Transcription Factor YY1 Represses Cell-Free Replication from Human Papillomavirus Origins

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J Virol, June 1998, p. 4911-4917, Vol. 72, No. 6
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Transcription Factor YY1 Represses Cell-Free Replication from Human Papillomavirus Origins

Kyung-Yeol Lee, Thomas R. Broker, and Louise T. Chow^*

Department of Biochemistry and Molecular Genetics, University of Alabama at Birmingham, Birmingham, Alabama 35294

Received 29 August 1997/Accepted 5 March 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

We have established cell-free replication for the human papillomavirus type 18 (HPV-18) origin of replication (ori)-containingDNA by using purified HPV-18 E1 and E2 gene products expressedas fusion proteins in Escherichia coli. The transcription factorYY1 has been shown to regulate RNA transcription by binding toa sequence overlapping the putative E1 protein binding site inthe HPV-18 ori. We show that exogenously added YY1 fusion proteininhibited HPV-18 ori replication. Cotransfection of YY1 expressionvectors also inhibited transient replication in 293 cells. However,inhibition did not appear to be mediated by binding to its cognatesite in the ori as YY1 also inhibited the replication of the HPV-11ori, which does not have a known or suspected YY1 binding site.Moreover, inhibition was not alleviated by the inclusion of YY1binding oligonucleotides in the replication reaction mixtures.Rather, we demonstrated a direct interaction between purifiedfusion E2 protein and fusion YY1 protein by the pull-down assayand a partial restoration of replication activity by an elevatedE2 protein concentration. These results suggest that YY1 can inhibitHPV ori replication by interfering with E2 protein functions.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

The small double-stranded DNA tumor viruses simian virus 40 (SV40), polyomavirus, and papillomaviruses are model systems forstudying eukaryotic DNA replication because they rely heavilyon host proteins. Many cellular replication proteins have beenidentified and cloned based on cell-free replication initiatedby the SV40 large T antigen (reviewed in reference 53). Humanpapillomaviruses (HPVs) are widespread pathogens that infect variousepithelia, causing warts (reviewed in reference 65). Infectionsby high-risk HPVs, including HPV type 18 (HPV-18), can developinto dysplasias and cancers in which the viral DNA often becomesintegrated into the host chromosomes, an event proposed to playan important role in disease progression (reviewed in reference10). In productively infected benign lesions, two distinct modesof DNA replication make this virus family attractive as a possibleparadigm for regulated host DNA replication. In these lesions,HPV DNA is maintained as low-copy-number, extrachromosomal plasmidsin the basal and parabasal cells of the squamous epithelium. Onlyin the differentiated upper strata does vegetative amplificationtake place. Viral transcription also increases dramatically withcellular differentiation. These two aspects of the infection processare undoubtedly interconnected but are not yet fully understood.

Because cloned genomic HPV DNA replicates poorly, if at all, in transfected cells, two strategies have been used to examinethe requirements for viral origin (ori)-specific replication (reviewedin references 9 and 52). One involves transient replicationof ori-containing plasmids in transfected cells in the presenceof vectors expressing viral replication proteins. E1 and E2 proteinsfrom the same viral type and certain mixed pairs from distincttypes can support replication from homologous and heterologouspapillomavirus ori's with varied efficiencies (8, 12, 18,55, 56, 59, 64). The second assay is cell-free replication,which has been established for HPV-11 and bovine papillomavirustype 1 (BPV-1), using cellular extracts supplemented with viralproteins purified from insect Sf9 cells infected with recombinantbaculoviruses (23, 61). These studies show that both the viralproteins and their ori's are highly conserved among HPVs and animalpapillomaviruses. Efficient ori replication requires both E1 andE2 proteins, with few exceptions (3, 18).

The functions of the papillomavirus replication proteins have been examined extensively. Briefly, the HPV-11 and the BPV-1E1 protein binds to an imperfect palindrome (the E1 binding site[E1BS]), which is flanked by E2BSs (Fig. 1) (30, 47, 54,60, 61). The E1 protein is an ATPase and helicase (5, 20,31, 49, 62) and also binds to the 180-kDa catalytic subunit(4, 41) and p70 subunit (11) of the host DNA polymerase $alpha$ . In cell-free replication, HPV-11 and BPV-1 E1 are requiredthroughout initiation and elongation, as expected of a helicaseat the replication fork (30). The E1 proteins also exhibit relativelyhigh nonspecific DNA binding, which undoubtedly contributes totheir ability to promote a low level of E2-independent as wellas ori-independent replication when present at elevated concentrationsin cell-free systems (23, 61, 62). The functions of theE2 proteins are severalfold. All E2 proteins are dimeric transcriptionfactors and bind to a consensus sequence ACCN₆GGT that existsin multiple copies in the upstream regulatory region (URR) ofall papillomaviruses (9, 52). The binding of E1 protein tothe E1BS is stabilized by interaction with the E2 proteins boundto nearby sites (17, 33, 36, 47, 48, 54). At low E1concentrations in the cell-free system, the assembly of initiationcomplex on the ori requires both E1 and E2 proteins (30). Theseinteractions provide specificity and increase the efficiency forori replication (7, 23, 36, 46). However, the E2 proteinappears to be dispensable for elongation (30).

