The Hinge of the Human Papillomavirus Type 11 E2 Protein Contains Major Determinants for Nuclear Localization and Nuclear Matrix Association

doi:10.1128/JVI.74.8.3761-3770.2000

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Journal of Virology, April 2000, p. 3761-3770, Vol. 74, No. 8
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

The Hinge of the Human Papillomavirus Type 11 E2 Protein Contains Major Determinants for Nuclear Localization and Nuclear Matrix Association

Nianxiang Zou,¹ Biing Yuan Lin,¹ Fenghai Duan,¹ Kyung-Yeol Lee,¹ Ge Jin,¹ Ran Guan,¹ Guang Yao,¹ Elliot J. Lefkowitz,² Thomas R. Broker,¹ and Louise T. Chow¹^,^*

Departments of Biochemistry and Molecular Genetics¹ and Microbiology and Immunology,² University of Alabama at Birmingham, Birmingham, Alabama 35294-0005

Received 27 August 1999/Accepted 7 January 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The E2 protein of papillomaviruses is a site-specific DNA binding nuclear protein. It functions as the primary replicationorigin recognition protein and assists in the assembly of thepreinitiation complex. It also helps regulate transcription fromthe native viral promoter. The E2 protein consists of an amino-terminal(N) trans-acting domain, a central hinge (H) domain, and a carboxyl-terminal(C) protein dimerization and DNA binding domain. The hinge ishighly divergent among papillomaviruses, and little is known aboutits functions. We fused the enhanced green fluorescent protein(GFP) with the full-length human papillomavirus type 11 (HPV-11)E2 protein and showed that the resultant fusion, called gfpE2,maintained transcription and replication functions of the wild-typeprotein and formed similar subnuclear foci. Using a series ofGFP fusion proteins, we showed that the hinge conferred strongnuclear localization, whereas the N or C domain was present inboth cytoplasm and nucleus. Biochemical fractionation demonstratedthat the N domain and hinge, but not the C domain, independentlyassociated with the nuclear matrix. Mutational analyses showedthat a cluster of basic amino acid residues, which is conservedamong many mucosotropic papillomaviruses, was required for efficientnuclear localization and nuclear matrix association. This mutationno longer repressed the HPV-11 upstream regulatory region-controlledreporter expression. However, a very small fraction of this mutantcolocalized with E1 in the nucleus, perhaps by a piggyback mechanism,and was able to support transient replication. We propose thatthe hinge is critical for the diverse regulatory functions ofthe HPV-11 E2 protein during mRNA transcription and viral DNAreplication.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The papillomavirus E2 protein is a multifunctional nuclear phosphoprotein with a molecular mass of approximately 40 kDa. Withhigh affinity and specificity, it functions as a dimer, bindingto multiple copies of a consensus E2 binding site (E2BS), ACCN₆GGT,located in the upstream regulatory region (URR) and regulatingboth viral DNA replication and mRNA transcription from the viralE6 promoter located immediately upstream of the E6 gene. The E2protein is the primary origin recognition protein and helps recruitthe viral replication initiator E1 protein (8, 30, 40,55, 64, 66, 70). It also plays a role in the assemblyof the preinitiation complex (39; K.-Y. Lee, T. R. Broker, andL. T. Chow, unpublished data). In vitro, E2 is able to excludenucleosome formation on the origin, which would otherwise inhibitthe initiation of DNA replication (36). Furthermore, E2 modulatesthe native human papillomavirus (HPV) URR-E6 promoter or a surrogatepromoter linked to the URR or to one or more copies of syntheticE2BS (16-18, 26, 59, 62, 63). The bovine papillomavirustype 1 (BPV-1) E2 protein tethers the BPV-1 DNA to mitotic chromosomes,ensuring plasmid segregation during mitosis (28, 35, 58).Moreover, the BPV-1 E2 has been postulated to play a role in virionmorphogenesis (14).

The full-length E2 protein consists of three distinct domains, the amino-terminal (N) trans-acting domain, a central, apparentlyunstructured hinge (also called the H domain), and the carboxyl-terminal(C) protein dimerization and DNA binding domain. The structureand function of the N and C domains are relatively conserved amonghuman and animal papillomaviruses, whereas the H domain is highlyvariable in sequence and length. Little is known about its function,and it is generally considered a flexible linker between the twofunctional domains (19). Alternative promoter usage and mRNAsplicing generate additional forms of E2 polypeptides. In theseE2-related proteins, the N domain is either truncated or substituted,but all contain the H and C domains. Each is a nuclear proteinand inhibits replication or transcription by competing for bindingto the E2BS (6, 7, 9, 10, 27, 32, 37, 39, 53).Since only the full-length E2 protein can activate a promoterand support replication, these observations indicate that theN domain plays a critical role in transcription activation andreplication by interacting with otherproteins.

Upon synthesis in the cytoplasm, proteins may enter the nucleus by passive diffusion or by energy-dependent active transport.All protein transport into and out of the nucleus occurs throughthe nuclear pore complexes in the nuclear envelope. Proteins largerthan 45 to 60 kDa require active transportation via nuclear localizationsignals (NLSs) encoded within the protein or by association withanother protein that is actively transported into the nucleusvia a piggyback mechanism (reviewed in reference 29). Althoughthere are no highly conserved consensus sequences for the NLS,peptide tracts rich in basic amino acid residues, exemplifiedby those in the simian virus 40 T antigen, can function as anNLS (56). In addition, phosphorylation can also play a rolein nuclear localization (29). Two NLSs have been identifiedin the BPV-1 E2 protein: residues 107 to 115 (KRCFKKGAR) in theN domain and residues 339 to 352 (KCYRFRVKKNHRHR) in the C domain(57). Partially homologous sequences exist in the N and C domainsof E2 proteins of many HPV types, including HPV type 11 (HPV-11).Whether they also function as NLSs has not beentested.

In a recent study using indirect immunofluorescence staining, we showed that the full-length HPV-11 E2 protein is locatedexclusively in the nucleus (61). Most prominent are the distinctsubnuclear foci. Furthermore, the virus-encoded E1 helicase (reviewedin references 11 and 60), which is required for both initiationand elongation (39), invariably colocalizes with the E2 proteinin these subnuclear foci. The E2 foci are observed in the presenceor absence of E1 or HPV origin-containing DNA. In contrast, E1,which is also a nuclear phosphoprotein, only infrequently exhibitsa similar punctate pattern when expressed alone. Thus, E2 appearsto play a role in recruiting E1 protein and the origin-containingDNA to certain subnuclear compartments. When E1 and E2 expressionvectors were cotransfected with an HPV origin-containing plasmid,some of these subnuclear foci became larger or merged. These largefoci are identified to be replication compartments by their colocalizationwith the single-stranded DNA binding protein RPA and with bromodeoxyuridineincorporated during pulse-labeling. They also colocalize withHPV origin-containing DNA, which is below the level of detectionelsewhere in the nucleus or in cells negative for E1 or E2 protein.We hypothesize that these subnuclear compartments are attributableto association with the nuclear matrix, but this hypothesis hasnot beenexamined.

Operationally, the eucaryotic nucleus is comprised of nucleoplasm, a soluble fraction of the nucleus, and two insoluble fractions:chromatin, which is composed of DNA and histones, and a fibrogranularstructure called the nuclear matrix (NM) or nuclear scaffold,which remains after the nucleus has been treated with DNase andhigh salt or lithium-3,5-diiodosalicylate (1, 51). NM iscomposed of lamin polymers, core filaments, and associated proteinsand is known to organize chromosomal DNA into looped domains viamatrix attachment regions. It is this scaffold on which RNA transcriptionand processing as well as DNA replication take place (1, 2,15).

In this study, we used the enhanced green fluorescent protein (GFP) as a tracer to delineate the domains of HPV-11 E2 responsiblefor its nuclear localization and to investigate the nature ofthe subnuclear E2 compartmentation. Our results show that, unexpectedly,the H domain contains a strong NLS and is responsible for nuclearlocalization of the protein. We also demonstrate that the E2 fociare indeed attributable to association with NM. Moreover, boththe N and H domains, but not the C domain, contain sequences thatbind to NM. Mutational analyses identified in the hinge a clusterof basic amino acids critical to NLS and for NM association. Theimplications of these findings in terms of HPV E2 protein functionswill bediscussed.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Plasmids. The enhanced GFP expression plasmid pEGFP-C1 (Clontech, Inc., Palo Alto, Calif.) was used to construct the GFP fusion proteinexpression plasmids. DNA fragments spanning the full-length HPV-11E2, or a portion of it, such as the N domain, the intact or truncatedhinge region, and the C domain, alone or in combinations (Fig.1), were amplified by PCR using DNA polymerase Pfu (Stratagene,La Jolla, Calif.). These fragments were each fused in frame tothe carboxyl terminus of the GFP coding gene via the BglII andSmaI cloning sites in plasmid pEGFP-C1. GFP fusion proteins containingmutations in the cluster of basic amino acids in the hinge (RKRARto AAAAA) (HPV-11 genomic nucleotides 3434 to 3458, correspondingto amino acid residues 238 to 242) were constructed by PCR-mediatedsite-directed mutagenesis. Fusion junctions and mutations wereconfirmed by DNA sequence analyses of up to 400 bases around thesite of interest. All constructs expressed proteins of the anticipatedmolecular masses in a Western blot.

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FIG. 1. Schematic representations of the GFP fusion proteins. The full-length HPV-11 E2 protein consists of the N, H, and C domains, each denoted by a different boxed symbol. The amino acid residues of the E2 protein expressed in each fusion protein are indicated. Mutations of the H domain are also illustrated. The GFP moiety is placed at the amino terminus of each fusion protein and is represented by an oval. The calculated molecular masses (kilodaltons) are given at the right; * signifies the dimeric form of the protein when the C domain is present.

