Mutant of L1 protein of human papillomavirus type 58
10940194 ยท 2021-03-09
Assignee
Inventors
- Shaowei Li (Xiamen, CN)
- Zhihai Li (Xiamen, CN)
- Shuo Song (Xiamen, CN)
- Maozhou He (Xiamen, CN)
- Ying Gu (Xiamen, CN)
- Ningshao Xia (Xiamen, CN)
Cpc classification
C12N2710/20043
CHEMISTRY; METALLURGY
C12N7/00
CHEMISTRY; METALLURGY
C12N2710/20022
CHEMISTRY; METALLURGY
C07K14/025
CHEMISTRY; METALLURGY
C12N15/70
CHEMISTRY; METALLURGY
International classification
C12N15/70
CHEMISTRY; METALLURGY
C12N7/00
CHEMISTRY; METALLURGY
Abstract
Provided are a mutated HPV58 L1 protein or a variant thereof, a sequence encoding the same, a method for preparing the same, and a virus-like particle comprising the same, wherein the protein or a variant thereof and the virus-like particle can induce the generation of neutralizing antibodies against at least two HPV types, and therefore can be used to prevent infection by said at least two HPV types, and a disease caused by said infection, such as cervical cancer and condyloma acuminatum. The invention further relates to the use of the protein and the virus-like particle in the manufacture of a pharmaceutical composition or a vaccine for preventing infection by said at least two HPV types, and a disease caused by said infection, such as cervical cancer and condyloma acuminatum.
Claims
1. A mutated HPV58 L1 protein, wherein as compared with a wild type HPV58 L1 protein, the mutated HPV58 L1 protein has the following mutations: (1) N-terminal truncation of 5-70 amino acids; and (2)(a) substitution of amino acid residues at positions 80-87 of the wild type HPV58 L1 protein with amino acid residues at the corresponding positions of the wild-type HPV33 L1 protein; or (2)(b) substitution of amino acid residues at positions 376-383 of the wild type HPV58 L1 protein with amino acid residues at the corresponding positions of the wild-type HPV33 L1 protein; wherein said wild type HPV58 L1 protein has an amino acid sequence as set forth in SEQ ID NO: 1 or a sequence having 95% or greater identity to SEQ ID NO: 1; and wherein said wild type HPV33 L1 protein has an amino acid sequence as set forth in SEQ ID NO: 2 or a sequence having 95% or greater identity to SEQ ID NO: 2.
2. An isolated nucleic acid, encoding the mutated HPV58 L1 protein according to claim 1.
3. A vector comprising the isolated nucleic acid according to claim 2.
4. An isolated host cell comprising the isolated nucleic acid according to claim 2 and/or a vector comprising the isolated nucleic acid.
5. A HPV virus-like particle, comprising or consisting of the mutated HPV58 L1 protein according to claim 1.
6. A pharmaceutical composition or vaccine, comprising the HPV virus-like particle according to claim 5, and a pharmaceutically acceptable carrier and/or excipient.
7. A method for preparing the mutated HPV58 L1 protein according to claim 1, comprising expressing the mutated HPV58 L1 protein in a host cell, and then recovering the mutated HPV58 L1 protein from a culture of the host cell.
8. A method for preparing a vaccine, comprising combining the HPV virus-like particle according to claim 5 with a pharmaceutically acceptable carrier and/or excipient.
9. A method for preventing HPV infection or a disease caused by HPV infection, comprising administering to a subject a prophylactically effective amount of the HPV virus-like particle according to claim 5 or a pharmaceutical composition or vaccine comprising the HPV virus-like particle and a pharmaceutically acceptable carrier and/or excipient.
10. The mutated HPV58 L1 protein according to claim 1, wherein the mutated HPV58 L1 protein is characterized by one or more of the following items: (i) the mutated HPV58 L1 protein has 5, 15, 27, 35, 40, 60 or 70 amino acids truncated at N-terminal, as compared with the wild type HPV58 L1 protein; (ii) the amino acid residues at the corresponding positions as described in claim 1 section (2)(a) are amino acid residues at positions 54-61 of the wild type HPV33 L1 protein; and (iii) the amino acid residues at the corresponding positions as described in claim 1 section (2)(b) are amino acid residues at positions 350-357 of the wild type HPV33 L1 protein.
11. The mutated HPV58 L1 protein according to claim 1, wherein the mutated HPV58 L1 protein has an amino acid sequence selected from the group consisting of: SEQ ID NOs: 4 and 10.
12. The method according to claim 7, wherein the host cell is E. coli.
13. The method according to claim 9, wherein: the HPV infection is HPV58 infection and/or HPV33 infection; and/or, the disease caused by HPV infection is selected from the group consisting of cervical cancer and condyloma acuminatum.
14. A mutated HPV58 L1 protein, wherein as compared with a wild type HPV58 L1 protein, the mutated HPV58 L1 protein has the following mutations: (1) N-terminal truncation of 5-70 amino acids; and (2)(a) substitution of amino acid residues at positions 80-87 of the wild type HPV58 L1 protein with amino acid residues at the corresponding positions of a wild-type HPV33 L1 protein; and (3)(a) substitution of amino acid residues at positions 375-383 of the wild type HPV58 L1 protein with the amino acid residues at the corresponding positions of a wild type HPV52 L1 protein; or (3)(b) substitution of amino acid residues at positions 144-168 of the wild type HPV58 L1 protein with amino acid residues at the corresponding positions of a wild type HPV52 L1 protein; wherein said wild type HPV58 L1 protein has an amino acid sequence as set forth in SEQ ID NO: 1 or a sequence having 95% or greater identity to SEQ ID NO:1; wherein said wild type HPV33 L1 protein has an amino acid sequence as set forth in SEQ ID NO: 2 or a sequence having 95% or greater identity to SEQ ID NO:2; and wherein said wild type HPV52 L1 protein has an amino acid sequence as set forth in SEQ ID NO: 3 or a sequence having 95% or greater identity to SEQ ID NO:3.
15. The mutated HPV58 L1 protein according to claim 14, wherein the mutated HPV58 L1 protein comprises one or more of the following items: (i) the mutated HPV58 L1 protein has 5, 15, 27, 35, 40, 60 or 70 amino acids truncated at N-terminus, as compared with a wild type HPV58 L1 protein; (ii) the amino acid residues at the corresponding positions as described in claim 14, section (2) are amino acid residues at positions 54-61 of the wild type HPV33 L1 protein; (iii) the amino acid residues at the corresponding positions as described in claim 14, section (3)(a) are amino acid residues at positions 380-388 of a wild type HPV52 L1 protein; and (iv) the amino acid residues at the corresponding positions as described in in claim 14, section (3)(b) are amino acid residues at positions 146-170 of a wild type HPV52 L1 protein.
16. The mutated HPV58 L1 protein according to claim 14, wherein the mutated HPV58 L1 protein has an amino acid sequence selected from the group consisting of: SEQ ID NOs: 11 and 14.
17. An isolated nucleic acid, encoding the mutated HPV58 L1 protein according to claim 14.
18. A vector comprising the isolated nucleic acid according to claim 17.
19. An isolated host cell comprising the isolated nucleic acid according to claim 17 and/or a vector comprising the isolated nucleic acid.
20. A HPV virus-like particle, comprising or consisting of the mutated HPV58 L1 protein according to claim 14.
21. A pharmaceutical composition or vaccine, comprising the HPV virus-like particle according to claim 20, and a pharmaceutically acceptable carrier and/or excipient.
22. A method for preparing the mutated HPV58 L1 protein according to claim 14, comprising expressing the mutated HPV58 L1 protein in a host cell, and then recovering the mutated HPV58 L1 protein from a culture of the host cell.
23. The method according to claim 22, wherein the host cell is E. coli.
24. A method for preparing a vaccine, comprising combining the HPV virus like particle according to claim 20 with a pharmaceutically acceptable carrier and/or excipient.
25. A method for preventing HPV infection or a disease caused by HPV infection, comprising administering to a subject a prophylactically effective amount of the HPV virus-like particle according to claim 20 or a pharmaceutical composition or vaccine comprising the HPV virus-like particle and a pharmaceutically acceptable carrier and/or excipient.
