DNA Replication of Human Papillomavirus Type 31 Is Modulated by Elements of the Upstream Regulatory Region That Lie 5' of the Minimal Origin

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Journal of Virology, March 1999, p. 1835-1845, Vol. 73, No. 3
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

DNA Replication of Human Papillomavirus Type 31 Is Modulated by Elements of the Upstream Regulatory Region That Lie 5' of the Minimal Origin

Walter G. Hubert, Taro Kanaya, and Laimonis A. Laimins^*

Department of Microbiology-Immunology, Northwestern University, Chicago, Illinois 60611-3008

Received 1 October 1998/Accepted 13 November 1998

	ABSTRACT

Top Abstract Introduction Materials and methods Results Discussion References

The viral replication factors E1 and E2 of papillomaviruses are necessary and sufficient to replicate plasmids containingthe minimal origin of DNA replication in transient assays. Underphysiological conditions, the upstream regulatory region (URR)governs expression of the early viral genes. To determine theeffect of URR elements on E1 and E2 expression specifically, andon the regulation of DNA replication during the various phasesof the viral life cycle, we carried out a systematic replicationstudy with entire genomes of human papillomavirus type 31 (HPV31),a high-risk oncogenic type. We constructed a series of URR deletions,spacer replacements, and point mutations to analyze the role ofthe keratinocyte enhancer (KE) element, the auxiliary enhancer(AE) domain, and the L1-proximal end of the URR (5'-URR domain)in DNA replication during establishment, maintenance, and vegetativeviral DNA amplification. Using transient and stable replicationassays, we demonstrate that the KE and AE are necessary for efficientE1 and E2 gene expression and that the KE can also directly modulateviral replication. KE-mediated activation of replication is dependenton the position and orientation of the element. Mutation of eitherone of the four Ap1 sites, the single Sp1 site, or the bindingsite for the uncharacterized footprint factor 1 reduced replicationefficiency through decreased expression of E1 and E2. Furthermore,the 5'-URR domain and the Oct1 DNA binding site are dispensablefor viral replication, since such HPV31 mutants are able to replicateefficiently in a transient assay, maintain a stable copy numberover several cell generations, and amplify viral DNA under vegetativeconditions. Interestingly, deletion of the 5'-URR domain leadsto increased transient and stable replication levels. These findingssuggest that elements in the HPV31 URR outside the minimal originmodulate viral replication through both direct and indirectmechanisms.

	INTRODUCTION

Top Abstract Introduction Materials and methods Results Discussion References

Papillomaviruses are small viruses that contain circular, double-stranded DNA genomes of about 8,000 bp and infect the cutaneousor mucosal epithelium. More than 70 types of human papillomaviruses(HPVs) have been identified to date. These viral genomes havea common genetic and functional organization, reflecting the useof common strategies during viral pathogenesis (12). Infectionby HPVs leads to benign proliferative lesions or warts, whichgenerally regress spontaneously. However, a subset of HPVs, referredto as high-risk HPVs are causally associated with the developmentof anogenital neoplasia (38). The productive life cycle of HPVsbegins with infection of basal keratinocytes, where the viralDNA is established as an autonomously replicating nuclear plasmidwith a low copy number. Expression of the viral early or regulatorygenes leads to an expansion of the infected keratinocyte populationand an alteration of the cellular differentiation program. Upondifferentiation, the late or structural genes of HPVs are expressed,viral DNA is amplified to a high copy number, and progeny virionsare produced (12).

Persistence of HPV DNA in the dividing basal cells is regulated by viral trans-acting factors which bind to sequences in theupstream regulatory region (URR) of the viral genome. These factorsinclude the E1 and E2 proteins, which are necessary for viralreplication (36). The URR of HPV31 can be divided into severalfunctional segments (Fig. 1A): a 5' region (5'-URR domain), anauxiliary enhancer (AE) domain, the cell-specific keratinocyteenhancer (KE) element, the minimal origin, and the P₉₇ promoterregion where early transcripts originate. The minimal origin wasidentified in transient replication assays and consists of anE1 binding site (E1BS), flanked upstream by E2BS2 and downstreamby E2BS3 and E2BS4 (5). Replication studies with HPV11, -16,and -18 have identified similar elements (3). In HPV31, theKE (nucleotides [nt] 7495 to 7789) is the major transcriptionalactivator of viral early gene expression and contains bindingsites for Ap1 and Oct1. In addition, a footprint which binds anuncharacterized factor (footprint 1 [Fp1] [14, 16]) is locatedat the 5' terminus of the KE. Directly upstream of the KE is anAE domain comprised of E2BS1 and YY1 and TEF1 sites that augmentsKE function (14). Such factor binding sites are found in theURRs of related HPVs and have been characterized for their rolein transcription (for a review, see reference 22). To date,the transcriptional activities of these elements in HPV31 haveonly been analyzed in transient transfection assays (14, 16,17).

Studies with the fibropapillomavirus bovine papillomavirus type 1 (BPV1) have identified the minimal URR sequences for stableplasmid replication, consisting of six binding sites for E2 andone for E1 (24). However, the functional organization of theURR of BPV1 is significantly different from that of the high-riskgenital HPVs (22, 37). Genital HPVs have four E2BS in thisregion, and it has been shown that only three of these sites arerequired for stable replication (33). The structure of the URRmay reflect the different mechanisms of pathogenesis for theseviruses; BPV1 infects both dermal and cutaneous epithelial cells,while genital HPVs persist exclusively in the mucosal epithelium.Methods for the genetic analysis of the productive viral lifecycle of HPV31 and HPV18 have recently been developed. In thesestable replication assays, cloned HPV DNA is excised from vectorsequences, unimolecularly ligated, and transfected into normalhuman keratinocytes. Immortalized cell lines can be established,which maintain the viral DNA as stably replicating plasmids (6,7). Upon differentiation in organotypic raft culture or suspensionin methylcellulose, these cells induce viral late functions, includingactivation of late gene expression and genome amplification (7,28).