Cell cultures and transient transfections. The simian virus 40-transformed monkey kidney epithelial cell line COS-7, adenovirus-transformed human kidney epithelial cellline 293, and human cervical carcinoma cell line C33A were maintainedin Dulbecco's modified Eagle's medium supplemented with 10% fetalbovine serum. Cells were grown at 37°C under 5% CO₂. Plasmidswere electroporated into 5 × 10⁶ human 293 cells at 960 µF and 180 V or into COS-7 and C33A cellsat 960 µF and 170 V (8). After electroporation, the cells werepelleted through 10 ml of medium, resuspended in fresh medium,and plated on 22- by 22-mm glass coverslips at a concentrationof 2 × 10⁵ per coverslip or on 60-mm plates at 5 × 10⁵ per plate and grown at 37°C for 24 or 48 h as specified for eachexperiment.

Transient HPV DNA replication and transcription regulation assays. Transient replication assays were performed as described elsewhere (8). Briefly, 0.5 µg of HPV-11 origin-containing plasmidp7730-99 (HPV-11 nucleotides 7730 to 7933 and 1 to 99), 5 µg ofan HPV-11 E1 protein expression vector (pMT2-11E1*) (70), and5 µg of an HPV-11 E2 protein expression vector (pMT2-11E2) (8),or alternatively 10 µg of pEGFP-E2, pEGFP-E2bm, or pEGFP thatexpressed the GFP-E2 fusion protein (here called gfpE2), gfpE2with mutations in the basic region of the hinge, or GFP, werecotransfected by electroporation into 5 × 10⁶ 293 cells, and half of the cells were cultured on a 100-mm-diameterplate for 48 h. Low-molecular-weight DNA was harvested via Hirtlysis as described elsewhere (8). Half of the DNA was subjectedto HindIII digestion, which linearizes pMT2-11E1*, pMT2-11E2,and p7730-99 but does not cut the pEGFP plasmids. The other halfwas digested with HindIII and DpnI, which cuts the unreplicatedinput plasmid DNA into small pieces. The digestion mixtures wereresolved by electrophoresis through 0.8% agarose gels, blottedonto nylon membranes, probed with [³²P]dCTP-labeled origin-containing plasmid, and documented by autoradiography.To perform the transcription regulation assay, 1 µg of pURR-LacZ,a plasmid which contains the bacterial lacZ gene driven by theHPV-11 URR-E6 promoter (50), was cotransfected into 293 cellswith 10 µg of vector, pMT2-11 E2, pEGFP-E2, or pEGFP-E2bm. After24 h, $beta$ -galactosidase activity was determined with an assay kit(Promega, Madison, Wis.).

Immunofluorescence detection of E1 and E2 proteins. Indirect immunofluorescence to detect the HPV-11 E1 protein was conducted as described previously (61), with slight modifications(14). Briefly, the transfected cells were grown on glass coverslipsfor 24 h, fixed with 1% paraformaldehyde in phosphate-bufferedsaline (PBS), washed three times with PBS containing 200 mM glycine,and then incubated with monoclonal antibody against the EE epitope(21) at a 1:500 dilution at room temperature for 2 h. Goat anti-mouseantibody conjugated with Texas red fluorophor (Southern BiotechnologyAssociates, Birmingham, Ala.) was used as the secondary antibodyat a 1:500 dilution. Incubation was conducted at room temperatureovernight, followed by extensive washing with PBS. Coverslipswere mounted on slides with DAPI (4',6-diamidino-2-phenylindole)-containingmounting medium (Vector Laboratories, Inc., Burlingame, Calif.).E1 protein was revealed by Texas red, and E2 was visualized viaGFP by using an Olympus IX70 fluorescence microscope, appropriatenarrow-band-pass filters, and a SenSys digital imagingcamera.

Subcellular fractionation. In situ fractionation was modified from the protocol described by McNeil et al. (46). Briefly, monolayer COS-7 cells transfectedwith expression plasmid were cultured on petri plates or coverslipsfor 24 h. Cells were then washed with PBS and extracted successivelyto generate various subcellular fractions as follows. The cytoplasmicfraction was obtained after incubation for 60 s on ice in CSKbuffer [10 mM piperazine-N,N'-bis(2-ethanesulfonic acid) (PIPES;pH 6.8), 300 mM sucrose, 100 mM NaCl, 3 mM MgCl₂, 1 mM EGTA] containing0.1% Triton X-100. The remaining material was washed once withcold PBS. An extraction solution containing 0.5% Triton X-100in CSK buffer was added and incubated on ice for 10 to 20 min.This solution was collected as the nucleoplasm fraction. Afterwashing with PBS, the residual nuclear structures, still attachedto the substratum, were incubated with DNase I at 100 µg/ml inCSK buffer at room temperature or 37°C for 15 min and then wereextracted in the same solution adjusted to 0.25 M (NH₄)₂SO₄ for10 min on ice or at room temperature. This solution was then collectedas the chromatin fraction. After final washing, residues lefton the substrate were NMs. To visualize directly the distributionof GFP fusion proteins after each extraction, the coverslips werefixed with 4% paraformaldehyde for 15 min and mounted on slideswith DAPI-containing mountingmedium.

For Western blots, the cytosol, nucleoplasm, and chromatin fractions were collected as described above. The whole cell extractand NM fraction on the substratum were solubilized in TES buffer(1% sodium dodecyl sulfate [SDS], 2 mM EDTA, 20 mM Tris-HCl [pH7.4]). Immunoblot analyses were performed after polyacrylamidegel electrophoresis (PAGE) through SDS-10% polyacrylamide gels.GFP and gfpE2 fusion proteins were detected with a monoclonalantibody against GFP at a 1:1,000 dilution (Clontech, Inc., PaloAlto, Calif.). Histone H1 and lamin A and C antibodies (SantaCruz Biotechnology, Santa Cruz, Calif.) were used at a 1:1,000dilution.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

GFP-tagged full-length E2 protein functions similarly to the native E2. We previously demonstrated that the HPV-18 glutathione S-transferase-E2 fusion protein can support cell-free HPV origin-specificreplication in the presence of HPV-18 E1 protein (34), indicatingthat it is possible for the E2 protein to accommodate a relativelylarge addition at its amino terminus without losing functions.To track the localization of HPV-11 E2 protein and to facilitateits subsequent genetic dissection into functional domains, wecreated gfpE2, a recombinant expression clone that encodes thefull-length HPV-11 E2 protein fused in frame to the carboxyl terminusof an enhanced GFP (Fig. 1). The GFP fusion proteins would bypassthe dependence on our polyclonal E2 antibody, which requires permeabilizationof the cell membrane and might recognize various E2 domains withdifferent efficiencies, thus confounding theanalyses.

To ascertain that the GFP moiety does not interfere with E2 protein functions, we tested the ability of gfpE2 to support HPV-11origin-dependent replication in the presence of HPV-11 E1 proteinin transiently transfected 293 cells. gfpE2 yielded a level ofreplication comparable to that of the wild-type E2 protein (Fig.2A, compare lanes 3 and 4 with lanes 1 and 2). In the presenceof E1 and GFP, no replication was observed (Fig. 2A, lanes 7 and8). In transfected COS-7 or C33A cells, gfpE2 colocalized withE1 protein to subnuclear foci in patterns identical to the previouslyreported replication complexes (61) (Fig. 3D and data not shown).Furthermore, the fusion protein was able to repress the HPV-11enhancer-E6 promoter activity to an extent similar to that imposedby the wild-type E2 (Fig. 2B). Thus, fusion to GFP does not significantlyaffect subnuclear localization or the replication and transcriptionfunctions of the E2 protein.

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FIG. 2. Regulatory functions of gfpE2 and gfpE2bm. (A) Transient replication of HPV-11 origin (ori) plasmid p7730-99 in the presence of HPV-11 E1 plus E2 (lanes 1 and 2), gfpE2 (lanes 3 and 4), gfpE2bm (lane 5 and 6), or GFP (lanes 7 and 8) expression vectors. An autoradiogram of one of two experiments reveals HindIII-linearized, total origin-containing DNA prior to DpnI digestion (lanes 1, 3, 5, and 7) and replicated, origin-containing DNA after DpnI digestion (lanes 2, 4, 6, and 8). (B) Repression of the HPV-11 URR-E6 promoter-driven lacZ reporter by E2, gfpE2, or gfpE2bm in transfected cells. The results shown were averages of two separate experiments, each performed in duplicate. Both functional assays were conducted in 293 cells as described in Materials and Methods.

The H region is required for exclusive nuclear localization. To determine the E2 domain responsible for its nuclear localization, we constructed a panel of GFP fusion proteins with oneor two of the three functional domains, each fused to the C terminusof GFP and designated gfpN, gfpH, gfpC, gfpNH, gfpHC, or gfpNC(Fig. 1). The calculated molecular mass or that of a dimer forfusion protein containing the C domain is also presented in Fig.1. The boundaries of the domains are based on a sequence alignmentof the E2 proteins of a large number of papillomavirus types aswell as the coding region of the E4 protein, which coincides withthe E2 H domain in a different reading frame (12, 48, 69).

COS-7 cells were transiently transfected with the expression plasmid for each fusion protein and, after 24 h of incubation,were fixed with paraformaldehyde. The cellular localization ofeach fusion protein was visualized directly via GFP with a fluorescencemicroscope, while nuclei were revealed by the fluorescence ofDAPI contained in the mounting medium (Fig. 3A). The same subcellulardistribution was observed in 293 and C33A cells. The examplesshown are for COS-7 cells because, of the three cells lines tested,COS-7 is the most suitable for in situ subcellular fractionation(described below); 293 cells do not attach to substrates securelyenough to allow fractionation, while C33A cells have a low transfectionefficiency such that the percentage of GFP-positive cells andthe signal intensities were low and not optimal for subcellularfractionation.