26. The method according to claim 25, wherein the HPV infection is selected from one or more of the following: HPV58 infection, HPV33 infection and HPV52 infection; and/or, the disease caused by HPV infection is selected from the group consisting of cervical cancer and condyloma acuminatum.
Description
DESCRIPTION OF DRAWINGS
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Sequence Information
(13) Some of the sequences involved in the invention are provided in the following Table 1.
(14) TABLE-US-00001 TABLE 1 Description of sequences SEQ ID NO: Description 1 wild type HPV58 L1 protein 2 wild type HPV33 L1 protein 3 wild type HPV52 L1 protein 4 the mutated HPV58 L1 protein comprising Segment 1 of HPV33 L1 protein, H58N35-33T1 5 H58N35-33T2-1 6 H58N35-33T2-2 7 the mutated HPV58 L1 protein comprising Segment 2 of HPV33 L1 protein, H58N35-33T2 8 the mutated HPV58 L1 protein comprising Segment 3 of HPV33 L1 protein, H58N35-33T3 9 the mutated HPV58 L1 protein comprising Segment 4 of HPV33 L1 protein, H58N35-33T4 10 the mutated HPV58 L1 protein comprising Segment 5 of HPV33 L1 protein, H58N35-33T5 11 the mutated HPV58 L1 protein comprising Segment 1 of HPV33 L1 protein and Segment 1 of HPV52 L1 protein, H58N35-33T1-52S1 12 the mutated HPV58 L1 protein comprising Segment 1 of HPV33 L1 protein and Segment 2 of HPV52 L1 protein, H58N35-33T1-52S2 13 the mutated HPV58 L1 protein comprising Segment 1 of HPV33 L1 protein and Segment 3 of HPV52 L1 protein, H58N35-33T1-52S3 14 the mutated HPV58 L1 protein comprising Segment 1 of HPV33 L1 protein and Segment 4 of HPV52 L1 protein, H58N35-33T1-52S4 15 the DNA sequence encoding SEQ ID NO: 1 16 the DNA sequence encoding SEQ ID NO: 2 17 the DNA sequence encoding SEQ ID NO: 3 18 the DNA sequence encoding SEQ ID NO: 4 19 the DNA sequence encoding SEQ ID NO: 5 20 the DNA sequence encoding SEQ ID NO: 6 21 the DNA sequence encoding SEQ ID NO: 7 22 the DNA sequence encoding SEQ ID NO: 8 23 the DNA sequence encoding SEQ ID NO: 9 24 the DNA sequence encoding SEQ ID NO: 10 25 the DNA sequence encoding SEQ ID NO: 11 26 the DNA sequence encoding SEQ ID NO: 12 27 the DNA sequence encoding SEQ ID NO: 13 28 the DNA sequence encoding SEQ ID NO: 14 59 the sequence of the amino acid residues at positions 54 to 61 of wild type HPV33 L1 protein 60 the sequence of the amino acid residues at positions 350 to 357 of wild type HPV33 L1 protein 61 the sequence of the amino acid residues at positions 146 to 170 of wild type HPV52 L1 protein 62 the sequence of the amino acid residues at positions 380 to 388 of wild type HPV52 L1 protein
(15) TABLE-US-00002 Sequence1(SEQIDNO:1): MVLILCCTLAILFCVADVNVFHIFLQMSVWRPSEATVYLPPVPVSKVVSTDEYVSRTSIYYYAGSSRLL AVGNPYFSIKSPNNNKKVLVPKVSGLQYRVFRVRLPDPNKFGFPDTSFYNPDTQRLVWACVGLEIGR GQPLGVGVSGHPYLNKFDDTETSNRYPAQPGSDNRECLSMDYKQTQLCLIGCKPPTGEHWGKGVAC NNNAAATDCPPLELFNSIIEDGDMVDTGFGCMDFGTLQANKSDVPIDICNSTCKYPDYLKMASEPYG DSLFFFLRREQMFVRHFFNRAGKLGEAVPDDLYIKGSGNTAVIQSSAFFPTPSGSIVTSESQLFNKPYW LQRAQGHNNGICWGNQLFVTVVDTTRSTNMTLCTEVTKEGTYKNDNFKEYVRHVEEYDLQFVFQLC KITLTAEIMTYIHTMDSNILEDWQFGLTPPPSASLQDTYRFVTSQAITCQKTAPPKEKEDPLNKYTFWE VNLKEKFSADLDQFPLGRKFLLQSGLKAKPRLKRSAPTTRAPSTKRKKVKK Sequence2(SEQIDNO:2): MSVWRPSEATVYLPPVPVSKVVSTDEYVSRTSIYYYAGSSRLLAVGHPYFSIKNPTNAKKLLVPKVSG LQYRVFRVRLPDPNICFGFPDTSFYNPDTQRLVWACVGLEIGRGQPLGVGISGHPLLNKFDDTETGNK YPGQPGADNRECLSMDYKQTQLCLLGCKPPTGEHWGKGVACINAAPANDCPPLELINTIIEDGDMVD TGFGCNIEDFKTLQANICSDVPIDICGSTCKYPDYLKMTSEPYGDSLFFFLRREQMFVRHFFNRAGTLGEA VPDDLYIKGSGTTASIQSSAFFPTPSGSMVTSESQLFNKPYWLQRAQGHNNGICWGNQVFVTVVDTTR STNMTLCTQVTSDSTYKNENFKEYIRHVEEYDLQFVFQLCKVTLTAEVMTYIHAMNPDILEDWQFGL TPPPSASLQDTYRFVTSQAITCQKTVPPKEKEDPLGKYTFWEVDLICEKFSADLDQFPLGRICFLLQAGL KAKPKLKRAAPTSTRTSSAICRICKVICK Sequence3(SEQIDNO:3): MVQILFYILVIFYYVAGVNVFHIFLQMSVWRPSEATVYLPPVPVSKVVSTDEYVSRTSIYYYAGSSRLL TVGHPYFSIKNTSSGNGKKVLVPKVSGLQYRVFRIKLPDPNKFGFPDTSFYNPETQRLVWACTGLEIG RGQPLGVGISGHPLLNKFDDTETSNKYAGKPGIDNRECLSMDYKQTQLCILGCKPPIGEHWGKGTPCN NNSGNPGDCPPLQL1NSVIQDGDMVDTGFGCMDFNTLQASKSDVPIDICSSVCKYPDYLQMASEPYGD SLFFFLRREQMFVRHFFNRAGTLGDPVPGDLYIQGSNSGNTATVQSSAFFPTPSGSMVTSESQLFNKPY WLQRAQGHNNGICWGNQLFVTVVDTTRSINMTLCAEVICKESTYKNENFICEYLRHGEEFDLQFIFQL CKITLTADVMTYIHKMDATILEDWQFGLTPPPSASLEDTYRFVTSTAITCQKNTPPKGKEDPLKDYMF WEVDLKEKFSADLDQFPLGRICFLLQAGLQARPKLKRPASSAPRTSTKICICKVICR Sequence4(SEQIDNO:4): MTVYLPPVPVSKVVSTDEYVSRTSIYYYAGSSRLLAVGNPYFSIKNPTNAKKLLVPKVSGLQYRVFRV RLPDPNICFGFPDTSFYNPDTQRLVWACVGLEIGRGQPLGVGVSGHPYLNKFDDTETSNRYPAQPGSD NRECLSMDYKQTQLCLIGCKPPTGEHWGKGVACNNNAAATDCPPLELFNSIIEDGDMVDTGFGCMD FGTLQANKSDVPIDICNSTCKYPDYLKMASEPYGDSLFFFLRREQMFVRHFFNRAGKLGEAVPDDLYI KGSGNTAVIQSSAFFPTPSGSIVTSESQLFNICPYWLQRAQGHNNGICWGNQLFVTVVDTIRSTNMTLC TEVTKEGTYKNDNFKEYVRHVEEYDLQFVFQLCKITLTAEIMTYIHTMDSNILEDWQFGLTPPPSASL QDTYRFVTSQAITCQKTAPPKEKEDPLNKYTFWEVNLICEKFSADLDQFPLGRKFLLQSGLKAKPRLK RSAPTTRAPSTKRKKVICK Sequence5(SEQIDNO:5): MTVYLPPVPVSKVVSTDEYVSRTSIYYYAGSSRLLAVGNPYFSIKSPNNNICKVLVPKVSGLQYRVFRV RLPDPNKFGFPDTSFYNPDTQRLVWACVGLEIGRGQPLGVGISGHPLLNKFDDTETSNRYPAQPGSDN RECLSMDYKQTQLCLIGCKPPTGEHWGKGVACNNNAAATDCPPLELFNSIIEDGDMVDTGFGCMDF GTLQANKSDVPIDICNSTCKYPDYLICMASEPYGDSLFFFLRREQMFVRHFFNRAGICLGEAVPDDLYIK GSGNTAVIQSSAFFPTPSGSIVTSESQLFNKPYWLQRAQGHNNGICWGNQLFVTVVDTTRSTNMTLCT EVTKEGTYKNDNFKEYVRHVEEYDLQFVFQLCKITLTAEIMTYIHTMDSNILEDWQFGLTPPPSASLQ DTYRFVTSQAITCQKTAPPKEKEDPLNKYTFWEVNLKEKFSADLDQFPLGRKFLLQSGLKAKPRLICRS APTTRAPSTKRKKVKK Sequence6(SEQIDNO:6): MTVYLPPVPVSKVVSTDEYVSRTSIYYYAGSSRLLAVGNPYFSIKSPNNNKICVLVPKVSGLQYRVFRV RLPDPNKFGFPDTSFYNPDTQRLVWACVGLEIGRGQPLGVGISGHPLLNKFDDTETGNKYPAQPGSDN RECLSMDYKQTQLCLIGCKPPTGEHWGKGVACNNNAAATDCPPLELFNSIIEDGDMVDTGFGCMDF GTLQANKSDVPIDICNSTCKYPDYLKMASEPYGDSLFFFLRREQMFVRHFFNRAGICLGEAVPDDLYIK GSGNTAVIQSSAFFPTPSGSIVTSESQLFNKPYWLQRAQGHNNGICWGNQLFVTVVDTTRSTNMTLCT EVTKEGTYKNDNFKEYVRHVEEYDLQFVFQLCKITLTAEIMTYIHTMDSNILEDWQFGLTPPPSASLQ DTYRFVTSQAITCQKTAPPICEKEDPLNKYTFWEVNLKEICFSADLDQFPLGRKFLLQSGLKAKPRLICRS APTTRAPSTKRKKVICK Sequence7(SEQIDNO:7): MTVYLPPVPVSKVVSTDEYVSRTSIYYYAGSSRLLAVGNPYFSIKSPNNNKKVLVPKVSGLQYRVFRV RLPDPNKFGFPDTSFYNPDTQRLVWACVGLEIGRGQPLGVGISGHPLLNICFDDTETGNKYPGQPGAD NRECLSMDYKQTQLCLIGCKPPTGEHWGKGVACNNNAAATDCPPLELFNSIIEDGDMVDTGFGCMD FGTLQANKSDVPIDICNSTCKYPDYLKMASEPYGDSLFFFLRREQMFVRHFFNRAGKLGEAVPDDLYI KGSGNTAVIQSSAFFPTPSGSIVTSESQLFNKPYWLQRAQGHNNGICWGNQLFVTVVDTIRSTNMTLC TEVTKEGTYICNDNFKEYVRHVEEYDLQFVFQLCKITLTAEIMTY1HTMDSNILEDWQFGLTPPPSASL QDTYRFVTSQAITCQKTAPPICEKEDPLNKYTFWEVNLKEKFSADLDQFPLGRKFLLQSGLKAKPRLK RSAPTTRAPSTKRICKVICK Sequence8(SEQIDNO:8): MTVYLPPVPVSKVVSTDEYVSRTSIYYYAGSSRLLAVGNPYFSIKSPNNNKKVLVPKVSGLQYRVFRV RLPDPNICFGFPDTSFYNPDTQRLVWACVGLEIGRGQPLGVGVSGHPYLNKFDDTETSNRYPAQPGSD NRECLSMDYKQTQLCLIGCKPPTGEHWGKGVACTNAAPANDCPPLELFNSIIEDGDMVDTGFGCMDF GTLQANKSDVPIDICNSTCKYPDYLICMASEPYGDSLFFFLRREQMFVRHFFNRAGKLGEAVPDDLYIK GSGNTAVIQSSAFFPTPSGSIVTSESQLFNICPYWLQRAQGHNNGICWGNQLFVTVVDTTRSTNMTLCT EVTKEGTYKNDNFKEYVRHVEEYDLQFVFQLCKITLTAEIMTYIHTMDSNILEDWQFGLTPPPSASLQ DTYRFVTSQAITCQKTAPPKEKEDPLNKYTFWEVNLKEKFSADLDQFPLGRKFLLQSGLKAKPRLKRS APTTRAPSTKRKKVKK Sequence9(SEQIDNO:9): MTVYLPPVPVSKVVSTDEYVSRTSIYYYAGSSRLLAVGNPYFSIKSPNNNKKVLVPKVSGLQYRVFRV RLPDPNKFGFPDTSFYNPDTQRLVWACVGLEIGRGQPLGVGVSGHPYLNICFDDTETSNRYPAQPGSD NRECLSMDYKQTQLCLIGCKPPTGEHWGKGVACNNNAAATDCPPLELFNSIIEDGDMVDTGFGCMD FGTLQANKSDVPIDICNSTCKYPDYLKMASEPYGDSLFFFLRREQMFVRHFFNRAGKLGEAVPDDLYI KGSGTTASIQSSAFFPTPSGSIVTSESQLFNKPYWLQRAQGHNNGICWGNQLFVTVVDTTRSTNMTLC TEVTKEGTYKNDNFKEYVRHVEEYDLQFVFQLCKITLTAEIMTYIEITMDSNILEDWQFGLTPPPSASL QDTYRFVTSQATTCQKTAPPKEKEDPLNKYTFWEVNLICEKFSADLDQFPLGRICFLLQSGLKAKPRLK RSAPTTRAPSTICRIUCVKK Sequence10(SEQIDNO:10): MTVYLPPVPVSKVVSTDEYVSRTSIYYYAGSSRLLAVGNPYFSIKSPNNNKKVLVPKVSGLQYRVFRV RLPDPNICFGFPDTSFYNPDTQRLVWACVGLEIGRGQPLGVGVSGHPYLNKFDDTETSNRYPAQPGSD NRECLSMDYKQTQLCLIGCKPPTGEHWGKGVACNNNAAATDCPPLELFNSIIEDGDMVDTGFGCMD FGTLQANICSDVPIDICNSTCKYPDYLKMASEPYGDSLFFFLRREQMFVRHFFNRAGICLGEAVPDDLYI KGSGNTAVIQSSAFFPTPSGSIVTSESQLFNICPYWLQRAQGHNNGICWGNQLFVTVVDTTRSTNMTLC TEVTSDSTYKNENFKEYVRHVEEYDLQFVFQLCKTTLTAEIMTYIHTMDSNILEDWQFGLTPPPSASLQ DTYRFVTSQAITCQKTAPPKEKEDPLNKYTFWEVNLKEKFSADLDQFPLGRKFLLQSGLKAKPRLKRS APTTRAPSTKRIUCVKK Sequence11(SEQIDNO:11): MTVYLPPVPVSKVVSTDEYVSRTSIYYYAGSSRLLAVGNPYFSIKNPTNAICKLLVPKVSGLQYRVFRV RLPDPNICFGFPDTSFYNPDTQRLVWACVGLEIGRGQPLGVGISGHPLLNICFDDTETSNKYAGKPGIDN RECLSMDYKQTQLCLIGCKPPTGEHWGKGVACNNNAAATDCPPLELFNSIIEDGDMVDTGFGCMDF GTLQANKSDVPIDICNSTCKYPDYLICMASEPYGDSLFFFLRREQMFVRHFFNRAGICLGEAVPDDLYIK GSGNTAVIQSSAFFPTPSGSIVTSESQLFNKPYWLQRAQGHNNGICWGNQLFVTVVDTTRSTNMTLCT EVTKEGTYKNDNFKEYVRHVEEYDLQFVFQLCKITLTAEIMTYIHTMDSNILEDWQFGLTPPPSASLQ DTYRFVTSQAITCQKTAPPKEICEDPLNKYTFWEVNLKEKFSADLDQFPLGRICFLLQSGLKAICPRLICRS