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FIG. 1. Replication origins of HPV-18 and HPV-11. Indicated are the binding sites for viral proteins E1 and E2 and for cellular transcription factors, YY1, Sp1, and TBP. The YY1BS in HPV-18 ori overlaps the putative E1BS (1, 25).

As expected from the properties of the E1 and E2 proteins, the papillomavirus ori regions are highly conserved and consistof several copies of the E2BS and one proven or putative E1BS,overlapping the transcription enhancers and E6 promoter. One ormore copies of the E2BS are critical to ori activity of genitalHPVs, such as HPV-11 and HPV-18, whereas deletion or mutationof E1BS reduces but does not abolish the activity (7, 23,31, 32, 43, 56). An efficient HPV-18 ori has been localizedby transient-replication assays to a 210-bp fragment spanningnucleotides (nt) 7766 to 7857 and 1 to 119 (43, 55, 56).It contains three copies of the E2BS and one putative E1BS asinferred by analogy to the HPV-11 and BPV-1 E1 protein bindingsequences (Fig. 1).

In the ori of SV40 or polyomavirus, the ori core binds the viral T antigen. In addition, transcription factor binding sitesflanking the core are auxiliary elements that enhance ori activities.Enhancement of replication in vivo is attributed to the abilityof bound transcription factors to prevent nucleosome formationaround the ori (reviewed in reference 13). The BPV-1 E2 proteinalso functions in this capacity (29). In the short HPV-18 ori,there are several host transcription factor binding sites, includingthose for yin-yang 1 (YY1), which overlaps the EIBS, for Sp1,and for TATA-box binding protein (TBP) (Fig. 1). The Sp1 and TBPsites are positive transcriptional elements (see references 1,14, 15, 42, and 57 and references therein), and mutationsin these sites have a negative effect on transient replication(25, 45). YY1 protein interacts with diverse proteins, includingTBP, transcription factor IIB, Sp1, c-Myc, and adenovirus E1Aproteins (for a review, see reference 51). In some instances,YY1 and other transcription factors compete for binding to adjacentor overlapping sites. Thus, depending on the sequence context,YY1 either functions as a transcription repressor, an activator,or an initiator binding protein. It is of great interest to determinewhether or how YY1 protein might regulate ori replication.

In this report, we describe our findings concerning the effect of YY1 in a cell-free replication system established with human293 cell extracts supplemented with HPV-18 E1 and E2 proteins,each expressed as a fusion protein in Escherichia coli. In thissystem, efficient HPV-18 ori replication is dependent on bothE1 and E2 proteins. We found that YY1 inhibited HPV-18 ori replicationin cell-free and in transient replication. Unexpectedly, evidencesuggests that inhibition is largely mediated via interferencewith the E2 protein functions and it does not appear to dependon binding to the ori. We show that YY1 protein interacts withE2 protein in vitro and inhibition can be relieved partially byelevated E2 protein concentrations or by an antibody to an intactYY1 protein.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Plasmid construction. The genomic HPV-18 clone was a gift of Harald zur Hausen. Prior to purifying E1 and E2 proteins from E. coli, we expressedboth as native proteins from the eukaryotic vector pMTX, a derivativeof pMT2 (22) with multiple-cloning sites (a gift from Jen-SingLiu of our laboratory), and established their functionality bytransient assays in human 293 cells as previously described (8).To generate pMTX-18E1, the TaqI-StuI fragment of HPV-18 (nt 838to 3070) was blunt ended with the Klenow fragment of the E. coliDNA polymerase I and inserted into the SmaI site of pMTX. To generatepMTX-18E2, the NsiI fragment (nt 2707 to 3975) was cloned intothe PstI site of pMTX. For expression in E. coli, the open readingframes (ORFs) were reconstituted from restriction fragments ofcloned DNA and amino terminal fragments of the E1 and E2 ORFsgenerated by PCR amplification. The E1 ORF was fused in frameat the carboxyl terminus of the hexahistidine encoded by the vectorpRSET (Invitrogen, Carlsbad, Calif.). A BamHI site (underlined)was introduced into the sense-strand primer 5'-TAAGGATCCATGGCTGATCCAG-3',while the antisense-strand primer 5'-AATGATAGCCCATATGTGTC-3' containsa native NdeI site (underlined). The BamHI-NdeI fragment of thePCR product (nt 905 to 1585) was ligated to the restriction fragmentNdeI (in the E1 ORF)-EcoRI (in pMTX) (nt 1586 to 2885) and thencloned into the BamHI and EcoRI sites of pRSET to generate pRSET-H18E1.HPV-18 E2 was fused in frame at the carboxyl terminus of the glutathioneS-transferase (GST) in pGEX2TM, a derivative of pGEX2T (Pharmacia,Uppsala, Sweden) with additional cloning sites (a gift from JeffreyKudlow) as follows. The sense-strand primer, 5'-AGAGGCATATGCAGACACCG-3',contains an introduced NdeI site, while the antisense-strand primer,5'-TTTGTGCAAGGCCTTGTAGG-3', contains a native StuI site (underlined).The NdeI-StuI fragment of the PCR product (nt 2817 to 3070) spanningthe amino terminus was ligated to the StuI-NdeI fragment (nt 3070to 3920) and then inserted into the NdeI site of pRSET to yieldpRSET-18E2. The NdeI fragment spanning the intact E2 ORF was thenblunt ended and cloned into the SmaI site of pGEX2TM.

