Positively Charged Termini of the L2 Minor Capsid Protein Are Necessary for Papillomavirus Infection

doi:10.1128/JVI.75.21.10493-10497.2001

This Article

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

Services

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

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Roden, R. B. S.
	Articles by Schiller, J. T.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Roden, R. B. S.
	Articles by Schiller, J. T.

Previous Article | Next Article

Journal of Virology, November 2001, p. 10493-10497, Vol. 75, No. 21
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.21.10493-10497.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Positively Charged Termini of the L2 Minor Capsid Protein Are Necessary for Papillomavirus Infection

Richard B. S. Roden,¹^,²^,^* Patricia M. Day,² Brian K. Bronzo,¹ William H. Yutzy IV,¹ Yanqin Yang,¹ Douglas R. Lowy,² and John T. Schiller²

Department of Pathology, The Johns Hopkins University, Baltimore, Maryland 21205-2196,¹ and Laboratory of Cellular Oncology, National Cancer Institute, Bethesda, Maryland 20892-4040²

Received 6 June 2001/Accepted 2 August 2001

	ABSTRACT

Top Abstract Text References

Coexpression of bovine papillomavirus L1 with L2 mutants lacking either eight N-terminal or nine C-terminal amino acids thatencode positively charged domains resulted in wild-type levelsof viral genome encapsidation. Despite wild-type binding to thecell surface, the resulting virions were noninfectious. An L2mutant encoding a scrambled version of the nine C-terminal residuesrestored infectivity, in contrast to an L2 mutant encoding a scrambledversion of the N-terminalresidues.

	TEXT

Top Abstract Text References

The papillomavirus capsid comprises two genetically unrelated viral proteins called L1 and L2 (2) surrounding an ~8-kbcircular DNA genome bound to histones. L1 is able to self-assembleinto virus-like particles (VLPs), morphologically and immunologicallyvery similar to virions (5), that are both necessary and sufficientfor binding to the cell surface (14). When coexpressed withL1, L2 is incorporated into VLPs in a similar ratio to virionspurified from warts (6, 26). L1 expressed in trans in mammaliancells harboring episomal DNA forms virions (19), although L2dramatically (>50-fold) (23) increases the efficiency of DNAencapsidation (12, 16, 24). Using a series of L2 deletionmutants, we have recently identified two domains in bovine papillomavirustype 1 (BPV1) L2 that participate in the interaction with L1 (11).One maps to residues 129 to 246, near the middle of L2, whilethe other involves residues 384 to 460, near the C terminus ofL2. Each L1 interaction domain of L2 was found to also affectthe efficiency of viral genomeencapsidation.

The positively charged residues at the N and C termini of human papillomavirus type 6 (HPV6) L2 function as redundant nuclearlocalization signals (17); furthermore, the residues at theN terminus of HPV16 L2, but not those at the C terminus, bindto DNA in a sequence-independent manner in vitro (25). BPV1L2 is 469 amino acids long, with groups of positively chargedresidues at the extreme N terminus and the extreme C terminus.With the goal of directly assessing the role of the positivelycharged termini in the generation of infectious virions, we constructeda BPV1 L2 with a deletion of either amino acids 2 to 9 (L2 $Delta$ 2-9)or the final nine amino acids (L2 $Delta$ 461-469). We also constructeda mutant with a deletion of internal L2 residues 422 to 431 (L2 $Delta$ 422-431)to serve as a control. These deletion mutants were cloned intovector pSFV-1, from which recombinant defective Semliki Forestviruses (SFVs) encoding these deletion mutants were generated(12). The activities of the mutants were then tested in severalL2-dependent assays, including one forinfectivity.

To examine L1-L2 interactions, BHK21 cells were coinfected with recombinant SFVs that express L1 and each mutant L2 (12).Cell lysates were prepared 24 h postinfection, and sequentialimmunoprecipitations were performed initially with preimmune rabbitserum, then rabbit anti-BPV1 L1 VLP (5), and finally rabbitanti-BPV1 L2-6His (15). The presence of L2 in immunoprecipitateswas detected by Western blotting with monoclonal antibody C6 (7)(Fig. 1). When expressed alone, L2 was not immunoprecipitatedby rabbit anti-BPV1 L1 VLP (Fig. 1, lane 2). L2 was absent frompreimmune rabbit serum immunoprecipitates, thus demonstratingspecificity (not shown). The three L2 deletion mutants were immunoprecipitatedwith anti-L1 as for wild-type L2 (Fig. 1), demonstrating equivalentassociation with L1 for L2, L2 $Delta$ 2-9, L2 $Delta$ 461-469 and L2 $Delta$ 422-431.Furthermore, equivalent quantities of L2 were detected upon subsequentimmunoprecipitation with antiserum to six-histidine-tagged full-lengthL2 (L2-6His), confirming equivalent expression in each sample(not shown).

