Chimaeric human papillomavirus 16 l1 virus like particles and a method for preparing the particles

Abstract
The invention describes a method for producing a chimaeric human papillomavirus (HPV) L1 polypeptide containing a heterologous peptide, and in particular, a HPV L2 peptide. The method comprises the steps of introducing a DNA sequence coding for the heterologous peptide into a DNA sequence coding for the L1 polypeptide; introducing the DNA sequence including the sequences for the L1 polypeptide and heterologous peptide into a host cell in which the DNA sequence can be expressed; causing expression of the DNA sequence; and recovering the resulting chimaeric L1 polypeptide which includes the heterologous peptide. Typically, the nucleotides encoding the heterologous peptide replace the nucleotides of the L1 polypeptide at the point of insertion. The invention also describes a vector for use in the method, a host cell containing the vector, and a vaccine including the chimaeric HPV L1 polypeptide produced according to the method.
Description
BACKGROUND OF THE INVENTION

The invention relates to a method for preparing polypeptides, and in particular virus-like particles (VLPs) or capsomers of human papillomavirus.


The papillomaviruses are a group of small DNA viruses, which induce warts and other lesions in a variety of higher vertebrates including humans.


Papillomaviruses (PV) are members of the genus Papillomavirus, family Papillomaviridae, and contain a double stranded circular DNA genome with a typical size of 7 900 base pairs (Seedorf et al., 1985). All PVs have a similar genomic organisation, with an early gene region encoding proteins involved in DNA replication and cellular transformation, and a late region encoding the viral capsid proteins (FIG. 1). A non-coding region known as the long control region (LCR) contains control elements for transcription and replication.


Papillomaviruses encode two viral structural proteins, L1 and L2. The virion contains 360 L1 molecules arranged as 72 capsomers, each of which is a pentamer composed of five L1 molecules (Baker et al., 1991). The ratio of L1 to L2 molecules has been estimated as approximately 30:1 (Doobar et al., 1987), which suggests that each virion would contain approximately twelve L2 molecules. The greater number of L1 molecules per virion has led to L1 being referred to as the ‘major’ capsid protein and L2 being referred to as the ‘minor’ capsid protein.


HPV-16 L1 is encoded by a 1.518 kb gene, giving rise to a protein of 504 amino acids. L1 has a molecular weight of 55 to 58 kD (Browne et al., 1988). Domains of L1 are likely to mediate cell binding and to contain antigenic determinants mediating antibody and T cell immune responses to the virus.


Among the genital human papillomaviruses (HPVs), there are low risk HPVs (for example, HPV 6 and HPV 11) that cause genital warts and cervical lesions that usually regress or do not progress to malignancy, and high risk (or oncogenic) genotypes (for example, HPV 16 and HPV 18), which are associated with high-grade cervical lesions and carcinomas. HPVs have also been implicated as the etiological agents in several other anogenital and upper aerodigestive tract cancers (Breitburd et al., 1999). A compelling body of clinical, molecular, experimental and epidemiological evidence has established that certain HPV types are the main cause of cercal cancer (Lowy et al, 1994; IARC, 1995). HPV 16 is present in most cases of cervical cancer cases and an additional three types (HPV 18, 31 and 45) are present in approximately an additional 30% of cases (IARC, 1999).


Although the incidence of cervical cancer is decreasing in the US, it is the most common malignancy in women in developing countries, with about 500 000 new cases diagnosed each year.


Traditionally most prophylactic vaccines have consisted of live, attenuated virus or formalin inactivated virus. Papillomavirus virions are highly immunogenic, inducing high titres (>10 000) of neutralising antibodies when systemically inoculated (Doretzky et al., 1980; Kirnbauer et al., 1991, 1992). However, due to the difficulties and risks involved in generating large quantities of these traditional vaccines there has been great emphasis on the development of viral protein subunit or virus-like particle (VLP) vaccines.