To prepare pBS-H18ori (nt 7766 to 7857 and 1 to 118), the BamHI fragment (nt 6929 to 118) of HPV-18 in pGEM-18URR (6) wascloned into pBluescript (Stratagene, La Jolla, Calif.). The fragmentbetween the AccI site (in the vector) and the AvaI site (in HPV-18URR) was then removed, and the vector was reclosed by blunt-endreligation. The HPV-11 ori-containing plasmid pUC7874-99 has beendescribed previously (23). The YY1 expression vector pCDNA-YY1was constructed by insertion of an XbaI-BamHI fragment of theYY1 cDNA plasmid (44) into an XbaI-BamHI site of the expressionvector pCDNA (Invitrogen). Additional YY1 expression vectors,pCMV-hYY1 and pCMV-hYY1DZnF, were kindly provided by K. Calame(44).

Antibodies and oligonucleotides. Polyclonal rabbit anti-YY1 antibodies were purchased from Santa Cruz Biotechnology (Santa Cruz, Calif.). C20 was raised againstthe C-terminal 20 residues, while H414 was raised against full-lengthYY1 protein. Oligonucleotides containing a strong YY1 bindingsite or a mutated YY1 binding site were also from Santa Cruz Biotechnology.

Transient replication assays. Transient replication of HPV-18 ori plasmid (pBS-H18ori containing nt 7766 to 7857 and 1 to 118) in transfected 293 cellswas conducted as described previously (8). Briefly, 5 millioncells were transfected by electroporation (capacitance, 960 µF;potential difference, 170 V) in 250 µl of growth medium with 5mM BES buffer (N,N-bis[2-hydroxyethyl]-2-aminoethane-sulfonicacid, pH 7.2) containing the ori plasmids, E1 and E2 expressionvectors, and carrier salmon sperm DNA. The HPV proteins were expressedfrom pMTX-18E1 and pMTX-18E2. For some experiments YY1 expressionvectors such as pCDNA-YY1, pCMV-hYY1, pCMV-hYY1DZnF, or the cloningvector pCDNA were also included.

Expression and purification of proteins from E. coli. To express the HPV-18 E1 protein, E. coli BL21(DE3) was transformed by pRSET-H18E1. The induction protocol and purificationthrough a nickel-nitrilotriacetic acid column (Qiagen, Santa Clarita,Calif.) and a heparin column (Bio-Rad, Hercules, Calif.) willbe described elsewhere (27). The fraction containing the E1protein was identified by Western blotting with antibody againstthe hexahistidine-containing epitope. The E1 protein was dialyzedagainst buffer D (20 mM HEPES-KOH [pH 7.5], 1 mM dithiothreitol,10% glycerol) and stored in aliquots at $-$ 80°C. To express HPV-18E2 protein, DH5 $alpha$ cells freshly transformed by the pGEX2TM-18E2plasmid were induced at mid-log phase by 0.5 mM of isopropylthio- $beta$ -galactoside(IPTG) for 20 h at 18°C. The bacteria were resuspended in bufferA (25 mM Tris [pH 7.5], 2 mM EDTA, 2 mM dithiothreitol), 10% glycerol,and 0.5 mM phenylmethylsulfonyl fluoride with 0.5 M NaCl and lysozyme(1 mg/ml). The lysates were sonicated and cleared of insolublematerials successively by centrifugation and ultrafiltration througha 0.45-µm-pore-size polysulfone filter. The filtrate was loadedonto a 0.5-ml GST column (Pharmacia) and washed with buffer Acontaining 0.8 M NaCl. The GST-E2 fusion protein was eluted with0.5 ml of buffer A containing 0.3 M NaCl and 20 mM glutathione.The eluent was dialyzed against buffer D and stored in aliquotsat $-$ 80°C.

The expression vectors for His-YY1 and GST-YY1 were gifts of Edward Seto and Yang Shi (26, 50). They were expressed inE. coli RR1 and DH5 $alpha$ , respectively, as soluble proteins by inductionat 18°C with 0.5 mM IPTG. Both proteins were purified by chelationon a nickel-nitrilotriacetic acid column, as the YY1 protein naturallycontains a polyhistidine domain. The fusion proteins were dialyzedand stored as described above. For the heat stability test, analiquot of His-YY1 protein solution was overlaid with mineraloil and heated to 100°C for 10 min. The solution was then quicklycooled on ice. A polyhistidine-tagged chloramphenicol acetyltransferase(CAT) (pTrcHisCAT; Invitrogen) was purified similarly.

