Activation of RNA Polymerase III Transcription in Cells Transformed by Simian Virus 40

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Molecular and Cellular Biology, July 1999, p. 4927-4934, Vol. 19, No. 7
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Activation of RNA Polymerase III Transcription in Cells Transformed by Simian Virus 40

Christopher G. C. Larminie, Josephine E. Sutcliffe, Kerrie Tosh, Andrew G. Winter, Zoe A. Felton-Edkins, and Robert J. White^*

Institute of Biomedical and Life Sciences, Division of Biochemistry and Molecular Biology, University of Glasgow, Glasgow G12 8QQ, United Kingdom

Received 19 February 1999/Returned for modification 24 March 1999/Accepted 16 April 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

RNA polymerase (Pol) III transcription is abnormally active in fibroblasts that have been transformed by simian virus 40 (SV40).This report presents evidence that two separate components ofthe general Pol III transcription apparatus, TFIIIB and TFIIIC2,are deregulated following SV40 transformation. TFIIIC2 subunitsare expressed at abnormally high levels in SV40-transformed cells,an effect which is observed at both protein and mRNA levels. Inuntransformed fibroblasts, TFIIIB is subject to repression throughassociation with the retinoblastoma protein RB. The interactionbetween RB and TFIIIB is compromised following SV40 transformation.Furthermore, the large T antigen of SV40 is shown to relieve repressionby RB. The E7 oncoprotein of human papillomavirus can also activatePol III transcription, an effect that is dependent on its abilityto bind to RB. The data provide evidence that both TFIIIB andTFIIIC2 are targets for activation by DNA tumorviruses.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

A broad range of transformed cell types display abnormally elevated levels of RNA polymerase (Pol) III transcripts (reviewedin references 53 and 54). This was first discovered with murinefibroblast lines that have been transformed by simian virus 40(SV40) (5, 36, 42). When different SV40-transformed clonesare compared, those which most efficiently induce tumors in nudemice also display the highest abundance of Pol III transcripts,whereas lower levels are detected in the less tumorigenic lines(36, 60). A tight link between transformation and Pol IIIinduction is suggested by analyses of two cell lines that weretransformed with temperature-sensitive mutants of the SV40 oncoproteinlarge T antigen; these cells down-regulate Pol III products atthe nonpermissive temperature while reverting to normal morphologyand phenotype (36). Large T antigen has also been shown to activatePol III transcription in transient transfection assays (9,28).

The activity of a general Pol III factor called TFIIIC2 has been shown to be greater in the SV40-transformed cell lines SV3T3Cl38 and SV3T3 Cl49 than in the untransformed parental 3T3 lineA31 (60). TFIIIC2 is a large DNA-binding factor that is requiredfor the expression of most class III genes (reviewed in reference53). It can relieve chromatin-mediated repression of Pol IIItranscription and has been shown to display histone acetyltransferaseactivity (18). TFIIIC2 can be detected in at least two forms,distinguishable by their differential migrations in electrophoreticmobility shift assays (EMSAs) (8, 15, 17, 43, 60).Whereas the high-mobility form predominates in untransformed A31cell extracts, the SV3T3 derivatives contain a greater proportionof TFIIIC2 in the slowly migrating form (60). Chromatographicfractionation of HeLa cells has revealed that the low-mobilityform is transcriptionally active, whereas the higher-mobilityspecies can bind DNA but is unable to support transcription (15,17). Following purification, the inactive form was found tobe missing a 110-kDa subunit, which was named TFIIIC $beta$ (17, 43).The abundance of TFIIIC $beta$ in HeLa cells has been shown to increasesubstantially following serum stimulation or adenovirus infection,two conditions which activate TFIIIC2 (43). In contrast, thelevel of TFIIIC $alpha$ , which is the DNA-binding subunit of TFIIIC2,remains constant under these conditions (43).

The large T antigen of SV40 can bind and neutralize RB, the protein product of the retinoblastoma susceptibility gene (11,13, 31). Mutations in T antigen that interfere with RB bindingalso abrogate its transforming activity (11, 13, 31). Genedisruption experiments have shown that endogenous RB repressesPol III transcription approximately fivefold in murine fibroblasts(61). The increased synthesis of tRNA and 5S rRNA that is observedin RB-knockout cells correlates with the deregulation of the generalPol III factor TFIIIB (24). TFIIIB is required for the expressionof all class III genes; it is recruited via TFIIIC2 and then servesto position the polymerase over the initiation site (reviewedin reference 53). TFIIIB activity has been shown to be inhibitedspecifically by recombinant RB in vitro (7, 24). Furthermore,immunoprecipitation, cofractionation, and pull-down experimentshave demonstrated that TFIIIB interacts with both endogenous andrecombinant RB (7, 24). The ability of large T antigen toneutralize RB therefore raises the possibility that TFIIIB isreleased from repression following SV40 transformation. We presentevidence that this is the case. We also demonstrate that SV40-transformedCl38 and Cl49 cells express much higher levels of TFIIIC $alpha$ andTFIIIC $beta$ than the untransformed parental A31 line. The data suggestthat at least two components of the general Pol III transcriptionapparatus become activated following transformation bySV40.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Tissue culture. SV3T3 Cl38 and Cl49 cell lines were generated by infection of BALB/c 3T3 A31 cells with SV40 (wt830 strain) and selected byfocus formation in low serum (35). All cell lines were grownin Dulbecco's modified Eagle's medium (Gibco) supplemented with10% fetal calf serum, 100 U of penicillin per ml, and 100 µg ofstreptomycin per ml and were harvested whensubconfluent.