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FIG. 3. Localization of GFP and GFP fusion proteins as visualized microscopically via GFP fluorescence. (A and C) Subcellular distribution of GFP and GFP fusion proteins in whole cells as indicated in each panel. COS cells were transfected with various expression vectors; 24 h posttransfection, cells were fixed with paraformaldehyde and treated with a mounting medium containing DAPI to reveal their nuclei. (B) Typical patterns of GFP fluorescence which remained in transfected COS-7 cells after in situ fractionation as described in Materials and Methods. (D and E) Typical COS-7 cells cotransfected with an origin-containing plasmid and plasmids expressing EE-E1 and gfpE2 (D) or gfpE2bm (E). E2 was directly visualized via GFP (left). The EE-E1 protein was revealed by the Texas red through indirect immunofluorescence after staining with a monoclonal antibody against the EE epitope (center). Merged images reveal colocalization (right). The images were acquired through a 40× (A and C) or 100× (B, D, and E) objective lens of a monochromatic camera, pseudo-colored, and digitally processed. Relative to panels A and C, images in panels B, D, and E have been enlarged to reveal detailed subnuclear structures.

The results are presented in Fig. 3A. Of all the fusion proteins, the signals from gfpE2, as well as the fraction of positivecells, were consistently the lowest. This low expression mightsuggest that E2 is unstable or overexpression is toxic to thecells. gfpE2 was detected virtually exclusively in the nucleusin a punctate pattern when visualized at a high magnificationas shown previously (61) (data not shown, but see Fig. 3B andD). In contrast, GFP alone was diffused throughout the cells.Unexpectedly, gfpN and gfpC fusion proteins were present in boththe cytoplasm and the nucleus, with a higher concentration inthe nucleus, indicative of an inward flux of the fusion proteinsto the nucleus greater than the outward flux. Since the calculatedmolecular masses of gfpN and dimerized gfpC are about 51 and 76kDa, respectively, near or above the approximately 45- to 60-kDalimit for passive diffusion through the nuclear pore complex,a weak NLS in the N and C domains or nuclear retention signalmay explain their biased subcellulardistribution.

Much to our surprise, virtually all of the 38-kDa gfpH was detected in the nucleus, with little or no cytoplasmic signals(Fig. 3A), indicating that the H, rather than N or C, domain containsa strong NLS or nuclear retention signal. To substantiate thisinterpretation, we expressed gfpNC, which has a molecular massof 120 kDa when dimerized. Highly efficient nuclear localizationsuch as that demonstrated by gfpE2 was abolished. Cytoplasmicdistribution of this protein ranged from very high to a levelsimilar to that exhibited by gfpN or gfpC. In contrast, when thehinge was linked to the N (gfpNH) or C (gfpHC) domain, strongand efficient nuclear localization was restored (Fig. 3A). Theformer has a molecular mass of 60 kDa, whereas the latter is 94kDa when dimerized, above the limit of passive diffusion intothe nucleus. Collectively, these results demonstrate that thehinge indeed confers highly effective nuclear localization toeach of the fusionproteins.

E2 nuclear foci are formed by association with NM. To ascertain whether the subnuclear foci observed with E2 and gfpE2 fusion proteins represent their association with NM, weexamined the partition of gfpE2 expressed in COS-7 cells. Thecells were fractionated while attached to the glass substratesby using an in situ protocol (46). Treatment with 0.5% TritonX-100 removed the cytoplasm, nuclear membrane, and soluble nucleoplasm,whereas chromatin and NM remained on the substrate as the insolublefraction. DNase I treatment and subsequent 0.25 M (NH₄)₂SO₄ extractionremoved chromatin, and only NM remained on the substrate. Thisfractionation protocol was confirmed by Western blotting of thevarious fractions of cells expressing GFP alone for the distributionof GFP, histone H1, and lamins A and C that represent the varioussubcellular fractions (reference 1 and references therein).GFP was detected only in the cytoplasm and nucleoplasm fractions,not in the chromatin or NM fraction (Fig. 4B, left panel). HistoneH1 was found only in the chromatin fraction, whereas lamins Aand C were restricted to the NM fraction (Fig. 4A).

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FIG. 4. Subcellular distribution of GFP and GFP fusion proteins as detected by immunoblotting. COS-7 cells were fractionated by an in situ protocol. The whole cell extracts (WC) as well as the sequentially collected cytoplasm (Cyt) and nucleoplasm (NP) or, alternatively, pooled cytoplasm and nucleoplasm (Ext), chromatin (Chr), and nuclear matrix (NM) fractions were solubilized in PAGE loading buffer, separated by SDS-PAGE, and Western blotted with a monoclonal antibody against H1 (A, left), lamins A and C (A, right), or GFP (B to D).

The partitioning of various GFP fusion proteins to the NM was then directly visualized with a fluorescence microscope afterin situ extraction (Fig. 3B). gfpE2 typically exhibited a punctatepattern in association with NM (Fig. 3B). The shape of the nucleuswas well preserved. The distribution of the gfpE2 fusion proteininto each subcellular fraction was further analyzed by SDS-PAGEand Western blotting with an antibody against GFP. In this andsubsequent Western blots, all of the antibody-reactive proteinsmigrated at the appropriate molecular masses of monomeric proteins.Virtually all of the gfpE2 was found in the NM fraction, whilethe cytoplasm, nucleoplasm, and chromatin fractions containedno detectable signal (Fig. 4B, right panel). Similar subcellularfractionation patterns were observed after Western blotting witha polyclonal antibody against E2 (data not shown). Collectively,these observations indicate that NM provides the basic structuralscaffold for the E2 protein subnuclear compartmentation and alsovalidate that direct visual inspection of the NM fraction is anaccurate means to assess the ability of GFP fusion proteins toassociate withNM.

gfpN and gfpH associate with the NM. To determine the E2 domain or domains required for the association with NM, the subcellular partitioning of GFP fusion proteinscontaining the individual E2 domains was examined following insitu fractionation as described above. Green fluorescence signalwas removed from all of the gfpC-transfected cells (Fig. 3B),and the result was confirmed by Western blotting (Fig. 4C). Onlytrace nonspecific green flluorescence signal was occasionallyobserved to associate with cell debris following in situ extraction.Similar background was also observed in cells expressing GFP aloneor other GFP fusion proteins, and it did not take on the shapeof a nucleus, as observed in cells expressing gfpE2, gfpN, orgfpH. About 90% of the gfpN- or gfpH-positive cells lost mostif not all of the green fluorescence after detergent extraction.These cells generally exhibited weaker signals before extraction.However, in the remaining 10% of GFP-positive cells that had relativelystrong signals before extraction, the fusion proteins were retainedon the NM (Fig. 3B). Consistent with the direct visualizationwith a fluorescence microscope, Western blot analysis revealedthat although a majority of gfpN and gfpH fusion proteins werepresent in the pooled cytoplasm and nucleoplasm fractions (Fig.4C, lanes labeled Ext), a small proportion was detected in theNM fraction. These results indicate that N and H domains can independentlyassociate with NM, but with a much reduced affinity relative tothe full-length E2protein.

A cluster of basic amino acids in the hinge region is critical for nuclear localization and NM association. To localize the sequence in the hinge region important for its nuclear localization and NM association, we used alignmentof the E2 hinge amino acid sequences of a large number of papillomavirusgenotypes (69). Although no extensive homology was found, thecentral portion of the E2 hinge of a number of mucosotropic HPVscontains three or four basic amino acids in close proximity, generallyflanked by proline and glycine residues (Fig. 5). In HPV-11, thissequence is PPRKRARPG (amino acid residues 236 to 244). To testwhether this region might be important for nuclear localization,we converted the basic amino acid residues to alanine (RKRAR toAAAAA) by site-directed mutagenesis in the context of gfpH aswell as gfpE2 (designated gfpHbm and gfpE2bm) (Fig. 1).

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FIG. 5. Alignment of a portion of the E2 H domain of 15 mucosotropic human and animal papillomaviruses spanning a cluster of basic amino acids residues. Pcpv, pigmy chimp papillomavirus; Rpv, rhesus monkey papillomavirus. Dashes represent gaps introduced for maximal alignment. The cluster of basic amino acids is marked by dots. The inner bracket denotes the pentapeptide mutated to alanine in the HPV-11 E2 fusion proteins. Note that the region is flanked by helix-breaking glycine and proline residues in many of the viruses (outer bracket).

These two fusion proteins were each transiently expressed in COS-7 cells. Both mutated proteins were efficiently expressed.gfpHbm was distributed in both the nucleus and cytoplasm (Fig.3C). In contrast, in the majority of the cells, gfpE2bm was detectedin the cytoplasm, although a small amount may have been locatedin the nucleus. We next examined by in situ fractionation whetherthis mutation affected NM association. Neither gfpHbm nor gfpE2bmwas associated with NM when probed by Western blotting (Fig. 4D)or viewed with a fluorescence microscope (data not shown). Collectively,these observations indicate that the cluster of basic amino acidsin the hinge is critical for nuclear localization and contributesto the binding to theNM.

A truncated hinge retains the NLS but no longer associates with NM. To delineate further the hinge region which contains the strong NLS and sequences that associate with NM, we expressed gfpH40.gfpH40 has a molecular mass of 33 kDa and contains amino acids(216 to 255) from the hinge region, including the basic peptideand the flanking proline and glycine residues (Fig. 1). In themajority of the transfected COS-7 cells, gfpH40 was primarilyobserved in the nucleus in a diffuse pattern with a much reducedcytoplasmic signal compared with gfpN or gfpC. However, significantcytoplasmic distribution was observed in some cells that overexpressedthe gfpH40 fusion protein (Fig. 3C). Upon in situ fractionation,all GFP signal was lost from the NM fraction when viewed witha fluorescence microscope (data not shown), similar to gfpC (Fig.3B). We thus conclude that this 40-amino-acid peptide still containsa strong NLS. However, an association with NM with an affinityhigh enough to be partially resistant to in situ fractionationrequires additional hinge region sequences. This loss of NM associationcould have contributed to their increased cytoplasmic distributionrelative togfpH.