The purity and identity of the proteins were determined by Coomassie blue staining following sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) and by Western blotting with antibodiesdirected against fusion tags of E1 or E2 proteins or with theanti-YY1 antibody (H414). The two YY1 proteins and the His-CATprotein were each more than 95% pure. The concentrations of proteinswere determined by Bradford assay (Bio-Rad) and Coomassie bluestaining following SDS-PAGE using known concentrations of bovineserum albumin as standards.

Cell-free DNA replication assays. The cultures of human 293 cells in monolayer or in suspension, the preparation of whole-cell extracts, and the implementationof cell-free replication assays were as described previously (23).Briefly, the reaction mixture of 25 µl containing 40 ng of freshlyprepared form I DNA template, 100 µg of cell extracts, viral proteinsas specified for each experiment, an ATP-regenerating system,and eight unlabeled nucleotide substrates in reaction buffer waspreincubated for 1 h at 37°C. [ $alpha$ -³²P]dCTP (2.5 µCi; 3,000 Ci/mmol) was then added, and incubationcontinued for another hour at 37°C. As described previously (23),little or no replicative synthesis occurred in the first hourof incubation. Delayed addition of the labeled substrate reducedbackground repair synthesis which was independent of viral proteinsand ori and approached a plateau during the 1-h preincubation(23; data not shown). In some assays, additional componentswere added prior to preincubation as described for each experiment.Reactions were terminated, and the products were analyzed by electrophoresisthrough 0.8% agarose gels as described previously (23). Autoradiogramswere exposed for 3 to 4 h with an intensifying screen at $-$ 80°C.The relative intensities of replication products (the sum of signalsfrom replication intermediates plus form I and form II DNA) werequantified by PhosphorImager (Molecular Dynamics, Sunnyvale, Calif.)after subtracting background obtained in the absence of E1 orE2 proteins, in the presence of the pBS cloning vector, or asdescribed in the figure legends.

GST pull-down assays. GST pull-down assays were performed as described previously (21, 24, 58). Aliquots (30 µg) of His-YY1 proteins weremixed with a constant amount of Sepharose-GST preloaded with increasingamounts of GST-H18 E2 protein or control Sepharose-GST. Afterextensive washing with a solution containing 20 mM Tris-HCl (pH8.0), 1 mM EDTA, 0.1 M NaCl, 0.5% Nonidet P-40, and 0.5% nonfatdry milk, the bound protein was recovered by centrifugation andsolubilized by boiling in loading buffer. Twenty percent of thesolubilized protein was separated by SDS-10% acrylamide gel electrophoresisand then detected after Western blotting by using an ECL kit (Amersham,Arlington Heights, Ill.) with anti-YY1 antibody (C20).

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Bacterially expressed HPV-18 E1 and E2 fusion proteins support HPV-18 ori replication. The HPV-18 E1 and E2 genes were individually cloned into a derivative of the mammalian expression vector described in Materialsand Methods. After confirming their ability to support transientreplication of an HPV-18 ori plasmid (pBS-H18ori containing nt7766 to 7857 and 1 to 118) in transfected 293 cells, we expressedand purified E1 and E2 proteins from E. coli. E1 was generatedas a fusion protein with a short polypeptide containing six histidineresidues at the amino terminus. E2 protein was translated as afusion protein with GST at the amino terminus. On the basis ofCoomassie blue staining, the purity of E1 protein was over 70%(Fig. 2A) and that of E2 was over 90% (Fig. 2B).

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FIG. 2. SDS-PAGE profiles of proteins expressed in and purified from E. coli. Lanes: A, purified His-H18E1; B, GST-H18E2; C, His-YY1; and D, GST-YY1. Proteins were purified as described in Materials and Methods, electrophoresed in SDS-polyacrylamide gels, and stained with Coomassie brilliant blue. Western blots using antibodies against the fusion tag (E1 and E2) or YY1 confirmed the identities (data not shown).

After preliminary tests that demonstrated the abilities of the E1 and E2 proteins to support cell-free replication of pBS-H18oriin the presence of 293 cell extracts, we optimized this systemby reiterated titration of E1 and E2 proteins needed to promoteori-specific replication in the presence of 40 ng of pBS-H18oriand 100 µg of cell extracts. Representative titration experimentsare shown in Fig. 3A. The optimal conditions included 180 ng ofHis-H18E1 protein and 14 ng of GST-H18E2 protein (Fig. 3A, lane16). Under these conditions, replication is ori dependent andproduced fast-migrating form I and form II and slow-migratingreplication intermediates as previously described (23, 61).In the absence of E1 or E2 or in the presence of the vector pBSplasmid only repair synthesis was detected, which generated onlylabeled form I DNA in the absence of any slow-migrating replicationintermediates (23). This background signal was less than 4.5%of that generated by pBS-H18ori, as quantified by a PhosphorImager(Fig. 3B).

