces cerevisiae. Genetics 168: 747-757 [Abstract] [Full Text]
Zhang, F., Sumibcay, L., Hinnebusch, A. G., Swanson, M. J. (2004). A Triad of Subunits from the Gal11/Tail Domain of Srb Mediator Is an In Vivo Target of Transcriptional Activator Gcn4p. Mol. Cell. Biol. 24: 6871-6886 [Abstract] [Full Text]
Fukuda, A., Nakadai, T., Shimada, M., Tsukui, T., Matsumoto, M., Nogi, Y., Meisterernst, M., Hisatake, K. (2004). Transcriptional Coactivator PC4 Stimulates Promoter Escape and Facilitates Transcriptional Synergy by GAL4-VP16. Mol. Cell. Biol. 24: 6525-6535 [Abstract] [Full Text]
Qiu, H., Hu, C., Yoon, S., Natarajan, K., Swanson, M. J., Hinnebusch, A. G. (2004). An Array of Coactivators Is Required for Optimal Recruitment of TATA Binding Protein and RNA Polymerase II by Promoter-Bound Gcn4p. Mol. Cell. Biol. 24: 4104-4117 [Abstract] [Full Text]
Malagon, F., Tong, A. H., Shafer, B. K., Strathern, J. N. (2004). Genetic Interactions of DST1 in Saccharomyces cerevisiae Suggest a Role of TFIIS in the Initiation-Elongation Transition. Genetics 166: 1215-1227 [Abstract] [Full Text]
Rani, P. G., Ranish, J. A., Hahn, S. (2004). RNA Polymerase II (Pol II)-TFIIF and Pol II-Mediator Complexes: the Major Stable Pol II Complexes and Their Activity in Transcription Initiation and Reinitiation. Mol. Cell. Biol. 24: 1709-1720 [Abstract] [Full Text]
Yoon, S., Qiu, H., Swanson, M. J., Hinnebusch, A. G. (2003). Recruitment of SWI/SNF by Gcn4p Does Not Require Snf2p or Gcn5p but Depends Strongly on SWI/SNF Integrity, SRB Mediator, and SAGA. Mol. Cell. Biol. 23: 8829-8845 [Abstract] [Full Text]
Cantin, G. T., Stevens, J. L., Berk, A. J. (2003). Activation domain-mediator interactions promote transcription preinitiation complex assembly on promoter DNA. Proc. Natl. Acad. Sci. USA 100: 12003-12008 [Abstract] [Full Text]
Lewis, B. A., Reinberg, D. (2003). The mediator coactivator complex: functional and physical roles in transcriptional regulation. J. Cell Sci. 116: 3667-3675 [Abstract] [Full Text]
Swanson, M. J., Qiu, H., Sumibcay, L., Krueger, A., Kim, S.-j., Natarajan, K., Yoon, S., Hinnebusch, A. G. (2003). A Multiplicity of Coactivators Is Required by Gcn4p at Individual Promoters In Vivo. Mol. Cell. Biol. 23: 2800-2820 [Abstract] [Full Text]
Park, J. M., Kim, J. M., Kim, L. K., Kim, S. N., Kim-Ha, J., Kim, J. H., Kim, Y.-J. (2003). Signal-Induced Transcriptional Activation by Dif Requires the dTRAP80 Mediator Module. Mol. Cell. Biol. 23: 1358-1367 [Abstract] [Full Text]
Balciunas, D., Hallberg, M., Bjorklund, S., Ronne, H. (2003). Functional Interactions within Yeast Mediator and Evidence of Differential Subunit Modifications. J. Biol. Chem. 278: 3831-3839 [Abstract] [Full Text]
Lau, J. F., Nusinzon, I., Burakov, D., Freedman, L. P., Horvath, C. M. (2003). Role of Metazoan Mediator Proteins in Interferon-Responsive Transcription. Mol. Cell. Biol. 23: 620-628 [Abstract] [Full Text]
Reeves, W. M., Hahn, S. (2003). Activator-Independent Functions of the Yeast Mediator Sin4 Complex in Preinitiation Complex Formation and Transcription Reinitiation. Mol. Cell. Biol. 23: 349-358 [Abstract] [Full Text]