Antibodies and Western blotting. Antibodies used were C-15 (Santa Cruz Biotechnology) and G99-549 (PharMingen) against RB, M-19 (Santa Cruz) against TAF_I48,330 and 128 against BRF (1, 4), SL30 against TATA-bindingprotein (TBP) (27), clone 46 (Transduction Laboratories) againstTFIIIC $beta$ , and Ab4 against TFIIIC $alpha$ (38). Western immunoblot analysiswas performed as previously described (56).

Reverse transcription-PCR (RT-PCR) analysis. RNA was extracted from subconfluent A31, Cl38, and Cl49 cells by using TRI reagent (Sigma) according to the manufacturer'sspecifications. Reverse transcription reactions were performedfor 1 h at 42°C, using 3 µg of RNA, 200 ng of random hexamers(Promega), and 400 U of Superscript II reverse transcriptase (LifeTechnologies) in a total volume of 40 µl of 1× First Strand Buffer(Life Technologies) containing 10 mM dithiothreitol (DTT) and0.5 mM each deoxynucleosidetriphosphate.

PCRs were carried out in a PTC-100 programmable thermal controller (MJ Research Inc.); 2 µl of cDNA was amplified with 20pmol of either glyceraldehyde-3-phosphate dehydrogenase (GAPDH)primers (5'-TCCACCACCCTGTTGCTGTA-3' and 5'-ACCACAGTCCATGCCATCAC-3')to give a 452-bp product, TFIIIC $beta$ primers (5'-CCAGAAGGGGTCTCAAAAGTCC-3'and 5'-CTTTCTTCAGAGATGTCAAAGG-3') to give a 303-bp product, TFIIIC $alpha$ primers (5'-TCCAGCGAGACCTTCACACC-3' and 5'-GGATTGAGTGTTGCTGGGCT-3')to give a 144-bp product, or BRF primers (5'-AAATTCTGTGAGCCTCTTCCGTAGTG-3'and 5'-AGACCCATGCTTGTACATTCCACG-3') to give a 260-bp product.Amplification reaction mixtures contained 0.5 U of Taq DNA polymerase(Promega) in a total volume of 20 µl of 1× Taq DNA polymerasebuffer (Promega) containing 1.5 mM MgCl₂ and 0.2 mM each deoxynucleosidetriphosphate. PCR was performed under the following cycling parameters:for GAPDH, (i) 94°C for 3 min, (ii) 18 cycles of 95°C for 30 s,66°C for 40 s, and 72°C for 1 min, (iii) 72°C for 5 min; for TFIIIC $beta$ ,(i) 94°C for 3 min, (ii) 6 cycles of 95°C for 1 min, 66°C for40 s, and 72°C for 40 s, (iii) 22 cycles of 95°C for 1 min, 62°Cfor 40 s, and 72°C for 40 s, (iv) 72°C 5 min; for TFIIIC $alpha$ , (i)95°C for 3 min, (ii) 30 cycles of 94°C for 20 s, 62°C for 30 s,and 72°C for 30 s, (iii) 72°C 10 min; for BRF, 95°C for 2 min,26 cycles of 95°C for 1 min, 60°C for 30 s, and 72°C for 1 min,(iv) 72°C 5 min. Reaction products were resolved on a 2% agarosegel and visualized by ethidium bromide staining. Gels were scanned,and the intensity of each band was quantitated by using a UVPimage analysis system and Adobe Photoshop 4.0software.

Plasmids. pVAI contains the adenovirus VA_I gene (10). pCAT (Promega) contains the chloramphenicol acetyltransferase (CAT) gene drivenby the SV40 promoter and enhancer. Expression constructs encodingthe E7 oncoprotein of human papillomavirus type 16 (HPV-16) andits mutant derivatives $Delta$ 21-35, PRO2, and GLY24 have been describedelsewhere (21).

Transfection assays. Cell lines were transiently transfected by the calcium phosphate precipitation method. DNA precipitates were left on the platesovernight, and then the cells were washed with phosphate-bufferedsaline and cultured for 24 h before harvesting. Total RNA wasextracted by using TRI reagent (Sigma) according to the manufacturer'sinstructions and then analyzed by primer extension using bothVA_I-specific (5'-CACGCGGGCGGTAACCGCATG-3') and CAT-specific (5'-CGATGCCATTGGGATATATCA-3')labeled primers. Primer extension reactions were conducted aspreviously described (61).

Transcription. Pol III transcription was carried out as described previously (59) except that pBR322 was not included and the incubationswere for 60 min at 30°C.