The best candidate protein for a prophylactic vaccine against HPV is the major capsid protein L1, which self-assembles into VLPs (Schiller and Lowy, 2001). These VLPs are very well characterised, and morphologically appear indistinguishable from whole virions (Chen et al., 2001; Rose et al., 1993). Injection of VLPs into experimental animals induces neutralising antibodies (Rose et al., 1998); preliminary human trials of injected VLP vaccines have also shown that these are well tolerated and highly immunogenic, and in the former case, stimulated robust B and T cell responses (Evans et al., 2001; Harro et al., 2001).


An effective, cheap prophylactic vaccine against oncogenic types of mucotropic HPVs could potentially have an impact on the world cancer burden, especially against HPV 16.


A common-neutralizing epitope for HPV types 6 and 16 has been found in the region (aa) 108-120 of the HPV 16 minor capsid protein, L2 (Kawana et al., 1998, 1999). Balb/c mice that were nasally immunised with a synthetic peptide corresponding to the epitope elicited an immune response that resulted in IgA and IgG antibodies cross-reacting with L1/L2 capsids of HPV 6, 16 and 18 (Kawana et al., 2001). Immunisation of rabbits with either of two overlapping peptides derived from the L2 sequence region 94-122 from either Rabbit oral papillomavirus (ROPV) or Cotttontail rabbit papillomavirus (CRPV) resulted in sera which reacted to purified cognate L2, specifically recognised L2 in infected cells, and neutralised virus in vitro. Rabbits immunised with CRPV peptides were immune to CRPV challenge (Embers et al., 2002).


The inventors therefore decided to further investigate the presentation of this L2 epitope on chimaeric L1 VLPs as a vaccine in its own right, and as a model for the presentation of other immunogenic peptide sequences.


SUMMARY OF THE INVENTION

According to a first embodiment of the invention, there is provided a method for producing a chimaeric human papillomavirus (HPV) L1 polypeptide containing a HPV L2 peptide, the method comprising the steps of:

    • introducing a DNA sequence coding for the L2 peptide into a DNA sequence coding for the L1 polypeptide;
    • introducing the DNA sequence including the sequences for the L1 polypeptide and L2 peptide into a host cell in which the DNA sequence can be expressed;
    • causing expression of the DNA sequence; and
    • recovering the resulting chimaeric L1 polypeptide which includes the L2 peptide.


The HPV L1 polypeptide and/or HPV L2 peptide may be a HPV-16 polypeptide or peptide.


The HPV L2 peptide may have the following amino acid sequence: LVEETSFIDAGAP (SEQ I.D. NO: 1), or a sequence which Is modification or derivative thereof, with the proviso that the modified or derived sequence is a sequence which has at least 80% homology to the sequence of SEQ l.D. NO:1 and codes for a peptide which elicits an immunogenic response against HPV.


One or more nucleotides of the L1 DNA sequence may be deleted at the point of introduction of the L2 DNA sequence, and typically the number of nucleotides deleted from the L1 sequence will correspond with the number of L2 nucleotides inserted.


The expression of the protein could either be in a prokaryotic or eukaryotic expression system.


The chimaeric polypeptide may have the amino acid sequence set out in any one of FIGS. 6, 8, 10, 12 and 14 (SEQ I.D. NOS: 5, 7, 9, 11 and 13), or a sequence which is at least 80% homologous to any one of the sequences set out in SEQ I.D. NOS: 5, 7, 9, 11 and 13 and which is capable of eliciting an immunogenic response against HPV. The DNA sequence coding for the chimaeric polypeptide may be the DNA sequence as set out in any one of FIGS. 5, 7, 9, 11 and 13 (SEQ I.D. NOS:4, 6, 8, 10 and 12), or a sequence having at least 80% homology to any one of these sequences and which codes for a polypeptide capable of eleiciting an immunogenic response against HPV.


The chimaeric L1 polypeptide may assemble into virus-like particles and/or capsomers. The virus-like particle or capsomer may be immunogenic.


According to a second embodiment of the invention, there is provided a chimaeric HPV L1 DNA sequence into which the DNA sequence coding for the above HPV L2 peptide has been inserted, the resulting HPV L1 sequence being capable of expressing the HPV L2 peptide.