View larger version (35K):
[in this window]
[in a new window]

FIG. 1. Coimmunoprecipitation of BPV1 L2 deletion mutants with L1. BHK21 cells were coinfected with recombinant SFV expressing BPV1 L1 and L2 deletion mutants, and 24 h postinfection, the cells were harvested and lysed. Immunopreciptation was performed with preimmune serum (not shown) and then rabbit anti-BPV1 L1 VLP (lanes 1 to 5). L2 was detected by Western blotting with monoclonal antibody C6 in anti-L1 VLP immunoprecipitates from lysates containing L1 (lanes 1 and 3 to 5) and full-length L2 (lanes 1 and 2), L2 $Delta$ 2-9 (lane 3), L2 $Delta$ 422-431 (lane 4), and L2 $Delta$ 461-469 (lane 5).

Before examining their infectivity, we sought to verify that the mutants behaved similarly to the wild type in several biochemicalassays. We previously demonstrated that BPV1 L2 traffics to thesubnuclear domains termed promonocytic leukemia protein (PML)-oncogenicdomains (PODs), also referred to as ND10 (1). L2 can also inducethe POD localization of BPV1 L1 and E2, two proteins that exhibita diffuse nuclear pattern in the absence of L2. To analyze theirsubcellular localization, the BPV1 L2 N-terminal and C-terminaldeletion mutants were expressed in BPHE-1 cells by infection withrecombinant SFV. The BPHE-1 line was clonally derived from BPV1-infectedprimary hamster embryo cells; it contains 50 to 200 BPV1 episomesper cell, but fails to express detectable levels of the capsidproteins (1, 12, 22). The BPV1 L2 deletion mutant proteinswere immunohistochemically stained with rabbit antiserum to 6His-L2and visualized by confocal fluorescence microscopy, as describedpreviously (1). L2 $Delta$ 2-9 and L2 $Delta$ 461-469 accumulated in the nucleusand associated with PODs (as assessed by colocalization with anti-PMLmonoclonal antibody 5E10 staining) as for wild-type L2 (Fig. 2).Colocalization of deletion mutant and wild-type L2 with anti-E2monoclonal antibody B202 or with anti-L1 monoclonal antibody 5B6staining was also assessed. The L2 deletion mutants were foundto retain the ability to localize E2 and L1 to PODs (data notshown) as described for wild-type L2 (1).

View larger version (59K):
[in this window]
[in a new window]

FIG. 2. Colocalization of BPV1 L2 deletion mutants with PML. BPHE-1 cells were infected with the L2-SFV recombinants. The cells were fixed, and double-staining immunolocalization against the L2 proteins and PML was performed. Infection of cells with full-length L2 is shown in panels A and B, infection with L2 $Delta$ 2-9 is shown in panels C and D, and infection with L2 $Delta$ 461-469 is shown in panels E and F. The same field is shown in each pair of panels. Anti-L2 staining is shown in panels A, C, and E, and anti-PML staining is shown in panels B, D, and F.

The capacity of the three L2 deletion mutants to encapsidate the viral genome was determined. BPHE-1 cells were coinfectedwith recombinant SFV expressing BPV1 L1 and mutant L2. Thirtyhours postinfection, the cells were harvested and lysed. The capsidproteins were immunoprecipitated with rabbit anti-BPV1 VLP, andthe immunoprecipitates were treated with DNase I to eliminatenonencapsulated genomes. Crude extract of bovine wart was usedas a positive control. The amount of DNase I-resistant BPV1 genomepresent in the immunoprecipitates was assessed by Southern blotting(Fig. 3). Consistent with similar papillomavirus assembly systems(16, 23), DNase I-resistant BPV genome, migrating as supercoiledDNA, was readily recovered from immunoprecipitates of BPHE-1 cellsexpressing BPV1 L1 together with BPV1 L2, although not with HPV16L2 (Fig. 3). Wild-type levels of genome encapsidation were observedwhen BPV1 L1 was coexpressed with each of the three deletionsof L2. As negative controls, no DNase I-resistant BPV genome wasobserved in immunoprecipitates from BPHE-1 cells expressing eitherL1 or L2 alone (Fig. 3, lanes 2 and 3), although on extended exposure,a weak band could be seen for L1 only (at least 50-fold lowerthan for L1 and L2 together), but not L2 (data not shown).