APTTRAPSTICRKKVICK Sequence12(SEQIDNO:12): MTVYLPPVPVSKVVSTDEYVSRTSIYYYAGSSRLLAVGNPYFSIKNPTNAKKLLVPKVSGLQYRVFRV RLPDPNKFGFPDTSFYNPDTQRLVWACVGLEIGRGQPLGVGVSGHPYLNICFDDTETSNRYPAQPGSD NRECLSMDYKQTQLCLIGCKPPTGEHWGKGTPCNNNSGNPGDCPPLELFNSIIEDGDMVDTGFGCMD FGTLQANKSDVPIDICNSTCKYPDYLKMASEPYGDSLFFFLRREQMFVRHFFNRAGKLGEAVPDDLYI KGSGNTAVIQSSAFFPTPSGSIVTSESQLFNKPYWLQRAQGHNNGICWGNQLFVTVVDTTRSTNMTLC TEVTKEGTYKNDNFKEYVRHVEEYDLQFVFQLCKITLTAEIMTYIFITMDSNILEDWQFGLTPPPSASL QDTYRFVTSQAITCQKTAPPKEKEDPLNKYTFWEVNLKEKFSADLDQFPLGRKFLLQSGLKAKPRLK RSAPTTRAPSTICRICKVICK Sequence13(SEQIDNO:13): MTVYLPPVPVSKVVSTDEYVSRTSIYYYAGSSRLLAVGNPYFSIKNPTNAKKLLVPKVSGLQYRVFRV RLPDPNKFGFPDTSFYNPDTQRLVWACVGLEIGRGQPLGVGVSGHPYLNICFDDTETSNRYPAQPGSD NRECLSMDYKQTQLCLIGCKPPTGEHWGKGVACNNNAAATDCPPLELFNSIIEDGDMVDTGFGCMD FGTLQANKSDVPIDICNSTCKYPDYLKMASEPYGDSLFFFLRREQMFVRHFFNRAGTLGDPVPGDLYI QGSNSGNTATVQSSAFFPTPSGSIVTSESQLFNKPYWLQRAQGHNNGICWGNQLFVTVVDTTRSTNM TLCTEVTKEGTYKNDNFKEYVRHVEEYDLQFVFQLCKITLTAEIMTYIHTMDSNILEDWQFGLTPPPS ASLQDTYRFVTSQAITCQKTAPPKEKEDPLNKYTFWEVNLKEKFSADLDQFPLGRKFLLQSGLKAKPR LKRSAPTTRAPSTKRKKVICK Sequence14(SEQIDNO:14): MTVYLPPVPVSICVVSTDEYVSRTSIYYYAGSSRLLAVGNPYFSIKNPTNAKICLLVPKVSGLQYRVFRV RLPDPNKFGFPDTSFYNPDTQRLVINACVGLEIGRGQPLGVGVSGHPYLNICFDDTETSNRYPAQPGSD NRECLSMDYKQTQLCLIGCKPPTGEHWGKGVACNNNAAATDCPPLELFNSIIEDGDMVDTGFGCMD FGTLQANKSDVPIDICNSTCKYPDYLKMASEPYGDSLFFFLRREQMFVRHFFNRAGKLGEAVPDDLYI KGSGNTAVIQSSAFFPTPSGSIVTSESQLFNKPYWLQRAQGHNNGICWGNQLFVTVVDTTRSTNMTLC TEVKKESTYKNENFKEYVRHVEEYDLQFVFQLCKITLTAEIMTYIHTMDSNILEDWQFGLTPPPSASLQ DTYRFVTSQAITCQKTAPPKEKEDPLNKYTFWEVNLKEKFSADLDQFPLGRKFLLQSGLKAKPRLKRS APTTRAPSTKRKKVKK Sequence15(SEQIDNO:15): ATGGTGCTGATCCTGTGCTGCACCCTGGCCATCCTGTTCTGCGTGGCCGACGTGAACGTGTTCCAC ATCTTCCTGCAGATGAGCGTGTGGAGGCCCAGCGAGGCCACCGTGTACCTGCCCCCCGTGCCCGT GAGCAAGGTGGTGAGCACCGACGAGTACGTGAGCAGGACCAGCATCTACTACTACGCCGGCAGC AGCAGGCTGCTGGCCGTGGGCAACCCCTACTTCAGCATCAAGAGCCCCAACAACAACAAGAAGG TGCTGGTGCCCAAGGTGAGCGGCCTGCAGTACAGGGTGTTCAGGGTGAGGCTGCCCGACCCCAA CAAGTTCGGCTTCCCCGACACCAGCTTCTACAACCCCGACACCCAGAGGCTGGTGTGGGCCTGCG TGGGCCTGGAGATCGGCAGGGGCCAGCCCCTGGGCGTGGGCGTGAGCGGCCACCCCTACCTGAA CAAGTTCGACGACACCGAGACCAGCAACAGGTACCCCGCCCAGCCCGGCAGCGACAACAGGGAG TGCCTGAGCATGGACTACAAGCAGACCCAGCTGTGCCTGATCGGCTGCAAGCCCCCCACCGGCG AGCACTGGGGCAAGGGCGTGGCCTGCAACAACAACGCCGCCGCCACCGACTGCCCCCCCCTGGA GCTGTTCAACAGCATCATCGAGGACGGCGACATGGTGGACACCGGCTTCGGCTGCATGGACTTCG GCACCCTGCAGGCCAACAAGAGCGACGTGCCCATCGACATCTGCAACAGCACCTGCAAGTACCC CGACTACCTGAAGATGGCCAGCGAGCCCTACGGCGACAGCCTGTTCTTCTTCCTGAGGAGGGAGC AGATGTTCGTGAGGCACTTCTTCAACAGGGCCGGCAAGCTGGGCGAGGCCGTGCCCGACGACCT GTACATCAAGGGCAGCGGCAACACCGCCGTGATCCAGAGCAGCGCCTTCTTCCCCACCCCCAGCG GCAGCATCGTGACCAGCGAGAGCCAGCTGTTCAACAAGCCCTACTGGCTGCAGAGGGCCCAGGG CCACAACAACGGCATCTGCTGGGGCAACCAGCTGTTCGTGACCGTGGTGGACACCACCAGGAGC ACCAACATGACCCTGTGCACCGAGGTGACCAAGGAGGGCACCTACAAGAACGACAACTTCAAGG AGTACGTGAGGCACGTGGAGGAGTACGACCTGCAGTTCGTGTTCCAGCTGTGCAAGATCACCCTG ACCGCCGAGATCATGACCTACATCCACACCATGGACAGCAACATCCTGGAGGACTGGCAGTTCG GCCTGACCCCCCCCCCCAGCGCCAGCCTGCAGGACACCTACAGGTTCGTGACCAGCCAGGCCATC ACCTGCCAGAAGACCGCCCCCCCCAAGGAGAAGGAGGACCCCCTGAACAAGTACACCTTCTGGG AGGTGAACCTGAAGGAGAAGTTCAGCGCCGACCTGGACCAGTTCCCCCTGGGCAGGAAGTTCCT GCTGCAGAGCGGCCTGAAGGCCAAGCCCAGGCTGAAGAGGAGCGCCCCCACCACCAGGGCCCCC AGCACCAAGAGGAAGAAGGTGAAGAAGTGA Sequence16(SEQIDNO:16): ATGAGCGTGTGGAGGCCCAGCGAGGCCACCGTGTACCTGCCCCCCGTGCCCGTGAGCAAGGTGG TGAGCACCGACGAGTACGTGAGCAGGACCAGCATCTACTACTACGCCGGCAGCAGCAGGCTGCT GGCCGTGGGCCACCCCTACTTCAGCATCAAGAACCCCACCAACGCCAAGAAGCTGCTGGTGCCC AAGGTGAGCGGCCTGCAGTACAGGGTGTTCAGGGTGAGGCTGCCCGACCCCAACAAGTTCGGCT TCCCCGACACCAGCTTCTACAACCCCGACACCCAGAGGCTGGTGTGGGCCTGCGTGGGCCTGGAG ATCGGCAGGGGCCAGCCCCTGGGCGTGGGCATCAGCGGCCACCCCCTGCTGAACAAGTTCGACG ACACCGAGACCGGCAACAAGTACCCCGGCCAGCCCGGCGCCGACAACAGGGAGTGCCTGAGCAT GGACTACAAGCAGACCCAGCTGTGCCTGCTGGGCTGCAAGCCCCCCACCGGCGAGCACTGGGGC AAGGGCGTGGCCTGCACCAACGCCGCCCCCGCCAACGACTGCCCCCCCCTGGAGCTGATCAACA CCATCATCGAGGACGGCGACATGGTGGACACCGGCTTCGGCTGCATGGACTTCAAGACCCTGCA GGCCAACAAGAGCGACGTGCCCATCGACATCTGCGGCAGCACCTGCAAGTACCCCGACTACCTG AAGATGACCAGCGAGCCCTACGGCGACAGCCTGTTCTTCTTCCTGAGGAGGGAGCAGATGTTCGT GAGGCACTTCTTCAACAGGGCCGGCACCCTGGGCGAGGCCGTGCCCGACGACCTGTACATCAAG GGCAGCGGCACCACCGCCAGCATCCAGAGCAGCGCCTTCTTCCCCACCCCCAGCGGCAGCATGGT GACCAGCGAGAGCCAGCTGTTCAACAAGCCCTACTGGCTGCAGAGGGCCCAGGGCCACAACAAC GGCATCTGCTGGGGCAACCAGGTGTTCGTGACCGTGGTGGACACCACCAGGAGCACCAACATGA CCCTGTGCACCCAGGTGACCAGCGACAGCACCTACAAGAACGAGAACTTCAAGGAGTACATCAG GCACGTGGAGGAGTACGACCTGrCAGTTCGTGTTCCAGCTGTGCAAGGTGACCCTGACCGCCGAG GTGATGACCTACATCCACGCCATGAACCCCGACATCCTGGAGGACTGGCAGTTCGGCCTGACCCC CCCCCCCAGCGCCAGCCTGCAGGACACCTACAGGTTCGTGACCAGCCAGGCCATCACCTGCCAGA AGACCGTGCCCCCCAAGGAGAAGGAGGACCCCCTGGGCAAGTACACCTTCTGGGAGGTGGACCT GAAGGAGAAGTTCAGCGCCGACCTGGACCAGTTCCCCCTGGGCAGGAAGTTCCTGCTGCAGGCC GGCCTGAAGGCCAAGCCCAAGCTGAAGAGGGCCGCCCCCACCAGCACCAGGACCAGCAGCGCCA AGAGGAAGAAGGTGAAGAAGTGA Sequence17(SEQIDNO:17): ATGGTGCAGATCCTGTTCTACATCCTGGTGATCTTCTACTACGTGGCCGGCGTGAACGTGTTCCAC ATCTTCCTGCAGATGAGCGTGTGGAGGCCCAGCGAGGCCACCGTGTACCTGCCCCCCGTGCCCGT GAGCAAGGTGGTGAGCACCGACGAGTACGTGAGCAGGACCAGCATCTACTACTACGCCGGCAGC AGCAGGCTGCTGACCGTGGGCCACCCCTACTTCAGCATCAAGAACACCAGCAGCGGCAACGGCA AGAAGGTGCTGGTGCCCAAGGTGAGCGGCCTGCAGTACAGGGTGTTCAGGATCAAGCTGCCCGA CCCCAACAAGTTCGGCTTCCCCGACACCAGCTTCTACAACCCCGAGACCCAGAGGCTGGTGTGGG CCTGCACCGGCCTGGAGATCGGCAGGGGCCAGCCCCTGGGCGTGGGCATCAGCGGCCACCCCCT GCTGAACAAGTTCGACGACACCGAGACCAGCAACAAGTACGCCGGCAAGCCCGGCATCGACAAC AGGGAGTGCCTGAGCATGGACTACAAGCAGACCCAGCTGTGCATCCTGGGCTGCAAGCCCCCCA TCGGCGAGCACTGGGGCAAGGGCACCCCCTGCAACAACAACAGCGGCAACCCCGGCGACTGCCC CCCCCTGCAGCTGATCAACAGCGTGATCCAGGACGGCGACATGGTGGACACCGGCTTCGGCTGC ATGGACTTCAACACCCTGCAGGCCAGCAAGAGCGACGTGCCCATCGACATCTGCAGCAGCGTGT GCAAGTACCCCGACTACCTGCAGATGGCCAGCGAGCCCTACGGCGACAGCCTGTTCTTCTTCCTG AGGAGGGAGCAGATGTTCGTGAGGCACTTCTTCAACAGGGCCGGCACCCTGGGCGACCCCGTGC CCGGCGACCTGTACATCCAGGGCAGCAACAGCGGCAACACCGCCACCGTGCAGAGCAGCGCCTT CTTCCCCACCCCCAGCGGCAGCATGGTGACCAGCGAGAGCCAGCTGTTCAACAAGCCCTACTGGC TGCAGAGGGCCCAGGGCCACAACAACGGCATCTGCTGGGGCAACCAGCTGTTCGTGACCGTGGT GGACACCACCAGGAGCACCAACATGACCCTGTGCGCCGAGGTGAAGAAGGAGAGCACCTACAA GAACGAGAACTTCAAGGAGTACCTGAGGCACGGCGAGGAGTTCGACCTGCAGTTCATCTTCCAG CTGTGCAAGATCACCCTGACCGCCGACGTGATGACCTACATCCACAAGATGGACGCCACCATCCT GGAGGACTGGCAGTTCGGCCTGACCCCCCCCCCCAGCGCCAGCCTGGAGGACACCTACAGGTTC GTGACCAGCACCGCCATCACCTGCCAGAAGAACACCCCCCCCAAGGGCAAGGAGGACCCCCTGA AGGACTACATGTTCTGGGAGGTGGACCTGAAGGAGAAGTTCAGCGCCGACCTGGACCAGTTCCC CCTGGGCAGGAAGTTCCTGCTGCAGGCCGGCCTGCAGGCCAGGCCCAAGCTGAAGAGGCCCGCC AGCAGCGCCCCCAGGACCAGCACCAAGAAGAAGAAGGTGAAGAGGTGA Sequence18(SEQIDNO:18): ATGACCGTGTACCTGCCCCCCGTGCCCGTGAGCAAGGTGGTGAGCACCGACGAGTACGTGAGCA GGACCAGCATCTACTACTACGCCGGCAGCAGCAGGCTGCTGGCCGTGGGCAACCCCTACTTCAGC ATCAAGAATCCCACTAACGCTAAAAAATTACTGGTGCCCAAGGTGAGCGGCCTGCAGTACAGGG TGTTCAGGGTGAGGCTGCCCGACCCCAACAAGTTCGGCTTCCCCGACACCAGCTTCTACAACCCC GACACCCAGAGGCTGGTGTGGGCCTGCGTGGGCCTGGAGATCGGCAGGGGCCAGCCCCTGGGCG TGGGCGTGAGCGGCCACCCCTACCTGAACAAGTTCGACGACACCGAGACCAGCAACAGGTACCC CGCCCAGCCCGGCAGCGACAACAGGGAGTGCCTGAGCATGGACTACAAGCAGACCCAGCTGTGC CTGATCGGCTGCAAGCCCCCCACCGGCGAGCACTGGGGCAAGGGCGTGGCCTGCAACAACAACG CCGCCGCCACCGACTGCCCCCCCCTGGAGCTGTTCAACAGCATCATCGAGGACGGCGACATGGTG GACACCGGCTTCGGCTGCATGGACTTCGGCACCCTGCAGGCCAACAAGAGCGACGTGCCCATCG ACATCTGCAACAGCACCTGCAAGTACCCCGACTACCTGAAGATGGCCAGCGAGCCCTACGGCGA CAGCCTGTTCTTCTTCCTGAGGAGGGAGCAGATGTTCGTGAGGCACTTCTTCAACAGGGCCGGCA AGCTGGGCGAGGCCGTGCCCGACGACCTGTACATCAAGGGCAGCGGCAACACCGCCGTGATCCA GAGCAGCGCCTTCTTCCCCACCCCCAGCGGCAGCATCGTGACCAGCGAGAGCCAGCTGTTCAACA AGCCCTACTGGCTGCAGAGGGCCCAGGGCCACAACAACGGCATCTGCTGGGGCAACCAGCTGTT CGTGACCGTGGTGGACACCACCAGGAGCACCAACATGACCCTGTGCACCGAGGTGACCAAGGAG GGCACCTACAAGAACGACAACTTCAAGGAGTACGTGAGGCACGTGGAGGAGTACGACCTGCAGT TCGTGTTCCAGCTGTGCAAGATCACCCTGACCGCCGAGATCATGACCTACATCCACACCATGGAC AGCAACATCCTGGAGGACTGGCAGTTCGGCCTGACCCCCCCCCCCAGCGCCAGCCTGCAGGACA CCTACAGGTTCGTGACCAGCCAGGCCATCACCTGCCAGAAGACCGCCCCCCCCAAGGAGAAGGA GGACCCCCTGAACAAGTACACCTTCTGGGAGGTGAACCTGAAGGAGAAGTTCAGCGCCGACCTG GACCAGTTCCCCCTGGGCAGGAAGTTCCTGCTGCAGAGCGGCCTGAAGGCCAAGCCCAGGCTGA AGAGGAGCGCCCCCACCACCAGGGCCCCCAGCACCAAGAGGAAGAAGGTGAAGAAGTAA Sequence19(SEQIDNO:19): ATGACCGTGTACCTGCCCCCCGTGCCCGTGAGCAAGGTGGTGAGCACCGACGAGTACGTGAGCA GGACCAGCATCTACTACTACGCCGGCAGCAGCAGGCTGCTGGCCGTGGGCAACCCCTACTTCAGC ATCAAGAGCCCCAACAACAACAAGAAGGTGCTGGTGCCCAAGGTGAGCGGCCTGCAGTACAGGG TGTTCAGGGTGAGGCTGCCCGACCCCAACAAGTTCGGCTTCCCCGACACCAGCTTCTACAACCCC GACACCCAGAGGCTGGTGTGGGCCTGCGTGGGCCTGGAGATCGGCAGGGGCCAGCCCCTGGGCG TCGGAATAAGCGGCCACCCCTTACTGAACAAGTTCGACGACACCGAGACCAGCAACAGGTACCC