Hall, D. B., Struhl, K. (2002). The VP16 Activation Domain Interacts with Multiple Transcriptional Components as Determined by Protein-Protein Cross-linking in Vivo. J. Biol. Chem. 277: 46043-46050 [Abstract] [Full Text]
Shim, E. Y., Walker, A. K., Blackwell, T. K. (2002). Broad Requirement for the Mediator Subunit RGR-1 for Transcription in the Caenorhabditis elegans Embryo. J. Biol. Chem. 277: 30413-30416 [Abstract] [Full Text]
Malik, S., Wallberg, A. E., Kang, Y. K., Roeder, R. G. (2002). TRAP/SMCC/Mediator-Dependent Transcriptional Activation from DNA and Chromatin Templates by Orphan Nuclear Receptor Hepatocyte Nuclear Factor 4. Mol. Cell. Biol. 22: 5626-5637 [Abstract] [Full Text]
Gu, J.-Y., Park, J. M., Song, E. J., Mizuguchi, G., Yoon, J. H., Kim-Ha, J., Lee, K.-J., Kim, Y.-J. (2002). Novel Mediator Proteins of the Small Mediator Complex in Drosophila SL2 Cells. J. Biol. Chem. 277: 27154-27161 [Abstract] [Full Text]
Carrozza, M. J., John, S., Sil, A. K., Hopper, J. E., Workman, J. L. (2002). Gal80 Confers Specificity on HAT Complex Interactions with Activators. J. Biol. Chem. 277: 24648-24652 [Abstract] [Full Text]
Lu, Z., Ansari, A. Z., Lu, X., Ogirala, A., Ptashne, M. (2002). A target essential for the activity of a nonacidic yeast transcriptional activator. Proc. Natl. Acad. Sci. USA 99: 8591-8596 [Abstract] [Full Text]
Howard, S. C., Budovskaya, Y. V., Chang, Y.-W., Herman, P. K. (2002). The C-terminal Domain of the Largest Subunit of RNA Polymerase II Is Required for Stationary Phase Entry and Functionally Interacts with the Ras/PKA Signaling Pathway. J. Biol. Chem. 277: 19488-19497 [Abstract] [Full Text]
Baek, H. J., Malik, S., Qin, J., Roeder, R. G. (2002). Requirement of TRAP/Mediator for Both Activator-Independent and Activator-Dependent Transcription in Conjunction with TFIID-Associated TAFIIs. Mol. Cell. Biol. 22: 2842-2852 [Abstract] [Full Text]
Hinnebusch, A. G., Natarajan, K. (2002). Gcn4p, a Master Regulator of Gene Expression, Is Controlled at Multiple Levels by Diverse Signals of Starvation and Stress. Eukaryot Cell 1: 22-32 [Full Text]
Kang, J. S., Kim, S. H., Hwang, M. S., Han, S. J., Lee, Y. C., Kim, Y.-J. (2001). The Structural and Functional Organization of the Yeast Mediator Complex. J. Biol. Chem. 276: 42003-42010 [Abstract] [Full Text]
Bhoite, L. T., Yu, Y., Stillman, D. J. (2001). The Swi5 activator recruits the Mediator complex to the HO promoter without RNA polymerase II. Genes Dev. 15: 2457-2469 [Abstract] [Full Text]
Gim, B. S., Park, J. M., Yoon, J. H., Kang, C., Kim, Y.-J. (2001). Drosophila Med6 Is Required for Elevated Expression of a Large but Distinct Set of Developmentally Regulated Genes. Mol. Cell. Biol. 21: 5242-5255 [Abstract] [Full Text]
Tansey, W. P. (2001). Transcriptional activation: risky business. Genes Dev. 15: 1045-1050 [Abstract] [Full Text]
Park, J. M., Gim, B. S., Kim, J. M., Yoon, J. H., Kim, H.-S., Kang, J.-G., Kim, Y.-J. (2001). Drosophila Mediator Complex Is Broadly Utilized by Diverse Gene-Specific Transcription Factors at Different Types of Core Promoters. Mol. Cell. Biol. 21: 2312-2323 [Abstract] [Full Text]