Preparation of extracts and protein fractions. Whole-cell extracts were prepared from exponentially growing cells by the method of Manley et al. (29). Nuclear extractswere purchased from the Computer Cell Culture Center (Mons, Belgium).PC-B is the 0.1 to 0.35 M KCl step fraction from a phosphocellulosecolumn and contains both TFIIIB and Pol III (37). PC-C is the0.35 to 0.6 M KCl step fraction from a phosphocellulose columnand contains both TFIIIC and Pol III (37). PC-D is the 0.6 to1.0 M KCl step fraction from a phosphocellulose column and containsTFIID (37). The CHep-1.0 fraction was generated as describedpreviously (56) by loading PC-C onto heparin-Sepharose CL-6Bin BC buffer (25 mM Tris-HCl [pH 7.9], 10% glycerol, 10 mM $beta$ -mercaptoethanol)plus 100 mM KCl (BC-100). The column was washed with BC-280 andeluted with BC-1000 to produce the CHep-1.0 fraction containingTFIIIC. The A25(0.15) fraction containing TFIIIB was generatedas described previously (56) by applying PC-B to an A25 DEAE-Sephadexcolumn in buffer A (20 mM HEPES-KOH [pH 7.9], 20% glycerol, 5mM MgCl₂, 3 mM DTT, 0.2 mM phenylmethylsulfonyl fluoride) plus50 mM (NH₄)₂SO₄. After extensive washing with this buffer, theA25(0.15) fraction containing TFIIIB was eluted in buffer A plus150 mM (NH₄)₂SO₄. Mono Q gradient-purified TFIIIB was preparedas described previously (27).

Recombinant glutathione S-transferase (GST) and GST-RB fusion proteins were expressed in bacteria and purified on glutathione-agaroseas previously described (24). GST-RB contains residues 379 to928 of RB. Immunoaffinity-purified recombinant SV40 large T antigenwas a generous gift from DavidLane.

Immunoprecipitation. Whole-cell extract (150 µg) was incubated at 4°C on an orbital shaker with 20 µl of protein A-Sepharose beads carrying equivalentamounts of prebound immunoglobulin G. Samples were then pelleted,supernatants were removed, and the beads were washed five timeswith 150 µl of LDB buffer (20 mM HEPES-KOH [pH 7.9], 17% glycerol,100 mM KCl, 12 mM MgCl₂, 0.1 mM EDTA, 2 mM DTT). The bound materialwas analyzed by Western blotting. In the experiments shown inFig. 5, reticulocyte lysate (15 µl) containing BRF translatedin the presence of [³⁵S]Met and [³⁵S]Cys was mixed with nuclear extract (150 µg) during immunoprecipitation.In this case, the precipitated material was analyzed by autoradiographyrather than Westernblotting.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

TFIIIC2 subunits are more abundant in SV3T3 Cl38 and Cl49 cell extracts than in parental 3T3 A31 cell extracts. Previous studies have shown that the SV40-transformed cell lines Cl38 and Cl49 express high levels of Pol III transcriptsrelative to the untransformed parental line A31 (36, 60).Nuclear run-on assays demonstrated that this up-regulation occursat the transcriptional level (60). EMSA analysis revealed thatthe DNA-binding activity of TFIIIC2 is significantly higher inCl38 and Cl49 cell extracts than in extracts of the A31 cells(60). This is a specific effect, since Sp1 activity is not elevatedin the transformed cell lines (60). In addition, the Cl38 andCl49 extracts were found to contain a greater proportion of TFIIIC2in the slowly migrating transcriptionally active form (60).It was proposed that these changes might account for the abnormallyhigh rates of Pol III transcription that are observed in theseSV3T3 cell lines (60).

Since the time of this previous analysis, the two forms of TFIIIC2 have been purified to homogeneity and shown to differ inthe presence of a 110-kDa subunit that is found only in the activeform and is referred to as TFIIIC $beta$ (17, 43). The availabilityof antibodies that recognize TFIIIC $beta$ (43) and the ~240-kDa DNA-bindingsubunit TFIIIC $alpha$ (20, 26) has provided the opportunity to investigatefurther the changes in TFIIIC2 that accompany SV40 transformation.We therefore carried out Western blot analyses to compare thelevels of these subunits in A31, Cl38, and Cl49 cell extracts.The level of TFIIIC $alpha$ was found to be higher in Cl38 and Cl49 cellextracts than in A31 cell extracts (Fig. 1A), consistent withthe increased DNA-binding activity detected by EMSA followingSV40 transformation (60). A striking change was also detectedwith the TFIIIC $beta$ subunit, which is substantially more abundantin the Cl38 and Cl49 cell extracts than in A31 cell extracts (Fig.1B). This increase in TFIIIC $beta$ may account for the higher proportionof TFIIIC2 that is found in the transcriptionally active formfollowing SV40 transformation (60).

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FIG. 1. The SV40-transformed cell lines Cl38 and Cl49 express elevated levels of TFIIIC2 subunits. (A) Whole-cell extracts (57 µg of protein) prepared from Cl38 (lane 1), A31 (lanes 2 and 4), and Cl49 (lane 3) cells were resolved on an SDS-7.8% polyacrylamide gel and then analyzed by Western immunoblotting with anti-TFIIIC $alpha$ antibody Ab4. Lanes 2 and 4 show extracts prepared from two separate batches of A31 cells. (B) CHep-1.0 fraction (15 µg of protein) containing TFIIIC2 (lane 1) and whole-cell extracts (38 µg of protein) prepared from HeLa (lane 2), Cl38 (lane 3), A31 (lane 4), and Cl49 (lane 5) cells were resolved on an SDS-7.8% polyacrylamide gel and then analyzed by Western immunoblotting with anti-TFIIIC $beta$ monoclonal antibody clone 46. (C) Whole-cell extracts (50 µg of protein) prepared from A31 (lane 1) and Cl38 (lane 2) cells, CHep-1.0 (12 µg of protein) TFIIIC2 fraction (lane 3), and A25(0.15) (1.6 µg of protein) TFIIIB fraction (lane 4) were resolved on an SDS-7.8% polyacrylamide gel and then analyzed by Western immunoblotting with anti-BRF antibody 330. (D) Whole-cell extracts (50 µg of protein) prepared from Cl38 (lane 1), A31 (lane 2), and Cl49 (lane 4) cells and PC-D (5.6 µg of protein) TFIID fraction (lane 3) were resolved on an SDS-7.8% polyacrylamide gel and then analyzed by Western immunoblotting with anti-TBP antibody SL30.