One or more nucleotides of the L1 DNA sequence at the point of introduction of the L2 DNA sequence may be deleted, and typically the number of nucleotides deleted from the L1 sequence will correspond with the number of L2 nucleotides inserted.


The chimaeric nucleic acid sequence may be a sequence as set out in any one of FIGS. 5, 7, 9, 11 and 13, or a DNA sequence which is a modification or derivative thereof, with the proviso that the modified or derived DNA sequence has at least 80% homology to any one of the sequences of SEQ I.D. NOS: 4, 6, 8, 10 and 12 and codes for a chimaeric L1 peptide which is capable of eliciting an immunogenic response against HPV.


According to a third embodiment of the invention, there is provided a vector including the nucleic acid sequence described above.


According to a fourth embodiment of the invention, there is provided a host cell including the vector described above.


According to yet a further embodiment of the invention, there is provided a chimaeric HPV L1 polypeptide that Includes the above HPV L2 peptide (SEQ I.D. NO: 1).


The chimaeric polypeptide may be a chimaeric HPV L1 virus-like particle or capsomer.


According to a further embodiment of the invention, there is provided an HPV polypeptide having the amino acid sequence set out in any one of FIGS. 6, 8, 10, 12 and 14 (SEQ I.D. NOS: 5, 7, 9, 11 and 13), or a sequence which is a modification or derivative thereof, the modification or derivative being a sequence which is at least 80% homologous to any one of the sequences set out in SEQ I.D. NOS: 5, 7, 9, 11 and 13 and which is capable of eliciting an immunogenic response against HPV.


According to another embodiment of the invention, there is provided a method for producing a chimaeric human papillomavirus (HPV) L1 polypeptide containing a heterologous peptide, the method comprising the steps of:

    • introducing a DNA sequence coding for the heterologous peptide into a DNA sequence coding for the L1 polypeptide;
    • introducing the DNA sequence including the sequences for the L1 polypeptide and heterologous peptide into a host cell in which the DNA sequence can be expressed;
    • causing expression of the DNA sequence; and
    • recovering the resulting chimaeric L1 polypeptide which includes the heterologous peptide.


The heterologous peptide sequence may be any other HPV sequence, or may be derived from any antigenic epitope, B-cell or T-cell specific.


One or more nucleotides of the L1 DNA sequence at the point of introduction of the heterologous DNA sequence may be deleted, and typically the number of nucleotides deleted from the L1 sequence will correspond with the number of heterologous nucleotides inserted.


According to yet a further embodiment of the invention, there is provided a vaccine including the chimeeric HPV L1 polypeptide or a DNA sequence coding for the polypeptide, substantially as described above. The vaccine may be for prophylactic or therapeutic treatment of HPV infection, in particular HPV 6, 16 and 18.


Preferably, the vaccine will be capable of inducing an immunogenic response to HPV and to the introduced peptide in a suitable host.


The vaccine may further include a pharmaceutical excipient and/or adjuvant.




DESCRIPTION OF THE DRAWINGS


FIG. 1 shows a diagrammatic representation of the genomic organisation of HPV 16;



FIG. 2 shows the monomer structure of HPV 16 L1;



FIG. 3 shows the nucleotide sequence of the native sequence of the HPV 16 L1 gene into which the L2 epitope was inserted to produce the chimaeric constructs of FIGS. 5 to 14 (SEQ I.D. NO: 2);



FIG. 4 shows the amino acid sequence of FIG. 3 (SEQ I.D. NO: 3);



FIG. 5 shows the nucleotide sequence of chimaeric construct A (SEQ I.D. NO: 4);



FIG. 6 shows the amino acid sequence of chimaeric construct A (SEQ I.D. NO: 5);



FIG. 7 shows the nucleotide sequence of chimaeric construct C (SEQ I.D. NO: 6);



FIG. 8 shows the amino acid sequence of chimaeric construct C (SEQ I.D. NO: 7);