Using these methods, we have systematically analyzed the role of URR sequences 5' to the minimal origin in plasmid replicationduring different phases of the HPV31 life cycle. Previous studieshave relied largely on transient assays using heterologous expressionvectors for E1 and E2. Our replication studies with entire HPV31genomes indicate that the KE directly modulates replication efficiencyand is essential for expression of E1 and E2. Multiple bindingsites in the URR for Ap1, Sp1, and Fp1 are necessary for transientand stable replication of HPV31 genomes. In contrast, the 5'-URRdomain and the Oct1 DNA binding site were found to be dispensablefor transient and stable viral replication as well as for viralDNA amplification under vegetativeconditions.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and methods Results Discussion References

Plasmids. All wild-type (wt) and mutated plasmids, are numbered according to the standard nucleotide number assignment as publishedfor HPV31 (8). Three parental HPV31 wt DNAs were used in thisstudy to facilitate the construction of mutants: (i) pBR322-HPV31(7), which contains the pBR322 vector at the unique EcoRI siteof HPV31; (ii) pBRmin-HPV31, which contains a pBR322 vector fragment(ClaI to Eco47III) at the unique EcoRI site of HPV31; and (iii)pUCmin-HPV31, which contains a pUC vector fragment (AflIII toSspI) at the unique XbaI site of HPV31. A schematic map of theURR is shown for each set of mutants in panels A of Fig. 1 through4. The locations of all DNA binding sites for cellular and viralfactors in the URR are numbered ascendingly in the sense directionof viral transcription (5' to 3'). The plasmid nomenclature forthe HPV31 genomes used in this study specifies the nature of amutation: deletion (d), spacer replacement (s), rearrangement(r), insertion (i), or point mutation (p). The size of a deletion,spacer, rearranged fragment, or insertion is indicated by thenumber of base pairs. Finally, deletions in the URR are classifiedas progressive (p) or internal (i), insertions are indicated asupstream (u) or downstream (d) with respect to the origin, andrearrangements of the KE are designated sense (s) or antisense(a). Mutations in DNA binding sites are denoted with the nameof the transcriptionfactor.

(i) Deletions. pBR322-HPV31 was used as the parental DNA for the following URR deletions ( $Delta$ ) between unique restriction sites: pHPV31-d1140p( $Delta$ BlpI to RsrII, $Delta$ nt 6274 to 7414), pHPV31-d1283p ( $Delta$ BlpI to SpeI, $Delta$ nt 6274 to 7557), pHPV31-d1515p ( $Delta$ BlpI to 3'-PmeI, $Delta$ nt 6274 to7789), and pHPV31-d294i ( $Delta$ 5'-PmeI to 3'-PmeI, $Delta$ nt 7495 to 7789).In each plasmid, the deletions were replaced with a BamHI linker(5'-dCGGATCCG). pHPV31-d143i ( $Delta$ RsrII to SpeI, nt 7414 to 7557)was prepared similarly but without a linker at the deletion. pHPV31-d102iwas prepared by replacing the corresponding wt sequences in pUCmin-HPV31with the Bst 1 107I-SpeI fragment from pBas102del (14).

(ii) Spacer replacements. pUCmin-HPV31 was used as parental DNA for the following spacer replacement mutants. pHPV31-s143i contains a PCR-generatedDNA spacer from the hygromycin resistance gene (nt 133 to 268of aminoglycoside phosphotransferase [Aph] coding sequence [9])inserted between the RsrII and SpeI sites. pHPV31-s294i was preparedby inserting a spacer (nt 133 to 412 of Aph coding sequence) intothe BamHI site of pHPV31-d294i and then transferring the BlpI-to-HindIIIfragment into pUCmin-HPV31. The DNA spacers do not contain consensussites for the common transcription factors that bind to the HPV31URR.

(iii) KE rearrangements and duplications. pBRmin-HPV31 was used as parental DNA for the following mutants. The KE fragment (5'-PmeI to 3'-PmeI, nt 7495 to 7789) wasdeleted and inserted at HpaI (nt 215) in sense orientation forpHPV31-r294s and in antisense orientation for pHPV31-r294a. Duplicationof the KE was performed with pBR322-HPV31. A second KE elementwas inserted in sense orientation at RsrII (nt 7414) for pHPV31-i294uor at HpaI for pHPV31-i294d.

(iv) URR binding site mutants. All mutants in this panel are based on pBR322-HPV31. pHPV31-pFp1 (defective Fp1 [17]), -pAp1.1 (defective Ap1 binding site1 [Ap1BS1]), -pAp1.2, -pOct1, -pAp1.3, -pAp1.4, and -pSp1 containmultiple point mutations within the indicated factor binding siteand were previously characterized in transient URR reporter andgel mobility shift assays (14, 17).

(v) Expression vectors. pSG-E1 and pSG-E2 are pSG5-based expression vectors (Stratagene) containing the HPV31 E1 and E2 coding sequences, respectively.These expression vectors support replication of HPV31 origin plasmidsin transient assays (5).

Transient replication assay. (i) DNA preparations. Bacterial vector sequences were first cleaved from the viral DNA (3 µg of 7,912-kbp wt or equimolar amounts of mutant) withthe appropriate restriction enzyme. Digested DNAs were unimolecularlyligated at 15°C overnight (850 µl, 7.5 Weiss units of T4 DNA ligasein 1× reaction buffer; GIBCO-BRL). Ligated DNAs were precipitatedwith 20 µg of sonicated salmon sperm DNA (Sigma), NaCl to 1 M(final concentration), and 0.6 volume of 2-propanol. DNAs werepelleted, washed with 70% ethanol, and resuspended in TE (10 mMTris [pH 8.0], 1 mM EDTA [pH 8.0]). For transfections with expressionvectors, equimolar (based on 7,912-kbp HPV31) amounts of pSG-E1and pSG-E2 were included in the final DNA mixture (20 µl).

(ii) Transient transfections and DNA isolation. Human squamous cell carcinoma (SCC13 [25]) cells were maintained in E medium on cocultured, mitomycin-treated J2-3T3 fibroblastfeeders as described previously (18). Transfection by electroporationwas carried out as described previously (5, 36), with thefollowing modifications. SCC13 cells (5 × 10⁶; 200 µl) in electroporation medium (complete E medium supplementedwith HEPES [pH 7.2] to 25 mM) were mixed with DNA in electroporationcuvettes (0.4-cm gap width) on ice, incubated at room temperaturefor 5 min, pulsed once (250 V, 960 µF; Bio-Rad GenePulser), andimmediately plated onto 10-cm-diameter dishes containing mitomycin-treatedJ2 feeder cells and electroporation medium. At 1, 2, and 4 daysafter transfection, cells were refed with fresh E medium. Low-molecular-weightDNA was isolated at 5 days posttransfection with a modified Hirtprotocol (11). Sample dishes were washed once with phosphate-bufferedsaline and placed on ice. Cells were scraped in resuspension buffer(0.6 ml; 300 mM NaCl, 20 mM EDTA), and transferred to an ultracentrifugetube (11 by 34 mm, thick-walled polycarbonate; Beckman). Sampleswere digested at 37°C for at least 3 h with proteinase K (to 0.2µg/µl) and sodium dodecyl sulfate (SDS; to 0.2% [wt/vol]). TheNaCl concentration of samples was adjusted to 1 M, high-molecular-weightDNA and cellular debris was precipitated by overnight incubationon ice. After ultracentrifugation (100,000 rpm, 20 min at 4°C,TLA100.2 rotor; Beckman), supernatants were extracted with phenoland chloroform and precipitated with 0.6 volume of 2-propanol.Samples were collected by centrifugation, washed with 70% (vol/vol)ethanol, and resuspended in TE (20 µl) with RNase A (to 20 µg/ml).One half of each sample was digested overnight with 8 U of DpnIand 7 U of linearizing enzyme (either HpaI, BanII, or AatII).