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FIG. 3. HPV-18 ori replication in the presence of E1 and E2 fusion proteins. In this and subsequent figures, cell-free replication was conducted with 100 µg of 293 cell extracts and 0 or 40 ng of template DNA (pBS-H18ori or pBS). (A) Effects of E1 and E2 protein concentrations on HPV-18 ori replication. Cell-free replication reaction mixtures containing 40 ng of pBSH18ori (all lanes) were conducted in the absence of His-H18E1 and GST-H18E2 (lane 1), in the presence of GST-H18E2 alone (lanes 2 to 4), in the presence of His-H18E1 alone (lanes 5 to 8), or in the presence of both His-H18E1 and GST-H18E2 (lanes 9 to 20). The amount of E1 fusion protein in the reaction mixtures was 22.5 ng (lanes 5, 9, 13, and 17), 45 ng (lanes 6, 10, 14, and 18), 90 ng (lanes 7, 11, 15, and 19), or 180 ng (lanes 8, 12, 16, and 20). The amount of GST-H18E2 protein was 7 ng (lanes 2 and 9 to 12), 14 ng (lanes 3 and 13 to 16), or 28 ng (lanes 4 and 17 to 20). (B) Specificity of cell-free HPV-18 ori replication under optimal conditions as defined for panel A. Replication was conducted in the presence (+) or absence ( $-$ ) of 180 ng of His-H18E1 and 14 ng of GST-H18E2 as indicated (lanes 2 to 6). form I (I), form II (II), and replication intermediates (R) are marked here and in Fig. 4 through 7. Incorporation in the absence of E1, E2, or both was due to repair synthesis, as evidenced by the lack of slow-migrating replication intermediates. The relative [ $alpha$ -³²P]dCTP incorporation of each reaction was quantified by using a PhosphorImager. The relative intensity (Rel I) was calculated by comparing isotope incorporation to that in lane 1 (with no exogenous DNA template).

YY1 fusion proteins inhibit HPV-18 E2-dependent cell-free ori replication. To examine whether YY1 might regulate HPV-18 ori replication, we purified both His-YY1 and GST-YY1 to near homogeneity (Fig.2C and D). The purified His-YY1 protein was able to form specificand stable complexes with the ori fragment but not with a neighboringfragment in an electrophoretic mobility shift assay (27). Whenadded to the cell-free replication reactions, both YY1 fusionproteins independently repressed the HPV-18 ori replication ina dose-dependent manner (Fig. 4A and data not shown). At 0.2 and0.4 µg of His-YY1, ori replication was reduced to 29 and 21% ofthe control (compare lanes 1, 4, and 5). To eliminate the possibilitythat repression was due to contaminating proteins in the YY1 proteinpreparations, we performed the following control experiments.Repression was not observed after the addition of the same amountsof His-tagged CAT, which was purified similarly (lanes 2 and 3).The addition of anti-YY1 antibody partially restored ori activity(lane 7), whereas addition of anti-YY1 antibody to a reactioncontaining no added YY1 protein had a small positive effect onreplication (lane 6). Since YY1 protein is heat resistant (63),we boiled His-YY1 protein for 10 min prior to addition to thereplication mixture. It retained the repression activity (seeFig. 6B; compare lanes 2 to 6). These results and additional experimentsdescribed below strongly argue for a YY1-specific repression andagainst a nonspecific repression by contaminants.

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FIG. 4. Specificity of repression of HPV-18 ori replication by exogenous YY1 protein. (A) Lane 1 contains a standard reaction mixture; the rest of the lanes contain the standard reaction mixture with the following additions: His-CAT protein (lanes 2 and 3), His-YY1 protein (lanes 4 and 5), anti-YY1 antibody (H414) raised against the intact YY1 protein (lane 6), and both YY1 and the H414 anti-YY1 antibody (lane 7). (B) Replication of pBSH18ori in 293 cell extracts supplemented with His-H18E1 alone (lane 1), GST-H18E2 alone (lane 2), or with both E1 and E2 proteins (lanes 4 to 6). To lane 5 was added exogenous his-YY1. Lane 6 contains both His-YY1 and antibody (C20) raised against the DNA-binding domain of the YY1 protein. Lane 3 contains the product of a replication reaction conducted with pBS cloning vector in 293 cells supplemented with both E1 and E2 proteins. The relative intensity (Rel I) values were calculated as percentages by comparing isotope incorporation to that in lane 1 (A) or lane 4 (B) as measured by a PhosphorImager. For both panels, the amounts (in µg) of protein or antibody added were as indicated.