To investigate the specificity of these effects, we also examined the abundance of two subunits of TFIIIB. Human TFIIIB hasbeen shown to contain TBP and an associated polypeptide of ~90kDa called TFIIIB90 or human BRF (27, 30, 40, 45, 51,57). Neither of these subunits was found to be significantlymore abundant in Cl38 cell extracts than in A31 cell extracts(Fig. 1C and D). We conclude that the up-regulation of TFIIIC $alpha$ and TFIIIC $beta$ in the SV40-transformed cells is a specificphenomenon.

SV40-transformed Cl38 and Cl49 cells express elevated levels of mRNA encoding TFIIIC $alpha$ and TFIIIC $beta$ . To determine the level at which TFIIIC $alpha$ and TFIIIC $beta$ become up-regulated, we carried out semiquantitative RT-PCR analyses oftheir mRNAs. The transcript encoding TFIIIC $beta$ was found to be significantlymore abundant in Cl38 and Cl49 cells than in A31 cells (Fig. 2A,top). Again, this is a specific phenomenon, since the mRNA encodingGAPDH is expressed at similar levels in these three cell lines(Fig. 2A, bottom). The TFIIIC $alpha$ transcript is also more abundantin Cl38 and Cl49 cells than in A31 cells (Fig. 2B, top). However,the mRNA for BRF shows little or no increase following SV40 transformation(Fig. 2B, bottom), consistent with the Western blotting data.After normalization to the level of GAPDH mRNA, the levels ofthe BRF transcript in Cl38 and Cl49 cells were 90 and 114%, respectively,of that seen in A31 cells. In contrast, expression of TFIIIC $alpha$ transcript was elevated four- to fivefold, whereas that of TFIIIC $beta$ was elevated seven- to eightfold in Cl38 and Cl49 cells, relativeto the parental A31 cells. The observed specific increases inthe mRNAs encoding TFIIIC $alpha$ and TFIIIC $beta$ may therefore account forthe elevated abundance of these subunits in the SV40-transformedcell lines.

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FIG. 2. The SV40-transformed cell lines Cl38 and Cl49 express elevated levels of transcripts encoding TFIIIC $alpha$ and TFIIIC $beta$ . (A) cDNAs generated by reverse transcription of 3 µg of RNA from A31 (lane 1), Cl38 (lane 2), and Cl49 (lane 3) cells were PCR amplified by using TFIIIC $beta$ (top) and GAPDH (bottom) primers. Amplification products were resolved on a 2% agarose gel. (B) cDNAs generated by reverse transcription of 3 µg of RNA from A31 (lane 1), Cl38 (lane 2), and Cl49 (lane 3) cells were PCR amplified by using TFIIIC $alpha$ (top) and BRF (bottom) primers. Amplification products were resolved on a 2% agarose gel.

SV40 large T antigen can activate Pol III transcription by overcoming the repressive effects of RB. The transforming protein of SV40 is its large T antigen, and this has been shown to be sufficient to stimulate Pol III transcriptionin transient transfection assays (9, 28). The ability ofT antigen to transform cells is dependent on its capacity to bindand inactivate RB (11, 13, 31). Since RB is a potent repressorof Pol III transcription in murine fibroblasts (61), we investigatedwhether T antigen can release Pol III from repression by RB (Fig.3). When recombinant T antigen was added to reactions that hadbeen reconstituted with partially purified factors, it causedno increase in the level of VA_I transcription by Pol III (lanes1 to 3). However, a different response was obtained after a recombinantGST-RB fusion protein had been added to depress transcription.In the presence of this added RB, titration of T antigen resultedin a significant stimulation of VA_I expression (lanes 4 to 6).The fact that T antigen increases Pol III transcription in thepresence of excess RB but not in its absence suggests that itsstimulatory effect in this system results from its ability toneutralize RB.

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FIG. 3. SV40 large T antigen can counteract the repressive effect of RB on Pol III transcription. Template pVAI (250 ng of DNA) was transcribed by using 2 µl of Mono Q-purified TFIIIB and 2 µl of CHep-1.0 fraction in the presence of 100 ng of either GST (lanes 1 to 3) or GST-RB (lanes 4 to 6) and 20 ng (lanes 2 and 5) or 40 ng (lanes 3 and 6) of immunoaffinity-purified recombinant large T antigen (TAg).

TFIIIB activity is abnormally elevated in the SV40-transformed cell lines Cl38 and Cl49. Previous studies have shown that the general Pol III factor TFIIIB is a target for repression by RB (7, 24). Since theT antigen present in SV40-transformed cells might be expectedto counteract the effects of RB, we investigated whether thisresults in an increase in TFIIIB activity. Extracts of 3T3 A31cells and SV3T3 Cl38 cells were subjected to chromatography onphosphocellulose. Equivalent TFIIIB fractions were then comparedfor their abilities to reconstitute transcription when mixed witha fraction containing TFIIIC and Pol III from HeLa cells (Fig.4A). No transcription was observed with this system in the absenceof added TFIIIB (lane 2). However, a robust transcription signalwas obtained following the addition of TFIIIB fractions derivedfrom HeLa or Cl38 cells (lanes 1 and 3, respectively). In contrast,an equal amount of the equivalent TFIIIB fraction derived from3T3 A31 cells gave much lower levels of Pol III transcription(lane 4).