(iii) DNA analysis. Digested DNAs were resolved on 0.8% agarose gels, blotted onto a neutral nylon membrane (Magna) by high-salt transfer (2),and immobilized by UV cross-linking (Stratagene). Hybridizationwas carried out with a subgenomic HPV31 DNA probe (HpaI-EcoRIfragment) radiolabeled by random priming (Pharmacia) in a nonaqueoussolution (50% [vol/vol] formamide, SSC [850 mM sodium chloride,100 mM sodium citrate {pH 7.0}], Denhardt's solution [0.1% {wt/vol}each of bovine serum albumin, polyvinyl alcohol, and Ficoll],5% [wt/vol] dextran sulfate, 1% [wt/vol] SDS, 100 µg of denaturedsonicated salmon sperm DNA per ml) at 42°C. Blots were washedunder stringent conditions (Magna), autoradiographed (AmershamHyperfilm MP), and quantified with a PhosphorImager (MolecularDynamics). Four independent transfections per sample were analyzedin separate transient replication assays which produced comparablerelative replication activities. To allow comparison between differenttransfections, all Southern blots contained DNA standards (500,25, 2.5, and 0.5 pg of 7,912-bp HPV31 DNA). Since not all cellstake up DNA in transient transfections, these standards do notrepresent copy numbers percell.

Stable replication assay. (i) Stable transfections. Viral DNAs were digested and unimolecularly ligated as described for the transient replication assay. Transfections and drugselection were carried out as published elsewhere (7), withthe following modifications. Samples were coprecipitated withequimolar amounts of the selectable marker plasmid pSV2neo (30)but without carrier DNA, collected by centrifugation, and resuspendedin TE (50 µl). Primary human foreskin keratinocytes (HFKs) weregrown to 60% confluence in 6-cm-diameter dishes with KGM medium(Clonetics). Transfection mixtures (500 µl) were prepared withthe sample DNAs and Lipofectamine (20 µl; GIBCO-BRL) in KGM mediumand incubated at room temperature for 30 min. Sample dishes werewashed with KGM medium and incubated with the transfection mixturein KGM medium (1.5 ml, total volume) for 5 h at 37°C. KGM mediumwas added to 5 ml, and incubation continued overnight. One dayposttransfection, transfected HFKs were plated into 10-cm-diameterdishes containing mitomycin-treated J2 feeder cells in E medium.Two days posttransfection, the growth medium was changed to Emedium supplemented with 200 ng of murine epidermal growth factorper ml (E+EGF medium). Transfected cells were selected for 5 dayswith G418 sulfate (200 µg/mL [wt/vol]; GIBCO) in E+EGF medium,and treated J2 feeder cells were replenished every 2 days. Afterselection, cells were grown in E+EGF medium until visible coloniesappeared (typically 2 weeks), trypsinized, and passed as masscultures into several 10-cm-diameter dishes for DNA and cell stockpreparation.

(ii) DNA analysis. Total cellular DNA was isolated from nearly confluent mass cultures by lysis with proteinase K and SDS as described elsewhere(29). Sheared DNA samples (5 µg) were digested with DpnI (20U) only; unsheared samples were digested with DpnI and a linearizingenzyme for the viral DNA (20 U of each). Samples were resolvedby agarose gel electrophoresis and analyzed by Southern hybridizationas described for the transient replicationassay.

DNA amplification assay. HFK-based cell lines with stably replicating wt or mutants of HPV31 were grown in semisolid medium (1.6% [wt/vol] methylcellulosein complete E medium with 25 mM HEPES [pH 7.2]) as described elsewhere(28). Cells were recovered immediately from the methylcellulosesuspension (0 h) or after 24 h, and total cellular DNA was isolatedand analyzed as describedabove.

	RESULTS

Top Abstract Introduction Materials and methods Results Discussion References

Loss of the central URR domains diminishes transient DNA replication efficiency. To investigate if URR sequences in addition to the minimal origin played a role in replication of HPV31, we constructed aseries of deletion mutants in the background of the entire viralgenome (Materials and Methods; Fig. 1A). Progressive deletionsextended from within the L1 open reading frame (from nt 6274)to sequences in the URR: pHPV31-d1140p (to nt 7414), pHPV31-d1283p(to nt 7557), or pHPV31-d1515p (to nt 7789). A mutant with aninternal deletion of the KE (pHPV31-d294i [from nt 7495 to 7789])was also constructed. These deletions mutants were first testedin a transient replication assay using HPV-negative human squamouscell carcinoma (SCC13) cells. Transient replication assays mostclosely mimic the establishment phase of the HPV life cycle. Therefore,analysis of transient replication activities of mutant viral genomesidentifies cis and trans replication defects. A previous studydemonstrated that the transient replication behavior of HPV31mutants in SCC13 cells is comparable to that in primary humankeratinocytes (15). Unimolecularly ligated HPV31 DNAs withoutbacterial vector sequences were transfected into 5 × 10⁶ SCC13 cells by electroporation, either by themselves or withexpression vectors for E1 and E2. Heterologous expression of theviral replication factors was necessary for those HPV31 mutantswhere mutation of the known transcriptional control elements wasexpected to diminish E1 and E2 expression and thus lead to lossof replication. Low-molecular-weight DNA was isolated from cells5 days posttransfection, and one half of each sample was analyzedby Southern blotting, autoradiography, and phosphorimaging (Materialsand Methods).