YY1 inhibition of HPV ori replication is independent of a YY1 binding site in ori. Because the YY1 site extensively overlaps the putative E1 binding site, it would be difficult to mutate the YY1 site withoutaffecting E1 binding to ori and, hence, ori replication (25).To examine whether YY1 inhibition is mediated by binding to thecognate site, we used two alternative approaches. First, a syntheticdouble-stranded oligonucleotide containing a known strong YY1binding site (YY1BS), GCCATCTTG, from the promoter in mouse ribosomalprotein rPL30 and rPL32 genes (19) or a mutated oligonucleotide,mYY1BS, ATTATCTTG, which no longer bound YY1 was added to thecell-free replication reaction in the presence or in the absenceof exogenous YY1 protein (Fig. 5A). The addition of mYY1BS hadno effect on replication (compare lanes 4 and 9) or on repression(compare lanes 5 and 7), but to our surprise the YY1BS oligonucleotidesdid not affect replication (lane 8) or repression (lane 6), contraryto what one might expect if YY1 had repressed replication viabinding to ori. The second approach is to test the effect of YY1on HPV-11 ori replication by using the same HPV-18 E1 and E2 proteins.HPV-11 ori (Fig. 1) does not contain a known or suspected YY1site, based on the consensus sequence of GACATNTT and VDCCATNWY(63). Replication repression was similarly observed (Fig. 5B).These results suggest that YY1 inhibition was mediated eitherthrough a cellular or a viral protein and that binding to oridid not significantly contribute to this repression.

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FIG. 5. YY1 inhibition of HPV ori replication is largely independent of binding to the ori. (A) Lack of discernible effects by the inclusion of YY1BS oligonucleotides in HPV-18 ori replication reaction mixtures containing exogenous YY1 protein. All the reactions were conducted under the optimal conditions described in the legend to Fig. 3B to replicate 40 ng of HPV-18 ori plasmid, which contains a YY1BS overlapping the E1BS, or HPV-11 ori plasmid, which does not have a known or suspected YY1BS (shown in panel B), except control reactions with a backbone plasmid (both panels, lanes 3). A double-stranded oligonucleotide containing YY1BS or mYY1BS was included in the cell-free replication reaction mixtures in the presence (+) or absence ( $-$ ) of exogenous YY1. Proteins (180 ng of E1, 14 ng of E2, and 0.2 µg of YY1) or oligonucleotides (20 ng) were included as indicated. (B) All reactions were conducted under the optimal conditions described in the legend to Fig. 3B. The amounts of His-tagged YY1 added to the reactions were 0.2 µg (lane 5) and 2 µg (lane 6).

Partial relief of YY1 repression of HPV-18 ori replication by an elevated level of HPV-18 E2 protein. Because YY1 interacts with a number of transcription factors, we examined the possibility that it also interacts with theE2 protein and that this interaction is part of the basis forrepression. We conducted a pull-down assay using purified GST-H18E2bound to GST-Sepharose. GST-H18E2 interacted with His-YY1 in thepresence or in the absence of ethidium bromide (30 µg/ml) (24),as demonstrated by a Western blot of bound protein (Fig. 6A, lanes2 and 3). Under the same condition, GST itself did not bind His-YY1protein (lane 1). These results suggest that replication repressionshould be at least partially relieved by increasing amounts ofE2 protein. We tested this prediction (Fig. 6B). In the absenceof YY1, the presence of 140 ng (a 10-fold excess) of E2 had littleeffect on ori replication relative to that in the standard reactionmixture, which contained 14 ng of E2 protein (compare lanes 2and 7). In comparison, addition of 140 ng of E2 protein to reactionmixtures containing 0.2 µg of His-YY1 protein restored activityfrom 25 to 70% (compare lanes 3 and 8). These results are consistentwith an interpretation that YY1 repression is at least partlycaused by interference with the HPV-18 E2 protein function.

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FIG. 6. Mechanism of YY1 repression of HPV ori replication. (A) Interaction of YY1 protein with GST-H18E2 protein. A Western blot following SDS-10% PAGE was used to reveal His-YY1 retained on glutathione-beads loaded with increasing amounts of GST-H18E2 fusion protein but not on beads loaded with GST alone. Purified His-YY1 (3 µg, one half of input amount) was loaded in lane 4. A similar result was obtained when the binding assay was performed in the presence of ethidium bromide (30 µg/ml), which eliminates potential nonspecific binding caused by interactions with DNA (24). (B) Partial restoration of HPV-18 ori replication in the presence of exogenous YY1 by elevated E2 protein. Replication reactions of pBS-H18ori was conducted in the absence of the viral replication proteins (lane 1) or in the presence of 180 ng of His-H18E1 plus 14 ng of GST-H18E2 (lanes 2 to 6) or plus 140 ng of E2 (lanes 7 and 8). His-YY1 (lanes 3 and 4) or His-YY1, which was boiled for 10 min under mineral oil (lanes 5 and 6), was added as indicated (in micrograms). The relative intensity (Rel I) values were calculated in percentages by comparing isotope incorporation to that in lane 2, after subtracting the background incorporation in lane 1, as measured by a PhosphorImager.