Park, J. M., Kim, H.-S., Han, S. J., Hwang, M.-S., Lee, Y. C., Kim, Y.-J. (2000). In Vivo Requirement of Activator-Specific Binding Targets of Mediator. Mol. Cell. Biol. 20: 8709-8719 [Abstract] [Full Text]
Boube, M., Faucher, C., Joulia, L., Cribbs, D. L., Bourbon, H.-M. (2000). Drosophila homologs of transcriptional mediator complex subunits are required for adult cell and segment identity specification. Genes Dev. 14: 2906-2917 [Abstract] [Full Text]
Costa, P. J., Arndt, K. M. (2000). Synthetic Lethal Interactions Suggest a Role for the Saccharomyces cerevisiae Rtf1 Protein in Transcription Elongation. Genetics 156: 535-547 [Abstract] [Full Text]
Lee, M., Chatterjee, S., Struhl, K. (2000). Genetic Analysis of the Role of Pol II Holoenzyme Components in Repression by the Cyc8-Tup1 Corepressor in Yeast. Genetics 155: 1535-1542 [Abstract] [Full Text]
Han, Y., Kodadek, T. (2000). Peptides Selected to Bind the Gal80 Repressor Are Potent Transcriptional Activation Domains in Yeast. J. Biol. Chem. 275: 14979-14984 [Abstract] [Full Text]
Kim, S., Cabane, K., Hampsey, M., Reinberg, D. (2000). Genetic Analysis of the Ydr1-Bur6 Repressor Complex Reveals an Intricate Balance among Transcriptional Regulatory Proteins in Yeast. Mol. Cell. Biol. 20: 2455-2465 [Abstract] [Full Text]
Kwon, J. Y., Park, J. M., Gim, B. S., Han, S. J., Lee, J., Kim, Y.-J. (1999). Caenorhabditis elegans Mediator complexes are required for developmental-specific transcriptional activation. Proc. Natl. Acad. Sci. USA 96: 14990-14995 [Abstract] [Full Text]
Sakurai, H., Fukasawa, T. (2000). Functional Connections between Mediator Components and General Transcription Factors of Saccharomyces cerevisiae. J. Biol. Chem. 275: 37251-37256 [Abstract] [Full Text]
Liu, Y., Ranish, J. A., Aebersold, R., Hahn, S. (2001). Yeast Nuclear Extract Contains Two Major Forms of RNA Polymerase II Mediator Complexes. J. Biol. Chem. 276: 7169-7175 [Abstract] [Full Text]
Chang, C., Gonzalez, F., Rothermel, B., Sun, L., Johnston, S. A., Kodadek, T. (2001). The Gal4 Activation Domain Binds Sug2 Protein, a Proteasome Component, in Vivo and in Vitro. J. Biol. Chem. 276: 30956-30963 [Abstract] [Full Text]
Han, S. J., Lee, J.-S., Kang, J. S., Kim, Y.-J. (2001). Med9/Cse2 and Gal11 Modules Are Required for Transcriptional Repression of Distinct Group of Genes. J. Biol. Chem. 276: 37020-37026 [Abstract] [Full Text]
Dotson, M. R., Yuan, C. X., Roeder, R. G., Myers, L. C., Gustafsson, C. M., Jiang, Y. W., Li, Y., Kornberg, R. D., Asturias, F. J. (2000). Structural organization of yeast and mammalian mediator complexes. Proc. Natl. Acad. Sci. USA 97: 14307-14310 [Abstract] [Full Text]

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Lee, Y. C.
	Articles by Kim, Y.-J.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Lee, Y. C.
	Articles by Kim, Y.-J.

1.	Apone, L. M., C. M. Virbasius, J. C. Reese, and M. R. Green. 1996. Yeast TAF(II)90 is required for cell-cycle progression through G2/M but not for general transcription activation. Genes Dev. 10:2368-2380[Abstract/Free Full Text].