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FIG. 1. Transient DNA replication of HPV31 mutants with progressive or internal URR-deletions. (A) The schematic shows the HPV31 URR with DNA binding sites for viral and cellular factors. The positions of known URR elements, such as the 5'-URR domain, AE domain, KE element, and minimal origin of DNA replication (Ori) are indicated by brackets. Solid bars denote the retained DNA sequences, and the numbers refer to deleted nucleotide positions (described in Materials and Methods). Deletion (d) mutants of HPV31 contain progressive (p) or internal (i) URR deletions of the indicated size: a, pHPV31-d1140p ( $Delta$ 6274 to 7414); b, pHPV31-d1283p ( $Delta$ 6274 to 7557); c, pHPV31-d1515p ( $Delta$ 6274 to 7789); and d, pHPV31-d294i ( $Delta$ 7495 to 7789). (B) Autoradiogram of representative Southern blot of replicated (DpnI-resistant) viral DNAs from a transient replication assay with HPV31 wt and mutants in SCC13 cells (50% of total sample analyzed for each). Viral DNAs (equimolar amounts based on 3 µg of 7,912-bp wt HPV31) were excised from vector sequences, unimolecularly ligated, and transfected without E1 or E2 expression vectors (see Materials and Methods). DNA standards (Stds) with linearized wt HPV31, shown on the left, contain 500, 25, 2.5, and 0.5 pg of 7,912-bp DNA, respectively. The arrow on the right denotes the migration of linearized (lin) wt DNA. The graph shows the relative (to wt) replication activities, quantified from a phosphorimage of the Southern blot. Relative replication activities were comparable in four independent transfections. (C) Autoradiogram and graph from cotransfections of viral DNAs with equimolar amounts of E1 and E2 expression vectors. The graph shows relative (to wt) replication activities, quantified as described for panel B. (D) Increasing amounts of E1 and E2 expression vectors were titrated (molar ratios of expression vector to viral DNA of 0.33, 1.0, and 3.0) in the presence of constant amounts of viral wt and mutant d DNAs. Graphs show amounts of replicated DNA as a function of expression vector ratio, quantified from a phosphorimage of the Southern blot.

As shown in Fig. 1B, replication efficiencies of HPV31 mutants with deletions that included the AE domain and/or the KE elementwere less than 10% of the wt level (lanes/columns 3 and 4). Similarly,the mutant with a deleted KE element also replicated at a lowlevel (lane/column 5), indicating that deletion of the centralURR domains can affect viral plasmid replication. To determineif the replication phenotype of these deletion mutants was theresult of reduced E1 and E2 expression, or rather reflected adirect modulation of replication, transient assays were also performedwith cotransfected expression vectors for E1 and E2. As shownin Fig. 1C, mutants with progressive deletions that include theAE domain (pHPV31-d1283p) and the KE element (pHPV31-d1515p) orthe KE alone (pHPV31-d294i) had much lower than wt levels of replicationwhen cotransfected with E1 and E2 vectors (lanes/columns 3 to5). All transient replication studies were carried out with fourindependent transfections per sample which produced comparablerelative replicationactivities.

To test if the low replication efficiency of pHPV31-d294i in the presence of expression E1 and E2 vectors was caused by insufficientamounts of the viral replication factors, we performed titrationswith increasing molar ratios of E1 and E2 vector DNAs based ona constant amount of viral genome. As shown in Fig. 1D, the replicationefficiency of the KE deletion mutant was not restored to wt levelseven when the ratio was increased 10-fold, from 0.33 to 3 (lanes/columns4 to 6). In contrast to the phenotypes of the central URR deletionmutants, removal of the 5' region from the viral genome (pHPV31-d1140p)increased replication efficiency above wt levels (Fig. 1B andC, lanes/columns 2), indicating that these DNA sequences may containelements that negatively regulate viral replication. The behaviorof the URR deletion mutants indicates that both the AE domainand the KE element are necessary for efficient transient plasmidreplication of HPV31. Mutants with AE and KE deletions also replicatesignificantly below wt levels when the E1 and E2 expression vectorsare cotransfected with the viral genomes, suggesting that thecentral URR domains can regulate expression of the viral replicationfactors as well as modulate replicationdirectly.

Replacement of URR deletions with spacers does not increase DNA replication efficiencies. The low-replication phenotype of most HPV31 mutants with a KE deletion (Fig. 1A, lanes/columns 3 to 5) could also have beencaused by bringing cis-acting elements closer to the minimal originthat could down-regulate E1 and E2 expression or replication.To test this possibility, we constructed a series of HPV31 genomesthat contained small internal deletions in the URR. For a subsetof these mutants, spacer DNA was inserted into the deletions whichwas derived from the Aph coding region (9). The selected regionsof Aph do not contain consensus sites for the known cellular transcriptionfactors that bind to the URR. Mutant pHPV31-d102i contains a deletion(nt 7281 to 7383) in the 5' segment of the URR between the latepolyadenylation signal and the 5'-most YY1 DNA binding site (Fig.2A) (14). In pHPV-d143i, the AE domain (nt 7414 to 7557) wasdeleted. This URR domain contains two YY1 sites, one TEF1 site,and the 5'-most E2BS and functions as a transcriptional activator(14). In mutants pHPV31-s143i and pHPV31-s294i, each deletionwas replaced with a DNA spacer of the same size.

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FIG. 2. Transient DNA replication of HPV31 mutants with internal URR deletions and spacer replacements. (A) The schematic elements of the HPV31 URR are the same as described in the legend to Fig. 1. Zigzag lines denote spacer DNA sequences inserted into the deletions (described in Materials and Methods). Deletion (d) and spacer (s) mutants of HPV31 with internal (i) URR deletions or spacer replacements of the indicated size: e, pHPV31-d102i ( $Delta$ 7281 to 7383); f, pHPV31-d143i ( $Delta$ 7414 to 7557); g, pHPV31-s143i ( $Delta$ 7495 to 7557 with spacer), d, pHPV31-d294i ( $Delta$ 7495 to 7789); h, pHPV31-s294i ( $Delta$ 7495 to 7789 with spacer). (B) Autoradiogram of representative Southern blot of replicated (DpnI-resistant) viral DNAs from a transient replication assay with HPV31 wt and mutants in SCC13 cells (50% of total sample analyzed for each). Viral DNAs (equimolar amounts based on 3 µg of 7,912-bp wt HPV31) were transfected without expression vectors. Wt1 and Wt2 pBR-based and pUC-based wt DNAs. (C) Autoradiogram and graph from cotransfections of viral DNAs with equimolar amounts of E1 and E2 expression vectors. DNA standards (Stds), migration of viral DNA, and quantification of the relative replication levels (B and C) are described in the legend to Fig. 1B.