CGCCCAGCCCGGCAGCGACAACAGGGAGTGCCTGAGCATGGACTACAAGCAGACCCAGCTGTGC CTGATCGGCTGCAAGCCCCCCACCGGCGAGCACTGGGGCAAGGGCGTGGCCTGCAACAACAACG CCGCCGCCACCGACTGCCCCCCCCTGGAGCTGTTCAACAGCATCATCGAGGACGGCGACATGGTG GACACCGGCTTCGGCTGCATGGACTTCGGCACCCTGCAGGCCAACAAGAGCGACGTGCCCATCG ACATCTGCAACAGCACCTGCAAGTACCCCGACTACCTGAAGATGGCCAGCGAGCCCTACGGCGA CAGCCTGTTCTTCTTCCTGAGGAGGGAGCAGATGTTCGTGAGGCACTTCTTCAACAGGGCCGGCA AGCTGGGCGAGGCCGTGCCCGACGACCTGTACATCAAGGGCAGCGGCAACACCGCCGTGATCCA GAGCAGCGCCTTCTTCCCCACCCCCAGCGGCAGCATCGTGACCAGCGAGAGCCAGCTGTTCAACA AGCCCTACTGGCTGCAGAGGGCCCAGGGCCACAACAACGGCATCTGCTGGGGCAACCAGCTGTT CGTGACCGTGGTGGACACCACCAGGAGCACCAACATGACCCTGTGCACCGAGGTGACCAAGGAG GGCACCTACAAGAACGACAACTTCAAGGAGTACGTGAGGCACGTGGAGGAGTACGACCTGCAGT TCGTGTTCCAGCTGTGCAAGATCACCCTGACCGCCGAGATCATGACCTACATCCACACCATGGAC AGCAACATCCTGGAGGACTGGCAGTTCGGCCTGACCCCCCCCCCCAGCGCCAGCCTGCAGGACA CCTACAGGTTCGTGACCAGCCAGGCCATCACCTGCCAGAAGACCGCCCCCCCCAAGGAGAAGGA GGACCCCCTGAACAAGTACACCTTCTGGGAGGTGAACCTGAAGGAGAAGTTCAGCGCCGACCTG GACCAGTTCCCCCTGGGCAGGAAGTTCCTGCTGCAGAGCGGCCTGAAGGCCAAGCCCAGGCTGA AGAGGAGCGCCCCCACCACCAGGGCCCCCAGCACCAAGAGGAAGAAGGTGAAGAAGTGA Sequence20(SEQIDNO:20): ATGACCGTGTACCTGCCCCCCGTGCCCGTGAGCAAGGTGGTGAGCACCGACGAGTACGTGAGCA GGACCAGCATCTACTACTACGCCGGCAGCAGCAGGCTGCTGGCCGTGGGCAACCCCTACTTCAGC ATCAAGAGCCCCAACAACAACAAGAAGGTGCTGGTGCCCAAGGTGAGCGGCCTGCAGTACAGGG TGTTCAGGGTGAGGCTGCCCGACCCCAACAAGTTCGGCTTCCCCGACACCAGCTTCTACAACCCC GACACCCAGAGGCTGGTGTGGGCCTGCGTGGGCCTGGAGATCGGCAGGGGCCAGCCCCTGGGCG TCGGAATAAGCGGCCACCCCTTACTGAACAAGTTCGACGACACCGAGACCGGAAACAAGTACCC CGCCCAGCCCGGCAGCGACAACAGGGAGTGCCTGAGCATGGACTACAAGCAGACCCAGCTGTGC CTGATCGGCTGCAAGCCCCCCACCGGCGAGCACTGGGGCAAGGGCGTGGCCTGCAACAACAACG CCGCCGCCACCGACTGCCCCCCCCTGGAGCTGTTCAACAGCATCATCGAGGACGGCGACATGGTG GACACCGGCTTCGGCTGCATGGACTTCGGCACCCTGCAGGCCAACAAGAGCGACGTGCCCATCG ACATCTGCAACAGCACCTGCAAGTACCCCGACTACCTGAAGATGGCCAGCGAGCCCTACGGCGA CAGCCTGTTCTTCTTCCTGAGGAGGGAGCAGATGTTCGTGAGGCACTTCTTCAACAGGGCCGGCA AGCTGGGCGAGGCCGTGCCCGACGACCTGTACATCAAGGGCAGCGGCAACACCGCCGTGATCCA GAGCAGCGCCTTCTTCCCCACCCCCAGCGGCAGCATCGTGACCAGCGAGAGCCAGCTGTTCAACA AGCCCTACTGGCTGCAGAGGGCCCAGGGCCACAACAACGGCATCTGCTGGGGCAACCAGCTGTT CGTGACCGTGGTGGACACCACCAGGAGCACCAACATGACCCTGTGCACCGAGGTGACCAAGGAG GGCACCTACAAGAACGACAACTTCAAGGAGTACGTGAGGCACGTGGAGGAGTACGACCTGCAGT TCGTGTTCCAGCTGTGCAAGATCACCCTGACCGCCGAGATCATGACCTACATCCACACCATGGAC AGCAACATCCTGGAGGACTGGCAGTTCGGCCTGACCCCCCCCCCCAGCGCCAGCCTGCAGGACA CCTACAGGTTCGTGACCAGCCAGGCCATCACCTGCCAGAAGACCGCCCCCCCCAAGGAGAAGGA GGACCCCCTGAACAAGTACACCTTCTGGGAGGTGAACCTGAAGGAGAAGTTCAGCGCCGACCTG GACCAGTTCCCCCTGGGCAGGAAGTTCCTGCTGCAGAGCGGCCTGAAGGCCAAGCCCAGGCTGA AGAGGAGCGCCCCCACCACCAGGGCCCCCAGCACCAAGAGGAAGAAGGTGAAGAAGTGA Sequence21(SEQIDNO:21): ATGACCGTGTACCTGCCCCCCGTGCCCGTGAGCAAGGTGGTGAGCACCGACGAGTACGTGAGCA GGACCAGCATCTACTACTACGCCGGCAGCAGCAGGCTGCTGGCCGTGGGCAACCCCTACTTCAGC ATCAAGAGCCCCAACAACAACAAGAAGGTGCTGGTGCCCAAGGTGAGCGGCCTGCAGTACAGGG TGTTCAGGGTGAGGCTGCCCGACCCCAACAAGTTCGGCTTCCCCGACACCAGCTTCTACAACCCC GACACCCAGAGGCTGGTGTGGGCCTGCGTGGGCCTGGAGATCGGCAGGGGCCAGCCCCTGGGCG TCGGAATAAGCGGCCACCCCTTACTGAACAAGTTCGACGACACCGAGACCGGAAACAAGTACCC CGGACAGCCCGGCGCTGACAACAGGGAGTGCCTGAGCATGGACTACAAGCAGACCCAGCTGTGC CTGATCGGCTGCAAGCCCCCCACCGGCGAGCACTGGGGCAAGGGCGTGGCCTGCAACAACAACG CCGCCGCCACCGACTGCCCCCCCCTGGAGCTGTTCAACAGCATCATCGAGGACGGCGACATGGTG GACACCGGCTTCGGCTGCATGGACTTCGGCACCCTGCAGGCCAACAAGAGCGACGTGCCCATCG ACATCTGCAACAGCACCTGCAAGTACCCCGACTACCTGAAGATGGCCAGCGAGCCCTACGGCGA CAGCCTGTTCTTCTTCCTGAGGAGGGAGCAGATGTTCGTGAGGCACTTCTTCAACAGGGCCGGCA AGCTGGGCGAGGCCGTGCCCGACGACCTGTACATCAAGGGCAGCGGCAACACCGCCGTGATCCA GAGCAGCGCCTTCTTCCCCACCCCCAGCGGCAGCATCGTGACCAGCGAGAGCCAGCTGTTCAACA AGCCCTACTGGCTGCAGAGGGCCCAGGGCCACAACAACGGCATCTGCTGGGGCAACCAGCTGTT CGTGACCGTGGTGGACACCACCAGGAGCACCAACATGACCCTGTGCACCGAGGTGACCAAGGAG GGCACCTACAAGAACGACAACTTCAAGGAGTACGTGAGGCACGTGGAGGAGTACGACCTGCAGT TCGTGTTCCAGCTGTGCAAGATCACCCTGACCGCCGAGATCATGACCTACATCCACACCATGGAC AGCAACATCCTGGAGGACTGGCAGTTCGGCCTGACCCCCCCCCCCAGCGCCAGCCTGCAGGACA CCTACAGGTTCGTGACCAGCCAGGCCATCACCTGCCAGAAGACCGCCCCCCCCAAGGAGAAGGA GGACCCCCTGAACAAGTACACCTTCTGGGAGGTGAACCTGAAGGAGAAGTTCAGCGCCGACCTG GACCAGTTCCCCCTGGGCAGGAAGTTCCTGCTGCAGAGCGGCCTGAAGGCCAAGCCCAGGCTGA AGAGGAGCGCCCCCACCACCAGGGCCCCCAGCACCAAGAGGAAGAAGGTGAAGAAGTAA Sequence22(SEQIDNO:22): ATGACCGTGTACCTGCCCCCCGTGCCCGTGAGCAAGGTGGTGAGCACCGACGAGTACGTGAGCA GGACCAGCATCTACTACTACGCCGGTAGCAGCAGGCTGCTGGCCGTGGGCAACCCCTACTTCAGC ATCAAGAGCCCCAACAACAACAAGAAGGTGCTGGTGCCCAAGGTGAGCGGCCTGCAGTACAGGG TGTTCAGGGTGAGGCTGCCCGACCCCAACAAGTTCGGCTTCCCCGACACCAGCTTCTACAACCCC GACACCCAGAGGCTGGTGTGGGCCTGCGTGGGCCTGGAGATCGGCAGGGGCCAGCCCCTGGGCG TGGGCGTGAGCGGCCACCCCTACCTGAACAAGTTCGACGACACCGAGACCAGCAACAGGTACCC CGCCCAGCCCGGCAGCGACAACAGGGAGTGCCTGAGCATGGACTACAAGCAGACCCAGCTGTGC CTGATCGGCTGCAAGCCCCCCACCGGCGAGCACTGGGGCAAGGGAGTAGCATGTACAAACGCTG CACCTGCCAACGACTGCCCCCCCCTGGAGCTGTTCAACAGCATCATCGAGGACGGCGACATGGTG GACACCGGCTTCGGCTGCATGGACTTCGGCACCCTGCAGGCCAACAAGAGCGACGTGCCCATCG ACATCTGCAACAGCACCTGCAAGTACCCCGACTACCTGAAGATGGCCAGCGAGCCCTACGGCGA CAGCCTGTTCTTCTTCCTGAGGAGGGAGCAGATGTTCGTGAGGCACTTCTTCAACAGGGCCGGCA AGCTGGGCGAGGCCGTGCCCGACGACCTGTACATCAAGGGCAGCGGCAACACCGCCGTGATCCA GAGCAGCGCCTTCTTCCCCACCCCCAGCGGCAGCATCGTGACCAGCGAGAGCCAGCTGTTCAACA AGCCCTACTGGCTGCAGAGGGCCCAGGGCCACAACAACGGCATCTGCTGGGGCAACCAGCTGTT CGTGACCGTGGTGGACACCACCAGGAGCACCAACATGACCCTGTGCACCGAGGTGACCAAGGAG GGCACCTACAAGAACGACAACTTCAAGGAGTACGTGAGGCACGTGGAGGAGTACGACCTGCAGT TCGTGTTCCAGCTGTGCAAGATCACCCTGACCGCCGAGATCATGACCTACATCCACACCATGGAC AGCAACATCCTGGAGGACTGGCAGTTCGGCCTGACCCCCCCCCCCAGCGCCAGCCTGCAGGACA CCTACAGGTTCGTGACCAGCCAGGCCATCACCTGCCAGAAGACCGCCCCCCCCAAGGAGAAGGA GGACCCCCTGAACAAGTACACCTTCTGGGAGGTGAACCTGAAGGAGAAGTTCAGCGCCGACCTG GACCAGTTCCCCCTGGGCAGGAAGTTCCTGCTGCAGAGCGGCCTGAAGGCCAAGCCCAGGCTGA AGAGGAGCGCCCCCACCACCAGGGCCCCCAGCACCAAGAGGAAGAAGGTGAAGAAGTAA Sequence23(SEQIDNO:23): ATGACCGTGTACCTGCCCCCCGTGCCCGTGAGCAAGGTGGTGAGCACCGACGAGTACGTGAGCA GGACCAGCATCTACTACTACGCCGGCAGCAGCAGGCTGCTGGCCGTGGGCAACCCCTACTTCAGC ATCAAGAGCCCCAACAACAACAAGAAGGTGCTGGTGCCCAAGGTGAGCGGCCTGCAGTACAGGG TGTTCAGGGTGAGGCTGCCCGACCCCAACAAGTTCGGCTTCCCCGACACCAGCTTCTACAACCCC GACACCCAGAGGCTGGTGTGGGCCTGCGTGGGCCTGGAGATCGGCAGGGGCCAGCCCCTGGGCG TGGGCGTGAGCGGCCACCCCTACCTGAACAAGTTCGACGACACCGAGACCAGCAACAGGTACCC CGCCCAGCCCGGCAGCGACAACAGGGAGTGCCTGAGCATGGACTACAAGCAGACCCAGCTGTGC CTGATCGGCTGCAAGCCCCCCACCGGCGAGCACTGGGGCAAGGGCGTGGCCTGCAACAACAACG CCGCCGCCACCGACTGCCCCCCCCTGGAGCTGTTCAACAGCATCATCGAGGACGGCGACATGGTG GACACCGGCTTCGGCTGCATGGACTTCGGCACCCTGCAGGCCAACAAGAGCGACGTGCCCATCG ACATCTGCAACAGCACCTGCAAGTACCCCGACTACCTGAAGATGGCCAGCGAGCCCTACGGCGA CAGCCTGTTCTTCTTCCTGAGGAGGGAGCAGATGTTCGTGAGGCACTTCTTCAACAGGGCCGGCA AGCTGGGCGAGGCCGTGCCCGACGACCTGTACATCAAGGGCAGCGGCACAACAGCAAGTATCCA GAGCAGCGCCTTCTTCCCCACCCCCAGCGGCAGCATCGTGACCAGCGAGAGCCAGCTGTTCAACA AGCCCTACTGGCTGCAGAGGGCCCAGGGCCACAACAACGGCATCTGCTGGGGCAACCAGCTGTT CGTGACCGTGGTGGACACCACCAGGAGCACCAACATGACCCTGTGCACCGAGGTGACCAAGGAG GGCACCTACAAGAACGACAACTTCAAGGAGTACGTGAGGCACGTGGAGGAGTACGACCTGCAGT TCGTGTTCCAGTTGTGCAAGATCACCCTGACCGCCGAGATCATGACCTACATCCACACCATGGAC AGCAACATCCTGGAGGACTGGCAGTTCGGCCTGACCCCCCCCCCCAGCGCCAGCCTGCAGGACA CCTACAGGTTCGTGACCAGCCAGGCCATCACCTGCCAGAAGACCGCCCCCCCCAAGGAGAAGGA GGACCCCCTGAACAAGTACACCTTCTGGGAGGTGAACCTGAAGGAGAAGTTCAGCGCCGACCTG GACCAGTTCCCCCTGGGCAGGAAGTTCCTGCTGCAGAGCGGCCTGAAGGCCAAGCCCAGGCTGA AGAGGAGCGCCCCCACCACCAGGGCCCCCAGCACCAAGAGGAAGAAGGTGAAGAAGTAA Sequence24(SEQIDNO:24): ATGACCGTGTACCTGCCCCCCGTGCCCGTGAGCAAGGTGGTGAGCACCGACGAGTACGTGAGCA GGACCAGCATCTACTACTACGCCGGCAGCAGCAGGCTGCTGGCCGTGGGCAACCCCTACTTCAGC ATCAAGAGCCCCAACAACAACAAGAAGGTGCTGGTGCCCAAGGTGAGCGGCCTGCAGTACAGGG TGTTCAGGGTGAGGCTGCCCGACCCCAACAAGTTCGGCTTCCCCGACACCAGCTTCTACAACCCC GACACCCAGAGGCTGGTGTGGGCCTGCGTGGGCCTGGAGATCGGCAGGGGCCAGCCCCTGGGCG TGGGCGTGAGCGGCCACCCCTACCTGAACAAGTTCGACGACACCGAGACCAGCAACAGGTACCC CGCCCAGCCCGGCAGCGACAACAGGGAGTGCCTGAGCATGGACTACAAGCAGACCCAGCTGTGC CTGATCGGCTGCAAGCCCCCCACCGGCGAGCACTGGGGCAAGGGCGTGGCCTGCAACAACAACG CCGCCGCCACCGACTGCCCCCCCCTGGAGCTGTTCAACAGCATCATCGAGGACGGCGACATGGTG GACACCGGCTTCGGCTGCATGGACTTCGGCACCCTGCAGGCCAACAAGAGCGACGTGCCCATCG ACATCTGCAACAGCACCTGCAAGTACCCCGACTACCTGAAGATGGCCAGCGAGCCCTACGGCGA CAGCCTGTTCTTCTTCCTGAGGAGGGAGCAGATGTTCGTGAGGCACTTCTTCAACAGGGCCGGCA AGCTGGGCGAGGCCGTGCCCGACGACCTGTACATCAAGGGCAGCGGCAACACCGCCGTGATCCA GAGCAGCGCCTTCTTCCCCACCCCCAGCGGCAGCATCGTGACCAGCGAGAGCCAGCTGTTCAACA AGCCCTACTGGCTGCAGAGGGCCCAGGGCCACAACAACGGCATCTGCTGGGGCAACCAGCTGTT CGTGACCGTGGTGGACACCACCAGGAGCACCAACATGACCCTGTGCACCGAGGTGACCAGCGAC AGCACGTACAAGAACGAGAACTTCAAGGAGTACGTGAGGCACGTGGAGGAGTACGACCTGCAGT TCGTGTTCCAGCTGTGCAAGATCACCCTGACCGCCGAGATCATGACCTACATCCACACCATGGAC