Functional assays of gfpE2bm. We then tested whether gfpE2bm might retain any of the regulatory functions. When cotransfected with HPV-11 URR-lacZ, thismutation no longer repressed the URR promoter (Fig. 2B). Thisis not surprising considering that little or no gfpE2bm was transportedinto the nucleus (Fig. 3C). Unexpectedly, when cotransfected withE1 expression vector in a transient replication assay, a verysmall fraction of the mutated E2 colocalized with E1 in the nucleus.Despite a more abundant total E2 protein, the amount of nucleargfpE2bm was significantly reduced relative to gfpE2 (compare Fig.3D to E and 4B to D). Interestingly, this amount was sufficientto support transient replication (Fig. 2A).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The extensive amino acid sequence homology and functional conservation exhibited by E2 proteins encoded by different papillomavirustypes are largely limited to the N and C domains. Other than beingconsidered a flexible linker, the highly variable central hingeregion has not been shown to serve any critical function (19).While high-resolution structures of the separated N and C domainshave been determined by X-ray crystallography (5, 23-25), theH domain or the full-length E2 has not, presumably due to an unstructurednature of the hinge. Nonetheless, the BPV-1 E2 hinge region containsa number of regulatory phosphorylation sites, and mutations inthese sites affect the association of E2 with mitotic chromosomesand extrachromosomal copy number (35, 45).

In this study, we prepared a panel of GFP fusion proteins containing the full-length HPV-11 E2 or one or two of the domainsas a means to delineate those responsible for the nuclear localizationand subnuclear focus formation exhibited by the full-length E2protein. Our results demonstrate, unexpectedly, that the hingeregion of HPV-11 E2 protein has a previously unrecognized criticalfunction in conferring nuclear localization. In addition, theH and N domains each independently associate with apparently differentcomponents of NM. These functions of the hinge region may partlyexplain why all forms of E2 proteins naturally truncated by theuse of alternative promoters or mRNA splice sites retain the hingeregion, even though the C domain alone has the same E2BS bindingproperty as the full-length E2 protein, critical for their inhibitoryfunctions.

We showed that only the GFP fusion proteins containing the hinge domain are localized exclusively to the nucleus, whereassignificant amounts of fusion proteins that do not have the hingeare found in the cytoplasm (Fig. 3A). These results indicate thatthe hinge contains a strong NLS and that the putative NLS in theN and C domains, as inferred by sequence homology to the NLS ofBPV-1 E2, are insufficient for efficient nuclear localization.In fact, less gfpNC than either gfpN or gfpC was targeted to thenucleus, and in some cells it was virtually excluded from thenucleus. One possible explanation is that because of its largedimeric size (120 kDa), gfpNC is not efficiently transported intothe nucleus in the absence of a strong NLS. Alternatively, theremay be a mutual interference of the weak NLSs in the N and C domainswhen they are brought into close proximity. Masking of the NLSin the C domain has also been proposed to explain the cytoplasmicdistribution of BPV-1 E2 in which the N-terminal NLS is mutatedor deleted (57). However, this masking effect cannot accountfor the primarily cytoplasmic distribution of gfpE2bm in whichthe spacing between the N and C domains remains unchanged (Fig.3C).

Mutagenic studies of the H domain revealed that the cluster of basic amino acids conserved among many of the mucosotropicHPVs (Fig. 5) is a critical element of the strong NLS of the HPV-11E2 protein. Further truncation of the H domain localizes the strongNLS to a 40-amino-acid peptide spanning these basic amino acids,as this small fusion protein was transported to the nucleus almostas efficiently as the intact H domain (compare Fig. 3C andA).

Biochemical fractionation followed by in situ visualization or by Western blot analysis demonstrated that the great majorityof the gfpE2 protein is associated with NM (Fig. 3B and 4). Therefore,we suggest that the specific subnuclear foci observed with HPV-11E2 are at least in part due to its association with NM. A fractionof the BPV-1 E2 protein has also been found to partition intothe NM fraction (27). Similar analyses of GFP fusions with thevarious HPV-11 E2 domains showed that the N and H domains eachcontain sequences that associate with NM, whereas C does not (Fig.3B and 4C). Relative to the full-length E2, the affinity for NMwas dramatically reduced when either the N or H domain was absent,suggesting that N and H domains may function synergistically ratherthanadditively.

The cluster of basic amino acids in the hinge region is not only a critical element of the NLS but is also important for NMassociation, as gfpHbm failed to associate with NM upon extraction(Fig. 4D). However, these basic residues are not sufficient forNM association. Additional sequences in the hinge contribute tothis affinity. This interpretation is suggested by the analysisof gfpH40, which retains the cluster of basic residues. Althoughprimarily localized to the nucleus, gfpH40 was no longer associatedwith NM. Why was gfpE2bm unable to associate with NM, despitethe ability of the N domain alone to bind to NM (Fig. 3B, 4C,and 4D)? This is likely because the NLS is largely incapacitatedby the mutations in the hinge. When, at best, only a small amountof the mutated protein was transported into the nucleus, it wasno longer possible to detect the weakened association with NM.Collectively, these data suggest that at least two activitiesare required to account for the subnuclear compartmentation exhibitedby the full-length E2 protein. The first is a strong NLS whichresides in the H domain primarily within a 40-amino-acid peptidespanning the cluster of basic residues. The second is a high affinityfor NM, which requires both the N and Hdomains.

gfpE2bm no longer functioned as a transcription repressor or activator because little of this protein was able to find itsway into the nucleus (Figs. 2B, 3C, and 4D). Unexpectedly, however,a small fraction of gfpE2bm was clearly colocalized with E1 inthe nucleus (compare Fig. 3E and D). We suggest that this mutationis able to piggyback on the coexpressed E1 protein which is activelytransported into the nucleus (61), as has been reported forother NLS-defective proteins (29). However, relative to gfpE2,only a fraction of the gfpE2bm formed distinct foci. Much of itexhibited a diffuse pattern (compare Fig. 3D and E), consistentwith the abolished or diminished ability of gfpHbm and the N domainalone to associate with NM. Nevertheless, some of the mutatedprotein did associate with focal NM proteins via the N domainor via interaction with E1 (Fig. 3E) and supported transient replicationof the HPV-11 origin-containing plasmid (Fig. 2A). We suggestthat only a small amount of the E2 protein is sufficient to supportDNA replication. Consistent with this interpretation, in a titrationexperiment, transfection of reduced amounts of gfpE2 or gfpE2bmexpression vector in the presence of a constant amount of E1 expressionvector increased rather than decreased transient replication (datanot shown). However, it is not possible to compare the specificreplication activity of the mutation relative to the wild-typeE2 protein. This is because the fraction of cells that expressedthese two proteins and the amounts of proteins expressed or transportedinto the nucleus were not comparable (compare Fig. 3A to C, 3Dto E, and 4B to D). We speculate that in vivo, when E1 and E2proteins were expressed at reduced levels from their native promotercompared to transfected cells, the probability of nuclear transportof E2 by piggybacking on E1 would be significantly reduced andthis mutated virus might bedefective.

We propose that, as is the case with cellular nucleic acid metabolism, NM is where HPV DNA replication and mRNA transcriptiontake place. Since E2 protein plays critical roles in both processes,the nuclear localization and proper subnuclear compartmentationconferred by the H and N domains are integral to these diversefunctions. We note that the N domain alone typically exhibitsa punctate pattern, similar to that of full-length E2, whereasthe H domain usually assumes a more fibrous pattern (Fig. 3B).Collectively, these results suggest that the N and H domains interactwith different components of the NM. We suggest that the N domainplays a major role in selecting focal NM-associated proteins whereasthe H domain helps anchor the protein to thescaffold.

We have no information on the focal components to which the N domain associates, but there are a number of potential candidates.For instance, our recent immunofluorescence studies of HPV replicationcompartments in transfected cells demonstrated that PML (or promyelocyticoncogenic domains), a component of nuclear domains 10 (ND10),is partially redistributed and colocalizes with HPV-11 E1 andE2 proteins (61). This colocalization is independent of HPVDNA replication and is thus dictated by one or both viral proteins.A variety of other DNA viruses, such as adenoviruses, polyomaviruses,and herpesviruses, also target to or disrupt ND10. To date, thesignificance of these relationships is not understood (reviewedin reference 44). We also note that many of the transcriptionfactors that bind to HPV URR (references 50, 67, and 68and references therein) also associate with NM (65), as do atleast some cellular replication proteins, such as RPA (47),DNA polymerase $alpha$ /primase (reference 42 and references therein),and topoisomerase II (reviewed in reference 33). Interestingly,our recent data indicated that E2 protein binds to RPA via the70-kDa subunit and enhances the single-stranded DNA binding activitiesof both (Lee et al., unpublished data). E1 also binds to the sameRPA subunit (22) as well as to DNA polymerase $alpha$ /primase (3,13, 43, 49).

Based on the above observations, we propose a model for the mechanics of how the E2 protein of HPV-11 functions (Fig. 6);this hypothesis may extend to some of the other mucosotropic HPVs,in view of the conservation of the cluster of basic amino acidsin the hinge region. The hinge region is involved in active transportof the E2 protein into the nucleus and helps anchor the proteinto the nuclear scaffold. The relative lack of structure and apparentflexibility due to the high proline and glycine content of theH domain enable the E2 protein to adopt new conformations whenthe C domain secures viral DNA, while the N domain associateswith focally located NM-associated proteins. Once anchored tothe NM, the E2 protein and viral DNA can then interact with additionalmatrix-associated proteins or recruit additional proteins to thecomplex, resulting in the regulation of viral mRNA transcriptionand DNA replication.