This panel of small deletion and spacer mutants was then analyzed in a transient replication assays. When transfected withoutE1 and E2 expression vectors, mutant pHPV31-d102i ( $Delta$ 7281 to 7385)was found to replicate at 40% of wt levels (Fig. 2B, lane/column3). Mutants with other deletions (pHPV31-d143i and -d294i) orspacers (pHPV31-s143i and -s294i) replicated with less than 10%of wt efficiency (lanes/columns 4 to 7). When these HPV31 DNAswere cotransfected with E1 and E2 expression vectors, the AE-specificdeletion and spacer mutants were found to replicate at about 50%of wt levels, while the KE-specific mutants were below 20% ofwt levels (Fig. 2C, lanes/columns 4 to 7). These observationsindicate that (i) deletions of either the AE domain (nt 7414 to7557) or the KE element (nt 7495 to 7789) diminish expressionof the viral replication factors, (ii) the AE domain has a smallerdirect effect on replication than the KE element, and (iii) thereplication efficiencies resulting from deletion of these URRsequences cannot be restored by inserting spacersequences.

The replication function of the KE is dependent on the position and orientation of the element and is not cooperative when present in multiple copies. Our analysis of HPV31 mutants with progressive deletions into the URR or smaller internal deletions indicated that the centralURR domains contain DNA sequences that modulate replication incis. In polyomaviruses, elements that overlap with the transcriptionalenhancer and augment replication of the minimal origin have beenidentified. This replication enhancer activity was shown to beindependent of the position or orientation of the element (4).To test if the KE (nt 7495 to 7789) of HPV31 could function asa replication enhancer, we generated a panel HPV31 mutants thatcontained repositioned or duplicated KE elements. In mutants pHPV31-r294sand pHPV31-r294a, the KE was deleted from its wt position andinserted at nt 215 in the same orientation as in a wt genome (sense)and antiparallel, respectively (Fig. 3A). The inserted KE elementis located about 210 nt 3' to the center of the palindromic E1BSin the origin, which is similar to the distance of a wt KE element5' of the origin (130 nt). To test potential cooperativity ofmultiple KE elements, a second KE was inserted upstream at nt7414 (pHPV31-i294u) or downstream at nt 215 (pHPV31-i294d).

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FIG. 3. Transient DNA replication of HPV31 mutants with deletions, rearrangements, or insertions of the KE. (A) The schematic elements of the HPV31 URR are the same as described in the legend to Fig. 1. In addition, KE elements inserted into the viral DNA at given nucleotide positions are shown as solid lines with arrow tips, indicating the normal KE orientation (described in Materials and Methods). Deletion (d), rearrangement (r), or insertion (i) mutants of HPV31 where the 294-bp KE fragment is deleted or placed in sense (s) or antisense (a) orientation, upstream (u) or downstream (d) of the origin: d, pHPV31-d294i ( $Delta$ 7495 to 7789); i, pHPV31-r294s ( $Delta$ 7495 to 7789, KE at nt 215 in sense); j, pHPV31-r294a ( $Delta$ 7495 to 7789, KE at nt 215 in antisense); k, pHPV31-i294u (new KE at nt 7414); l pHPV31-i294d (new KE at nt 215). (B) Autoradiogram of representative Southern blot of replicated (DpnI-resistant) viral DNAs from a transient replication assay with HPV31 wt and mutants in SCC13 cells (50% of total sample analyzed for each). Viral wt and mutant k DNAs (equimolar amounts based on 3 µg of 7,912-bp wt HPV31) were transfected without expression vectors. (C) Autoradiogram and graph from cotransfections of viral DNAs with equimolar amounts of E1 and E2 expression vectors. DNA standards (Stds), migration of viral DNA, and quantification of the relative replication levels (B and C) are described for Fig. 1B.

All KE rearrangement mutants were analyzed in a transient replication assay with cotransfected E1 and E2 expression vectorsas described in Materials and Methods. Since pHPV31-i294u is theonly mutant genome that contains an intact early transcriptionunit, it was also tested without E1 and E2 expression vectors.Duplication of the KE element in pHPV31-i294u diminished replicationto 20% of wt levels (Fig. 3B, lane/column 2) in the absence ofE1 and E2 expression vectors, indicating that viral gene expressionwas possibly affected by this mutation. When expression vectorswere cotransfected with pHPV31-i294u, replication was not completelyrestored to wt levels, suggesting that the duplication of theKE element also interfered directly with replication (Fig. 3C,lane/column 5). When the KE element was duplicated at both sidesof the minimal origin in pHPV31-i294d, the replication efficiencywith E1 and E2 expression vectors was similar to wt levels (lane/column6).

In cotransfections with E1 and E2 expression vectors, the mutant genomes containing a KE element downstream of the minimalorigin, pHPV31-r294s and pHPV31-r294a, replicated as inefficientlyas the KE deletion mutant pHPV31-d294i (Fig. 3C, lanes/columns2 to 4). Replication of these KE rearrangement mutants at lessthan 20% of wt levels, therefore, indicates that the replicationefficiency of HPV31 genomes that lack a wt KE cannot be restoredby inserting a KE element downstream of the origin. These findingsdemonstrate that activation of replication by the KE element isposition and orientation dependent. Since duplication of the elementalso did not cooperatively activate replication, it appears thatthe entire KE element, which was mapped in earlier transcriptionalstudies, does not act as a replicationenhancer.

DNA binding of transcription factors to their cognate sites in the URR activates DNA replication primarily through an increase in viral gene expression. To test if binding of specific transcription factors to the URR could contribute to the activation of DNA replication, HPV31genomes with mutated factor binding sites were tested in a transientreplication assay. Previous transient studies with reporter plasmidsthat contained mutated URR sequences identified specific bindingsites that can activate transcription. These include four bindingsites for Ap1, one each for Sp1 and Oct1, and the uncharacterizedFp1 (14, 16). The following panel of viral genomes containpoint mutations which abrogate binding of the factors to the specifiedsites (in 5'-to-3' direction on the HPV31 sense strand [Fig. 4A]):pHPV31-pFp1, pHPV31-pAp1.1 (Ap1BS1), pHPV31-pAp1.2, pHPV31-pOct1,pHPV31-pAp1.3, pHPV31-pAp1.4, and pHPV31-pSp1. These binding sitemutations were previously tested in gel mobility shift assaysand found to be defective for factor binding (14, 16).

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FIG. 4. Transient replication of HPV31 DNAs with point mutations in the URR. (A) The schematic elements of the HPV31 URR are the same as described in the legend to Fig. 1. In addition, specific DNA binding sites of transcription factors marked with × are mutated (described in Materials and Methods). Point mutations (p) are designated with factor name and binding site number (5' to 3' on HPV31 sense strand): m, pHPV31-pFp1; n, pHPV31-pAp1.1; o, pHPV31-Ap1.2; p, pHPV31-Oct1; q, pHPV31-Ap1.3; r pHPV31-Ap1.4; s, pHPV31-Sp1. (B) Autoradiogram of representative Southern blot of replicated (DpnI-resistant) viral DNAs from a transient replication assay with HPV31 wt and mutants in SCC13 cells (50% of total sample analyzed for each). Viral DNAs (equimolar amounts based on 3 µg of 7,912-bp wt HPV31) were transfected without expression vectors. (C) Autoradiogram and graph from cotransfections of viral DNAs with equimolar amounts of E1 and E2 expression vectors. DNA standards (Stds), migration of viral DNA, and quantification of the relative replication levels (B and C) are described for Fig. 1B.