YY1 expression vectors inhibit transient replication of HPV-18 ori. We note that the addition of anti-YY1 antibody to a reaction mixture containing no added YY1 protein slightly, but consistently,stimulated cell-free replication (Fig. 4A; compare lanes 6 and1). This observation might be an indication that the endogenousYY1 has an inhibitory effect. To substantiate this hypothesis,we performed transient-replication assays in 293 cells after cotransfectionof an expression vector of YY1. The results are reproducible andare presented in Fig. 7. Upon cotransfection of the empty cloningvector pCDNA, there was a slight stimulation of ori replication,whereas when pCDNA-YY1 was cotransfected, there was a dose-dependentrepression (Fig. 7A). Furthermore, repression persisted when theYY1 lacking the DNA binding domain was cotransfected (Fig. 7B).Thus, in vivo, high levels of YY1 can also inhibit replicationand the ability of YY1 to bind to ori is not essential. Consistentwith the latter result and interpretation, we also observed thatonly the polyclonal antibody raised against the intact YY1, butnot another polyclonal antibody raised against the DNA bindingdomain (Fig. 4B), can partially restore the replication activity.

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FIG. 7. Cotransfection of YY1 expression vectors represses HPV-18 ori replication in transient replication. (A) Repression of HPV-18 ori replication by YY1 in transfected 293 cells. Increasing amounts of pCDNA (lanes 3 to 5) or pCDNA-hYY1 (lanes 6 to 8) were cotransfected into 293 cells with expression vectors of viral E1 and E2 proteins (pMTX-H18E1 and pMTXH18E2), and the origin-containing vector (pBS-H18ori). Replicated DNA was revealed by Southern blotting after digestion with DpnI and BamHI as described in Materials and Methods. Cotransfection with pBS without viral ori (lane 1) was used as a negative control for transient replication assays. Lane M, 200 pg of linearized pBS-H18ori. (B) Repression of HPV-18 ori replication by YY1 mutated in the DNA-binding domain. An expression vector of the full-length YY1 protein (pCMV-hYY1) or of a truncated YY1 lacking the zinc finger DNA-binding domain (pCMV-hYY1DZnF) was cotransfected into 293 cells. The intensity of replication in each transfection containing YY1 expression vectors was compared to that of a control transfection. Data were collected from three independent experiments. Open bars indicate averages, and error bars indicate standard deviations.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Replication-competent epitope-tagged BPV-1 and HPV-11 E1 proteins have been expressed previously in insect Sf9 cells froma recombinant baculovirus system (23, 61). In addition, afterenzymatic cleavage to remove the GST amino-terminal tag, bacteriallyexpressed BPV-1 E1 protein supported ori replication in the presenceof native E2 protein purified from Sf9 cells or from E. coli (35,37). This report demonstrates that bacterially expressed HPVE1 and E2 fusion proteins function in cell-free replication assayswithout first removing the fusion protein moiety (Fig. 3). Thereplication properties of the bacterially expressed HPV-18 fusionproteins are similar to those of HPV-11 and BPV-1 expressed inSf9 cells. Efficient ori replication depends on both E1 and E2proteins.

YY1 protein binds to many transcription factors and displays diverse functions in regulating transcription (51). Transcriptionfactors that function as auxiliary replication factors in vivonormally do not affect ori replication in cell-free systems dueto a paucity of histones. In contrast, the addition of YY1 significantlyinhibited HPV-18 ori replication, a novel observation in the controlof ori replication (Fig. 4). Repression is specific, as it washeat resistant (Fig. 6), a property of YY1, and was partiallyrelieved by a polyclonal antibody against the intact YY1 protein(Fig. 4A). Unexpectedly, despite the overlapping nature of theYY1BS and putative E1BS, our data strongly suggest that bindingto the YY1 site is not the primary cause for the repression basedon several pieces of evidence. (i) First, the inclusion of anoligonucleotide containing a known strong YY1BS or mutated oligonucleotidesdid not restore ori replication in the presence of exogenous YY1protein (Fig. 5A). (ii) YY1 also inhibited HPV-11 ori replicationwhich is not known to have a YY1BS (Fig. 5B). (iii) The additionof an antibody raised against the DNA-binding domain of YY1 failedto restore activity (Fig. 4B). Rather, our data showed that interactionwith E2 protein was at least largely responsible for the ori repression.We demonstrated that E2 interacted with YY1 in a pull-down assayand repression was partially alleviated by E2 protein at 10-foldexcess concentrations (Fig. 6). Since E2 plays important rolesduring the assembly of the initiation complex (30) by interactingwith both the E1 protein and host proteins, such as RP-A (28),we suggest that the E2-YY1 interaction might adversely affectthese E2 protein functions. That YY1 is indeed capable of inhibitingHPV ori replication in vivo by mechanisms independent of bindingto the ori is substantiated by transient replication assays incells transfected with an expression vector of either the intactYY1 or a YY1 mutant with the DNA binding zinc finger domain truncated(Fig. 7).