AGCAACATCCTGGAGGACTGGCAGTTCGGCCTGACCCCCCCCCCCAGCGCCAGCCTGCAGGACA CCTACAGGTTCGTGACCAGCCAGGCCATCACCTGCCAGAAGACCGCCCCCCCCAAGGAGAAGGA GGACCCCCTGAACAAGTACACCTTCTGGGAGGTGAACCTGAAGGAGAAGTTCAGCGCCGACCTG GACCAGTTCCCCCTGGGCAGGAAGTTCCTGCTGCAGAGCGGCCTGAAGGCCAAGCCCAGGCTGA AGAGGAGCGCCCCCACCACCAGGGCCCCCAGCACCAAGAGGAAGAAGGTGAAGAAGTAA Sequence25(SEQIDNO:25): ATGACCGTGTACCTGCCCCCCGTGCCCGTGAGCAAGGTGGTGAGCACCGACGAGTACGTGAGCA GGACCAGCATCTACTACTACGCCGGCAGCAGCAGGCTGCTGGCCGTGGGCAACCCCTACTTCAGC ATCAAGAATCCCACTAACGCTAAAAAATTACTGGTGCCCAAGGTGAGCGGCCTGCAGTACAGGG TGTTCAGGGTGAGGCTGCCCGACCCCAACAAGTTCGGCTTCCCCGACACCAGCTTCTACAACCCC GACACCCAGAGGCTGGTGTGGGCCTGCGTGGGCCTGGAGATCGGCAGGGGCCAGCCCCTGGGCG TGGGCATCAGCGGCCACCCCCTGCTGAACAAGTTCGACGACACCGAGACCAGCAACAAGTACGC CGGCAAGCCCGGCATCGACAACAGGGAGTGCCTGAGCATGGACTACAAGCAGACCCAGCTGTGC CTGATCGGCTGCAAGCCCCCCACCGGCGAGCACTGGGGCAAGGGCGTGGCCTGCAACAACAACG CCGCCGCCACCGACTGCCCCCCCCTGGAGCTGTTCAACAGCATCATCGAGGACGGCGACATGGTG GACACCGGCTTCGGCTGCATGGACTTCGGCACCCTGCAGGCCAACAAGAGCGACGTGCCCATCG ACATCTGCAACAGCACCTGCAAGTACCCCGACTACCTGAAGATGGCCAGCGAGCCCTACGGCGA CAGCCTGTTCTTCTTCCTGAGGAGGGAGCAGATGTTCGTGAGGCACTTCTTCAACAGGGCCGGCA AGCTGGGCGAGGCCGTGCCCGACGACCTGTACATCAAGGGCAGCGGCAACACCGCCGTGATCCA GAGCAGCGCCTTCTTCCCCACCCCCAGCGGCAGCATCGTGACCAGCGAGAGCCAGCTG.TTCAACA AGCCCTACTGGCTGCAGAGGGCCCAGGGCCACAACAACGGCATCTGCTGGGGCAACCAGCTGTT CGTGACCGTGGTGGACACCACCAGGAGCACCAACATGACCCTGTGCACCGAGGTGACCAAGGAG GGCACCTACAAGAACGACAACTTCAAGGAGTACGTGAGGCACGTGGAGGAGTACGACCTGCAGT TCGTGTTCCAGCTGTGCAAGATCACCCTGACCGCCGAGATCATGACCTACATCCACACCATGGAC AGCAACATCCTGGAGGACTGGCAGTTCGGCCTGACCCCCCCCCCCAGCGCCAGCCTGCAGGACA CCTACAGGTTCGTGACCAGCCAGGCCATCACCTGCCAGAAGACCGCCCCCCCCAAGGAGAAGGA GGACCCCCTGAACAAGTACACCTTCTGGGAGGTGAACCTGAAGGAGAAGTTCAGCGCCGACCTG GACCAGTTCCCCCTGGGCAGGAAGTTCCTGCTGCAGAGCGGCCTGAAGGCCAAGCCCAGGCTGA AGAGGAGCGCCCCCACCACCAGGGCCCCCAGCACCAAGAGGAAGAAGGTGAAGAAGTAA Sequence26(SEQIDNO:26): ATGACCGTGTACCTGCCCCCCGTGCCCGTGAGCAAGGTGGTGAGCACCGACGAGTACGTGAGCA GGACCAGCATCTACTACTACGCCGGCAGCAGCAGGCTGCTGGCCGTGGGCAACCCCTACTTCAGC ATCAAGAATCCCACTAACGCTAAAAAATTACTGGTGCCCAAGGTGAGCGGCCTGCAGTACAGGG TGTTCAGGGTGAGGCTGCCCGACCCCAACAAGTTCGGCTTCCCCGACACCAGCTTCTACAACCCC GACACCCAGAGGCTGGTGTGGGCCTGCGTGGGCCTGGAGATCGGCAGGGGCCAGCCCCTGGGCG TGGGCGTGAGCGGCCACCCCTACCTGAACAAGTTCGACGACACCGAGACCAGCAACAGGTACCC CGCCCAGCCCGGCAGCGACAACAGGGAGTGCCTGAGCATGGACTACAAGCAGACCCAGCTGTGC CTGATCGGCTGCAAGCCCCCCACCGGCGAGCACTGGGGCAAGGGCACCCCCTGCAACAACAACA GCGGCAACCCCGGCGACTGCCCCCCCCTGGAGCTGTTCAACAGCATCATCGAGGACGGCGACAT GGTGGACACCGGCTTCGGCTGCATGGACTTCGGCACCCTGCAGGCCAACAAGAGCGACGTGCCC ATCGACATCTGCAACAGCACCTGCAAGTACCCCGACTACCTGAAGATGGCCAGCGAGCCCTACG GCGACAGCCTGTTCTTCTTCCTGAGGAGGGAGCAGATGTTCGTGAGGCACTTCTTCAACAGGGCC GGCAAGCTGGGCGAGGCCGTGCCCGACGACCTGTACATCAAGGGCAGCGGCAACACCGCCGTGA TCCAGAGCAGCGCCTTCTTCCCCACCCCCAGCGGCAGCATCGTGACCAGCGAGAGCCAGCTGTTC AACAAGCCCTACTGGCTGCAGAGGGCCCAGGGCCACAACAACGGCATCTGCTGGGGCAACCAGC TGTTCGTGACCGTGGTGGACACCACCAGGAGCACCAACATGACCCTGTGCACCGAGGTGACCAA GGAGGGCACCTACAAGAACGACAACTTCAAGGAGTACGTGAGGCACGTGGAGGAGTACGACCTG CAGTTCGTGTTCCAGCTGTGCAAGATCACCCTGACCGCCGAGATCATGACCTACATCCACACCAT GGACAGCAACATCCTGGAGGACTGGCAGTTCGGCCTGACCCCCCCCCCCAGCGCCAGCCTGCAG GACACCTACAGGTTCGTGACCAGCCAGGCCATCACCTGCCAGAAGACCGCCCCCCCCAAGGAGA AGGAGGACCCCCTGAACAAGTACACCTTCTGGGAGGTGAACCTGAAGGAGAAGTTCAGCGCCGA CCTGGACCAGTTCCCCCTGGGCAGGAAGTTCCTGCTGCAGAGCGGCCTGAAGGCCAAGCCCAGG CTGAAGAGGAGCGCCCCCACCACCAGGGCCCCCAGCACCAAGAGGAAGAAGGTGAAGAAGTAA Sequence27(SEQIDNO:27): ATGACCGTGTACCTGCCCCCCGTGCCCGTGAGCAAGGTGGTGAGCACCGACGAGTACGTGAGCA GGACCAGCATCTACTACTACGCCGGCAGCAGCAGGCTGCTGGCCGTGGGCAACCCCTACTTCAGC ATCAAGAATCCCACTAACGCTAAAAAATTACTGGTGCCCAAGGTGAGCGGCCTGCAGTACAGGG TGTTCACrGGTGAGGCTGCCCGACCCCAACAAGTTCGGCTTCCCCGACACCAGCTTCTACAACCCC GACACCCAGAGGCTGGTGTGGGCCTGCGTGGGCCTGGAGATCGGCAGGGGCCAGCCCCTGGGCG TGGGCGTGAGCGGCCACCCCTACCTGAACAAGTTCGACGACACCGAGACCAGCAACAGGTACCC CGCCCAGCCCGGCAGCGACAACAGGGAGTGCCTGAGCATGGACTACAAGCAGACCCAGCTGTGC CTGATCGGCTGCAAGCCCCCCACCGGCGAGCACTGGGGCAAGGGCGTGGCCTGCAACAACAACG CCGCCGCCACCGACTGCCCCCCCCTGGAGCTGTTCAACAGCATCATCGAGGACGGCGACATGGTG GACACCGGCTTCGGCTGCATGGACTTCGGCACCCTGCAGGCCAACAAGAGCGACGTGCCCATCG ACATCTGCAACAGCACCTGCAAGTACCCCGACTACCTGAAGATGGCCAGCGAGCCCTACGGCGA CAGCCTGTTCTTCTTCCTGAGGAGGGAGCAGATGTTCGTGAGGCACTTCTTCAACAGGGCCGGCA CCCTGGGCGACCCCGTGCCCGGCGACCTGTACATCCAGGGCAGCAACAGCGGCAACACCGCCAC CGTGCAGAGCAGCGCCTTCTTCCCCACCCCCAGCGGCAGCATCGTGACCAGCGAGAGCCAGCTGT TCAACAAGCCCTACTGGCTGCAGAGGGCCCAGGGCCACAACAACGGCATCTGCTGGGGCAACCA GCTGTTCGTGACCGTGGTGGACACCACCAGGAGCACCAACATGACCCTGTGCACCGAGGTGACC AAGGAGGGCACCTACAAGAACGACAACTTCAAGGAGTACGTGAGGCACGTGGAGGAGTACGAC CTGCAGTTCGTGTTCCAGCTGTGCAAGATCACCCTGACCGCCGAGATCATGACCTACATCCACAC CATGGACAGCAACATCCTGGAGGACTGGCAGTTCGGCCTGACCCCCCCCCCCAGCGCCAGCCTGC AGGACACCTACAGGTTCGTGACCAGCCAGGCCATCACCTGCCAGAAGACCGCCCCCCCCAAGGA GAAGGAGGACCCCCTGAACAAGTACACCTTCTGGGAGGTGAACCTGAAGGAGAAGTTCAGCGCC GACCTGGACCAGTTCCCCCTGGGCAGGAAGTTCCTGCTGCAGAGCGGCCTGAAGGCCAAGCCCA GGCTGAAGAGGAGCGCCCCCACCACCAGGGCCCCCAGCACCAAGAGGAAGAAGGTGAAGAAGT AA Sequence28(SEQIDNO:28): ATGACCGTGTACCTGCCCCCCGTGCCCGTGAGCAAGGTGGTGAGCACCGACGAGTACGTGAGCA GGACCAGCATCTACTACTACGCCGGCAGCAGCAGGCTGCTGGCCGTGGGCAACCCCTACTTCAGC ATCAAGAATCCCACTAACGCTAAAAAATTACTGGTGCCCAAGGTGAGCGGCCTGCAGTACAGGG TGTTCAGGGTGAGGCTGCCCGACCCCAACAAGTTCGGCTTCCCCGACACCAGCTTCTACAACCCC GACACCCAGAGGCTGGTGTGGGCCTGCGTGGGCCTGGAGATCGGCAGGGGCCAGCCCCTGGGCG TGGGCGTGAGCGGCCACCCCTACCTGAACAAGTTCGACGACACCGAGACCAGCAACAGGTACCC CGCCCAGCCCGGCAGCGACAACAGGGAGTGCCTGAGCATGGACTACAAGCAGACCCAGCTGTGC CTGATCGGCTGCAAGCCCCCCACCGGCGAGCACTGGGGCAAGGGCGTGGCCTGCAACAACAACG CCGCCGCCACCGACTGCCCCCCCCTGGAGCTGTTCAACAGCATCATCGAGGACGGCGACATGGTG GACACCGGCTTCGGCTGCATGGACTTCGGCACCCTGCAGGCCAACAAGAGCGACGTGCCCATCG ACATCTGCAACAGCACCTGCAAGTACCCCGACTACCTGAAGATGGCCAGCGAGCCCTACGGCGA CAGCCTGTTCTTCTTCCTGAGGAGGGAGCAGATGTTCGTGAGGCACTTCTTCAACAGGGCCGGCA AGCTGGGCGAGGCCGTGCCCGACGACCTGTACATCAAGGGCAGCGGCAACACCGCCGTGATCCA GAGCAGCGCCTTCTTCCCCACCCCCAGCGGCAGCATCGTGACCAGCGAGAGCCAGCTGTTCAACA AGCCCTACTGGCTGCAGAGGGCCCAGGGCCACAACAACGGCATCTGCTGGGGCAACCAGCTGTT CGTGACCGTGGTGGACACCACCAGGAGCACCAACATGACCCTGTGCACCGAGGTGAAGAAGGAG AGCACCTACAAGAACGAGAACTTCAAGGAGTACGTGAGGCACGTGGAGGAGTACGACCTGCAGT TCGTGTTCCAGCTGTGCAAGATCACCCTGACCGCCGAGATCATGACCTACATCCACACCATGGAC AGCAACATCCTGGAGGACTGGCAGTTCGGCCTGACCCCCCCCCCCAGCGCCAGCCTGCAGGACA CCTACAGGTTCGTGACCAGCCAGGCCATCACCTGCCAGAAGACCGCCCCCCCCAAGGAGAAGGA GGACCCCCTGAACAAGTACACCTTCTGGGAGGTGAACCTGAAGGAGAAGTTCAGCGCCGACCTG GACCAGTTCCCCCTGGGCAGGAAGTTCCTGCTGCAGAGCGGCCTGAAGGCCAAGCCCAGGCTGA AGAGGAGCGCCCCCACCACCAGGGCCCCCAGCACCAAGAGGAAGAAGGTGAAGAAGTAA Sequence59(SEQIDNO:59): NPTNAKKL Sequence60(SEQIDNO:60): SDSTYKNE Sequence61(SEQIDNO:61): ISGHPLLNKFDDTETSNKYAGKPGI Sequence62(SEQIDNO:62): KKESTYKNE
Specific Modes for Carrying Out the Invention
(16) The present invention is further described by reference to the examples as follows, wherein the examples are used only for the purpose of illustrating the present invention, rather than limiting the present invention.
(17) Unless indicated otherwise, the molecular biological experimental methods and immunological assays used in the present invention are carried out substantially in accordance with the methods as described in Sambrook J et al., Molecular Cloning: A Laboratory Manual (Second Edition), Cold Spring Harbor Laboratory Press, 1989, and F. M. Ausubel et al., Short Protocols in Molecular Biology, 3rd Edition, John Wiley & Sons, Inc., 1995; and restriction enzymes are used under the conditions recommended by the manufacturers. Those skilled in the art understand that the examples are used for illustrating the present invention, but not intended to limit the protection scope of the present invention.
EXAMPLE 1. EXPRESSION AND PURIFICATION OF THE MUTATED HPV58 L1 PROTEINS
(18) Construction of Expression Vectors
(19) An expression vector encoding the mutated HPV58 L1 protein comprising a segment from HPV33 L1 protein was constructed by PCR for multi-site mutagenesis, wherein the initial template used was the plasmid pTO-T7-HPV58L1N35C (encoding the HPV58 L1 protein having 35 amino acids truncated at N-terminal; abbreviated as 58L1N35 in Table 2). The templates and primers for each PCR were shown in Table 2, and the amplification conditions for PCR were as followed: denaturation at 94 C. for 10 min; 25 cycles (denaturation at 94 C. for 50 sec, annealing at a given temperature for a certain period of time, and extension at 72 C. for 7.5 min); and final extension at 72 C. for 10 min. The sequences of the PCR primers used were listed in Table 3.