View larger version (70K):
[in this window]
[in a new window]

FIG. 3. Encapsidation of the BPV1 genome by L1 and L2 deletion mutants in BPHE-1 cells. BPHE-1 cells, which harbor 50 to 200 BPV1 episomes per cell, were coinfected with recombinant SFV expressing BPV1 L1 and L2 deletion mutants, and 30 h postinfection, the cells were harvested and lysed. By using rabbit anti-BPV1 L1 VLP, L1 was immunoprecipitated from lysates containing L1 (lanes 2 and 4 to 8) and full-length L2 (lanes 3 and 4), full-length HPV16 L2 (lane 5), L2 $Delta$ 2-9 (lane 6), L2 $Delta$ 461-469 (lane 7), and L2 $Delta$ 422-431 (lane 8) or from crude extract of bovine wart (lane 9). The immunoprecipitates were treated with DNase I for 1 h and washed. Undigested DNA present in the immunoprecipitates was recovered and separated on a 0.8% agarose gel with a biotinylated HindIII digest of $lambda$ (lane 1). The presence of viral DNA was detected by Southern blotting with a biotinylated probe corresponding to the EcoRI-BamHI large fragment of the BPV1 genome.

Having found that the mutants behaved as did the wild type with regard to localization to PODs, recruitment of L1 and E2,and viral genome encapsidation, the ability of each L2 deletionmutant to produce infectious BPV was also determined. Each L2mutant was coexpressed with wild-type BPV1 L1 in BPHE-1 cellswith recombinant SFV (12), the BPHE-1 cells were harvested andlysed 30 h postinfection, and the resulting BPV1 infectivity inthe extracts was assayed by using in vitro focal transformationof C127C mouse fibroblasts (3). The focus-forming activityresulting from BPHE-1 extracts from cells coexpressing wild-typeL1 with the L2 $Delta$ 422-431 mutant was similar to that obtained fromextracts that coexpressed L1 with wild-type L2 (Table 1). Thisresult indicates that infectivity can be retained despite a 10-amino-aciddeletion in at least one region of L2. In contrast to L2 $Delta$ 422-431,neither L2 $Delta$ 2-9 nor L2 $Delta$ 461-469 generated infectious BPV1 when coexpressedwith L1 in BPHE-1 cells (Table 1). These results indicate thatcoexpression of L1 with L2 $Delta$ 2-9 or L2 $Delta$ 461-469 in BPHE-1 cells hasgenerated defective virions, thus implying a new role for L2 inviral infection.

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

TABLE 1. Generation of infectious BPV1 by coexpression of BPV1 L1 and L2 deletion mutants in BPHE-1 cells^a

One possible explanation for the lack of infectivity by L2 $Delta$ 2-9 or L2 $Delta$ 461-469 could be that the presence of mutant L2 in virionsmight have interfered with the efficiency of virion binding tocells. This possibility has become more plausible, following therecent demonstration that L2 alone is able to bind to cell surfacesin a sequence-dependent manner (4), although other studieshave suggested that L2 may function in a postbinding step (9,13-15, 20). To examine whether L2 $Delta$ 2-9 or L2 $Delta$ 461-469 in virionsmight interfere with binding to cell surfaces, L1 was coexpressedwith either L2, L2 $Delta$ 2-9, or L2 $Delta$ 461-469 in BPHE-1 cells. The resultantvirions were separated from pentamers and empty VLPs by rate zonalcentrifugation through a 20 to 40% (wt/vol) sucrose gradient for90 min at 160,000 x g at 4°C. Equivalent quantities of virionsor buffer alone were incubated with mouse C127C cells for 1 hat 4°C. The cells were washed, and bound virions were detectedby indirect immunofluorescence with monoclonal antibody 5B6 toL1. Levels of binding of L1/L2, L1/L2 $Delta$ 2-9, and L1/L2 $Delta$ 461-469 virionsto C127C cells were equivalent (Fig. 4A, B, and C, respectively),each forming a speckled pattern on the cell surface that was absentfrom control cells (Fig. 4D). The quality and quantity of theL1/L2, L1/L2 $Delta$ 2-9, and L1/L2 $Delta$ 461-469 virion preparations were verysimilar when compared by Western blot analysis with rabbit antiserumto BPV1 L1/L2 VLPs (Fig. 4E). Therefore, incorporation of theL2 deletion mutants into virions did not prevent them from bindingto cell surfaces, implying that the deletion mutants did not inducemisfolding of the virions and that the L2 termini function duringinfection after virion binding to cell surfaces.