FIG. 9 shows the nucleotide sequence of chimaeric construct E (SEQ I.D. NO: 8);



FIG. 10 shows the amino acid sequence of chimaeric construct E (SEQ I.D. NO: 9);



FIG. 11 shows the nucleotide sequence of chimaeric construct F (SEQ I.D. NO: 10);



FIG. 12 shows the amino acid sequence of chimaeric construct F (SEQ I.D. NO: 11);



FIG. 13 shows the nucleotide sequence of chimaeric construct H (SEQ I.D. NO: 12);



FIG. 14 shows the amino acid sequence of chimaeric construct H (SEQ I.D. NO: 13);



FIG. 15 shows a diagrammatic representation of the chimaeric construct A;



FIG. 16 shows a diagrammatic representation of the chimaeric construct C;



FIG. 17 shows a diagrammatic representation of the chimaeric construct E;



FIG. 18 shows a diagrammatic representation of the chimaeric construct F;



FIG. 19 shows a diagrammatic representation of the chimaeric construct H;



FIG. 20 shows data obtained from end point titrations of mice inoculated with chimaeric VLPs obtained from construct A;



FIG. 21 shows data obtained from end point titrations of mice inoculated with chimaeric VLPs obtained from construct C;



FIG. 22 shows data obtained from end point titrations of mice inoculated with chimaeric VLPs obtained from construct E;



FIG. 23 shows data obtained from end point titrations of mice inoculated with chimaeric VLPs obtained from construct F;



FIG. 24 shows data obtained from end point titrations of mice inoculated with chimaeric VLPs obtained from construct H;



FIG. 25 shows data obtained from end point titrations of mice inoculated with VLPs obtained from a non-chimaeric HPV 16 L1 (SA-opt);



FIG. 26 shows the response of mice to boosters following initial immunisation;



FIG. 27 shows the nucleotide sequence of the L2 peptide which was inserted into the L1 sequence (SEQ I.D. NO: 14); and



FIG. 28 shows the amino acid sequence of the L2 peptide which was inserted into the L1 sequence (SEQ I.D. NO: 1).




DETAILED DESCRIPTION OF AN EMBODIMENT OF THE INVENTION

Design of Chimaeric Constructs


Primers encoding the peptide:

LVEETSFIDAGAP(SEQ I.D. NO:1)


which is a common-neutralising epitope for HPV 6 and 16 in the region (aa) 108-120 of the HPV minor capsid protein, L2, were synthesised.


According to the HPV 16 L1 monomer structure published by Chen et al. (2000) (FIG. 2), various surface loops and regions are exposed when pentamers and high order structures are formed.


Based on the epitope mapping of the V5 antibody (neutralising antibody raised to L1), various regions/loops were selected for the insertion of the L2 peptide so as to maintain the V5 antibody binding region of the L1 VLPs.


The major antigenic region (V5 binding region) of the L1 molecule has been mapped with amino acid residues A266, (with F50 being located beneath the surface residue V271) and S282 (Roden et al., 1996, White et al., 1999). Based on these residues, the inventors decided not to alter the B loop of the molecule, as this would alter the antigenic region and possibly destroy vital L1 epitopes.


The following L1 regions were therefore selected for insertion of the L2 peptide:

    • A: E-F loop (SEQ I.D. NO: 4 and 5)
    • C: D-E loop (SEQ I.D. NO: 6 and 7)
    • E: region between the h4 helix and J region of L1 (SEQ I.D. NO: 8 and 9)
    • F: h4 helix (SEQ I.D. NO: 10 and 11)
    • H: internal C-D loop (SEQ I.D. NO: 12 and 13)


      Synthesis of Chimaeric Constructs


Chimaeric constructs were prepared by PCR with the primers being designed with the 3′ end coding for the L2 peptide. The HPV 16 SA-opt L1 gene (FIGS. 3 and 4) cloned in the pSK plasmid vector was used as a template. The following DNA sequence was used to encode the L2 peptide:

(SEQ I.D. NO:14)5′-TTAGTGGAAGAAACTAGTTTTATTGATGCTGGTGCACCA-3′.