(20) To the amplification product (50 L), 2 L restriction endonuclease DpnI was added, and the resultant mixture was incubated at 37 C. for 60 min. 10 L of the product of digestion was used to transform 40 L competent E. coli ER2566 (purchased from New England Biolabs) prepared by the Calcium chloride method. The transformed E. coli was spread onto solid LB medium (the components of the LB medium: 10 g/L peptone, 5 g/L yeast powder, 10 g/L NaCl, the same hereinafter) containing kanamycin (at a final concentration of 25 mg/mL, the same hereinafter), and was subjected to static culture at 37 C. for 10-12 h until single colonies could be observed clearly. Single colony was picked and inoculated into a tube containing 4 mL liquid LB medium (containing kanamycin), and cultured with shaking at 220 rpm for 10 h at 37 C., and then 1 ml bacterial solution was taken and stored at 70 C. Plasmids were extracted from E. coli, and T7 primer was used to sequence the nucleotide sequences of the fragments of interest inserted into the plasmids. The sequencing result showed that the nucleotide sequences of the fragments of interest inserted into the constructed plasmids (expression vectors) were SEQ ID NO: 18, 19, 20, 21, 22, 23, and 24, respectively, and their encoded amino acid sequences were SEQ ID NO: 4, 5, 6, 7, 8, 9, and 10, respectively (the corresponding proteins were designated as H58N35-33T1, H58N35-33T2-1, H58N35-33T2-2, H58N35-33T2, H58N35-33T3, H58N35-33T4 and H58N35-33T5, respectively).
(21) The mutated protein H58N35-33T1 differs from HPV58N35 by: the substitution of the amino acid residues from positions 80 to 87 of wild type HPV58 L1 protein with the amino acid residues from positions 54 to 61 of wild type HPV33 L1 protein. The mutated protein H58N35-33T2 differs from HPV58N35 by: the substitution of the amino acid residues from positions 144 to 168 of wild type HPV58 L1 protein with the amino acid residues from positions 118 to 142 of wild type HPV33 L1 protein. The mutated protein H58N35-33T3 differs from HPV58N35 by: the substitution of the amino acid residues from positions 203 to 209 of wild type HPV58 L1 protein with the amino acid residues from positions 177 to 183 of wild type HPV33 L1 protein. The mutated protein H58N35-33T4 differs from HPV58N35 by: the substitution of the amino acid residues from positions 308 to 311 of wild type HPV58 L1 protein with the amino acid residues from positions 282 to 285 of wild type HPV33 L1 protein. The mutated protein H58N35-33T5 differs from HPV58N35 by: the substitution of the amino acid residues from positions 376 to 383 of wild type HPV58 L1 protein with the amino acid residues from positions 350 to 357 of wild type HPV33 L1 protein.
(22) Gibson assembly (Gibson D G, Young L, Chuang R Y, Venter J C, Hutchison C A, Smith H O. Enzymatic assembly of DNA molecules up to several hundred kilobases. Nat Methods. 2009; 6:343-5. doi: 10.1038/ntneth.1318) was used to construct the expression vector encoding the mutated HPV58 L1 protein having double substitutions, wherein the mutated HPV58 L1 protein comprised a segment from HPV33 L1 and a segment from HPV52L1. In brief, a short fragment comprising mutations and a long fragment comprising no mutation were obtained by PCR, and Gibson assembly system was then used to ligate the two fragments to form a ring. The initial template used comprised the plasmid pTO-T7-H58N35-33T1 (encoding the mutated protein H58N35-33T1; abbreviated as H58N35-33T1 in Table 2) and the plasmid pTO-T7-HPV52N40C (encoding the HPV52 L1 protein having 40 amino acids truncated at N-terminal; abbreviated as 52L1N40 in Table 2). The templates and primers for each PCR were shown in Table 2, and, the amplification conditions for PCR for amplifying the short fragment were as followed: denaturation at 94 C. for 10 min; 25 cycles (denaturation at 94 C. for 50 sec, annealing at a given temperature for a certain period of time, and extension at 72 C. for 1 min); and final extension at 72 C. for 10 min. The amplification conditions for PCR for amplifying the long fragment were as followed: denaturation at 94 C. for 10 min; 25 cycles (denaturation at 94 C. for 50 sec, annealing at a given temperature for a certain period of time, and extension at 72 C. for 7.5 min); and final extension at 72 C. for 10 min. The sequences of the PCR primers used were listed in Table 3. The amplification product was subjected to electrophoresis, the fragment of interest was then recovered by using DNA Extraction Kit, and its concentration was determined. The short fragment and long fragment obtained by amplification were mixed at a molar ratio of 2:1 (a total volume of 3 L), and 34 of 2 Gibson Assembly Master Mix (purchased from NEB, containing 15 exonuclease, Phusion DNA polymerase, Taq DNA ligase) was then added, and reacted at 50 C. for 1 h.
(23) The assembled product (64) was used to transform 40 L competent E. coli ER2566 (purchased from New England Biolabs) prepared by the Calcium chloride method. The transformed E. coli were spread onto solid LB medium containing kanamycin, and were subjected to static culture at 37 C. for 10-12 h until single colonies could be observed clearly. Single colony was picked and inoculated into a tube containing 4 mL liquid LB medium (containing kanamycin), and cultured with shaking at 220 rpm for 10 h at 37 C., and then 1 ml bacterial solution was taken and stored at 70 C. Plasmids were extracted from E. coli, and T7 primer was used to sequence the nucleotide sequences of the fragments of interest inserted into the plasmids. The sequencing result showed that the nucleotide sequences of the fragments of interest inserted into the constructed plasmids (expression vectors) were SEQ ID NO: 25, 26, 27, and 28, respectively, and their encoded amino acid sequences were SEQ ID NO: 11, 12, 13, and 14, respectively (the corresponding proteins were designated as H58N35-33T1-52S1, H58N35-33T1-52S2, 1-158N35-33T1-52S3, and H58N35-33T1-52S4, respectively).
(24) The mutated protein H58N35-33T1-52S1 differs from HPV58N35 by: the substitution of the amino acid residues from positions 80 to 87 of wild type HPV58 L1 protein with the amino acid residues from positions 54 to 61 of wild type HPV33 L1 protein, and the substitution of the amino acid residues from positions 144 to 168 of wild type HPV58 L1 protein with the amino acid residues from positions 146 to 170 of wild type HPV52 L1 protein. The mutated protein H58N35-33T1-52S2 differs from HPV58N35 by: the substitution of the amino acid residues from positions 80 to 87 of wild type HPV58 L1 protein with the amino acid residues from positions 54 to 61 of wild type HPV33 L1 protein, and the substitution of the amino acid residues from positions 200 to 209 of wild type HPV58 L1 protein with the amino acid residues from positions 202 to 212 of wild type HPV52 L1 protein. The mutated protein H58N35-33T1-52S3 differs from HPV58N35 by: the substitution of the amino acid residues from positions 80 to 87 of wild type HPV58 L1 protein with the amino acid residues from positions 54 to 61 of wild type HPV33 L1 protein, and the substitution of the amino acid residues from positions 292 to 312 of wild type HPV58 L1 protein with the amino acid residues from positions 295 to 317 of wild type HPV52 L1 protein. The mutated protein H58N35-33T1-52S4 differs from HPV58N35 by: the substitution of the amino acid residues from positions 80 to 87 of wild type HPV58 L1 protein with the amino acid residues from positions 54 to 61 of wild type HPV33 L1 protein, and the substitution of the amino acid residues from positions 375 to 383 of wild type HPV58 L1 protein with the amino acid residues from positions 380 to 388 of wild type HPV52 L1 protein.
(25) TABLE-US-00003 TABLE 2 PCR templates and primers for constructing expression vectors Template Upstream primer Downstream primer Product 58L1N35 H58N35-33T1-F H58N35-33T1-R H58N35-33T1 58L1N35 H58N35-33T2-1F H58N35-33T2-1R H58N35-33T2-1 H58N35-33T2-1 H58N35-33T2-2F H58N35-33T2-2R H58N35-33T2-2 H58N35-33T2-2 H58N35-33T2-3F H58N35-33T2-3R H58N35-33T2 58L1N35 H58N35-33T3-F H58N35-33T3-R H58N35-33T3 58L1N35 H58N35-33T4-F H58N35-33T4-R H58N35-33T4 58L1N35 H58N35-33T5-F H58N35-33T5-R H58N35-33T5 H58N35-33T1 G-V-H58N35-33T1-52S1-F G-V-H58N35-33T1-52S1-R H58N35-33T1-52S1 long fragment H58N35-33T1 G-V-H58N35-33T1-52S2-F G-V-H58N35-33T1-52S2-R H58N35-33T1-52S2 long fragment H58N35-33T1 G-V-H58N35-33T1-52S3-F G-V-H58N35-33T1-52S3-R H58N35-33T1-52S3 long fragment H58N35-33T1 G-V-H58N35-33T1-52S4-F G-V-H58N35-33T1-52S4-R H58N35-33T1-52S4 long fragment 52L1N40 G-H58N35-33T1-52S1-F G-H58N35-33T1-52S1-R H58N35-33T1-52S1 short fragment 52L1N40 G-H58N35-33T1-52S2-F G-H58N35-33T1-52S2-R H58N35-33T1-52S2 short fragment 52L1N40 G-H58N35-33T1-52S3-F G-H58N35-33T1-52S3-R H58N35-33T1-52S3 short fragment 52L1N40 G-H58N35-33T1-52S4-F G-H58N35-33T1-52S4-R H58N35-33T1-52S4 short fragment
(26) TABLE-US-00004 TABLE3 Sequencesoftheprimersused(SEQIDNOs:29-58) SEQIDNO: Primername Primersequence(5-3) 29 H58N35-33T1-F CTTCAGCATCAAGAATCCCACTAACGCTAAAAAATTA CTGGTGCCCAAGG 30 H58N35-33T1-R CCTTGGGCACCAGTAATTTTTTAGCGTTAGTGGGATTC TTGATGCTGAAG 31 H58N35-33T2-1F CCTGGGCGTCGGAATAAGCGGCCACCCCTTACTGAAC AAGTTCG 32 H58N35-33T2-1R CGAACTTGTTCAGTAAGGGGTGGCCGCTTATTCCGAC GCCCAGG 33 H58N35-33T2-2F CGACACCGAGACCGGAAACAAGTACCCCGCCCAGC 34 H58N35-33T2-2R GCTGGGCGGGGTACTTGTTTCCGGTCTCGGTGTCG 35 H58N35-33T2-3F AACAAGTACCCCGGACAGCCCGGCGCTGACAACAGG GAGT 36 H58N35-33T2-3R ACTCCCTGTTGTCAGCGCCGGGCTGTCCGGGGTACTTG TT 37 H58N35-33T3-F GGGGCAAGGGAGTAGCATGTACAAACGCTGCACCTGC CAACGACTGC 38 H58N35-33T3-R GCAGTCGTTGGCAGGTGCAGCGTTTGTACATGCTACT CCCTTGCCCC 39 H58N35-33T4-F CAAGGGCAGCGGCACAACAGCAAGTATCCAGAGCAG CG 40 H58N35-33T4-R CGCTGCTCTGGATACTTGCTGTTGTGCCGCTGCCCTTG 41 H58N35-33T5-F CCGAGGTGACCAGCGACAGCACGTACAAGAACGAGA ACTTCAAGGAG 42 H58N35-33T5-R CTCCTTGAAGTTCTCGTTCTTGTACGTGCTGTCGCTGG TCACCTCGG 43 G-V-H58N35-33T1- CTGATCGGCTGCAAGCCCCCCAC 52S1-F 44 G-V-H58N35-3311- CACGCAGGCCCACACCAGCC 52S1-R 45 G-V-H58N35-33T1- GAGCTGTTCAACAGCATCATCGAGG 52S2-F 46 G-V-H58N35-33T1- GGTGGGGGGCTTGCAGCCGATC 52S2-R 47 G-V-H58N35-33T1- ATCGTGACCAGCGAGAGCCAGC 52S3-F 48 G-V-H58N35-33T1- CTTCAGGTAGTCGGGGTACTTGC 52S3-R 49 G-V-H58N35-33T1- GTGAGGCACGTGGAGGAGTACG 52S4-F 50 G-V-H58N35-33T1- GGTGCACAGGGTCATGTTGGTG 52S4-R 51 G-H58N35-33T1-52S1- GAGGCTGGTGTGGGCCTGCGTGGGCCTGGAGATCGGC F AGG 52 G-H58N35-33T1-52S1- TGGGGGGCTTGCAGCCGATCAGGCACAGCTGGGTCTG R CTTG 53 G-H58N35-33T1-52S2- TGATCGGCTGCAAGCCCCCCACCGGCGAGCACTGGGG F CAAGGG 54 G-H58N35-33T1-52S2- TCGATGATGCTGTTGAACAGCTCCAGGGGGGGGCAGT R CGCCG 55 G-H58N35-33T1-52S3- GCAAGTACCCCGACTACCTGAAGATGGCCAGCGAGCC F CT 56 G-H58N35-33T1-52S3- GCTGGCTCTCGCTGGTCACGATGCTGCCGCTGGGGGT R G 57 G-H58N35-33T1-52S4- CACCAACATGACCCTGTGCACCGAGGTGAAGAAGGA F GAG 58 G-H58N35-33T1-52S4- CGTACTCCTCCACGTGCCTCACGTACTCCTTGAAGTTC R TCG
(27) Expression of the Mutated Proteins on a Large Scale
(28) The E. coli solutions comprising the recombinant plasmid pTO-T7-H58N35-33T1, pTO-T7-H58N35-33T2, pTO-T7-H58N35-33T3, pTO-T7-H58N35-33T4, pTO-T7-H58N35-33T5, pTO-T7-H58N35-33T1-52S1, pTO-T7-H58N35-33T1-52S2, pTO-T7-H58N35-33T1-52S3, and pTO-T7-H58N35-33T1-52S4, respectively, were taken from 70 C. refrigerator, were seeded in 100 mL LB liquid medium containing kanamycin, and incubated at 200 rpm and 37 C. for about 8 h. Then, the culture was transferred to 500 mL LB medium containing kanamycin (1 ml bacterial solution was transferred), and was further incubated. When the bacterial concentration reached an OD.sub.600 of about 0.6, the culturing temperature was lowered to 25 C. and 500 L IPTG was added to each culture bottle. The incubation was further performed for 8 h. After the incubation was finished, the bacteria were collected by centrifugation. The bacteria expressing H58N35-33T1, H58N35-33T2, H58N35-33T3, H58N35-33T4, H58N35-33T5, H58N35-33T1-52S1, H58N35-33T1-52S2, H58N35-33T1-52S3, and H58N35-33T1-52S4 protein, were obtained, respectively.