2.	Berger, S. L., W. D. Cress, A. Cress, S. J. Triezenberg, and L. Guarente. 1990. Selective inhibition of activated but not basal transcription by the acidic activation domain of VP16: evidence for transcriptional adaptors. Cell 61:1199-1208[Medline].
3.	Bjorklund, S., and Y. J. Kim. 1996. Mediator of transcriptional regulation. Trends Biochem. Sci. 21:335-337[Medline].
4.	Brown, S. A., C. S. Weirich, E. M. Newton, and R. E. Kingston. 1998. Transcriptional activation domains stimulate initiation and elongation at different times and via different residues. EMBO J. 17:3146-3154[Medline].
5.	Chasman, D. I., J. Leatherwood, M. Carey, M. Ptashne, and R. D. Kornberg. 1989. Activation of yeast polymerase II transcription by herpesvirus VP16 and GAL4 derivatives in vitro. Mol. Cell. Biol. 9:4746-4749[Abstract/Free Full Text].
6.	Estojak, J., R. Brent, and E. A. Golemis. 1995. Correlation of two-hybrid affinity data with in vitro measurements. Mol. Cell. Biol. 15:5820-5829[Abstract].
7.	Flanagan, P. M., R. J. Kelleher III, M. H. Sayre, H. Tschochner, and R. D. Kornberg. 1991. A mediator required for activation of RNA polymerase II transcription in vitro. Nature 350:436-438[Medline].
8.	Goodrich, J. A., G. Cutler, and R. Tjian. 1996. Contacts in context: promoter specificity and macromolecular interactions in transcription. Cell 84:825-830[Medline].
9.	Goodrich, J. A., and R. Tjian. 1994. TBP-TAF complexes: selectivity factors for eukaryotic transcription. Curr. Opin. Cell Biol. 6:403-409[Medline].
10.	Guarente, L. 1983. Yeast promoters and lacZ fusions designed to study expression of cloned genes in yeast. Methods Enzymol. 101:181-191[Medline].
11.	Guarente, L., R. R. Yocum, and P. Gifford. 1982. A GAL10-CYC1 hybrid yeast promoter identifies the GAL4 regulatory region as an upstream site. Proc. Natl. Acad. Sci. USA 79:7410-7414[Abstract/Free Full Text].
12.	Gustafsson, C. M., L. C. Myers, J. Beve, H. Spahr, M. Lui, H. Erdjument-Bromage, P. Tempst, and R. D. Kornberg. 1998. Identification of new mediator subunits in the RNA polymerase II holoenzyme from Saccharomyces cerevisiae. J. Biol. Chem. 273:30851-30854[Abstract/Free Full Text].
13.	Gustafsson, C. M., L. C. Myers, Y. Li, M. J. Redd, M. Lui, H. Erdjument-Bromage, P. Tempst, and R. D. Kornberg. 1997. Identification of Rox3 as a component of mediator and RNA polymerase II holoenzyme. J. Biol. Chem. 272:48-50[Abstract/Free Full Text].
14.	Gyuris, J., E. Golemis, H. Chertkov, and R. Brent. 1993. Cdi1, a human G1 and S phase protein phosphatase that associates with Cdk2. Cell 75:791-803[Medline].
15.	Han, S. J., Y. C. Lee, B. S. Gim, G.-H. Ryu, S. J. Park, W. S. Lane, and Y.-J. Kim. 1999. Activator-specific requirement of yeast Mediator proteins for RNA polymerase II transcriptional activation. Mol. Cell. Biol. 19:979-988[Abstract/Free Full Text].
16.	Hengartner, C. J., C. M. Thompson, J. Zhang, D. M. Chao, S. M. Liao, A. J. Koleske, S. Okamura, and R. A. Young. 1995. Association of an activator with an RNA polymerase II holoenzyme. Genes Dev. 9:897-910[Abstract/Free Full Text].