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FIG. 6. A model for the structure and function of the dimeric HPV-11 E2 protein. The N domain (oval) binds to focal NM-associated proteins, while the flexible hinge (H; bold zig zag lines) helps anchor the protein by association with the fibrous matrix scaffold (thin lines). The C domain (fans) secures the supercoiled viral DNA (ribbon). The E2 protein and the viral DNA then interact with additional proteins on NM or recruit proteins to the matrix-bound DNA, leading to the regulation of viral mRNA transcription or DNA replication. The cluster of basic residues in the hinge is an important element for both nuclear localization and for NM association.

It is worth noting that papillomaviruses appear to use different NLS and NM attachment sequences to target E2 to the propernuclear loci. For instance, the hinge of BPV-1 E2 can be approximatelyaligned with that of a number of cutaneous animal and human papillomavirustypes but not with the mucosotropic HPVs (69). This lack ofhomology would perhaps explain the different NLS between HPV-11and BPV-1 E2 proteins (this work and reference 57). Similarly,only the full-length BPV-1 E2, not the other N-terminus-truncatedforms of E2, associates with NM (27). Our results are also differentfrom those for the mucosotropic HPV-16. When expressed in insectcells, the HPV-16 E2 peptide truncated of the C domain was foundin the cytoplasm, whereas the C domain peptide was found in boththe nucleus and the cytoplasm (54). We note that among the mucosotropicHPVs, HPV-16 has the least homology in the corresponding hingeregion, with only two basic residues (Fig. 5). This distinctionmay explain their different distribution in insect cells. Interestingly,the cutaneous HPV-5 E2 protein appears to have properties thatare similar partially to those of HPV-11 and partially to thoseof BPV-1 E2 proteins. It colocalizes with an mRNA splicing coactivatorin a speckled nuclear pattern (31), similar to the punctatenuclear pattern exhibited by HPV-11 E2 (reference 61 and thiswork). Since no common cellular antigens were used in their andour studies, it remains to be determined whether both E2 proteinsindeed associate with the same cellular proteins. As with BPV-1E2, the hinge of HPV-5 E2 had little homology to that of HPV-11E2. However, an HPV-5 E2 peptide lacking the hinge region is observedin the nucleus, but in a diffuse pattern (31). Evidently, theN or C domain or both of HPV-5 E2 contain the NLS, but the H domainappears to be critical to its association with NM, as it is forHPV-11E2.

It is intriguing that in all papillomaviruses, the hinge region overlaps and coincides with the coding region of the E4 proteinin a different translation frame. The E4 protein is very abundantin productively infected tissues (4). It is directly or indirectlyassociated with cytokeratins, but its precise function has yetto be defined (52). The E2 hinge and the E4 proteins of manypapillomaviruses have several features in common. Both are hypervariable.Both are rich in proline and glycine residues that are helix breakers,indicating that both are rather unstructured or flexible peptides.These properties apparently enable them to associate with theirrespective interacting protein partners in the nuclear or cytoplasmicskeletons (this work and reference 52). Both are also rich inserine and threonine residues, and some of these residues in HPV-1E4 and BPV-1 E2 are substrates for kinases (20, 35, 45).HPV-11 E2 protein is a substrate of cyclin E-, A-, or B-dependentkinases (CDKs) in vitro in a complex which also contains the HPV-11E1 protein (41). However, only cyclin E/cdk2 plays a uniquerole in initiation of replication that cannot be fulfilled byother CDKs (38). We note that several candidate CDK phosphorylationsites are located in the hinge region. Whether phosphorylationof these residues modulates the association with NM or its regulatoryfunctions in the context of the full-length E2 will be of interestfor futureinvestigations.

	ACKNOWLEDGMENTS

This research was supported by USPHS grants CA36200 and CA83679 and the Cystic Fibrosis Foundation. The Digital Imaging MicroscopyFacility was established with grant funds provided in large measuresby the UAB Health Services Foundation and by Oral Cancer ResearchCenter grant DE/CA11910.

The DNA sequence was determined by a core facility of the UAB Center for AIDSResearch.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biochemistry and Molecular Genetics, University of Alabama at Birmingham,510 McCallum Basic Health Sciences Building, 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 and Methods
Results
Discussion
References

1. Berezney, R., and X. Wei. 1998. The new paradigm: integrating genomic function and nuclear architecture. J. Cell. Biochem. Suppl. 30-31:238-242.

2. Blencowe, B. J., J. A. Nickerson, R. Issner, S. Penman, and P. A. Sharp. 1994. Association of nuclear matrix antigens with exon-containing splicing complexes. J. Cell Biol. 127:593-607[Abstract/Free Full Text].

3. 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].

4. Brown, D. R., M. T. Chin, and D. G. Strike. 1988. Identification of human papillomavirus type 11 E4 gene products in human tissue implants from athymic mice. Virology 165:262-267[CrossRef][Medline].

5. Bussiere, D. E., X. Kong, D. A. Egan, K. Walter, T. F. Holzman, F. Lindh, T. Robins, and V. L. Giranda. 1998. Structure of the E2 DNA-binding domain from human papillomavirus serotype 31 at 2.4 Å. Acta Crystallogr. Sect. D 54:1367-1376[CrossRef][Medline].

6. Chiang, C.-M., T. R. Broker, and L. T. Chow. 1991. An E1ME2C fusion protein encoded by human papillomavirus type 11 is a sequence-specific transcription repressor. J. Virol. 65:3317-3329[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. Chin, M. T., R. Hirochika, H. Hirochika, T. R. Broker, and L. T. Chow. 1988. Regulation of human papillomavirus type 11 enhancer and E6 promoter by activating and repressing proteins from the E2 open reading frame: functional and biochemical studies. J. Virol. 62:2994-3002[Abstract/Free Full Text].

10. Choe, J., P. Vaillancourt, A. Stenlund, and M. Botchan. 1989. Bovine papillomavirus type 1 encodes two forms of a transcriptional repressor: structural and functional analysis of new viral cDNAs. J. Virol. 63:1743-1755[Abstract/Free Full Text].

11. Chow, L. T., and T. R. Broker. 1994. Papillomavirus DNA replication. Intervirology 37:150-158[Medline].

12. Chow, L. T., M. Nasseri, S. M. Wolinsky, and T. R. Broker. 1987. Human papillomavirus types 6 and 11 mRNAs from genital condylomata acuminata. J. Virol. 61:2581-2588[Abstract/Free Full Text].

13. Conger, K. L., J.-S. Liu, S.-R. Kuo, L. T. Chow, and T. S.-F. Wang. 1999. Human papillomavirus DNA replication. Interactions between the viral E1 protein and two subunits of human DNA polymerase alpha/primase. J. Biol. Chem. 274:2696-2705[Abstract/Free Full Text].

14. Day, P. M., R. B. Roden, D. R. Lowy, and J. T. Schiller. 1998. The papillomavirus minor capsid protein, L2, induces localization of the major capsid protein, L1, and the viral transcription/replication protein, E2, to PML oncogenic domains. J. Virol. 72:142-150[Abstract/Free Full Text].

15. de Jong, L., M. A. Grande, K. A. Mattern, W. Schul, and R. van Driel. 1996. Nuclear domains involved in RNA synthesis, RNA processing, and replication. Crit. Rev. Eukaryotic Gene Expr. 6:215-246[Medline].

16. Demeret, C., C. Desaintes, M. Yaniv, and F. Thierry. 1997. Different mechanisms contribute to the E2-mediated transcriptional repression of human papillomavirus type 18 viral oncogenes. J. Virol. 71:9343-9349[Abstract].

17. Dong, G., T. R. Broker, and L. T. Chow. 1994. Human papillomavirus type 11 E2 proteins repress the homologous E6 promoter by interfering with the binding of host transcription factors to adjacent elements. J. Virol. 68:1115-1127[Abstract/Free Full Text].

18. Dostatni, N., P. F. Lambert, R. Sousa, J. Ham, P. M. Howley, and M. Yaniv. 1991. The functional BPV-1 E2 trans-activating protein can act as a repressor by preventing formation of the initiation complex. Genes Dev. 5:1657-1671[Abstract/Free Full Text].

19. Gauthier, J. M., J. Dillner, and M. Yaniv. 1991. Structural analysis of the human papillomavirus type 16-E2 transactivator with antipeptide antibodies reveals a high mobility region linking the transactivation and the DNA-binding domains. Nucleic Acids Res. 19:7073-7079[Abstract/Free Full Text].

20. Grand, R. J., J. Doorbar, K. J. Smith, I. Coneron, and P. H. Gallimore. 1989. Phosphorylation of the human papillomavirus type 1 E4 proteins in vivo and in vitro. Virology 170:201-213[CrossRef][Medline].

21. Grüssenmeyer, T., K. H. Scheidtmann, M. A. Hutchinson, W. Eckhart, and G. Walter. 1985. Complexes of polyoma virus medium T antigen and cellular proteins. Proc. Natl. Acad. Sci. USA 82:7952-7954[Abstract/Free Full Text].

22. Han, Y., Y. M. Loo, K. T. Militello, and T. Melendy. 1999. Interactions of the papovavirus DNA replication initiator proteins, bovine papillomavirus type 1 E1 and simian virus 40 large T antigen, with human replication protein A. J. Virol. 73:4899-4907[Abstract/Free Full Text].

23. Harris, S. F., and M. R. Botchan. 1999. Crystal structure of the human papillomavirus type 18 E2 activation domain. Science 284:1673-1677[Abstract/Free Full Text].

24. Hegde, R. S., and E. J. Androphy. 1998. Crystal structure of the E2 DNA-binding domain from human papillomavirus type 16: implications for its DNA binding-site selection mechanism. J. Mol. Biol. 284:1479-1489[CrossRef][Medline].

25. Hegde, R. S., A. F. Wang, S. S. Kim, and M. Schapira. 1998. Subunit rearrangement accompanies sequence-specific DNA binding by the bovine papillomavirus-1 E2 protein. J. Mol. Biol. 276:797-808[CrossRef][Medline].