(29) Disruption of Bacteria Expressing the Mutated Proteins
(30) The bacteria obtained were re-suspended at a ratio of 1 g bacteria to 10 mL lysis buffer (20 mM Tris buffer, pH7.2, 300 mM NaCl). The bacteria were disrupted by using an ultrasonic apparatus for 30 min. The lysis solution containing the disrupted bacteria were centrifuged at 13500 rpm (30000 g) for 15 min, and the supernatant (i.e. the supernatant of disrupted bacteria) was obtained.
(31) Chromatographic Purification of the Mutated Protein
(32) Equipment: AKTA Explorer 100 preparative liquid chromatography system produced by GE Healthcare (i.e. the original Amershan Pharmacia Co.)
(33) Chromatographic media: SP Sepharose 4 Fast Flow (GE Healthcare Co.), CHT-II (purchased from Bio-RAD) and Butyl Sepharose 4 Fast Flow (GE Healthcare Co.)
(34) Buffer: 20 mM phosphate buffer, pH8.0, 20 mM DTT; and, 20 mM phosphate buffer, pH8.0, 20 mM DTT, 2 M NaCl.
(35) Sample: the supernatants of disrupted bacteria containing H58N35-33T1, H58N35-33T2, H58N35-33T3, H58N35-33T4, H58N35-33T5, H58N35-33T1-52S1, H58N35-33T1-52S2, H58N35-33T1-52S3, and H58N35-33T1-52S4, respectively, as obtained above.
(36) Elution Protocol
(37) (1) Cation exchange purification of the supernatant of disrupted bacteria by SP Sepharose 4 Fast Flow: the sample was loaded on the column, undesired proteins were then eluted with a buffer containing 400 mM NaCl, followed by the elution of the protein of interest with a buffer containing 800 mM NaCl, and the fraction eluted with the buffer containing 800 mM NaCl was collected;
(38) (2) Chromatographic purification of the elution fraction obtained in the step (1) by CHTII (hydroxyapatite chromatography): the elution fraction obtained in the step (1) was diluted so that the NaCl concentration was decreased to 0.5 M; the sample was loaded on the column, undesired proteins were then eluted with a buffer containing 500 mM NaCl, followed by the elution of the protein of interest with a buffer containing 1000 mM NaCl, and the fraction eluted with the buffer containing 1000 mM NaCl was collected;
(39) (3) Chromatographic purification of the elution fraction obtained in the step (2) by HIC (hydrophobic interaction chromatography): the sample was loaded on the column, undesired proteins were then eluted with a buffer containing 1000 mM NaCl, followed by the elution of the protein of interest with a buffer containing 200 mM NaCl, and the fraction eluted with the buffer containing 200 mM NaCl was collected.
(40) 150 L elution fraction obtained in the step (3) was added to 30 L of 6 Loading Buffer. The resultant solution was mixed homogeneously and incubated in 80 C. water bath for 10 mM. 10 l of the resultant sample was then subjected to 10% SDS-PAGE at 120V for 120 mM; and the electrophoretic bands were stained by Coomassie brilliant blue. The electrophoretic result was shown in
(41) By similar methods, HPV58N35 protein was prepared and purified by using E. coli and the plasmid pTO-T7-HPV58L1N35C; HPV52N40 protein was prepared and purified by using E. coli and the plasmid pTO-T7-HPV52N40C; and HPV33N9 protein was prepared and purified by using E. coli and the plasmid pTO-T7-HPV33L1N9C (encoding HPV33N9 protein).
(42) Western Blot Assay of the Mutated Proteins
(43) The H58N35-33T1, H58N35-33T2, H58N35-33T3, H58N35-33T4, H58N35-33T5, H58N35-33T1-52S1, H58N35-33T1-52S2, H58N35-33T1-52S3, and H58N35-33T1-52S4 purified by the method above were subjected to electrophoresis. After electrophoresis, Western Blot assay was carried out by using a broad-spectrum antibody 4B3 against HPV L1 protein, and the result was shown in
EXAMPLE 2: ASSEMBLY OF HPV VIRUS-LIKE PARTICLES AND MORPHOLOGICAL DETECTION OF PARTICLES
(44) Assembly of HPV Virus-Like Particles
(45) A given volume (about 2 ml) of the protein H58N35-33T1, H58N35-33T2, H58N35-33T3, H58N35-33T4, H58N35-33T5, H58N35-33T1-52S1, H58N35-33T1-52S2, H58N35-33T1-52S3, or H58N35-33T1-52S4, was dialyzed to (1) 2 L storage buffer (20 mM sodium phosphate buffer pH 6.5, 0.5 M NaCl); (2) 2 L renaturation buffer (50 mM sodium phosphate buffer pH 6.0, 2 mM CaCl.sub.2, 2 mM MgCl.sub.2, 0.5 M NaCl); and (3) 20 mM sodium phosphate buffer pH 7.0, 0.5 M NaCl, successively. The dialysis was performed in each of the three buffers for 12 h.
(46) By similar methods, the HPV58N35, HPV33N9 and HPV52N40 protein were assembled into HPV58N35 VLP, HPV33N9 VLP and HPV52N40 VLP, respectively.
(47) Molecular Sieve Chromatographic Analysis
(48) The dialyzed sample was subjected to molecular sieve chromatographic analysis by 1120 Compact LC High Performance Liquid Chromatographic System (Agilent Technologies), wherein the analytical column used was TSK Gel PW5000xl 7.8300 mm. The analysis results were shown in
(49) Sedimentation Velocity Analysis
(50) The apparatus for sedimentation velocity analysis was Beckman XL-A Analytical Ultracentrifuge, equipped with optical inspection system and An-50Ti and An-60Ti rotor. The sedimentation coefficient of H58N35 VLP, HPV33N9 VLP and H58N35-33T1 VLP was analyzed by sedimentation velocity method. The results were shown in
(51) Morphological Test of Virus-Like Particles
(52) A 100 L sample comprising VLP was observed by transmission electron microscope (TEM). The equipment used was a 100 kV Transmission Electron Microscope supplied by JEOL Ltd. (100,000 magnification). In brief, a 13.5 L sample was negatively stained with 2% phosphotungstic acid (pH 7.0), fixed on a carbon-coated copper grid, and then observed by TEM. The results were shown in
EXAMPLE 3: EVALUATION OF THERMOSTABILITY OF VIRUS-LIKE PARTICLES
(53) The VLPs formed by H58N35-33T1, H58N35-33T1-52S1, H58N35-33T1-52S2, H58N35-33T1-52S3, and H58N35-33T1-52S4 were evaluated for their thermostability by using a differential scanning calorimeter VP Capillary DSC purchased from GE Company (i.e. the MicroCal Co.), wherein the storage buffer for the protein was used as control, and the proteins were scanned at a heating rate of 1.5 C./min within a temperature range of 10 C.-90 C. The detection results were shown in
EXAMPLE 4: EVALUATION 1 OF IMMUNE PROTECTION OF VIRUS-LIKE PARTICLES IN ANIMALS
(54) The immune protection of the VLPs formed by H58N35-33T1, H58N35-33T3, H58N35-33T4, H58N35-33T5, H58N35-33T1-52S1, H58N35-33T1-52S2, H58N35-33T1-52S3, and H58N35-33T1-52S4, was evaluated in mice. Animals for vaccination were BALB/c mice (ordinary grade), 5-6 weeks old (purchased from Shanghai SLAC Laboratory Animal Co. LTD.).
(55) The H58N35-33T1 VLP, H58N35-33T3 VLP, H58N35-33T4 VLP, H58N35-33T5 VLP, HPV58N35 VLP and HPV33N9 VLP as prepared above were absorbed onto Freund's adjuvant, respectively. Mice were divided into 6 groups depending on immunogen, and each group included 3 mice. Vaccination procedure was as followed: the first vaccination at Week 0, and the booster vaccination at Weeks 2 and 4, respectively. Mice were vaccinated via subcutaneous injection. The immunogens used and doses thereof were shown in Table 4. At Week 8 after the first vaccination, venous blood was collected from eyeball, and serum was separated. The titers of neutralizing antibodies in the serum were determined. The detection result was shown in
(56) TABLE-US-00005 TABLE 4 Vaccination schedule Vaccination Antigen for Immunizing procedure vaccination Adjuvant dose Number (week) HPV33N9 VLP Freund's 100 g 3 0, 2, 4 adjuvant HPV58N35 VLP Freund's 100 g 3 0, 2, 4 adjuvant H58N35-33T1VLP Freund's 100 g 3 0, 2, 4 adjuvant H58N35-33T3 VLP Freund's 100 g 3 0, 2, 4 adjuvant H58N35-33T4 VLP Freund's 100 g 3 0, 2, 4 adjuvant H58N35-33T5 VLP Freund's 100 g 3 0, 2, 4 adjuvant
(57) In addition, the H58N35-33T1-52S1 VLP, H58N35-33T1-52S2 VLP, H58N35-33T1-52S3 VLP, H58N35-33T1-52S4 VLP, HPV58N35 VLP, HPV33N9 VLP, HPV52N40 VLP and a mixed HPV58/HPV33/HPV52 VLP (i.e. a mixture of HPV58N35 VLP, HPV33N9 VLP and HPV52N40 VLP) as prepared above were absorbed onto aluminum adjuvant. Mice were divided into 8 groups depending on immunogen, and each group included 4 mice. Vaccination procedure was as followed: the first vaccination at Week 0, and the booster vaccination at Weeks 2 and 4, respectively. Mice were vaccinated via intraperitoneal injection. The immunogens and doses thereof were shown in Table 5. At Week 8 after the first vaccination, venous blood was collected from eyeball, and serum was separated. The titers of neutralizing antibodies in the serum were determined. The detection result was shown in
(58) TABLE-US-00006 TABLE 5 Vaccination schedule Vaccination Antigen for Immunizing procedure vaccination Adjuvant dose Number (week) HPV33N9 VLP aluminum 5 g 4 0, 2, 4 adjuvant HPV52N40 VLP aluminum 5 g 4 0, 2, 4 adjuvant HPV58N35 VLP aluminum 5 g 4 0, 2, 4 adjuvant H58N35-33T1-52S1 VLP aluminum 5 g 4 0, 2, 4 adjuvant H58N35-33T1-52S2 VLP aluminum 5 g 4 0, 2, 4 adjuvant H58N35-33T1-52S3 VLP aluminum 5 g 4 0, 2, 4 adjuvant H58N35-33T1-52S4 VLP aluminum 5 g 4 0, 2, 4 adjuvant HPV58/HPV33/HPV52 VLP aluminum 5 g for each VLP 4 0, 2, 4 adjuvant
EXAMPLE 5: EVALUATION 2 OF IMMUNE PROTECTION OF VIRUS-LIKE PARTICLES IN ANIMALS
(59) ED.sub.50 of H58N35-33T1 VLP
(60) 6-week old BalB/c female mice (8 mice) were vaccinated with aluminum adjuvant by single intraperitoneal injection, wherein H58N35-33T1 VLP was used in the Experimental groups, and HPV58N35 VLP alone or HPV33N9 VLP alone was used in the Control groups; the immunizing dose was 0.300 g, 0.100 g, 0.033 g, 0.011 g or 0.004 g; the immunizing volume was 1 mL. At Week 5 after vaccination, venous blood was collected from eyeball. Antibodies against HPV in the blood were detected, and by Reed-Muench method (Reed L J M H. A simple method of estimating fifty percent endpoints. Am J Hyg. 1938; 27:493-7), ED.sub.50 for inducing seroconversion (i.e. inducing the generation of antibodies in mice) was calculated for each sample. The results were shown in Tables 6-8.
(61) TABLE-US-00007 TABLE 6 ED.sub.50 of HPV33N9 VLP for inducing the generation of antibodies against HPV33, HPV58 in mice Number of mice with Positive Dose Total number positive conversion ED.sub.50 Type (g) of mice conversion rate (g) HPV33 0.300 8 8 100.00% 0.066 0.100 8 5 70.00% 0.033 8 1 16.67% 0.011 8 1 5.56% 0.004 8 0 0.00% HPV58 0.300 8 0 0.00% >0.3 0.100 8 0 0.00% 0.033 8 0 0.00% 0.011 8 0 0.00% 0.004 8 0 0.00%
(62) TABLE-US-00008 TABLE 7 ED.sub.50 of H58N35-33T1 VLP for inducing the generation of antibodies against HPV33, HPV58 in mice Number of mice with Positive Dose Total number positive conversion ED50 Type (g) of mice conversion rate (g) HPV33 0.300 8 7 94.74% 0.043 0.100 8 6 78.57% 0.033 8 4 41.67% 0.011 8 0 6.25% 0.004 8 1 4.35% HPV58 0.300 8 8 100.00% 0.019 0.100 8 8 100.00% 0.033 8 7 88.89% 0.011 8 1 11.11% 0.004 8 0 0.00%
(63) TABLE-US-00009 TABLE 8 ED.sub.50 of HPV58N35 VLP for inducing the generation of antibodies against HPV33, HPV58 in mice Number of mice with Positive Dose Total number positive conversion ED.sub.50 Type (g) of mice conversion rate (g) HPV33 0.300 8 0 0.00% >0.3 0.100 8 0 0.00% 0.033 8 0 0.00% 0.011 8 0 0.00% 0.004 8 0 0.00% HPV58 0.300 8 8 100.00% 0.006 0.100 8 8 100.00% 0.033 8 7 94.12% 0.011 8 6 75.00% 0.004 8 3 27.27%
(64) The results showed that 5 weeks after vaccination of mice, ED.sub.50 of H58N35-33T1 VLP for inducing the generation of antibodies against HPV58 in mice was comparable to that of HPV58N35 VLP alone, and was significantly superior to that of HPV33N9 VLP alone; and its ED.sub.50 for inducing the generation of antibodies against HPV33 in mice was comparable to that of HPV33N9 VLP alone, and was significantly superior to that of HPV58N35 VLP alone. This showed that H58N35-33T1 VLP had good cross-immunogenicity and cross-protection against HPV58 and HPV33.
(65) ED.sub.50 of H58N35-33T1-52S1 VLP and H58N35-58T1-52S4 VLP
(66) 6-week old BalB/c female mice (8 mice) were vaccinated with aluminum adjuvant by single intraperitoneal injection, wherein H58N35-33T1-52S1 VLP or H58N35-58T1-52S4 VLP was used in the Experimental groups (at an immunizing dose of 0.900 g, 0.300 g, 0.100 g, 0.033 g, 0.011 g or 0.004 g); HPV33N9 VLP alone, HPV58N35 VLP alone or HPV52N40 VLP alone (at an immunizing dose of 0.300 g, 0.100 g, 0.033 g, 0.011 g or 0.004 g), or a mixture of HPV33N9 VLP, HPV58N35 VLP and HPV52N40 VLP (for each VLP, the immunizing dose was 0.300 g, 0.100 g, 0.033 g, 0.011 g or 0.004 g) was used in the Control groups; and the immunizing volume was 1 mL. At Week 5 after vaccination, venous blood was collected from eyeball. Antibodies against HPV in the blood were detected, and by Reed-Muench method (Reed L J M H. A simple method of estimating fifty percent endpoints. Am J Hyg. 1938; 27:493-7), ED.sub.50 for inducing seroconversion (i.e. inducing the generation of antibodies in mice) was calculated for each sample. The results were shown in Tables 9-14.