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

FIG. 4. Binding of BPV1 virions containing L2 deletion mutants to the cell surface. L1 was coexpressed with recombinant SFV with either wild-type L2, L2 $Delta$ 2-9, or L2 $Delta$ 461-49 in BPHE-1 cells. Upon cell lysis by sonication, virions were separated from pentamers and empty VLPs by rate zonal centrifugation through a 20 to 40% (wt/vol) sucrose gradient for 90 min at 160,000 × g at 4°C. L1/L2 (A and E, lane 1), L1/L2 $Delta$ 2-9 (B and E, lane 2), and L1/L2 $Delta$ 461-49 (C and E, lane 3) virion preparations and buffer alone (D) were incubated at equivalent concentrations for 1 h at 4°C with mouse C127C cells. The cells were washed, and bound virions were detected by indirect immunofluorescence with monoclonal antibody 5B6 to L1. The quality and quantity of virion preparations was estimated by Western blot analysis with rabbit antiserum to BPV1 L1/L2 VLPs (E). In panel E, molecular masses are given to the left in kilodaltons.

It was also possible that the absence of charge resulting from deletion of the amino acids at the N or C terminus might accountfor the loss of infectivity. To examine this possibility, twoadditional mutants were generated. One encoded the N-terminalamino acids in scrambled form (L2mix2-9, which replaces MSARKRVKRwith MRVKSKRAR). The other encoded the 9 C-terminal amino acidsin scrambled form (L2mix461-469, which replaces RKRKKRKHA withKRKHRARKK). When L2mix461-469 was coexpressed with L1 in BPHE-1,the resulting extract was found to be as infectious as wild-typeL2 (Table 1). Thus, compared with the noninfectious L2 $Delta$ 461-469mutant, restoration of the positive charge at the L2 C terminus,even in scrambled form, was able to restore infectivity. SinceL2 $Delta$ 422-431 retains the ability to form infectious virions, thelength of L2 does not appear to be critical, but further testingof neutral or acid substitutions in residues 461 to 469 is warrantedto confirm the significance of the positive charge in infectivity.In contrast, the L2mix2-9 mutant, when coexpressed with L1 inBPHE-1, did not produce infectious virus. This negative resultsuggests that the extreme N terminus makes a sequence-specificcontribution toinfectivity.

In addition to its relationship to virion assembly (11, 12, 24), L2 in virions has been shown to participate in pseudoviralinfectivity in systems in which pseudovirions are formed in vitrowith either L1 alone or the combination of L1 and L2, with nakedreporter DNA that is either encapsidated or bound to the capsidsurface (4, 9, 18, 21). L2 is not absolutely necessaryfor infectivity in these systems, but its presence enhances theefficiency of infection. The presence of L2 enhances the infectivityof HPV33 pseudovirion generated in COS-7 cells by ~10-fold (19).When an L2 protein in which residues 108 to 111 have been mutatedis substituted for wild-type L2 in HPV16 L1/L2 pseudovirions,their infectivity approximates that of pseudovirions with onlyL1 (4). This suggests that the effect of L2 is mediated bysequences near the middle of L2 that are exposed at the capsidsurface (4).

We have in the current report identified a function for L2 in infectivity that also appears to be independent of the abilityof L2 to participate in virion assembly. The infectivity functionwas revealed by using two L2 deletion mutants, one lacking aminoacids 2 through 9 (L2 $Delta$ 2-9) and the other lacking the final nineC-terminal amino acids (L2 $Delta$ 461-469). Both mutants behaved as thewild type for each assay related to virion assembly, includingthe genome encapsidation assay, but both mutants were deficientfor infectivity. Since both mutant proteins retain the exposedL2 amino acids identified by Kawana et al. (4) as requiredfor the L2-dependent infectivity of the pseudovirions and bothmutant proteins appear to be incorporated into virions with thesame efficiency as wild-type L2, it is likely that the L2 infectivityfunction described here isdistinct.

Since both termini of L2 contain several positively charged amino acids, we assessed the possible role of the charge, ratherthan sequence, by reconstituting the charge at each terminus ofL2 with a scrambled version of the authentic peptide. Infectivitywas restored with the scrambled C-terminal mutant L2mix461-469,while the scrambled N-terminal mutant, L2mix2-9, remained deficientfor infectivity. Thus, at the C terminus, where 8 of the 9 aminoacids are charged, a positive charge seems to be the main determinantof infectivity. In contrast, sequence specificity at the N terminus,where only 5 of the 8 amino acids are charged, appears to be criticalforinfectivity.

We speculate that the function we have identified for L2 operates after the initial binding of virions to the cell surface.This inference is consistent with earlier studies, suggestingthat L1 is both necessary and sufficient for virion binding tocell surfaces (9, 13, 14, 20) and that L2-specific antibodiescan neutralize infection without inhibiting such binding (14,15). Since L2 alone can bind and enter cells (4), L2 maybind a secondary receptor. L2 also interacts in vitro throughpositively charged side chains with DNA independently of nucleotidesequence (8, 25), and L2 is associated with episomes in vivo(16). We therefore speculate that L2 may function in the uncoatingof virions and delivery of the viral genome to the nucleus, viaa combination of the putative L2 receptor and the positively chargedL2 termini bound to the viral genome (4, 25). During infectionby the papovavirus simian virus 40, cytoplasmic or nuclear microinjectionof antibody to the minor capsid protein VP3 can prevent infection(10), suggesting that this minor capsid protein targeted tothe nucleus could play a role in infection similar to that postulatedforL2.