The L2 peptide was inserted into the gene by replacing the regions shown in Table 1. This method of replacing the existing nucleotides, rather than merely inserting the L2 nucleotides into the L1 sequence without any replacement, is advantageous in that disturbances of the tertiary structure are kept to a minimum, and the possibility of steric effects or interference with antibody binding to nearby sequences due to extra peptide “loops” is minimised.


The position of the inserted L2 epitope is depicted for the chimaeric constructs in FIGS. 15 to 19 respectively.


The chimaeric genes from the sequenced pSK constructs were cloned into a pFastbac1 vector (Sal I/Xba I site). The DNA from the pFastbac1 clones was used to transfect DH10bac cells to prepare bacmid clones.


The chimaeric constructs were expressed in insect cells using the Bac-to-Bac® baculovirus expression system (Life Technologies).

TABLE 1Insertion of L2 peptideNucleotideAmino acidChimaericposition of L2Shown in Figure No.positionShown in Figure No.constructpeptide(SEQ I.D. NO)of L2 peptide(SEQ I.D. NO)A520-5585 (4)174-1866 (5)C391-4297 (6)131-1438 (7)E1291-13299 (8)431-44310 (9) F1240-127811 (10)414-42612 (11)H241-27913 (12)81-9314 (13)


The bacmid DNA was transferred Into sf21 (Spodoptera frugiperda) insect cells using cellfectin. The basic Bac-to-Bac® protocol was followed to amplify the recombinant virus and infect the sf21 insect cells for expression of the chimaeric VLPs.


A basic HPV 16 L1 VLP purification protocol was followed. The infected insect cells were spun down at 3 000 rpm and resuspended in phosphate buffered saline (PBS) with 0.5 M NaCl. The suspension was sonicated 4 times at 5 second intervals. This was then overlayed onto a 40% sucrose cushion and pelleted at 100 000×g for 3 hrs. The pellet was resuspended in CsCl buffer (PBS with 0.4 g/ml CsCl) and resuspended by drawing up through 18 and 26 gauge needles to reduce the viscosity before sonication (4 times at 5 second intervals). The suspension was centrifuged at 100 000×g at 10° C. for 24 hrs.


No distinct bands were observed in CsCl gradients. 500 μl fractions were therefore collected and analysed by ELISA using conformation specific V5 and D9 (linear epitope) monoclonal antibodies. Fractions that were found to react to the V5 and/or D9 antibodies were pooled and dialysed against PBS at 4° C. overnight.


Results


Western blots showed that a polygonal L2 antibody raised to the peptide in rabbits (obtained from Dr. Neil Christensen of The Jake Gittlen Cancer Research Institute, The Milton S. Hershey Medical Centre, Hersey Pa., USA) bound to the chimaeric L1 particles (55 kD), showing that the L2 epitope is expressed by the chimaeric constructs.


Antibody characterisation of the purified VLPs was carried out by ELISA using a panel of antibodies provided by Dr. Neil Christensen (Chistensen et al., 1996, 2001). Table 2 summarises the data.

TABLE 2V5E70U49AD9I23L2A++++++C+++++E+++++++F+++++++H+++SA-opt+++++L1


A brief description of the antibodies and their binding regions is given in table 3 below.

TABLE 3V5Monoclonal, conformation specificantibody; aa 266 and 282 being criticalE70Monoclonal, conformation specificantibody; aa 50, 266 and 282 being criticalU4Monoclonal, conformation specificantibody9AMonoclonal, binds a linear regionin the are aa 1-171D9Monoclonal, binds denatured L1proteinI23Monoclonal, binds in the regionaa 111-130L2Polyclonal antibody that bindingthe L2 epitope (aa 108-120)


Electron Microscopy of the Chimaeric Particles


EM results showed that the particles formed from the chimaeric constructs are not identical to those produced by the wild type HPV L1 gene. The particles formed are mainly in a partially broken down or partially disassembled state and are generally seen to clump together


Animal Experimentation with Chimaeric Antigen


Six sets of 5 Balb/c mice were used for the animal experimentation to determine if inoculation with the chimaeric VLPs elicited an Immune response. Chimaeric VLPs produced from the 5 chimaeric constructs and VLPs produced from a non-chimaeric HPV 16 L1 (SA-opt) were injected at a concentration of 100 μg at two sub-cutaneous sites. The animals were inoculated at weeks 0, 2 and 4. Blood samples and vaginal washes were taken at various time periods.