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FIG. 4. Cl38 and Cl49 cell extracts contain higher TFIIIB activity than A31 cell extracts. (A) Template pVAI (250 ng of DNA) was transcribed by using 2 µl of HeLa-derived PC-C fraction and buffer alone (lane 2) or PC-B fraction (6.4 µg of protein) derived from HeLa (lane 1), Cl38 (lane 3), or A31 (lane 4) cell extracts. (B) Template pVA1 (500 ng DNA) was transcribed by using 4 µl of HeLa-derived PC-C fraction supplemented with 10 ng of recombinant TBP and 6 µl of heat-treated Mono Q-purified TFIIIB (lane 1), buffer alone (lanes 2 and 6), or 7.5 µg of heat-treated extract from Cl38 (lane 3), A31 (lane 4), or Cl49 (lane 5) cells.

The reduced activity of A31 cell-derived TFIIIB fractions could conceivably result from differential recovery or inactivationduring chromatography. We therefore also conducted complementationassays to measure TFIIIB activity in unfractionated extracts.These assays make use of the differential sensitivity of Pol IIItranscription factors to inactivation by mild heat treatment.When an extract is heated at 47°C for 15 min, TFIIIC and TBP becomeinactivated whereas the other components of the Pol III machineryare not compromised (17, 41, 57, 58). The activity ofTFIIIB in an unfractionated extract can therefore be assayed byheat treating the extract and then measuring its ability to reconstitutetranscription when added to a complementing fraction containingTFIIIC, TBP, and Pol III (1, 24, 55, 56). Using suchassays, we found that A31 cell extracts contain significantlyless TFIIIB activity than extracts of Cl38 or Cl49 cells (Fig.4B). We conclude that SV40 transformation of A31 cells is accompaniedby an increase in TFIIIB activity, even though the levels of TBPand BRF do notincrease.

The interaction between RB and TFIIIB is compromised following SV40 transformation. Previous genetic analyses have shown that TFIIIB is subject to repression by RB in murine fibroblasts (24). Coimmunoprecipitationexperiments were therefore carried out to test whether the physicalinteraction between RB and TFIIIB is diminished following SV40transformation. The BRF subunit of the TFIIIB complex was synthesizedby using a reticulocyte lysate in the presence of [³⁵S]cysteine and [³⁵S]methionine. The radiolabeled protein was then incubated withwhole-cell extracts under conditions which allow complex assembly(4). The mixtures were subjected to immunoprecipitation usinga monoclonal antibody that is specific for RB, and the precipitateswere analyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis(SDS-PAGE) and autoradiography (Fig. 5A). Significant amountsof radiolabeled BRF were coprecipitated with RB from an A31 cellextract (lane 5). This was not due to cross-reaction with theantibody, since only background levels of BRF were detected whenbuffer was used in place of the whole-cell extract (lane 2). Similarbackground levels were also obtained using extracts of SAOS2 osteosarcomacells (lane 3), which express an inactive truncated mutant formof RB (39). Furthermore, very little BRF was coimmunoprecipitatedwith RB when it was mixed with an extract of SV3T3 Cl38 cells(lane 4), despite the fact that Cl38 cells contain full-lengthRB that is no less abundant than the RB present in A31 cells (25).A similar analysis using a different RB antibody revealed thatthe interaction between BRF and RB is also compromised in SV3T3Cl49 cell extracts (Fig. 5B). Identical results were obtainedin assays using a third antibody against a different region ofRB (44). In contrast, irrelevant control antibodies failed tocoprecipitate BRF (44).

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FIG. 5. The BRF subunit of TFIIIB coimmunoprecipitates with endogenous RB present in A31 extracts, but this interaction is compromised in extracts of Cl38 and Cl49 cells. (A) Reticulocyte lysate (15 µl) containing in vitro-translated BRF was immunoprecipitated (IP) with anti-RB antibody G3-245 in the presence of buffer alone (lane 2) or 150 µg of whole-cell extract prepared from SAOS2 (lane 3), Cl38 (lane 4), or A31 (lane 5) cells. Proteins retained after extensive washing were resolved on an SDS-7.8% polyacrylamide gel and then visualized by autoradiography. Lane 1 shows 10% of the input reticulocyte lysate containing in vitro-translated BRF. (B) Reticulocyte lysate (15 µl) containing in vitro-translated BRF was immunoprecipitated with anti-RB antibody C-15 in the presence of buffer alone (lane 1) or 150 µg of whole-cell extract prepared from A31 (lane 2) or Cl49 (lane 3) cells. Proteins retained after extensive washing were resolved on an SDS-7.8% polyacrylamide gel and then visualized by autoradiography.