17.	Henry, N. L., A. M. Campbell, W. J. Feaver, D. Poon, P. A. Weil, and R. D. Kornberg. 1994. TFIIF-TAF-RNA polymerase II connection. Genes Dev. 8:2868-2878[Abstract/Free Full Text].
18.	Ingles, C. J., M. Shales, W. D. Cress, S. J. Triezenberg, and J. Greenblatt. 1991. Reduced binding of TFIID to transcriptionally compromised mutants of VP16. Nature 351:588-590[Medline].
19.	Kaelin, W. G., Jr., W. Krek, W. R. Sellers, J. A. DeCaprio, F. Ajchenbaum, C. S. Fuchs, T. Chittenden, Y. Li, P. J. Farnham, M. A. Blanar, D. M. Livingston, and E. K. Flemington. 1992. Expression cloning of a cDNA encoding a retinoblastoma-binding protein with E2F-like properties. Cell 70:351-364[Medline].
20.	Kelleher, R. J., III, P. M. Flanagan, and R. D. Kornberg. 1990. A novel mediator between activator proteins and the RNA polymerase II transcription apparatus. Cell 61:1209-1215[Medline].
21.	Kim, Y. J., S. Bjorklund, Y. Li, M. H. Sayre, and R. D. Kornberg. 1994. A multiprotein mediator of transcriptional activation and its interaction with the C-terminal repeat domain of RNA polymerase II. Cell 77:599-608[Medline].
22.	Koh, S. S., A. Z. Ansari, M. Ptashne, and R. A. Young. 1998. An activator target in the RNA polymerase II holoenzyme. Mol. Cell 1:895-904[Medline].
23.	Lee, T. I., J. J. Wyrick, S. S. Koh, E. G. Jennings, E. L. Gadbois, and R. A. Young. 1998. Interplay of positive and negative regulators in transcription initiation by RNA polymerase II holoenzyme. Mol. Cell. Biol. 18:4455-4462[Abstract/Free Full Text].
24.	Lee, Y. C., and Y.-J. Kim. 1998. Requirement for a functional interaction between mediator components Med6 and Srb4 in RNA polymerase II transcription. Mol. Cell. Biol. 18:5364-5370[Abstract/Free Full Text].
25.	Lee, Y. C., S. Min, B. S. Gim, and Y. J. Kim. 1997. A transcriptional mediator protein that is required for activation of many RNA polymerase II promoters and is conserved from yeast to humans. Mol. Cell. Biol. 17:4622-4632[Abstract].
26.	Li, Y., S. Bjorklund, Y. W. Jiang, Y. J. Kim, W. S. Lane, D. J. Stillman, and R. D. Kornberg. 1995. Yeast global transcriptional regulators Sin4 and Rgr1 are components of mediator complex/RNA polymerase II holoenzyme. Proc. Natl. Acad. Sci. USA 92:10864-10868[Abstract/Free Full Text].
27.	Liao, S. M., J. Zhang, D. A. Jeffery, A. J. Koleske, C. M. Thompson, D. M. Chao, M. Viljoen, H. J. van Vuuren, and R. A. Young. 1995. A kinase-cyclin pair in the RNA polymerase II holoenzyme. Nature 374:193-196[Medline].
28.	Lin, Y. S., and M. R. Green. 1991. Mechanism of action of an acidic transcriptional activator in vitro. Cell 64:971-981[Medline].
29.	Moqtaderi, Z., Y. Bai, D. Poon, P. A. Weil, and K. Struhl. 1996. TBP-associated factors are not generally required for transcriptional activation in yeast. Nature 383:188-191[Medline].
30.	Myers, L. C., C. M. Gustafsson, D. A. Bushnell, M. Lui, H. Erdjument-Bromage, P. Tempst, and R. D. Kornberg. 1998. The Med proteins of yeast and their function through the RNA polymerase II carboxy-terminal domain. Genes Dev. 12:45-54[Abstract/Free Full Text].
31.	Nonet, M. L., and R. A. Young. 1989. Intragenic and extragenic suppressors of mutations in the heptapeptide repeat domain of Saccharomyces cerevisiae RNA polymerase II. Genetics 123:715-724[Abstract/Free Full Text].