YY1 is thought to be a ubiquitous protein (16, 19, 40, 50). Although the distribution of YY1 in differentiating epitheliumhas not been determined, the existence of multiple YY1BSs in HPV-8,HPV-16, and HPV-18 (34, 38, 39) regulatory regions suggestthat this factor may play some role in modulating viral activities.Indeed, in epithelial cell lines, YY1 negatively regulates theURR promoter of HPV-16. It has been postulated that deletion orother mutations of YY1 sites in the HPV-16 URR observed in severalcases of carcinomas might have contributed to the enhanced expressionof viral oncogenes, leading to the development of the carcinomas.In HPV-18, YY1 switched from being a transcription repressor toan activator when the transcription factor CREB was bound to aswitch site (1, 2). E2 protein also regulates the viralenhancer-promoter, either positively or negatively in epithelialcells and cell lines, depending on the amounts of E2 protein andinteractions with host factors bound to the URR (see references14, 15, and 57 and references therein). The E2-YY1 interactionand YY1 repression of the HPV-18 ori described in this reportadd another level of intricate cross-talk between the viral andthe host proteins in the regulation of viral transcription andreplication during epithelial cell growth and differentiation.

In conclusion, we describe the establishment of a cell-free replication system for the HPV-18 ori by using HPV-18 E1 and E2fusion proteins purified from E. coli and report the novel E2-mediatedrepression of HPV-18 ori replication by YY1. The functionalityof bacterially expressed fusion viral proteins should facilitatefuture studies of the mechanisms and regulation of papillomavirusDNA replication and should also be useful for drug discovery assays.

	ACKNOWLEDGMENTS

This work is supported by USPHS grant CA36200. We thank Jen-Sing Liu and Shu-Ru Kuo for many helpful discussions, Harald zurHausen for HPV-18 DNA, Edward Seto and Yang Shi for the YY1 expressionvectors, Kathryn Calame for pCMV-hYY1 and pCMV-hYY1DZnF, and JeffreyKudlow for vector pGEX2TM.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biochemistry and Molecular Genetics, University of Alabama at Birmingham,1918 University Blvd., Birmingham, AL 35294-0005. Phone: (205)975-8300. Fax: (205) 975-6075. E-mail: LTChow{at}uab.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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1.	Bauknecht, T., F. Jundt, I. Herr, T. Oehler, H. Delius, Y. Shi, P. Angel, and H. zur Hausen. 1995. A switch region determines the cell type-specific positive or negative action of YY1 on the activity of the human papillomavirus type 18 promoter. J. Virol. 69:1-12[Abstract].
2.	Bauknecht, T., R. H. See, and Y. Shi. 1996. A novel C/EBP $beta$ -YY1 complex controls the cell-type-specific activity of the human papillomavirus type 18 upstream regulatory region. J. Virol. 70:7695-7705[Abstract].
3.	Bonne-Andrea, C., S. Santucci, and P. Clertant. 1995. Bovine papillomavirus E1 protein can, by itself, efficiently drive multiple rounds of DNA synthesis in vitro. J. Virol. 69:3201-3205[Abstract].
4.	Bonne-Andrea, C., S. Santucci, P. Clertant, and F. Tillier. 1995. Bovine papillomavirus E1 protein binds specifically DNA polymerase $alpha$ but not replication protein A. J. Virol. 69:2341-2350[Abstract].
5.	Bream, G. L., C. A. Ohmstede, and W. C. Phelps. 1993. Characterization of human papillomavirus type 11 E1 and E2 proteins expressed in insect cells. J. Virol. 67:2655-2663[Abstract/Free Full Text].
6.	Cheng, S., D.-C. Schmidt-Grimminger, T. Murant, T. R. Broker, and L. T. Chow. 1995. Differentiation-dependent up-regulation of the human papillomavirus E7 gene reactivates cellular DNA replication in suprabasal differentiated keratinocytes. Genes Dev. 9:2335-2349[Abstract/Free Full Text].
7.	Chiang, C.-M., G. Dong, T. R. Broker, and L. T. Chow. 1992. Control of human papillomavirus type 11 origin of replication by the E2 family of transcription regulatory proteins. J. Virol. 66:5224-5231[Abstract/Free Full Text].
8.	Chiang, C. M., M. Ustav, A. Stenlund, T. F. Ho, T. R. Broker, and L. T. Chow. 1992. Viral E1 and E2 proteins support replication of homologous and heterologous papillomaviral origins. Proc. Natl. Acad. Sci. USA 89:5799-5803[Abstract/Free Full Text].
9.	Chow, L. T., and T. R. Broker. 1994. Papillomavirus DNA replication. Intervirology 37:150-158[Medline].
10.	Chow, L. T., and T. R. Broker. 1997. Small DNA tumor viruses, p. 267-302. In N. Nathanson (ed.), Viral pathogenesis. Lippincott-Raven, Philadelphia, Pa.
11.	Conger, K. L., J.-S. Liu, S.-R. Kuo, L. T. Chow, and T. S.-F. Wang. Submitted for publication.
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