The previous experiments suggest that the BRF subunit of TFIIIB is much less able to associate with cellular RB followingSV40 transformation. As these results were obtained in studiesusing exogenous radiolabeled BRF, we also carried out coimmunoprecipitationanalyses to compare the extent to which endogenous TFIIIB is boundby RB in 3T3 and SV3T3 cells. Extracts of A31 and Cl38 cells wereimmunoprecipitated with either an anti-RB antibody or an irrelevantcontrol antibody against the TAF_I48 subunit of the Pol I factorSL1. Immunoprecipitated material was then resolved by SDS-PAGEand probed for the presence of BRF by Western blotting (Fig. 6A).Substantial amounts of endogenous BRF were found to coprecipitatewith RB from A31 cell extracts, an effect that was specific sincenone was detected in the control immunoprecipitates. In contrast,significantly less BRF was coprecipitated with RB from the Cl38cell extracts. Similarly, anti-RB immunoprecipitates from Cl49cell extracts contained much less BRF than those obtained in parallelfrom A31 cell extracts (Fig. 6B). These results reinforce thedata obtained in assays using radiolabeled BRF and indicate thatthe interaction between endogenous RB and TFIIIB is diminishedfollowing SV40 transformation.

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FIG. 6. The association between endogenous RB and endogenous TFIIIB is greater in A31 cells than in Cl38 and Cl49 cells. (A) Cl38 (lanes 1 and 2) and A31 (lanes 3 and 4) cell extracts (150 µg of protein) were immunoprecipitated (IP) with anti-TAF_I48 antibody M-19 (lanes 1 and 3) or anti-RB antibody C-15 (lanes 2 and 4). Precipitated material was resolved on an SDS-7.8% polyacrylamide gel and then analyzed by Western blotting with anti-BRF antiserum 128. (B) Cl49 (lanes 1 and 2) and A31 (lanes 3 and 4) cell extracts (150 µg of protein) were immunoprecipitated with anti-TAF_I48 antibody M-19 (lanes 1 and 3) or anti-RB antibody C-15 (lanes 2 and 4). Precipitated material was resolved on an SDS-7.8% polyacrylamide gel and then analyzed by Western blotting with anti-BRF antiserum 128.

The E7 oncoprotein of HPV-16 can also activate Pol III transcription. The data described above suggest that T antigen can activate TFIIIB by releasing it from the repressive influence of RB. TheRB-binding site within T antigen has been mapped to an LXCXE motif,where X can be any amino acid (11, 64, 65). HPV-16 encodesan oncoprotein called E7 that has also been shown to bind andneutralize RB by means of an LXCXE motif (12, 32, 48). Wetherefore tested whether E7 resembles T antigen in being ableto activate Pol IIItranscription.

The untransformed murine fibroblast cell line NIH 3T3 was transfected with expression vectors encoding either wild-type E7or several mutant forms of E7 (Fig. 7). Primer extension analysiswas used to determine the levels of Pol III transcription of acotransfected VA_I gene; a cotransfected control plasmid, in whichthe CAT gene is driven by the SV40 early promoter, was used tonormalize for transfection efficiency. Specific VA_I expressionwas stimulated substantially by the wild-type E7 protein (lane2) relative to empty vector (lane 1). The ability of E7 to activateVA_I transcription was severely compromised by deletion of residues21 to 35, which removes the LXCXE motif that is located betweenamino acids 22 and 26 (lane 4). Indeed, substitution of the C24residue to glycine is sufficient to abrogate the ability of E7to stimulate VA_I expression (lane 5). In contrast, mutant PRO2,which carries a proline substitution in its second residue andhas an intact LXCXE motif, remains fully capable of activatingPol III transcription (lane 3). The PRO2 mutant is significant,because it has lost the ability to transform although it can stillbind and neutralize RB (21). The fact that the PRO2 mutant canactivate VA_I expression indicates that the effect of E7 on PolIII transcription is not an indirect consequence of cell transformation.These E7 proteins are all expressed at comparable levels in NIH3T3 cells (21). We conclude that E7 can activate Pol III transcriptionin vivo in a manner that is dependent on its RB-binding LXCXEmotif.

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FIG. 7. Transfected HPV E7 activates Pol III transcription in vivo in a manner that is dependent on its RB-binding domain. NIH 3T3 cells were transfected with pVAI (2 µg), pCAT (2 µg), and 6 µg of empty vector (lane 1) or vector encoding wild-type E7 (E7 WT; lane 2), PRO2 mutant E7 (lane 3), $Delta$ 21-35 mutant E7 (lane 4), or GLY24 mutant E7 (lane 5). (A) VA_I primer extension products. (B) VA_I transcription levels that have been normalized to the levels of CAT expression to correct for transfection efficiency and are expressed relative to the value obtained for the empty vector control (designated 1.0).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Abnormally high levels of Pol III transcripts are observed in SV40-transformed cells (5, 36, 42, 60). The presentstudy has provided evidence that more than one mechanism contributesto this effect and that two distinct Pol III factors, TFIIIB andTFIIIC2, are both targeted for activation bySV40.

The deregulation of TFIIIC2 in SV3T3 cells was first detected by EMSA, which revealed an overall increase in DNA-binding activityand a greater proportion of the transcriptionally active form(60). These observations can be explained by our new data whichshow that SV40 transformation is accompanied by an increase inthe abundance of both TFIIIC $alpha$ and TFIIIC $beta$ , two of the principalcomponents of the TFIIIC2 complex. Cross-linking has demonstratedthat the TFIIIC $alpha$ subunit is responsible for contacting promoterDNA (3, 17, 63). In contrast, the presence of TFIIIC $beta$ isnot required for DNA binding but is necessary for transcriptionalactivity (17, 43). Both the $alpha$ and $beta$ subunits have been reportedto display histone acetyltransferase activity (18). TFIIIC2also contains three other subunits (17, 63), but the cloningof cDNAs encoding these subunits has not yet been reported andtheir roles have yet to be established. In the absence of molecularreagents that recognize the uncharacterized components of TFIIIC2,we cannot determine whether these are also up-regulated in SV3T3cells. However, it seems probable that they would be, in orderto allow an overall increase in the level of functional TFIIIC2.Our RT-PCR analyses have demonstrated that the transcripts encodingTFIIIC $alpha$ and TFIIIC $beta$ are more abundant in Cl38 and Cl49 cells thanthey are in the parental A31 cells. This is likely to account,at least in part, for the elevated levels of the TFIIIC $alpha$ and TFIIIC $beta$ polypeptides.