	ACKNOWLEDGMENTS

We are most grateful to Elliot Androphy and the late Jian Zhou for providing monoclonal antibodies B202 and C6. We also thankCarl Olson for the bovine papillomavirus. We are grateful to JonYewdell, Jack Bennink, and the Laboratory of Viral Diseases atthe National Institutes of Health (NIH) for the use of their confocalmicroscope.

This work was supported by NIH intramural funding and grant 1 PO1 AI48203-01 to R.B.S.R., the Richard TeLinde endowment, andthe Cancer Research Institute (R.B.S.R.).

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Pathology, Room 656, Ross Research Building, The Johns Hopkins University,720 Rutland Ave., Baltimore, MD 21205-2196. Phone: (410) 502-5161.Fax: (410) 614-3548. E-mail: roden{at}jhmi.edu.

REFERENCES

Top
Abstract
Text
References

1. Day, P. M., R. B. S. 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].

2. Doorbar, J., and P. H. Gallimore. 1987. Identification of proteins encoded by the L1 and L2 open reading frames of human papillomavirus 1a. J. Virol. 61:2793-2799[Abstract/Free Full Text].

3. Dvoretzky, I., R. Shober, S. K. Chattopadhyay, and D. R. Lowy. 1980. A quantitative in vitro focus assay for bovine papilloma virus. Virology 103:369-375[CrossRef][Medline].

4. Kawana, Y., K. Kawana, H. Yoshikawa, Y. Taketani, K. Yoshiike, and T. Kanda. 2001. Human papillomavirus type 16 minor capsid protein L2 N-terminal region containing a common neutralization epitope binds to the cell surface and enters the cytoplasm. J. Virol. 75:2331-2336[Abstract/Free Full Text].

5. Kirnbauer, R., F. Booy, N. Cheng, D. R. Lowy, and J. T. Schiller. 1992. Papillomavirus L1 major capsid protein self-assembles into virus-like particles that are highly immunogenic. Proc. Natl. Acad. Sci. USA 89:12180-12184[Abstract/Free Full Text].

6. Kirnbauer, R., J. Taub, H. Greenstone, R. Roden, M. Dürst, L. Gissmann, D. R. Lowy, and J. T. Schiller. 1993. Efficient self-assembly of human papillomavirus type 16 L1 and L1-L2 into virus-like particles. J. Virol. 67:6929-6936[Abstract/Free Full Text].

7. Liu, W. J., L. Gissmann, X. Y. Sun, A. Kanjanahaluethai, M. Muller, J. Doorbar, and J. Zhou. 1997. Sequence close to the N-terminus of L2 protein is displayed on the surface of bovine papillomavirus type 1 virions. Virology 227:474-483[CrossRef][Medline].

8. Mallon, R. G., D. Wojciechowicz, and V. Defendi. 1987. DNA-binding activity of papillomavirus proteins. J. Virol. 61:1655-1660[Abstract/Free Full Text].

9. Muller, M., L. Gissmann, R. J. Cristiano, X.-Y. Sun, I. H. Frazer, A. B. Jenson, A. Alonso, H. Zentgraf, and J. Zhou. 1995. Papillomavirus capsid binding and uptake by cells from different tissues and species. J. Virol. 69:948-954[Abstract].

10. Nakanishi, A., J. Clever, M. Yamada, P. P. Li, and H. Kasamatsu. 1996. Association with capsid proteins promotes nuclear targeting of simian virus 40 DNA. Proc. Natl. Acad. Sci. USA 93:96-100[Abstract/Free Full Text].

11. Okun, M. M., P. M. Day, H. L. Greenstone, F. P. Booy, D. R. Lowy, J. T. Schiller, and R. B. S. Roden. 2001. L1 interaction domains of papillomavirus L2 necessary for viral genome encapsidation. J. Virol. 75:4332-4342[Abstract/Free Full Text].

12. Roden, R. B. S., H. L. Greenstone, R. Kirnbauer, F. P. Booy, J. Jessie, D. R. Lowy, and J. T. Schiller. 1996. In vitro generation and type-specific neutralization of a human papillomavirus type 16 virion pseudotype. J. Virol. 70:5875-5883[Abstract].

13. Roden, R. B. S., N. L. Hubbert, R. Kirnbauer, F. Breitburd, D. R. Lowy, and J. T. Schiller. 1995. Papillomavirus L1 capsids agglutinate mouse erythrocytes through a proteinaceous receptor. J. Virol. 69:5147-5151[Abstract].