The mouse sera from each group was pooled and analysed by ELISA using VLPs produced in insect cells by recombinant baculoviruses. End point titrations for each group of mice were carried out to determine the extent of the response and give a better reflection of the response (FIGS. 20 to 26).


The results indicate that a high immune response was achieved.


REFERENCES



  • Baker, T. S., W. W. Newcomb, N. H. Olson, L. M. Cowsert, C. Olson, and J. C. Brown. 1991. Biophys. J. 60:1445-1456.

  • Breltburd, F. and P. Coursaget. 1999. Cancer Biology 9:431-445.

  • Browne, H. M., M. J. Churcher, M. A. Stanley, G. L. Smith, and A. C. Minson. 1988. J. Gen. Virol. 69, 1263-1273.

  • Chen, X. S., Garcea, R. L., Goldberg, I., Casini, G., and Harrison, S. C. (2000). Mol Cell 5, 557-567.

  • Chen, X. S., Casini, G., Harrison, S. C and Garcea, R. (2001). Journal of Molecular Biology 307, 173-182.

  • Christensen, N. D., J. Diller, C. Eklund, J. J. Carter, G. C. Wlpf, C. A. Reed, N. M. Ciadel, and D. A. Galloway. 1996. Virol.223, 174-184.

  • Christensen N D, Cladel N M, Reed C A, Budgeon L R, Embers M E, Skulsky D M, McClements W L, Ludmerer S W, Jansen K U. 2001, 20; 291(2): 324-34.

  • Doorbaar, J., and P. H. Gallimore. 1987. J. Virol. 61:2793-2799.

  • Doretzky, I., R. Shober, S. K. Chattopadhyay, and D. R. Lowy. 1980. Virology 103:369-375.

  • M E Embers, L R Budgeon, M Pickel, N D Christensen, 2002, J. Virol., 76 (19): 9798-9805.

  • Evans, T. G., Bonnez, W., Rose, R. C., Koenig, S., Demeter, L., Suzich, J. A., O'Brien, D., Campbell, M., White, W. I., Balsley, J., and Reichman, R. C. 2001. J Infect. Dis. 183, 1485-1493.

  • Harro, C. D., Pang, Y. Y., Roden, R. B., Hildesheim, A., Wang, Z., Reynolds, M. J., Mast, T. C., Robinson, R., Murphy, B. R., Karron, R. A., Dillner, J., Schiller, J. T., and Lowy, D. R. 2001. J Natl. Cancer Inst. 93, 284-292.

  • IARC, World Health Organization. 1995. WHO Report of a technical meeting, Geneva. Ref Type: Report

  • IARC, World Health Organization. 1999. WHO. Report of a technical meeting, Geneva, 16-18 Feb 1999. 1999. Ref Type: Report

  • Kawana, K., Matsumoto, K., Yoshikawa, H., Taketani, Y., Kawana, T., Yoshiike, K., and Kanda, T. 1998. Virology 245, 353-359.

  • Kawana, K., Yoshikawa, H., Takentani, Y., Yoshiike, K., and Kanda, T. (1999). Jouranl of Virology 73, 6188-6190.

  • Kawana, K., Kawana, Y., Yoshikawa, H., Takentani, Y., Yoshiike, K., and Kanda, T. (2001). Vaccine 19, 1496-1502.

  • Kimbauer, R., F. Booy, N. Cheng, D. R. Lowy, and J. T. Schiller. 1992. Proc. Nab. Acad. Sci USA. 89, 12180-12184.