SV40 transformation of A31 cells also results in the activation of TFIIIB. In contrast to TFIIIC2, this does not appear toresult from an increase in the abundance of TFIIIB subunits. Thus,Western blotting reveals little or no change in the levels ofTBP and BRF when A31 extracts are compared with Cl38 and Cl49extracts. Human TFIIIB is incompletely characterized at presentbut is believed to contain at least one additional subunit besidesTBP and BRF (27, 30, 46, 47). We cannot exclude the possibilitythat the abundance of one or more uncharacterized component(s)of the complex becomes elevated in response to SV40 transformation.However, it is not necessary to invoke such a contingency in orderto explain the observed activation of TFIIIB. Both biochemicaland genetic data have shown that TFIIIB is subject to negativeregulation in untransformed murine fibroblasts through a physicalinteraction with RB (24, 61). Coimmunoprecipitation analysesreveal that much less of the TFIIIB in SV3T3 cells is associatedwith RB (Fig. 5 and 6). The higher specific activity of TFIIIBthat is observed in Cl38 and Cl49 cells (Fig. 4) is thereforelikely due, at least in part, to a partial release from repressionby RB. This interpretation is supported strongly by the fact thatrecombinant SV40 T antigen can stimulate Pol III transcriptionin a partially purified system in an RB-dependent fashion (Fig.3). These data are consistent with a model in which T antigencounteracts the inhibitory influence of RB onTFIIIB.

This study has described two distinct mechanisms which allow SV40-transformed cells to maintain abnormally high levels ofPol III transcription, namely, the increased abundance of TFIIIC2and the release of TFIIIB from repression by RB. Given the complexityof gene regulation by SV40, it is entirely possible that additionallevels of control are also involved. For example, T antigen hasbeen shown to bind and neutralize the tumor suppressor p53, andthis capability is important for the transformation of some celltypes (22, 48, 65). Among its many functions, p53 has beenfound to interact with TFIIIB and repress Pol III transcription(4, 6). Inactivation of p53 might therefore provide an additionalmechanism whereby T antigen is able to deregulate TFIIIB. However,this may not have a major effect in the 3T3 system investigatedhere, since p53 levels are extremely low in unstressed A31 cells(25).

Damania et al. have reported recently that T antigen can be found in a complex with TFIIIB, a conclusion based on both cofractionationand coimmunoprecipitation experiments with extracts prepared fromHeLa cells that had been infected with a recombinant adenoviruswhich overexpresses SV40 large T antigen (9). The authors suggestedthat binding to TFIIIB may allow T antigen to activate Pol IIItranscription directly, although no evidence was presented toestablish this model (9). Our experiments with partially purifiedfactors are not consistent with a direct effect on TFIIIB, sinceT antigen was found to activate Pol III transcription only inthe presence of added RB (Fig. 3). It is possible that T antigenacts directly on TFIIIB under different experimental conditions.However, we have been unable to detect T antigen associated withTFIIIB in extracts of SV3T3 cells. Thus, T antigen is not detectedin anti-BRF immunoprecipitates, nor is BRF detected in anti-Timmunoprecipitates from Cl38 or Cl49 cells, even though both celllines express high levels of T antigen (44). We can thereforefind no evidence that T antigen acts directly on TFIIIB in theSV3T3 cellsystem.

The up-regulation of both TFIIIB and TFIIIC2 is likely to ensure that SV40-transformed cells maintain high rates of Pol IIItranscription. At present it is not clear which target is of greaterimportance in determining the overall level of class III geneexpression. Add-back experiments carried out previously with crudefractions have suggested that TFIIIC activity is limiting in extractsprepared from A31, Cl38, and Cl49 cells (60). If TFIIIC is alsolimiting for Pol III transcription in vivo, then the up-regulationof this factor may make the principal contribution to the activationobserved in SV3T3 cells. However, much of the complexity of thesituation is likely to be concealed when asynchronous cell populationsare analyzed. Thus, experiments with synchronized HeLa populationshave revealed that alternative Pol III factors can be limitingduring different phases of the cell cycle (55). Whereas TFIIICactivity limits the rate of VA_I expression in extracts of S- orG₂-phase HeLa cells, TFIIIB is the limiting factor in extractsof cells that were harvested during early G₁ phase (55). Underthese circumstances, stimulation of TFIIIB or TFIIIC alone mightinfluence the transcriptional output only during a restrictedinterval of the cell cycle. If a similar situation pertains in3T3 cells, then the activation of both TFIIIB and TFIIIC mightallow SV40 to sustain elevated rates of Pol III transcriptionthroughoutinterphase.