14. Roden, R. B. S., R. Kirnbauer, A. B. Jenson, D. R. Lowy, and J. T. Schiller. 1994. Interaction of papillomaviruses with the cell surface. J. Virol. 68:7260-7266[Abstract/Free Full Text].

15. Roden, R. B. S., E. M. Weissinger, D. W. Henderson, F. Booy, R. Kirnbauer, J. F. Mushinski, D. R. Lowy, and J. T. Schiller. 1994. Neutralization of bovine papillomavirus by antibodies to L1 and L2 capsid proteins. J. Virol. 68:7570-7574[Abstract/Free Full Text].

16. Stauffer, Y., K. Raj, K. Masternak, and P. Beard. 1998. Infectious human papillomavirus type 18 pseudovirions. J. Mol. Biol. 283:529-536[CrossRef][Medline].

17. Sun, X. Y., I. Frazer, M. Muller, L. Gissmann, and J. Zhou. 1995. Sequences required for the nuclear targeting and accumulation of human papillomavirus type 6B L2 protein. Virology 213:321-327[CrossRef][Medline].

18. Touze, A., and P. Coursaget. 1998. In vitro gene transfer using human papillomavirus-like particles. Nucleic Acids Res. 26:1317-1323[Abstract/Free Full Text].

19. Unckell, F., R. E. Streeck, and M. Sapp. 1997. Generation and neutralization of pseudovirions of human papillomavirus type 33. J. Virol. 71:2934-2939[Abstract].

20. Volpers, C., F. Unckell, P. Schirmacher, R. E. Streeck, and M. Sapp. 1995. Binding and internalization of human papillomavirus type 33 virus-like particles by eukaryotic cells. J. Virol. 69:3258-3264[Abstract].

21. Yeager, M. D., M. Aste-Amezaga, D. R. Brown, M. M. Martin, M. J. Shah, J. C. Cook, N. D. Christensen, C. Ackerson, R. S. Lowe, J. F. Smith, P. Keller, and K. U. Jansen. 2000. Neutralization of human papillomavirus (HPV) pseudovirions: a novel and efficient approach to detect and characterize HPV neutralizing antibodies. Virology 278:570-577[CrossRef][Medline].

22. Zhang, Y.-L., A. Lewis, Jr., M. Wade-Glass, and R. Schlegel. 1987. Levels of bovine papillomavirus RNA and protein expression correlate with variations in the tumorigenic phenotype of hamster cells. J. Virol. 61:2924-2928[Abstract/Free Full Text].

23. Zhao, K. N., X. Y. Sun, I. H. Frazer, and J. Zhou. 1998. DNA packaging by L1 and L2 capsid proteins of bovine papillomavirus type 1. Virology 243:482-491[CrossRef][Medline].

24. Zhou, J., D. J. Stenzel, X. Y. Sun, and I. H. Frazer. 1993. Synthesis and assembly of infectious bovine papillomavirus particles in vitro. J. Gen. Virol. 74:763-768[Abstract/Free Full Text].

25. Zhou, J., X.-Y. Sun, K. Louis, and I. H. Frazer. 1994. Interaction of human papillomavirus (HPV) type 16 capsid proteins with HPV DNA requires an intact L2 N-terminal sequence. J. Virol. 68:619-625[Abstract/Free Full Text].

26. Zhou, J., X. Y. Sun, D. J. Stenzel, and I. H. Frazer. 1991. Expression of vaccinia recombinant HPV 16 L1 and L2 ORF proteins in epithelial cells is sufficient for assembly of HPV virion-like particles. Virology 185:251-257[CrossRef][Medline].

This article has been cited by other articles:

Florin, L., Becker, K. A., Lambert, C., Nowak, T., Sapp, C., Strand, D., Streeck, R. E., Sapp, M. (2006). Identification of a Dynein interacting domain in the papillomavirus minor capsid protein l2.. J. Virol. 80: 6691-6696 [Abstract] [Full Text]
Richards, R. M., Lowy, D. R., Schiller, J. T., Day, P. M. (2006). Cleavage of the papillomavirus minor capsid protein, L2, at a furin consensus site is necessary for infection. Proc. Natl. Acad. Sci. USA 103: 1522-1527 [Abstract] [Full Text]
Kamper, N., Day, P. M., Nowak, T., Selinka, H.-C., Florin, L., Bolscher, J., Hilbig, L., Schiller, J. T., Sapp, M. (2006). A Membrane-Destabilizing Peptide in Capsid Protein L2 Is Required for Egress of Papillomavirus Genomes from Endosomes. J. Virol. 80: 759-768 [Abstract] [Full Text]
Bossis, I., Roden, R. B. S., Gambhira, R., Yang, R., Tagaya, M., Howley, P. M., Meneses, P. I. (2005). Interaction of tSNARE Syntaxin 18 with the Papillomavirus Minor Capsid Protein Mediates Infection. J. Virol. 79: 6723-6731 [Abstract] [Full Text]
Fay, A., Yutzy, W. H. IV, Roden, R. B. S., Moroianu, J. (2004). The Positively Charged Termini of L2 Minor Capsid Protein Required for Bovine Papillomavirus Infection Function Separately in Nuclear Import and DNA Binding. J. Virol. 78: 13447-13454 [Abstract] [Full Text]
Darshan, M. S., Lucchi, J., Harding, E., Moroianu, J. (2004). The L2 Minor Capsid Protein of Human Papillomavirus Type 16 Interacts with a Network of Nuclear Import Receptors. J. Virol. 78: 12179-12188 [Abstract] [Full Text]
Day, P. M., Baker, C. C., Lowy, D. R., Schiller, J. T. (2004). Establishment of papillomavirus infection is enhanced by promyelocytic leukemia protein (PML) expression. Proc. Natl. Acad. Sci. USA 101: 14252-14257 [Abstract] [Full Text]
Yang, R., Yutzy, W. H. IV, Viscidi, R. P., Roden, R. B. S. (2003). Interaction of L2 with beta -Actin Directs Intracellular Transport of Papillomavirus and Infection. J. Biol. Chem. 278: 12546-12553 [Abstract] [Full Text]
Yang, R., Day, P. M., Yutzy, W. H. IV, Lin, K.-Y., Hung, C.-F., Roden, R. B. S. (2003). Cell Surface-Binding Motifs of L2 That Facilitate Papillomavirus Infection. J. Virol. 77: 3531-3541 [Abstract] [Full Text]
Bousarghin, L., Touze, A., Combita-Rojas, A.-L., Coursaget, P. (2003). Positively charged sequences of human papillomavirus type 16 capsid proteins are sufficient to mediate gene transfer into target cells via the heparan sulfate receptor. J. Gen. Virol. 84: 157-164 [Abstract] [Full Text]

This Article

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

Services

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

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Roden, R. B. S.
	Articles by Schiller, J. T.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Roden, R. B. S.
	Articles by Schiller, J. T.