26. Hirochika, H., R. Hirochika, T. R. Broker, and L. T. Chow. 1988. Functional mapping of the human papillomavirus type 11 transcriptional enhancer and its interaction with the trans-acting E2 proteins. Genes Dev. 2:54-67[Abstract/Free Full Text].

27. Hubbert, N. L., J. T. Schiller, D. R. Lowy, and E. J. Androphy. 1988. Bovine papilloma virus-transformed cells contain multiple E2 proteins. Proc. Natl. Acad. Sci. USA 85:5864-5868[Abstract/Free Full Text].

28. Ilves, I., S. Kivi, and M. Ustav. 1999. Long-term episomal maintenance of bovine papillomavirus type 1 plasmids is determined by attachment to host chromosomes, which is mediated by the viral E2 protein and its binding sites. J. Virol. 73:4404-4412[Abstract/Free Full Text].

29. Jans, D. A., and S. Hubner. 1996. Regulation of protein transport to the nucleus: central role of phosphorylation. Physiol. Rev. 76:651-685[Abstract/Free Full Text].

30. Kuo, S.-R., J.-S. Liu, T. R. Broker, and L. T. Chow. 1994. Cell-free replication of the human papillomavirus DNA with homologous viral E1 and E2 proteins and human cell extracts. J. Biol. Chem. 269:24058-24065[Abstract/Free Full Text].

31. Lai, M. C., B. H. Teh, and W. Y. Tarn. 1999. A human papillomavirus E2 transcriptional activator. The interactions with cellular splicing factors and potential function in pre-mRNA processing. J. Biol. Chem. 274:11832-11841[Abstract/Free Full Text].

32. Lambert, P. F., N. L. Hubbert, P. M. Howley, and J. T. Schiller. 1989. Genetic assignment of multiple E2 gene products in bovine papillomavirus-transformed cells. J. Virol. 63:3151-3154[Abstract/Free Full Text].

33. Larsen, A. K., A. Skladanowski, and K. Bojanowski. 1996. The roles of DNA topoisomerase II during the cell cycle. Prog. Cell Cycle Res. 2:229-239[Medline].

34. Lee, K.-Y., T. R. Broker, and L. T. Chow. 1998. Transcription factor YY1 represses cell-free replication from human papillomavirus origins. J. Virol. 72:4911-4917[Abstract/Free Full Text].

35. Lehman, C. W., and M. R. Botchan. 1998. Segregation of viral plasmids depends on tethering to chromosomes and is regulated by phosphorylation. Proc. Natl. Acad. Sci. USA 95:4338-4343[Abstract/Free Full Text].

36. Li, R., and M. R. Botchan. 1994. Acidic transcription factors alleviate nucleosome-mediated repression of DNA replication of bovine papillomavirus type 1. Proc. Natl. Acad. Sci. USA 91:7051-7055[Abstract/Free Full Text].

37. Lim, D. A., M. Gossen, C. W. Lehman, and M. R. Botchan. 1998. Competition for DNA binding sites between the short and long forms of E2 dimers underlies repression in bovine papillomavirus type 1 DNA replication control. J. Virol. 72:1931-1940[Abstract/Free Full Text].

38. Lin, B. Y., T. Ma, J.-S. Liu, S.-R. Kuo, G. Jin, T. R. Broker, J. W. Harper, and L. T. Chow. HeLa cells are phenotypically limiting in cyclin E/cdk2 for efficient human papillomavirus DNA replication. J. Biol. Chem., in press.

39. Liu, J.-S., S.-R. Kuo, T. R. Broker, and L. T. Chow. 1995. The functions of human papillomavirus type 11 E1, E2, and E2C proteins in cell-free DNA replication. J. Biol. Chem. 270:27283-27291[Abstract/Free Full Text].

40. Lusky, M., J. Hurwitz, and Y.-S. Seo. 1994. The bovine papillomavirus E2 protein modulates the assembly of but is not stably maintained in a replication-competent multimeric E1-replication origin complex. Proc. Natl. Acad. Sci. USA 91:8895-8899[Abstract/Free Full Text].

41. Ma, T., N. Zou, B.-Y. Lin, L. T. Chow, and J. W. Harper. 1999. Interaction between cyclin-dependent kinases and human papillomavirus replication-initiation protein E1 is required for efficient viral replication. Proc. Natl. Acad. Sci. USA 96:382-387[Abstract/Free Full Text].

42. Martelli, A. M., S. Capitani, and L. M. Neri. 1998. Prereplicative increase of nuclear matrix-bound DNA polymerase-alpha and primase activities in HeLa S3 cells following dilution of long-term cultures. J. Cell. Biochem. 71:11-20[CrossRef][Medline].

43. Masterson, P. J., M. A. Stanley, A. P. Lewis, and M. A. Romanos. 1998. A C-terminal helicase domain of the human papillomavirus E1 protein binds E2 and the DNA polymerase alpha-primase p68 subunit. J. Virol. 72:7407-7419[Abstract/Free Full Text].

44. Maul, G. G. 1998. Nuclear domain 10, the site of DNA virus transcription and replication. Bioessays 20:660-667[CrossRef][Medline].

45. McBride, A. A., and P. M. Howley. 1991. Bovine papillomavirus with a mutation in the E2 serine 301 phosphorylation site replicates at a high copy number. J. Virol. 65:6528-6534[Abstract/Free Full Text].

46. McNeil, S., B. Guo, J. L. Stein, J. B. Lian, S. Bushmeyer, E. Seto, M. L. Atchison, S. Penman, A. J. van Wijnen, and G. S. Stein. 1998. Targeting of the YY1 transcription factor to the nucleolus and the nuclear matrix in situ: the C-terminus is a principal determinant for nuclear trafficking. J. Cell. Biochem. 68:500-510[CrossRef][Medline].

47. Murti, K. G., D. C. He, B. R. Brinkley, R. Scott, and S. H. Lee. 1996. Dynamics of human replication protein A subunit distribution and partitioning in the cell cycle. Exp. Cell Res. 223:279-289[CrossRef][Medline].

48. Nasseri, M., R. Hirochika, T. R. Broker, and L. T. Chow. 1987. A human papilloma virus type 11 transcript encoding an E1E4 protein. Virology 159:433-439[CrossRef][Medline].

49. Park, P., W. Copeland, L. Yang, T. Wang, M. R. Botchan, and I. J. Mohr. 1994. The cellular DNA polymerase alpha-primase is required for papillomavirus DNA replication and associates with the viral E1 helicase. Proc. Natl. Acad. Sci. USA 91:8700-8704[Abstract/Free Full Text].

50. Parker, J. N., W. Zhao, K. J. Askins, T. R. Broker, and L. T. Chow. 1997. Mutational analyses of differentiation-dependent human papillomavirus type 18 enhancer elements in epithelial raft cultures of neonatal foreskin keratinocytes. Cell Growth Differ. 8:751-762[Abstract].

51. Pederson, T. 1998. Thinking about a nuclear matrix. J. Mol. Biol. 277:147-159[CrossRef][Medline].

52. Roberts, S., I. Ashmole, S. M. Rookes, and P. H. Gallimore. 1997. Mutational analysis of the human papillomavirus type 16 E1-E4 protein shows that the C terminus is dispensable for keratin cytoskeleton association but is involved in inducing disruption of the keratin filaments. J. Virol. 71:3554-3562[Abstract].

53. Rotenberg, M. O., L. T. Chow, and T. R. Broker. 1989. Characterization of rare human papillomavirus type 11 mRNAs coding for regulatory and structural proteins, using the polymerase chain reaction. Virology 172:489-497[CrossRef][Medline].

54. Sanders, C. M., P. L. Stern, and N. J. Maitland. 1995. Characterization of human papillomavirus type 16 E2 protein and subdomains expressed in insect cells. Virology 211:418-433[CrossRef][Medline].

55. Seo, Y.-S., F. Müller, M. Lusky, E. Gibb, H. Y. Kim, B. Phillips, and J. Hurwitz. 1993. Bovine papilloma virus (BPV)-encoded E2 protein enhances binding of E1 protein to the BPV replication origin. Proc. Natl. Acad. Sci. USA 90:2865-2869[Abstract/Free Full Text].

56. Silver, P. A. 1991. How proteins enter the nucleus. Cell 64:489-497[CrossRef][Medline].

57. Skiadopoulos, M. H., and A. A. McBride. 1996. The bovine papillomavirus type 1 E2 transactivator and repressor proteins use different nuclear localization signals. J. Virol. 70:1117-1124[Abstract].

58. Skiadopoulos, M. H., and A. A. McBride. 1998. Bovine papillomavirus type 1 genomes and the E2 transactivator protein are closely associated with mitotic chromatin. J. Virol. 72:2079-2088[Abstract/Free Full Text].

59. Spalholz, B. A., Y. C. Yang, and P. M. Howley. 1985. Transactivation of a bovine papilloma virus transcriptional regulatory element by the E2 gene product. Cell 42:183-191[CrossRef][Medline].

60. Stenlund, A. 1996. Papillomavirus DNA replication, p. 679-697. In M. L. DePamphilis (ed.), DNA replication in eukaryotic cells. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

61. Swindle, C. S., N. Zou, B. A. Van Tine, G. M. Shaw, J. A. Engler, and L. T. Chow. 1999. Human papillomavirus DNA replication compartments in a transient DNA replication system. J. Virol. 73:1001-1009[Abstract/Free Full Text].

62. Tan, S. H., L. E. Leong, P. A. Walker, and H. U. Bernard. 1994. The human papillomavirus type 16 E2 transcription factor binds with low cooperativity to two flanking sites and represses the E6 promoter through displacement of Sp1 and TFIID. J. Virol. 68:6411-6420[Abstract/Free Full Text].

63. Thierry, F., and M. Yaniv. 1987. The BPV1-E2 trans-acting protein can be either an activator or a repressor of the HPV18 regulatory region. EMBO J. 6:3391-3397[Medline].