  • Kirnbauer, R., J. Taub, H. Greenstone, R. Roden, M. Durst, L. Gissman, D. R. Lowy, and J. T. Schiller. 1993. J. Virol. 67, 6929-6936.

  • Lowy, D. R., R. Kimbauer, and J. T. Schiller. 1994. Proc Natl Acad Sci USA 91:2436-2440.

  • Roden, R. B. S., H. L. Greenstone, R. Kirnbauer, F. P. Booy, J. Jessie, D. R. Lowy, and J. T. Schiller. 1996. J. Virol. 70, 5875-5883.

  • Rose, R. C., Bonnez, W., Reichman, R. C., and Garcea, R. L. 1993. J Virol 67, 1936-1944.

  • Rose, R. C., White, W. I., Li, M., Suzich, J. A, Lane, C., and Garcea, R. L. 1998. Journal of Virology 72, 6151-6154.

  • Schiller, J. T. and Lowy, D. R. 2001. Expert. Opin. Biol. Ther. 1, 571-581.

  • Seedorf, K., G. Krämmer, M. Dürst, S. Suhai, and W. G. R{overscore (o)}wekamp, 1985. Virol. 145, 181-185.

  • White, W. I., Wilson, S. D., Palmer-Hill, F. J., Woods, R. M., Ghim, S.-J., Hewitt, L A., Goldman, D. M., Burke, S. J., Jenson, A. B., Koenig, S., and Suzich, J. A. 1999. J. Virol. 73, 4882-488.