1.	Day, P. M., R. B. S. 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].
2.	Doorbar, J., and P. H. Gallimore. 1987. Identification of proteins encoded by the L1 and L2 open reading frames of human papillomavirus 1a. J. Virol. 61:2793-2799[Abstract/Free Full Text].
3.	Dvoretzky, I., R. Shober, S. K. Chattopadhyay, and D. R. Lowy. 1980. A quantitative in vitro focus assay for bovine papilloma virus. Virology 103:369-375[CrossRef][Medline].
4.	Kawana, Y., K. Kawana, H. Yoshikawa, Y. Taketani, K. Yoshiike, and T. Kanda. 2001. Human papillomavirus type 16 minor capsid protein L2 N-terminal region containing a common neutralization epitope binds to the cell surface and enters the cytoplasm. J. Virol. 75:2331-2336[Abstract/Free Full Text].
5.	Kirnbauer, R., F. Booy, N. Cheng, D. R. Lowy, and J. T. Schiller. 1992. Papillomavirus L1 major capsid protein self-assembles into virus-like particles that are highly immunogenic. Proc. Natl. Acad. Sci. USA 89:12180-12184[Abstract/Free Full Text].
6.	Kirnbauer, R., J. Taub, H. Greenstone, R. Roden, M. Dürst, L. Gissmann, D. R. Lowy, and J. T. Schiller. 1993. Efficient self-assembly of human papillomavirus type 16 L1 and L1-L2 into virus-like particles. J. Virol. 67:6929-6936[Abstract/Free Full Text].
7.	Liu, W. J., L. Gissmann, X. Y. Sun, A. Kanjanahaluethai, M. Muller, J. Doorbar, and J. Zhou. 1997. Sequence close to the N-terminus of L2 protein is displayed on the surface of bovine papillomavirus type 1 virions. Virology 227:474-483[CrossRef][Medline].
8.	Mallon, R. G., D. Wojciechowicz, and V. Defendi. 1987. DNA-binding activity of papillomavirus proteins. J. Virol. 61:1655-1660[Abstract/Free Full Text].
9.	Muller, M., L. Gissmann, R. J. Cristiano, X.-Y. Sun, I. H. Frazer, A. B. Jenson, A. Alonso, H. Zentgraf, and J. Zhou. 1995. Papillomavirus capsid binding and uptake by cells from different tissues and species. J. Virol. 69:948-954[Abstract].
10.	Nakanishi, A., J. Clever, M. Yamada, P. P. Li, and H. Kasamatsu. 1996. Association with capsid proteins promotes nuclear targeting of simian virus 40 DNA. Proc. Natl. Acad. Sci. USA 93:96-100[Abstract/Free Full Text].
11.	Okun, M. M., P. M. Day, H. L. Greenstone, F. P. Booy, D. R. Lowy, J. T. Schiller, and R. B. S. Roden. 2001. L1 interaction domains of papillomavirus L2 necessary for viral genome encapsidation. J. Virol. 75:4332-4342[Abstract/Free Full Text].
12.	Roden, R. B. S., H. L. Greenstone, R. Kirnbauer, F. P. Booy, J. Jessie, D. R. Lowy, and J. T. Schiller. 1996. In vitro generation and type-specific neutralization of a human papillomavirus type 16 virion pseudotype. J. Virol. 70:5875-5883[Abstract].
13.	Roden, R. B. S., N. L. Hubbert, R. Kirnbauer, F. Breitburd, D. R. Lowy, and J. T. Schiller. 1995. Papillomavirus L1 capsids agglutinate mouse erythrocytes through a proteinaceous receptor. J. Virol. 69:5147-5151[Abstract].
14.	Roden, R. B. S., R. Kirnbauer, A. B. Jenson, D. R. Lowy, and J. T. Schiller. 1994. Interaction of papillomaviruses with the cell surface. J. Virol. 68:7260-7266[Abstract/Free Full Text].
15.	Roden, R. B. S., E. M. Weissinger, D. W. Henderson, F. Booy, R. Kirnbauer, J. F. Mushinski, D. R. Lowy, and J. T. Schiller. 1994. Neutralization of bovine papillomavirus by antibodies to L1 and L2 capsid proteins. J. Virol. 68:7570-7574[Abstract/Free Full Text].
16.	Stauffer, Y., K. Raj, K. Masternak, and P. Beard. 1998. Infectious human papillomavirus type 18 pseudovirions. J. Mol. Biol. 283:529-536[CrossRef][Medline].
17.	Sun, X. Y., I. Frazer, M. Muller, L. Gissmann, and J. Zhou. 1995. Sequences required for the nuclear targeting and accumulation of human papillomavirus type 6B L2 protein. Virology 213:321-327[CrossRef][Medline].
18.	Touze, A., and P. Coursaget. 1998. In vitro gene transfer using human papillomavirus-like particles. Nucleic Acids Res. 26:1317-1323[Abstract/Free Full Text].
19.	Unckell, F., R. E. Streeck, and M. Sapp. 1997. Generation and neutralization of pseudovirions of human papillomavirus type 33. J. Virol. 71:2934-2939[Abstract].
20.	Volpers, C., F. Unckell, P. Schirmacher, R. E. Streeck, and M. Sapp. 1995. Binding and internalization of human papillomavirus type 33 virus-like particles by eukaryotic cells. J. Virol. 69:3258-3264[Abstract].
21.	Yeager, M. D., M. Aste-Amezaga, D. R. Brown, M. M. Martin, M. J. Shah, J. C. Cook, N. D. Christensen, C. Ackerson, R. S. Lowe, J. F. Smith, P. Keller, and K. U. Jansen. 2000. Neutralization of human papillomavirus (HPV) pseudovirions: a novel and efficient approach to detect and characterize HPV neutralizing antibodies. Virology 278:570-577[CrossRef][Medline].
22.	Zhang, Y.-L., A. Lewis, Jr., M. Wade-Glass, and R. Schlegel. 1987. Levels of bovine papillomavirus RNA and protein expression correlate with variations in the tumorigenic phenotype of hamster cells. J. Virol. 61:2924-2928[Abstract/Free Full Text].
23.	Zhao, K. N., X. Y. Sun, I. H. Frazer, and J. Zhou. 1998. DNA packaging by L1 and L2 capsid proteins of bovine papillomavirus type 1. Virology 243:482-491[CrossRef][Medline].
24.	Zhou, J., D. J. Stenzel, X. Y. Sun, and I. H. Frazer. 1993. Synthesis and assembly of infectious bovine papillomavirus particles in vitro. J. Gen. Virol. 74:763-768[Abstract/Free Full Text].
25.	Zhou, J., X.-Y. Sun, K. Louis, and I. H. Frazer. 1994. Interaction of human papillomavirus (HPV) type 16 capsid proteins with HPV DNA requires an intact L2 N-terminal sequence. J. Virol. 68:619-625[Abstract/Free Full Text].
26.	Zhou, J., X. Y. Sun, D. J. Stenzel, and I. H. Frazer. 1991. Expression of vaccinia recombinant HPV 16 L1 and L2 ORF proteins in epithelial cells is sufficient for assembly of HPV virion-like particles. Virology 185:251-257[CrossRef][Medline].