Mutating one of the four Ap1 sites in the URR diminished replication to less than 10% (site 1, 3, or 4) or 30% (site 2) ofwt levels in the absence of E1 and E2 expression vectors (Fig.4B, lanes/columns 3, 4, 6, and 7). Similarly, abrogation of DNAbinding by Sp1 or the factors comprising Fp1 also reduced replicationto about 20% of wt levels (lanes/columns 8 and 2). The only mutatedgenome in the panel that replicated better than wt was pHPV31-pOct1(lane/column 5). When these viral DNAs were cotransfected withE1 and E2 expression vectors, the replication efficiencies ofmost mutants increased to 40% or more of the wt level (Fig. 4C,lanes/columns 4, 5, 7, and 8). Only pHPV31-pFp1, -pAp1.1, and-pAp1.3 replicated inefficiently at about 20% of wt levels withE1 and E2 vectors (lanes/columns 2, 3, and 6). These results indicatethat (i) most transcription factors binding in the URR of HPV31modulate viral replication through expression of the E1 and E2genes and (ii) mutations in Fp1, Ap1BS1, or Ap1BS3 affect viraltranscription as well as replicationdirectly.

Deletions of the 5'-URR domain do not diminish stable DNA replication. We next sought to identify sequences within the URR that in addition to the minimal origin are required for stable replication.In contrast to transient replication assays which mimic the establishmentphase of HPV infection, stable replication assays with primaryhuman keratinocytes allow the examination of the requirementsfor maintenance. Stable replication of HPV genomes as autonomouslyreplicating nuclear plasmids depends on the complex interactionof viral and cellular processes. Previous studies have demonstratedsignificant differences between transient and stable assays (15,32, 33).

To test which URR sequences were necessary for stable replication, we carried out stable replication assays with a subsetof the HPV31 mutants analyzed in the transient studies (see Materialsand Methods). Typically, primary cell lines established by transfectionwith wt HPV31 contain 20 to 50 viral genomes per cell (7).The following groups of mutated HPV31 genomes all contain intactE6 and E7 genes which are required for full immortalization ofprimary cells (20): progressive URR deletion mutants pHPV31-d1140p,-d1283p, and -d1515p (Fig. 1A); internal URR deletion and spacermutants pHPV31-d102i, -d143i, -s143i, -d294i, and -s294i (Fig.2A); the KE duplication mutant pHPV31-i294u (Fig. 3A); and allof the URR point mutants pHPV31-pFp1, -pAp1.1, -pAp1.2, -pOct1,-pAp1.3, -pAp1.4, and -pSp1 (Fig. 4A). HPV31 plasmids were digestedto cleave the bacterial vector sequences from the viral DNA, unimolecularlyligated, and transfected into primary HFKs with a selectable markerand no expression vectors for E1 and E2. Transfected cells wereselected; drug-resistant colonies were pooled and expanded. Totalcellular DNA was isolated from these mass culture cell lines atpassage 3 posttransfection and analyzed by Southern blotting.Several different topological forms of viral DNA can be distinguishedin sheared total cellular DNA: (i) slowly migrating, high-molecular-weightsmears (hmw), (ii) open-circle monomers (oc), and (iii) fast-migratingsupercoiled monomers (sc) (Fig. 5). Hybridization signals at positioni generally indicate integrated or highly multimeric viral plasmidDNA, while those at positions ii and iii demonstrate autonomousviral replication. To estimate viral copy number per cell, totalunsheared cellular DNA was digested with an enzyme that linearizesviral plasmid monomers or reduces tandemly integrated speciesto unit length.

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FIG. 5. Stable DNA replication of HPV31 mutants. Autoradiograms of representative Southern blots show HPV31 mutants tested in stable replication assays. Total cellular DNA was isolated from mass cultures of stably transfected primary cells and analyzed for the presence of viral DNA (Materials and Methods). All panels show sheared/undigested DNA (5 µg) on the left, unit-length DNA standards (500, 25, 2.5, and 0.5 pg of 7,912-bp wt HPV31 DNA; equivalent to about 100, 5, 0.25, and 0.1 viral genomes per cell) in the center, and unsheared/linearized DNA (5 µg) on the right. Autonomous viral plasmid replication is indicated by supercoiled monomeric (sc1) and open-circle monomeric (oc1) bands (arrows on left). Hybridization of high-molecular-weight DNA (hmw) generally indicates the presence of plasmid multimers or integrated viral DNA. Unit-length viral DNAs (lin) from digestion with a unique restriction enzyme is obtained from autonomously replicating plasmid DNA or tandemly integrated viral DNA and is an indicator of viral copy number (arrows on the right). (A) HPV31 mutants with progressive URR deletions (maps in Fig. 1A): sheared samples (lanes 1 through 8) of wt and mutant pHPV31-d1140p (a) from three independent transfections, and mutants pHPV31-d1283p (b) and pHPV31-d1515p (c). Linearized samples are shown in the same order (9 through 16). (B) HPV31 mutants with internal URR deletions, DNA spacers, or KE insertion (maps in Fig. 2A and 3A): sheared samples (lanes 1 through 7) of wt and mutants pHPV31-d102i (e), pHPV31-d143i (f), pHPV31-s143i (g), pHPV31-d294i (d), pHPV31-s294i (h), and pHPV31-i294u (b). Linearized samples are shown in the same order (8 through 14). (C) HPV31 mutants with defective factor binding sites (maps in Fig. 4A): sheared samples (lanes 1 through 8) of wt, pHPV31-pFp1 (m), pHPV31-pAp1.1 (n), pHPV31-Ap1.2 (o), pHPV31-Oct1 (p), pHPV31-Ap1.3 (q), pHPV31-Ap1.4 (r), and pHPV31-Sp1 (s). Linearized samples are shown in the same order (9 through 16).