32.	O'Neil, K., J. D. Shuman, C. Ampe, and W. F. DeGrado. 1991. DNA-induced increase in the alpha-helical content of C/EBP and GCN4. Biochemistry 30:9030-9034[Medline].
33.	Piruat, J. I., S. Chavez, and A. Aguilera. 1997. The yeast HRS1 gene is involved in positive and negative regulation of transcription and shows genetic characteristics similar to SIN4 and GAL11. Genetics 147:1585-1594[Abstract].
34.	Roberts, S. G., I. Ha, E. Maldonado, D. Reinberg, and M. R. Green. 1993. Interaction between an acidic activator and transcription factor TFIIB is required for transcriptional activation. Nature 363:741-744[Medline].
35.	Roeder, R. G. 1996. The role of general initiation factors in transcription by RNA polymerase II. Trends Biochem. Sci. 21:327-335[Medline].
36.	Sakurai, H., Y. Hiraoka, and T. Fukasawa. 1993. Yeast GAL11 protein is a distinctive type transcription factor that enhances basal transcription in vitro. Proc. Natl. Acad. Sci. USA 90:8382-8386[Abstract/Free Full Text].
37.	Santos-Rosa, H., B. Clever, W. D. Heyer, and A. Aguilera. 1996. The yeast HRS1 gene encodes a polyglutamine-rich nuclear protein required for spontaneous and hpr1-induced deletions between direct repeats. Genetics 142:705-716[Abstract].
38.	Shen, W. C., and M. R. Green. 1997. Yeast TAF(II)145 functions as a core promoter selectivity factor, not a general coactivator. Cell 90:615-624[Medline].
39.	Stringer, K. F., C. J. Ingles, and J. Greenblatt. 1990. Direct and selective binding of an acidic transcriptional activation domain to the TATA-box factor TFIID. Nature 345:783-786[Medline].
40.	Thompson, C. M., A. J. Koleske, D. M. Chao, and R. A. Young. 1993. A multisubunit complex associated with the RNA polymerase II CTD and TATA-binding protein in yeast. Cell 73:1361-1375[Medline].
41.	Thompson, C. M., and R. A. Young. 1995. General requirement for RNA polymerase II holoenzymes in vivo. Proc. Natl. Acad. Sci. USA 92:4587-4590[Abstract/Free Full Text].
42.	Verrijzer, C. P., and R. Tjian. 1996. TAFs mediate transcriptional activation and promoter selectivity. Trends Biochem. Sci. 21:338-342[Medline].
43.	Vinson, C. R., K. L. LaMarco, P. F. Johnson, W. H. Landschulz, and S. L. McKnight. 1988. In situ detection of sequence-specific DNA binding activity specified by a recombinant bacteriophage. Genes Dev. 2:801-806[Abstract/Free Full Text].
44.	Walker, S. S., J. C. Reese, L. M. Apone, and M. R. Green. 1996. Transcription activation in cells lacking TAF(II)s. Nature 383:185-188[Medline].
45.	Walker, S. S., W. C. Shen, J. C. Reese, L. M. Apone, and M. R. Green. 1997. Yeast TAF(II)145 required for transcription of G1/S cyclin genes and regulated by the cellular growth state. Cell 90:607-614[Medline].
46.	Wilson, C. J., D. M. Chao, A. N. Imbalzano, G. R. Schnitzler, R. E. Kingston, and R. A. Young. 1996. RNA polymerase II holoenzyme contains SWI/SNF regulators involved in chromatin remodeling. Cell 84:235-244[Medline].
47.	Xiao, H., A. Pearson, B. Coulombe, R. Truant, S. Zhang, J. L. Regier, S. J. Triezenberg, D. Reinberg, O. Flores, C. J. Ingles, and J. Greenblatt. 1994. Binding of basal transcription factor TFIIH to the acidic activation domains of VP16 and p53. Mol. Cell. Biol. 14:7013-7024[Abstract/Free Full Text].