64. Ustav, M., and A. Stenlund. 1991. Transient replication of BPV-1 requires two viral polypeptides encoded by the E1 and E2 open reading frames. EMBO J. 10:449-457[Medline].

65. van Wijnen, A. J., J. P. Bidwell, E. G. Fey, S. Penman, J. B. Lian, J. L. Stein, and G. S. Stein. 1993. Nuclear matrix association of multiple sequence-specific DNA binding activities related to SP-1, ATF, CCAAT, C/EBP, OCT-1, and AP-1. Biochemistry 32:8397-8402[CrossRef][Medline].

66. Yang, L., R. Li, I. J. Mohr, R. Clark, and M. R. Botchan. 1991. Activation of BPV-1 replication in vitro by the transcription factor E2. Nature 353:628-632[CrossRef][Medline].

67. Zhao, W., T. R. Broker, and L. T. Chow. 1997. Transcriptional activities of human papillomavirus type 11 promoter-proximal elements in raft and submerged cultures of foreskin keratinocytes. J. Virol. 71:8832-8840[Abstract].

68. Zhao, W., L. T. Chow, and T. R. Broker. 1999. A distal element in the HPV-11 upstream regulatory region contributes to promoter repression in basal keratinocytes of squamous epithelium. Virology 253:219-229[CrossRef][Medline].

69. Zhu, Q. L., T. F. Smith, E. J. Lefkowitz, L. T. Chow, and T. R. Broker. 1994. Nucleic acid and protein sequence alignments of human and animal papillomaviruses constrained by functional sites. University of Alabama at Birmingham.

70. Zou, N., J.-S. Liu, S.-R. Kuo, T. R. Broker, and L. T. Chow. 1998. The carboxyl-terminal region of the human papillomavirus type 16 E1 protein determines E2 protein specificity during DNA replication. J. Virol. 72:3436-3441[Abstract/Free Full Text].