Deleting URR sequences 5' of nt 7414 did not adversely affect stable replication. In three independent experiments with primaryHFKs from different donors, the mutant pHPV31-d1140p replicatedextrachromosomally as an intact monomeric (Fig. 5A, lanes 2 and4) or, in one case, rearranged (lane 6) plasmid. Its estimatedDNA copy number per cell was, on average, about 1.8-fold higherthan that for wt DNA. In addition, a smaller deletion in the 5'-URRdomain was found to replicate stably at wt levels (Fig. 5B, lane2). HPV31 genomes which contained deletions of the AE domain (pHPV31-d1283pand -d143i) or the KE element (pHPV31-d1515p and -d294i) or hadDNA spacers in the respective deletions (pHPV31-s143i and -s294i)did not replicate stably. Although the detection limit of ourassay was better than 0.1 viral copy per cell (0.5 pg [Fig. 5A,center]), consistently, no viral signal was detectable in thetotal DNA samples (Fig. 5A, lanes 7 and 8; Fig. 5B, lanes 3 through6). Similarly, the HPV31 mutant containing an upstream duplicationof the KE element (pHPV31-i294u) did not replicate stably (Fig.5B, lane 7). The inability of these mutants to replicate stablythus correlated with their low levels of replication in the transientassays without E1 and E2 expression vectors. Finally, we testedthe panel of HPV31 genomes with inactivated factor binding sites(pHPV31-pFp1, -pAp1.1, -pAp1.2, -pOct1, -pAp1.3, -pAp1.4, and-pSp1 [Fig. 4A]) in a stable replication assay. Again, only pHPV31-pOct1,which could replicate efficiently in the transient assay, wasalso able to replicate stably (Fig. 5C, lane 5). Genomes containingmutations in other binding sites produced high-molecular-weighthybridization signals in the stable replication assay, indicatingthat the viral DNA was integrated into the cellular genome (Fig.5C, lanes 2 to 4 and 6 to 8). In all stable replication assaysthat were performed, we observed some integrated viral DNA withwt DNA (Fig. 5A, lanes 1, 3, and 5; Fig. 5B, lane 1; Fig. 5C,lane 1). However in all cases, wt HPV31 replicated as a monomericplasmid with prominent supercoiled and open-circle bands (Fig.5). Occasionally, both monomeric and rearranged species of wtor mutant HPV31 DNA were found in the same sample (Fig. 5B, lanes1 and 2), which may have been caused by improper recircularizationof the viral genomes prior totransfection.

The 5'-URR domain and the Oct1 DNA binding site are not required for viral DNA amplification. Differentiation of the HPV-infected host cells is necessary for the ability of papillomaviruses to amplify viral genomes andinduce late gene expression (1, 7, 13, 19). HPV31-harboringkeratinocytes grown in semisolid medium (10) undergo cellulardifferentiation and induce viral genome amplification in about20% of cells (27, 28). To test the effects of specific mutationson the ability to amplify viral DNA, the cell lines that couldbe established with stably replicating HPV31 mutants in our precedinganalyses were subjected to growth in methylcellulose (see Materialsand Methods). At 0- and 24-h time points, total cellular DNA wasisolated and analyzed by Southernblotting.

The HPV31 genomes that contain deletions in the 5'-URR (pHPV31-d1140p and -d102i [Fig. 1A and 2A]) were able to amplify theircopy number about twofold above the levels in undifferentiatedmonolayer cultures (Fig. 6A and B, lanes 2 versus lanes 1). Thisratio of increase was similar to the observed amplification ofwt DNA (Fig. 6A, compare lanes 2 and 4) and is equivalent to abouta 10-fold increase in viral genomes in amplification-competentcells. The pHPV31-pOct1 point mutant (Fig. 4A) could also amplifyits copy number (Fig. 6A, lane 6 versus lane 5). We thereforeconclude that the 5'-URR domain and the Oct1 binding site arenonessential for HPV31 genome amplification.

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FIG. 6. DNA amplification of stably replicating HPV31 mutants. Autoradiograms of representative Southern blots show stably replicating HPV31 mutants in differentiating primary keratinocytes. Cells were grown in semisolid medium for 0 h (odd lane numbers) and 24 h (even lane numbers) to induce differentiation and viral DNA amplification. Total cellular DNA was isolated, analyzed for viral DNA, and arranged on the blots as described in Materials and Methods and the legend to Fig. 5. All panels show sheared/undigested DNA (5 µg) on the left, unit-length DNA standards (500, 25, 2.5, and 0.5 pg of 7,912-bp wt HPV31 DNA; equivalent to about 100, 5, 0.25, and 0.1 viral genomes per cell) in the center, and unsheared/linearized DNA (5 µg) on the right. (A) Sheared (lanes 1 through 6) and linearized (7 through 12) samples of mutant pHPV31-d1140p (a [Fig. 1A]), wt, and mutant pHPV31-Oct1 (p [Fig. 4A]), uninduced (lanes 1, 3, and 5) and induced (lanes 2, 4, and 6). (B) Sheared (lanes 1 and 2) and linearized (lanes 3 and 4) samples of mutant pHPV31-d102i (e [Fig. 2A]), uninduced (lanes 1 and 3) and induced (lanes 2 and 4).

	DISCUSSION

Top Abstract Introduction Materials and methods Results Discussion References

We have systematically examined the effects of URR sequences outside the minimal origin on the replication activity of HPV31in different phases of the viral life cycle by carrying out transient,stable, and DNA amplification assays with a series of viral genomescontaining URR deletions, spacer replacements, or point mutations.Consistent with the previous findings that the KE is necessaryfor efficient transcription of the early viral genes in general,we demonstrate here that it is specifically required for expressionof the replication proteins E1 and E2 and that it also modulatesreplication activity in cis, since addition of expression vectorsfor E1 and E2 does not restore the replication efficiencies ofKE mutants to wt levels. The E1 and E2 expression vectors usedin this study have been shown to support replication of an HPV31minimal origin plasmid (5). While our URR mutations of thetranscriptional enhancer sequences of HPV31 likely affect theexpression of most early genes, the observed reduction of transientreplication efficiency in SCC13 cells is, we believe, caused bydecreased E1 and E2 levels. Since HPV31 mutants defective forE6 or E7 expression can replicate in transiently transfected SCC13cells comparable to wt levels (35), altered expression of theseoncoproteins does not play a major role in modulating the transientreplication activities of HPV31 enhancermutants.