Like SV40, adenovirus appears able to use more than one mechanism to stimulate the production of Pol III products. Adenovirusinfection results in a marked increase in TFIIIC2 activity (15,16, 43, 62). Western blotting revealed that the infectedcells express elevated levels of TFIIIC $beta$ , although TFIIIC $alpha$ wasnot induced under these circumstances (43). Induction of TFIIIC $beta$ requires the adenoviral transforming protein E1A (43). In additionto its effect on TFIIIC $beta$ , E1A has also been shown to relieve PolIII transcription from repression by RB, both in vitro and invivo (61). Adenovirus therefore resembles SV40 in employingat least two distinct mechanisms to activate the Pol III machinery.The present study has provided evidence to suggest that a thirdDNA tumor virus, HPV, can also stimulate Pol III transcriptionby overcoming the repressive influence of RB. We have shown thatthe E7 oncoprotein of HPV activates VA_I expression in transfectedfibroblasts (Fig. 7). This capacity is abolished by mutationsthat specifically prevent E7 from binding and neutralizing RB.Previous work has shown that hepatitis B virus and human T-cellleukemia virus type 1 can also stimulate Pol III transcriptionby activating TFIIIB (2, 14, 19, 34, 49, 50). Ittherefore seems that TFIIIB is a frequent target for transformingviruses (reviewed in reference 54). High rates of Pol III transcriptionare a prerequisite of rapid growth, in order to sustain the productionof tRNA and 5S rRNA. It has therefore been suggested that repressionof the Pol III system may provide a mechanism for restrainingcell growth (23, 33, 52). The fact that this system is targetedby two unrelated tumor suppressors, RB and p53, provides strongsupport for this contention. Additional support is provided bythe range of oncogenic viruses that have evolved mechanisms tostimulate Pol IIItranscription.

	ACKNOWLEDGMENTS

We are extremely grateful to K. Vousden and R. Watson for the E7 expression vectors, D. Lane for recombinant T antigen, N.Hernandez for antibody SL30, and Y. Shen and A. Berk for antibodiesAb2 andAb4.

This work was funded by grant SP2314/0101 to R.J.W. from the Cancer Research Campaign and grant 98-46 to R.J.W. from the Associationfor International Cancer Research. J.E.S. and Z.A.F-E. are supportedby postgraduate studentships from the Biotechnology and BiologicalSciences Research Council and the Medical Research Council, respectively.R.J.W. is a Jenner Research Fellow of the Lister Institute ofPreventiveMedicine.

	FOOTNOTES

^* Corresponding author. Mailing address: Institute of Biomedical and Life Sciences, Division of Biochemistry and Molecular Biology,Davidson Building, University of Glasgow, Glasgow G12 8QQ, UnitedKingdom. Phone: 0141-330-4628. Fax: 0141-330-4620. E-mail: rwhite{at}udcf.gla.ac.uk.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Alzuherri, H. M., and R. J. White. 1998. Regulation of a TATA-binding protein-associated factor during cellular differentiation. J. Biol. Chem. 273:17166-17171[Abstract/Free Full Text].
2.	Aufiero, B., and R. J. Schneider. 1990. The hepatitis B virus X-gene product trans-activates both RNA polymerase II and III promoters. EMBO J. 9:497-504[Medline].
3.	Boulanger, P. A., S. K. Yoshinaga, and A. J. Berk. 1987. DNA-binding properties and characterization of human transcription factor TFIIIC2. J. Biol. Chem. 262:15098-15105[Abstract/Free Full Text].
4.	Cairns, C. A., and R. J. White. 1998. p53 is a general repressor of RNA polymerase III transcription. EMBO J. 17:3112-3123[Medline].
5.	Carey, M. F., K. Singh, M. Botchan, and N. R. Cozzarelli. 1986. Induction of specific transcription by RNA polymerase III in transformed cells. Mol. Cell. Biol. 6:3068-3076[Abstract/Free Full Text].
6.	Chesnokov, I., W.-M. Chu, M. R. Botchan, and C. W. Schmid. 1996. p53 inhibits RNA polymerase III-directed transcription in a promoter-dependent manner. Mol. Cell. Biol. 16:7084-7088[Abstract].
7.	Chu, W.-M., Z. Wang, R. G. Roeder, and C. W. Schmid. 1997. RNA polymerase III transcription repressed by Rb through its interactions with TFIIIB and TFIIIC2. J. Biol. Chem. 272:14755-14761[Abstract/Free Full Text].
8.	Clark, M. E., and A. Dasgupta. 1990. A transcriptionally active form of TFIIIC is modified in poliovirus-infected HeLa cells. Mol. Cell. Biol. 10:5106-5113[Abstract/Free Full Text].
9.	Damania, B., R. Mital, and J. C. Alwine. 1998. Simian virus 40 large T antigen interacts with human TFIIB-related factor and small nuclear RNA-activating protein complex for transcriptional activation of TATA-containing polymerase III promoters. Mol. Cell. Biol. 18:1331-1338[Abstract/Free Full Text].
10.	Dean, N., and A. J. Berk. 1988. Ordering promoter binding of class III transcription factors TFIIIC1 and TFIIIC2. Mol. Cell. Biol. 8:3017-3025[Abstract/Free Full Text].
11.	DeCaprio, J. A., J. W. Ludlow, J. Figge, J.-Y. Shew, C.-M. Huang, W.-H. Lee, E. Marsilio, E. Paucha, and D. M. Livingston. 1988. SV40 large tumour antigen forms a specific complex with the product of the retinoblastoma susceptibility gene. Cell 54:275-283[Medline].
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