(67) TABLE-US-00010 TABLE 9 ED.sub.50 of HPV33N9 VLP for inducing the generation of antibodies against HPV33, HPV58 and HPV52 in mice Number of mice with Positive Dose Total number positive conversion ED50 Type (g) of mice conversion rate (g) HPV33 0.300 8 8 100.00% 0.013 0.100 8 7 94.74% 0.033 8 6 78.57% 0.011 8 5 45.45% 0.004 8 0 0.00% HPV58 0.300 8 0 0.00% >0.3 0.100 8 0 0.00% 0.033 8 0 0.00% 0.011 8 0 0.00% 0.004 8 0 0.00% HPV52 0.300 8 0 0.00% >0.3 0.100 8 0 0.00% 0.033 8 0 0.00% 0.011 8 0 0.00% 0.004 8 0 0.00%
(68) TABLE-US-00011 TABLE 10 ED.sub.50 of HPV58N35 VLP for inducing the generation of antibodies against HPV33, HPV58 and HPV52 in mice Number of mice with Positive Dose Total number positive conversion ED50 Type (g) of mice conversion rate (g) HPV33 0.300 8 1 12.50% >0.3 0.100 8 0 0.00% 0.033 8 0 0.00% 0.011 8 0 0.00% 0.004 8 0 0.00% HPV58 0.300 8 8 100.00% 0.021 0.100 8 7 93.75% 0.033 8 7 80.00% 0.011 8 1 10.00% 0.004 8 0 0.00% HPV52 0.300 8 0 0.00% >0.3 0.100 8 0 0.00% 0.033 8 0 0.00% 0.011 8 0 0.00% 0.004 8 0 0.00%
(69) TABLE-US-00012 TABLE 11 ED.sub.50 of HPV52N40 VLP for inducing the generation of antibodies against HPV33, HPV58 and HPV52 in mice Number of mice with Positive Dose Total number positive conversion ED50 Type (g) of mice conversion rate (g) HPV33 0.300 8 0 0.00% >0.3 0.100 8 0 0.00% 0.033 8 0 0.00% 0.011 8 0 0.00% 0.004 8 0 0.00% HPV58 0.300 8 0 0.00% >0.3 0.100 8 0 0.00% 0.033 8 0 0.00% 0.011 8 0 0.00% 0.004 8 0 0.00% HPV52 0.300 8 8 100.00% 0.046 0.100 8 7 90.91% 0.033 8 3 33.33% 0.011 8 0 0.00% 0.004 8 0 0.00%
(70) TABLE-US-00013 TABLE 12 ED.sub.50 of a mixture of HPV33N9 VLP, HPV58N35 VLP and HPV52N40 VLP for inducing the generation of antibodies against HPV33, HPV58 and HPV52 in mice Number of mice with Positive Dose Total number positive conversion ED50 Type (g) of mice conversion rate (g) HPV33 0.300 for each VLP 8 6 93.33% 0.009 0.100 for each VLP 8 8 91.67% 0.033 for each VLP 8 6 77.78% 0.011 for each VLP 8 7 61.54% 0.004 for each VLP 8 1 7.69% HPV58 0.300 for each VLP 8 6 93.10% 0.009 0.100 for each VLP 8 8 91.30% 0.033 for each VLP 8 5 72.22% 0.011 for each VLP 8 8 61.54% 0.004 for each VLP 8 0 0.00% HPV52 0.300 for each VLP 8 6 92.31% 0.017 0.100 for each VLP 8 8 90.00% 0.033 for each VLP 8 5 66.67% 0.011 for each VLP 8 5 38.46% 0.004 for each VLP 8 0 0.00%
(71) TABLE-US-00014 TABLE 13 ED.sub.50 of H58N35-33T1-52S1 VLP for inducing the generation of antibodies against HPV33, HPV58 and HPV52 in mice Number of mice with Positive Dose Total number positive conversion ED50 Type (g) of mice conversion rate (g) HPV33 0.900 8 8 100.00% 0.009 0.300 8 8 100.00% 0.100 8 7 95.24% 0.033 8 5 76.47% 0.011 8 6 57.14% 0.004 8 2 14.29% HPV58 0.900 8 8 100.00% 0.014 0.300 8 7 96.15% 0.100 8 7 90.00% 0.033 8 4 64.71% 0.011 8 6 46.67% 0.004 8 1 6.25% HPV52 0.900 8 7 91.67% 0.341 0.300 8 4 44.44% 0.100 8 0 0.00% 0.033 8 0 0.00% 0.011 8 0 0.00% 0.004 8 0 0.00%
(72) TABLE-US-00015 TABLE 14 ED.sub.50 of H58N35-33T1-52S4 VLP for inducing the generation of antibodies against HPV33, HPV58 and HPV52 in mice Number of mice with Positive Dose Total number positive conversion ED50 Type (g) of mice conversion rate (g) HPV33 0.900 8 8 100.00% 0.065 0.300 8 8 100.00% 0.100 8 5 70.00% 0.033 8 2 18.18% 0.011 8 0 0.00% 0.004 8 0 0.00% HPV58 0.900 8 8 100.00% 0.041 0.300 8 8 100.00% 0.100 8 7 91.67% 0.033 8 3 40.00% 0.011 8 1 7.14% 0.004 8 0 0.00% HPV52 0.900 8 8 100.00% 0.058 0.300 8 8 100.00% 0.100 8 6 80.00% 0.033 8 2 20.00% 0.011 8 0 0.00% 0.004 8 0 0.00%
(73) The results showed that 5 weeks after vaccination of mice, ED.sub.50 of H58N35-33T1-52S1 VLP and H58N35-33T1-52S4 VLP for inducing the generation of antibodies against HPV58 in mice was comparable to that of HPV58N35 VLP alone and of a mixture of HPV58N35 VLP, HPV33N9 VLP and HPV52N40 VLP, and was significantly superior to that of HPV33N9 VLP alone and HPV52N40 VLP alone; and their ED.sub.50 for inducing the generation of antibodies against HPV33 in mice was comparable to that of HPV33N9 VLP alone and of a mixture of HPV58N35 VLP, HPV33N9 VLP and HPV52N40 VLP, and was significantly superior to that of HPV58N35 VLP alone and of HPV52N40 VLP alone; and their ED.sub.50 for inducing the generation of antibodies against HPV52 in mice was comparable to that of HPV52N40 VLP alone and of a mixture of HPV58N35 VLP, HPV33N9 VLP and HPV52N40 VLP, and was significantly superior to that of HPV33N9 VLP alone and of HPV58N35 VLP alone. This showed that H33N9-58T5-52S2 VLP and H33N9-58T5-52S4 VLP had good cross-immunogenicity and cross-protection against HPV58, HPV33 and HPV52.
(74) Evaluation of Neutralizing Antibody Titer in Serum of Mice Vaccinated with H58N35-33T1 VLP
(75) In this experiment, vaccination schedule was shown in Table 15. All the mice (6-week old BalB/c female mice) were divided into 4 groups: Freund's adjuvant group (at an immunizing dose of 1 g, using Freund's adjuvant), Aluminum adjuvant group 1 (at an immunizing dose of 10 g, using aluminum adjuvant), Aluminum adjuvant group 2 (at an immunizing dose of 1 g, using aluminum adjuvant), and Aluminum adjuvant group 3 (at an immunizing dose of 0.1 g, using aluminum adjuvant). Each group was further divided into 3 subgroups. The Control subgroups 1 and 2 were vaccinated with HPV33N9 VLP alone and HPV58N35 VLP alone, respectively, and the Experimental subgroup was vaccinated with H58N35-33T1 VLP.
(76) In Freund's adjuvant group, 6 mice/subgroup were vaccinated by subcutaneous injection, at an immunizing dose of 1 g, and an injection volume of 200 l. In Aluminum adjuvant groups 1-3, 6 mice/subgroup were vaccinated by intraperitoneal injection, at an immunizing dose 10 g, 1 g, and 0.1 g, respectively, and an injection volume of 1 mL. All the mice were subjected to the first vaccination at Week 0, and then subjected to the booster vaccination at Weeks 2 and 4, respectively. At Week 8, blood sample was collected via orbital bleeding, and the titers of antibodies against HPV58 and HPV33 in serum were analyzed. The analysis results were shown in
(77) TABLE-US-00016 TABLE 15 Vaccination schedule Vaccination Antigen for Immunizing procedure Group vaccination Adjuvant dose Number (week) Freund's adjuvant HPV58N35 VLP Freund's 1 g 6 0, 2, 4 group adjuvant HPV33N9 VLP Freund's 1 g 6 0, 2, 4 adjuvant H58N35-33T1 VLP Freund's 1 g 6 0, 2, 4 adjuvant Aluminum adjuvant HPV58N35 VLP aluminum 10 g 6 0, 2, 4 group 1 adjuvant HPV33N9 VLP aluminum 10 g 6 0, 2, 4 adjuvant H58N35-33T1 VLP aluminum 10 g 6 0, 2, 4 adjuvant Aluminum adjuvant HPV58N35 VLP aluminum 1 g 6 0, 2, 4 group 2 adjuvant HPV33N9 VLP aluminum 1 g 6 0, 2, 4 adjuvant H58N35-33T1 VLP aluminum 1 g 6 0, 2, 4 adjuvant Aluminum adjuvant HPV58N35 VLP aluminum 0.1 g 6 0, 2, 4 group 3 adjuvant HPV33N9 VLP aluminum 0.1 g 6 0, 2, 4 adjuvant H58N35-33T1 VLP aluminum 0.1 g 6 0, 2, 4 adjuvant
(78) Evaluation of Neutralizing Antibody Titer in Serum of Mice Vaccinated with H58N35-33T1-52S1 VLP or H58N35-33T1-52S4 VLP
(79) In this experiment, vaccination schedule was shown in Table 16. All the mice (6-week old BalB/c female mice) were divided into 3 groups: Aluminum adjuvant group 1 (at an immunizing dose of 10 g, using aluminum adjuvant), Aluminum adjuvant group 2 (at an immunizing dose of 1 g, using aluminum adjuvant), and Aluminum adjuvant group 3 (at an immunizing dose of 0.1 g, using aluminum adjuvant). Each group was further divided into 6 subgroups. The Control subgroups 1, 2 and 3 were vaccinated with HPV58N35 VLP alone, HPV33N9 VLP alone and HPV52N40 VLP alone, respectively; the Control subgroup 4 was vaccinated with a mixture of HPV58N35 VLP, HPV33N9 VLP and HPV52N40 VLP; and the Experimental subgroups 1 and 2 were vaccinated with H58N35-33T1-52S1 VLP alone and H58N35-33T1-52S4 VLP alone, respectively.
(80) In Aluminum adjuvant groups 1-3, 6 mice/subgroup were vaccinated by intraperitoneal injection, at an immunizing dose of 10 g, 1 g, and 0.1 g, respectively, and an injection volume of 1 mL. All the mice were subjected to the first vaccination at Week 0, and then subjected to the booster vaccination at Weeks 2 and 4, respectively. At Week 8, blood sample was collected via orbital bleeding, and the titers of antibodies against HPV58, HPV33 and HPV52 in serum were analyzed. The analysis results were shown in
(81) TABLE-US-00017 TABLE 16 Vaccination schedule Vaccination Antigen for Immunizing procedure Group vaccination Adjuvant dose Number (week) Aluminum HPV33N9 VLP aluminum 10 g 6 0, 2, 4 adjuvant adjuvant group 1 HPV58N35 VLP aluminum 10 g 6 0, 2, 4 adjuvant HPV52N40 VLP aluminum 10 g 6 0, 2, 4 adjuvant HPV58/HPV33/HPV52 VLP aluminum 10 g for each VLP 6 0, 2, 4 adjuvant H58N35-33T1-52S1 VLP aluminum 10 g 6 0, 2, 4 adjuvant H58N35-33T1-52S4 VLP aluminum 10 g 6 0, 2, 4 adjuvant Aluminum HPV33N9 VLP aluminum 1 g 6 0, 2, 4 adjuvant adjuvant group 2 HPV58N35 VLP aluminum 1 g 6 0, 2, 4 adjuvant HPV52N40 VLP aluminum 1 g 6 0, 2, 4 adjuvant HPV58/HPV33/HPV52 VLP aluminum 1 g for each VLP 6 0, 2, 4 adjuvant H58N35-33T1-52S1 VLP aluminum 1 g 6 0, 2, 4 adjuvant H58N35-33T1-52S4 VLP aluminum 1 g 6 0, 2, 4 adjuvant Aluminum HPV33N9 VLP aluminum 0.1 g 6 0, 2, 4 adjuvant adjuvant group 3 HPV58N35 VLP aluminum 0.1 g 6 0, 2, 4 adjuvant HPV52N40 VLP aluminum 0.1 g 6 0, 2, 4 adjuvant HPV58/HPV33/HPV52 VLP aluminum 0.1 g for each VLP 6 0, 2, 4 adjuvant H58N35-33T1-52S1 VLP aluminum 0.1 g 6 0, 2, 4 adjuvant H58N35-33T1-52S4 VLP aluminum 0.1 g 6 0, 2, 4 adjuvant
EXAMPLE 6: EVALUATION OF IMMUNE PROTECTION OF H58N35-33T1-52S4 VLP IN CYNOMOLGUS MONKEY
(82) This experiment was carried out in the Yunnan Key Laboratory of Primate Biomedical Research. Vaccination schedule was shown in Table 17. 14 cynomolgus monkeys were randomly divided into two groups: the Control group was vaccinated with a mixture of HPV58N35 VLP, HPV33N9 VLP and HPV52N40 VLP, at a dose of 5 g for each VLP, and an injection volume of 1 mL; the Experimental group was vaccinated with H58N35-33T1-52S4 VLP alone, at a dose of 5 g, and an injection volume of 1 mL. The adjuvant used was aluminum adjuvant, and the cynomolgus monkeys were vaccinated by intramuscular injection. All the cynomolgus monkeys were subjected to the first vaccination at Week 0, and then subjected to the booster vaccination at Week 8. Blood was collected from cynomolgus monkeys at Week 10, and the titers of antibodies against HPV58, HPV33 and HPV52 in serum were analyzed. The analysis result was shown in
(83) TABLE-US-00018 TABLE 17 Vaccination schedule Vaccination Antigen for Immunizing procedure vaccination Adjuvant dose Number (week) H58N35-33T1-52S4 VLP aluminum 5 g 7 0, 8 adjuvant HPV58/HPV33/HPV52 VLP aluminum 5 g for each VLP 7 0, 8 adjuvant
EXAMPLE 7: RECONSTRUCTION OF THREE-DIMENSIONAL STRUCTURES OF H58N35-33T1 VLP AND H58N35-33T1-52S4 VLP
(84) The three-dimensional structures of H58N35-33T1 VLP and H58N35-33T1-52S4 VLP were reconstructed by three-dimensional structure reconstruction experiment using cryo-electron microscopy (cryoEM) (Wolf M, Garcea R L, Grigorieff N. et al. Proc Natl Acad Sci USA. (2010), 107(14): 6298-303). In brief, in the cryo-electron microscopy (cryoEM) photograph of H58N35-33T1 VLP (
(85) Although the specific embodiments of the present invention have been described in details, those skilled in the art would understand that, according to the teachings disclosed in the specification, various modifications and changes can be made thereto, and that such modifications and changes are within the scope of the present invention. The scope of the present invention is given by the appended claims and any equivalents thereof.