Our observation that the replication activities of HPV31 genomes that contain a deletion of the KE or a neutral DNA spacerare comparable and below wt levels suggests that the KE elementmay contain sequences that directly activate replication. However,unlike the function of the replication enhancer in polyomavirus(21), activation of HPV31 replication by the KE is dependenton the specific position and orientation of the element in theviral genome, indicating that the KE is not a replication enhancer.The inefficient replication of HPV31 genomes containing pointmutations in transcription factor binding sites demonstrated thatthe primary function of these sites is in the regulation of E1and E2 expression. However, even in the presence of E1 and E2expression vectors, viral genomes with defective Ap1BS1 or Ap1BS3replicated only at about 30% of wt levels. These results indicatethat these two Ap1 sites, which are equidistant from each otherand the minimal origin, appear to modulate replication directly.Such a role for Ap1 in HPV31 replication would be consistent withthe function of the murine Ap1 homologue in polyomavirus DNA replication(26). Among all of the HPV31 mutants with defective factor bindingsites that were analyzed, only the Oct1 site mutant replicatedsimilarly to wt in transient and stable replication as well asDNA amplification. While binding of Oct1 to its cognate site inthe URR may not be necessary for viral DNA replication or DNAamplification, it may still play a role in the modulation of differentiation-dependentlate gene expression. Further studies using a minimal origin withadded factor binding sites may be necessary to determine the exactmechanism by which specific cellular factors that bind to theURR modulate origin activity. Possible mechanisms include thealteration of chromatin structure, to produce nucleosome freeregions on the viral minichromosome, or DNA looping, to providecontact between origin-proximal and -distal replicationfactors.

Adjacent to the KE is the AE domain, which contains multiple YY1 binding sites and E2BS1. In transient reporter assays, theseYY1 sites have been shown to complement KE activation of earlygene expression (14). Consistent with this role, our presentfindings also indicate that the AE moderately affects replicationfunction directly. A previous study demonstrated that E2BS1 isrequired for transient and stable replication of HPV31 (33).This E2BS could also modulate replication by augmenting viralgene expression as has been shown for the related HPV18 (31).

Our analysis of HPV31 genomes which contained deletions in the 5'-URR domain demonstrated that these DNA sequences are notessential for transient and stable replication or differentiation-dependentDNA amplification. Interestingly, we found that the HPV31 mutantwith a large 5'-URR deletion consistently replicated more efficientlythan wt in transient assays and maintained a higher copy numberin stable replication. One plausible explanation for the increasedreplication efficiency of pHPV31-d1140p is that the smaller plasmidsize of this mutant (6,778 bp) could result in more favorablereplication kinetics than for the wt DNA (7,912 bp). More likely,however, is the possibility that the 5'-URR domain modulates eitherE1 and E2 expression or replication directly. Previous studieswith the low-risk mucosal HPV6 have identified negative regulatorysequences in this region which bind the CCAAT displacement factor(23). In transient reporter assays with HPV31, a similar elementthat weakly represses transcription from P₉₇, the major viralearly promoter, was found (14). In light of these transcriptionaldata, the results of our replication studies suggest that the5'-URR domain down-modulates HPV31 DNA replication through differentmechanisms. Recently, an attachment site for the nuclear matrixwas mapped to the 5'-URR domain in the closely related HPV16 (34).Since we demonstrated that this region of the viral genome isnot required in transient or stable replication of HPV31, ourdata suggest that attachment to the nuclear matrix as a mechanismfor plasmid segregation may be facilitated through multiple redundantsites.

In this study, we have demonstrated the importance of URR sequences other than the minimal origin in regulating HPV31 plasmidreplication in keratinocytes. The AE domain and the KE elementcan modulate replication in two ways: (i) indirectly through specificactivation of E1 and E2 expression and (ii) directly through ayet unidentified mechanism. Both enhancer regions are requiredfor transient and stable replication, while the 5'-URR domainor binding of Oct1 to the URR was nonessential for viral replicationand DNA amplification. Independent of the type of mutation, HPV31genomes which exhibited defects in either E1 and E2 gene expressionor direct activation of replication replicated at low levels intransient assays and, invariably, were unable to replicate stably.Further dissection of the cis- and trans-acting components ofthe viral genome that regulate plasmid replication await the developmentof an efficient trans-complementing transfection system forHPVs.

	ACKNOWLEDGMENTS

We thank the members of the Laimins laboratory for advice and helpful comments, and we thank R. Longnecker and K. Rundellfor critically reading themanuscript.

W.G.H. is supported by INRSA grant F32-CA73087 from the National Cancer Institute. This work was supported by a grant fromthe NCI (CA74202) to L.A.L.

	FOOTNOTES

^* Corresponding author. Mailing address: Dept. of Microbiology- Immunology, Northwestern University, 303 E. Chicago Ave., Chicago,IL 60611-3008. Phone: (312) 503-0648. Fax: (312) 503-0649. E-mail:lal{at}merle.acns.nwu.edu.

Present address: Department of Obstetrics and Gynecology, Kanazawa University School of Medicine, Kanazawa,Japan.

REFERENCES

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Abstract
Introduction
Materials and methods
Results
Discussion
References

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Hubert, W. G., Laimins, L. A. (2002). Human Papillomavirus Type 31 Replication Modes during the Early Phases of the Viral Life Cycle Depend on Transcriptional and Posttranscriptional Regulation of E1 and E2 Expression. J. Virol. 76: 2263-2273 [Abstract] [Full Text]
Pena, L. d. M., Laimins, L. A. (2001). Differentiation-Dependent Chromatin Rearrangement Coincides with Activation of Human Papillomavirus Type 31 Late Gene Expression. J. Virol. 75: 10005-10013 [Abstract] [Full Text]
Terhune, S. S., Hubert, W. G., Thomas, J. T., Laimins, L. A. (2001). Early Polyadenylation Signals of Human Papillomavirus Type 31 Negatively Regulate Capsid Gene Expression. J. Virol. 75: 8147-8157 [Abstract] [Full Text]
Newhouse, C. D., Silverstein, S. J. (2001). Orientation of a Novel DNA Binding Site Affects Human Papillomavirus-Mediated Transcription and Replication. J. Virol. 75: 1722-1735 [Abstract] [Full Text]
Stubenrauch, F., Hummel, M., Iftner, T., Laimins, L. A. (2000). The E8 ˆE2C Protein, a Negative Regulator of Viral Transcription and Replication, Is Required for Extrachromosomal Maintenance of Human Papillomavirus Type 31 in Keratinocytes. J. Virol. 74: 1178-1186 [Abstract] [Full Text]
O'Connor, M. J., Stünkel, W., Koh, C.-H., Zimmermann, H., Bernard, H.-U. (2000). The Differentiation-Specific Factor CDP/Cut Represses Transcription and Replication of Human Papillomaviruses through a Conserved Silencing Element. J. Virol. 74: 401-410 [Abstract] [Full Text]
Thomas, J. T., Hubert, W. G., Ruesch, M. N., Laimins, L. A. (1999). Human papillomavirus type 31 oncoproteins E6 and E7 are required for the maintenance of episomes during the viral life cycle in normal human keratinocytes. Proc. Natl. Acad. Sci. USA 96: 8449-8454 [Abstract] [Full Text]

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