Claims
  • 1. A method for producing a chimaeric human papillomavirus (HPV) L1 polypeptide containing a HPVL2 peptide, the method comprising the steps of: introducing a DNA sequence coding for the L2 peptide into a DNA sequence coding for the L1 polypeptide; introducing the DNA sequence including the sequences for the L1 polypeptide and L2 peptide into a host cell in which the DNA sequence can be expressed; causing expression of the DNA sequence; and recovering the resulting chimaeric L1 polypeptide which includes the L2 peptide.
  • 2. A method according to claim 1, wherein the HPV L1 polypeptide and/or HPV L2 peptide is/are a HPV-16 polypeptide or peptide.
  • 3. A method according to claim 1, wherein the HPV L2 peptide has the following amino acid sequence: LVEETSFIDAGAP (SEQ ID NO: 1), or a sequence which is a modification or derivative thereof, with the proviso that the modified or derived sequence has at least 80% homology to the sequence of SEQ ID NO: 1 and codes for a peptide capable of eliciting an immunogenic response against HPV.
  • 4. A method according to claim 1, wherein one or more nucleotides of the L1 DNA sequence are deleted at the point of introduction of the L2 DNA sequence.
  • 5. A method according to claim 4, wherein the number of nucleotides deleted from the L1 DNA sequence corresponds with the number of L2 nucleotides inserted.
  • 6. A method according to claim 1, wherein expression of the polypeptide is in either of a prokaryotic or eukaryotic expression system.
  • 7. A method according to claim 1, wherein the chimaeric polypeptide has an amino acid sequence set out in any one of FIGS. 6, 8, 10, 12 and 14 (SEQ ID NOS: 5, 7, 9, 11 and 13), or a sequence which is at least 80% homologous to any one of the sequences set out in SEQ ID NOS: 5, 7, 9, 11 and 13 and which is capable of eliciting an immunogenic response against HPV.
  • 8. A method according to claim 1, wherein the DNA sequence coding for the chimaeric polypeptide had a DNA sequence set out in any one of FIGS. 5, 7, 9, 11 and 13 (SEQ ID NOS: 4, 6, 8, 10 and 12), or a sequence having at least 80% homology to any one of these sequences and which codes for a polypeptide capable of eliciting an immunogenic response against HPV.
  • 9. A method according to claim 1, wherein the chimaeric L1 polypeptide is capable of assembling into virus-like particles and/or capsomers.
  • 10. A method according to claim 9, wherein the virus-like particles or capsomers are immunogenic.
  • 11. A chimaeric human papilloma virus (HPV) L1 DNA sequence into which a DNA sequence coding for a HPV L2 peptide (SEQ ID NO: 1) has been inserted, which is capable of expressing the HPV L2 peptide.
  • 12. A HPV L1 DNA sequence according to claim 11, wherein one or more nucleotides of the L1 DNA sequence have been deleted at the point of introduction of the L2 DNA sequence.
  • 13. A HPV L1 DNA sequence according to claim 12, wherein the number of nucleotides deleted from the L1 sequence corresponds with the number of L2 nucleotides inserted.
  • 14. A human papillomavirus (HPV) nucleic acid sequence, which codes for a chimaeric L1 peptide presenting an immunogenic HPV peptide sequence, wherein the chimaeric HPV L1 sequence has a DNA sequence set out in any one of FIGS. 5, 7, 9, 11 and 13 (SEQ ID NOS 4, 6, 8, 10 and 12), or a DNA sequence which is a modification or derivative thereof, with the proviso that the modified or derived DNA sequence codes for a peptide having at least 80% homology to the sequence of SEQ ID NO: 1 and which is capable of eliciting an immunogenic response against HPV.
  • 15. A vector including a nucleic acid sequence as described in claim 11.
  • 16. A host cell including a vector as claimed in claim 15.
  • 17. A chimaeric human papilloma virus (HPV) L1 polypeptide including a peptide having the amino acid sequence:
  • 18. A polypeptide according to claim 17, which is a chimaeric HPV L1 virus-like particle or capsomer.
  • 19. A human papilloma virus (HPV) polypeptide having an amino acid sequence set out in any one of FIGS. 6, 8, 10, 12 and 14 (SEQ ID NOS: 5,7,9, 11 and 13), or a sequence which is a modification or derivative thereof, with the proviso that the modified or derived amino acid sequence has at least 80% homology to any one of the sequences set out in SEQ ID NOS: 5, 7, 9, 11 and 13 and is capable of eliciting an immunogenic response against HPV.
  • 20. A method for producing a chimaeric human papillomavirus (HPV) L1 polypeptide containing a heterologous peptide, the method comprising the steps of: introducing a DNA sequence coding for the heterologous peptide into a DNA sequence coding for the L1 polypeptide at nucleotide positions 241-279, 391-429, 520-558, 1240-1278 or 1291-1329; introducing the DNA sequence including the sequences for the L1 polypeptide and heterologous peptide into a host cell in which the DNA sequence can be expressed; causing expression of the DNA sequence; and recovering the resulting chimaeric L1 polypeptide which includes the heterologous peptide.
  • 21. A method according to claim 20, wherein the heterologous peptide sequence is any other HPV sequence or is derived from any antigenic epitope, B-cell or T-cell specific.
  • 22. A method according to claim 20, wherein one or more nucleotides of the L1 DNA sequence are deleted at the point of introduction of the heterologous DNA sequence.
  • 23. A method according to claim 22, wherein the number of nucleotides deleted from the L1 sequence corresponds with the number of heterologous nucleotides inserted.
  • 24. A vaccine including a chimaeric human papilloma virus (HPV) L1 polypeptide as described in claim 17 or a DNA sequence as described in claim 14.
  • 25. A vaccine according to claim 24, which is for use in the prophylactic or therapeutic treatment of HPV infection.
  • 26. A vaccine according to claim 25, which is for use in the treatment of HPV 6, 16 or 18.
  • 27. A vaccine according to claim 24, which is capable of inducing an immunogenic response to HPV and/or to the introduced peptide in a suitable host.
  • 28. A vaccine according to claim 24, which further comprises a pharmaceutical excipient and/or adjuvant.
  • 29. (canceled)
  • 30. A vector including a nucleic acid sequence as described in claim 14.
  • 31. A host cell including a vector as claimed in claim 30.
Priority Claims (1)
Number Date Country Kind
2002/3957 May 2002 ZA national
PCT Information
Filing Document Filing Date Country Kind 371c Date
PCT/IB03/01912 5/19/2003 WO 3/18/2005