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1.	Berezney, R., and X. Wei. 1998. The new paradigm: integrating genomic function and nuclear architecture. J. Cell. Biochem. Suppl. 30-31:238-242.
2.	Blencowe, B. J., J. A. Nickerson, R. Issner, S. Penman, and P. A. Sharp. 1994. Association of nuclear matrix antigens with exon-containing splicing complexes. J. Cell Biol. 127:593-607[Abstract/Free Full Text].
3.	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].
4.	Brown, D. R., M. T. Chin, and D. G. Strike. 1988. Identification of human papillomavirus type 11 E4 gene products in human tissue implants from athymic mice. Virology 165:262-267[CrossRef][Medline].
5.	Bussiere, D. E., X. Kong, D. A. Egan, K. Walter, T. F. Holzman, F. Lindh, T. Robins, and V. L. Giranda. 1998. Structure of the E2 DNA-binding domain from human papillomavirus serotype 31 at 2.4 Å. Acta Crystallogr. Sect. D 54:1367-1376[CrossRef][Medline].
6.	Chiang, C.-M., T. R. Broker, and L. T. Chow. 1991. An E1ME2C fusion protein encoded by human papillomavirus type 11 is a sequence-specific transcription repressor. J. Virol. 65:3317-3329[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.	Chin, M. T., R. Hirochika, H. Hirochika, T. R. Broker, and L. T. Chow. 1988. Regulation of human papillomavirus type 11 enhancer and E6 promoter by activating and repressing proteins from the E2 open reading frame: functional and biochemical studies. J. Virol. 62:2994-3002[Abstract/Free Full Text].
10.	Choe, J., P. Vaillancourt, A. Stenlund, and M. Botchan. 1989. Bovine papillomavirus type 1 encodes two forms of a transcriptional repressor: structural and functional analysis of new viral cDNAs. J. Virol. 63:1743-1755[Abstract/Free Full Text].
11.	Chow, L. T., and T. R. Broker. 1994. Papillomavirus DNA replication. Intervirology 37:150-158[Medline].
12.	Chow, L. T., M. Nasseri, S. M. Wolinsky, and T. R. Broker. 1987. Human papillomavirus types 6 and 11 mRNAs from genital condylomata acuminata. J. Virol. 61:2581-2588[Abstract/Free Full Text].
13.	Conger, K. L., J.-S. Liu, S.-R. Kuo, L. T. Chow, and T. S.-F. Wang. 1999. Human papillomavirus DNA replication. Interactions between the viral E1 protein and two subunits of human DNA polymerase alpha/primase. J. Biol. Chem. 274:2696-2705[Abstract/Free Full Text].
14.	Day, P. M., R. B. Roden, D. R. Lowy, and J. T. Schiller. 1998. The papillomavirus minor capsid protein, L2, induces localization of the major capsid protein, L1, and the viral transcription/replication protein, E2, to PML oncogenic domains. J. Virol. 72:142-150[Abstract/Free Full Text].
15.	de Jong, L., M. A. Grande, K. A. Mattern, W. Schul, and R. van Driel. 1996. Nuclear domains involved in RNA synthesis, RNA processing, and replication. Crit. Rev. Eukaryotic Gene Expr. 6:215-246[Medline].
16.	Demeret, C., C. Desaintes, M. Yaniv, and F. Thierry. 1997. Different mechanisms contribute to the E2-mediated transcriptional repression of human papillomavirus type 18 viral oncogenes. J. Virol. 71:9343-9349[Abstract].
17.	Dong, G., T. R. Broker, and L. T. Chow. 1994. Human papillomavirus type 11 E2 proteins repress the homologous E6 promoter by interfering with the binding of host transcription factors to adjacent elements. J. Virol. 68:1115-1127[Abstract/Free Full Text].
18.	Dostatni, N., P. F. Lambert, R. Sousa, J. Ham, P. M. Howley, and M. Yaniv. 1991. The functional BPV-1 E2 trans-activating protein can act as a repressor by preventing formation of the initiation complex. Genes Dev. 5:1657-1671[Abstract/Free Full Text].
19.	Gauthier, J. M., J. Dillner, and M. Yaniv. 1991. Structural analysis of the human papillomavirus type 16-E2 transactivator with antipeptide antibodies reveals a high mobility region linking the transactivation and the DNA-binding domains. Nucleic Acids Res. 19:7073-7079[Abstract/Free Full Text].
20.	Grand, R. J., J. Doorbar, K. J. Smith, I. Coneron, and P. H. Gallimore. 1989. Phosphorylation of the human papillomavirus type 1 E4 proteins in vivo and in vitro. Virology 170:201-213[CrossRef][Medline].
21.	Grüssenmeyer, T., K. H. Scheidtmann, M. A. Hutchinson, W. Eckhart, and G. Walter. 1985. Complexes of polyoma virus medium T antigen and cellular proteins. Proc. Natl. Acad. Sci. USA 82:7952-7954[Abstract/Free Full Text].
22.	Han, Y., Y. M. Loo, K. T. Militello, and T. Melendy. 1999. Interactions of the papovavirus DNA replication initiator proteins, bovine papillomavirus type 1 E1 and simian virus 40 large T antigen, with human replication protein A. J. Virol. 73:4899-4907[Abstract/Free Full Text].
23.	Harris, S. F., and M. R. Botchan. 1999. Crystal structure of the human papillomavirus type 18 E2 activation domain. Science 284:1673-1677[Abstract/Free Full Text].
24.	Hegde, R. S., and E. J. Androphy. 1998. Crystal structure of the E2 DNA-binding domain from human papillomavirus type 16: implications for its DNA binding-site selection mechanism. J. Mol. Biol. 284:1479-1489[CrossRef][Medline].
25.	Hegde, R. S., A. F. Wang, S. S. Kim, and M. Schapira. 1998. Subunit rearrangement accompanies sequence-specific DNA binding by the bovine papillomavirus-1 E2 protein. J. Mol. Biol. 276:797-808[CrossRef][Medline].
26.	Hirochika, H., R. Hirochika, T. R. Broker, and L. T. Chow. 1988. Functional mapping of the human papillomavirus type 11 transcriptional enhancer and its interaction with the trans-acting E2 proteins. Genes Dev. 2:54-67[Abstract/Free Full Text].
27.	Hubbert, N. L., J. T. Schiller, D. R. Lowy, and E. J. Androphy. 1988. Bovine papilloma virus-transformed cells contain multiple E2 proteins. Proc. Natl. Acad. Sci. USA 85:5864-5868[Abstract/Free Full Text].
28.	Ilves, I., S. Kivi, and M. Ustav. 1999. Long-term episomal maintenance of bovine papillomavirus type 1 plasmids is determined by attachment to host chromosomes, which is mediated by the viral E2 protein and its binding sites. J. Virol. 73:4404-4412[Abstract/Free Full Text].
29.	Jans, D. A., and S. Hubner. 1996. Regulation of protein transport to the nucleus: central role of phosphorylation. Physiol. Rev. 76:651-685[Abstract/Free Full Text].
30.	Kuo, S.-R., J.-S. Liu, T. R. Broker, and L. T. Chow. 1994. Cell-free replication of the human papillomavirus DNA with homologous viral E1 and E2 proteins and human cell extracts. J. Biol. Chem. 269:24058-24065[Abstract/Free Full Text].
31.	Lai, M. C., B. H. Teh, and W. Y. Tarn. 1999. A human papillomavirus E2 transcriptional activator. The interactions with cellular splicing factors and potential function in pre-mRNA processing. J. Biol. Chem. 274:11832-11841[Abstract/Free Full Text].
32.	Lambert, P. F., N. L. Hubbert, P. M. Howley, and J. T. Schiller. 1989. Genetic assignment of multiple E2 gene products in bovine papillomavirus-transformed cells. J. Virol. 63:3151-3154[Abstract/Free Full Text].
33.	Larsen, A. K., A. Skladanowski, and K. Bojanowski. 1996. The roles of DNA topoisomerase II during the cell cycle. Prog. Cell Cycle Res. 2:229-239[Medline].
34.	Lee, K.-Y., T. R. Broker, and L. T. Chow. 1998. Transcription factor YY1 represses cell-free replication from human papillomavirus origins. J. Virol. 72:4911-4917[Abstract/Free Full Text].
35.	Lehman, C. W., and M. R. Botchan. 1998. Segregation of viral plasmids depends on tethering to chromosomes and is regulated by phosphorylation. Proc. Natl. Acad. Sci. USA 95:4338-4343[Abstract/Free Full Text].
36.	Li, R., and M. R. Botchan. 1994. Acidic transcription factors alleviate nucleosome-mediated repression of DNA replication of bovine papillomavirus type 1. Proc. Natl. Acad. Sci. USA 91:7051-7055[Abstract/Free Full Text].
37.	Lim, D. A., M. Gossen, C. W. Lehman, and M. R. Botchan. 1998. Competition for DNA binding sites between the short and long forms of E2 dimers underlies repression in bovine papillomavirus type 1 DNA replication control. J. Virol. 72:1931-1940[Abstract/Free Full Text].
38.	Lin, B. Y., T. Ma, J.-S. Liu, S.-R. Kuo, G. Jin, T. R. Broker, J. W. Harper, and L. T. Chow. HeLa cells are phenotypically limiting in cyclin E/cdk2 for efficient human papillomavirus DNA replication. J. Biol. Chem., in press.
39.	Liu, J.-S., S.-R. Kuo, T. R. Broker, and L. T. Chow. 1995. The functions of human papillomavirus type 11 E1, E2, and E2C proteins in cell-free DNA replication. J. Biol. Chem. 270:27283-27291[Abstract/Free Full Text].
40.	Lusky, M., J. Hurwitz, and Y.-S. Seo. 1994. The bovine papillomavirus E2 protein modulates the assembly of but is not stably maintained in a replication-competent multimeric E1-replication origin complex. Proc. Natl. Acad. Sci. USA 91:8895-8899[Abstract/Free Full Text].
41.	Ma, T., N. Zou, B.-Y. Lin, L. T. Chow, and J. W. Harper. 1999. Interaction between cyclin-dependent kinases and human papillomavirus replication-initiation protein E1 is required for efficient viral replication. Proc. Natl. Acad. Sci. USA 96:382-387[Abstract/Free Full Text].
42.	Martelli, A. M., S. Capitani, and L. M. Neri. 1998. Prereplicative increase of nuclear matrix-bound DNA polymerase-alpha and primase activities in HeLa S3 cells following dilution of long-term cultures. J. Cell. Biochem. 71:11-20[CrossRef][Medline].
43.	Masterson, P. J., M. A. Stanley, A. P. Lewis, and M. A. Romanos. 1998. A C-terminal helicase domain of the human papillomavirus E1 protein binds E2 and the DNA polymerase alpha-primase p68 subunit. J. Virol. 72:7407-7419[Abstract/Free Full Text].
44.	Maul, G. G. 1998. Nuclear domain 10, the site of DNA virus transcription and replication. Bioessays 20:660-667[CrossRef][Medline].
45.	McBride, A. A., and P. M. Howley. 1991. Bovine papillomavirus with a mutation in the E2 serine 301 phosphorylation site replicates at a high copy number. J. Virol. 65:6528-6534[Abstract/Free Full Text].
46.	McNeil, S., B. Guo, J. L. Stein, J. B. Lian, S. Bushmeyer, E. Seto, M. L. Atchison, S. Penman, A. J. van Wijnen, and G. S. Stein. 1998. Targeting of the YY1 transcription factor to the nucleolus and the nuclear matrix in situ: the C-terminus is a principal determinant for nuclear trafficking. J. Cell. Biochem. 68:500-510[CrossRef][Medline].
47.	Murti, K. G., D. C. He, B. R. Brinkley, R. Scott, and S. H. Lee. 1996. Dynamics of human replication protein A subunit distribution and partitioning in the cell cycle. Exp. Cell Res. 223:279-289[CrossRef][Medline].
48.	Nasseri, M., R. Hirochika, T. R. Broker, and L. T. Chow. 1987. A human papilloma virus type 11 transcript encoding an E1E4 protein. Virology 159:433-439[CrossRef][Medline].
49.	Park, P., W. Copeland, L. Yang, T. Wang, M. R. Botchan, and I. J. Mohr. 1994. The cellular DNA polymerase alpha-primase is required for papillomavirus DNA replication and associates with the viral E1 helicase. Proc. Natl. Acad. Sci. USA 91:8700-8704[Abstract/Free Full Text].
50.	Parker, J. N., W. Zhao, K. J. Askins, T. R. Broker, and L. T. Chow. 1997. Mutational analyses of differentiation-dependent human papillomavirus type 18 enhancer elements in epithelial raft cultures of neonatal foreskin keratinocytes. Cell Growth Differ. 8:751-762[Abstract].
51.	Pederson, T. 1998. Thinking about a nuclear matrix. J. Mol. Biol. 277:147-159[CrossRef][Medline].
52.	Roberts, S., I. Ashmole, S. M. Rookes, and P. H. Gallimore. 1997. Mutational analysis of the human papillomavirus type 16 E1-E4 protein shows that the C terminus is dispensable for keratin cytoskeleton association but is involved in inducing disruption of the keratin filaments. J. Virol. 71:3554-3562[Abstract].
53.	Rotenberg, M. O., L. T. Chow, and T. R. Broker. 1989. Characterization of rare human papillomavirus type 11 mRNAs coding for regulatory and structural proteins, using the polymerase chain reaction. Virology 172:489-497[CrossRef][Medline].
54.	Sanders, C. M., P. L. Stern, and N. J. Maitland. 1995. Characterization of human papillomavirus type 16 E2 protein and subdomains expressed in insect cells. Virology 211:418-433[CrossRef][Medline].
55.	Seo, Y.-S., F. Müller, M. Lusky, E. Gibb, H. Y. Kim, B. Phillips, and J. Hurwitz. 1993. Bovine papilloma virus (BPV)-encoded E2 protein enhances binding of E1 protein to the BPV replication origin. Proc. Natl. Acad. Sci. USA 90:2865-2869[Abstract/Free Full Text].
56.	Silver, P. A. 1991. How proteins enter the nucleus. Cell 64:489-497[CrossRef][Medline].
57.	Skiadopoulos, M. H., and A. A. McBride. 1996. The bovine papillomavirus type 1 E2 transactivator and repressor proteins use different nuclear localization signals. J. Virol. 70:1117-1124[Abstract].
58.	Skiadopoulos, M. H., and A. A. McBride. 1998. Bovine papillomavirus type 1 genomes and the E2 transactivator protein are closely associated with mitotic chromatin. J. Virol. 72:2079-2088[Abstract/Free Full Text].
59.	Spalholz, B. A., Y. C. Yang, and P. M. Howley. 1985. Transactivation of a bovine papilloma virus transcriptional regulatory element by the E2 gene product. Cell 42:183-191[CrossRef][Medline].
60.	Stenlund, A. 1996. Papillomavirus DNA replication, p. 679-697. In M. L. DePamphilis (ed.), DNA replication in eukaryotic cells. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
61.	Swindle, C. S., N. Zou, B. A. Van Tine, G. M. Shaw, J. A. Engler, and L. T. Chow. 1999. Human papillomavirus DNA replication compartments in a transient DNA replication system. J. Virol. 73:1001-1009[Abstract/Free Full Text].
62.	Tan, S. H., L. E. Leong, P. A. Walker, and H. U. Bernard. 1994. The human papillomavirus type 16 E2 transcription factor binds with low cooperativity to two flanking sites and represses the E6 promoter through displacement of Sp1 and TFIID. J. Virol. 68:6411-6420[Abstract/Free Full Text].
63.	Thierry, F., and M. Yaniv. 1987. The BPV1-E2 trans-acting protein can be either an activator or a repressor of the HPV18 regulatory region. EMBO J. 6:3391-3397[Medline].
64.	Ustav, M., and A. Stenlund. 1991. Transient replication of BPV-1 requires two viral polypeptides encoded by the E1 and E2 open reading frames. EMBO J. 10:449-457[Medline].
65.	van Wijnen, A. J., J. P. Bidwell, E. G. Fey, S. Penman, J. B. Lian, J. L. Stein, and G. S. Stein. 1993. Nuclear matrix association of multiple sequence-specific DNA binding activities related to SP-1, ATF, CCAAT, C/EBP, OCT-1, and AP-1. Biochemistry 32:8397-8402[CrossRef][Medline].
66.	Yang, L., R. Li, I. J. Mohr, R. Clark, and M. R. Botchan. 1991. Activation of BPV-1 replication in vitro by the transcription factor E2. Nature 353:628-632[CrossRef][Medline].
67.	Zhao, W., T. R. Broker, and L. T. Chow. 1997. Transcriptional activities of human papillomavirus type 11 promoter-proximal elements in raft and submerged cultures of foreskin keratinocytes. J. Virol. 71:8832-8840[Abstract].
68.	Zhao, W., L. T. Chow, and T. R. Broker. 1999. A distal element in the HPV-11 upstream regulatory region contributes to promoter repression in basal keratinocytes of squamous epithelium. Virology 253:219-229[CrossRef][Medline].
69.	Zhu, Q. L., T. F. Smith, E. J. Lefkowitz, L. T. Chow, and T. R. Broker. 1994. Nucleic acid and protein sequence alignments of human and animal papillomaviruses constrained by functional sites. University of Alabama at Birmingham.
70.	Zou, N., J.-S. Liu, S.-R. Kuo, T. R. Broker, and L. T. Chow. 1998. The carboxyl-terminal region of the human papillomavirus type 16 E1 protein determines E2 protein specificity during DNA replication. J. Virol. 72:3436-3441[Abstract/Free Full Text].