Identification of a conserved JEV serocomplex B-cell epitope by screening a phage-display peptide library with a mAb generated against West Nile virus capsid protein.

Szczegóły
Abstrakt

Tytuł:: Identification of a conserved JEV serocomplex B-cell epitope by screening a phage-display peptide library with a mAb generated against West Nile virus capsid protein.
Autorzy:: Sun EC; The Key Laboratory of Veterinary Public Health, Ministry of Agriculture, State Key Laboratory of Veterinary Biotechnology, Harbin Veterinary Research Institute, Chinese Academy of Agricultural Sciences, Harbin 150001, PR China.
Zhao J
Yang T
Liu NH
Geng HW
Qin YL
Wang LF
Bu ZG
Yang YH
Lunt RA
Wang LF
Wu DL
Źródło:: Virology journal [Virol J] 2011 Mar 06; Vol. 8, pp. 100. Date of Electronic Publication: 2011 Mar 06.
Typ publikacji:: Journal Article; Research Support, Non-U.S. Gov't
Język:: English
Imprint Name(s):: Original Publication: [London] : BioMed Central, 2004-
MeSH Terms:: Conserved Sequence*
Peptide Library*
Antibodies, Monoclonal/*analysis
Capsid Proteins/*chemistry
Encephalitis Virus, Japanese/*chemistry
Epitopes, B-Lymphocyte/*chemistry
West Nile virus/*chemistry
Amino Acid Sequence ; Capsid Proteins/genetics ; Capsid Proteins/immunology ; Encephalitis Virus, Japanese/genetics ; Encephalitis Virus, Japanese/immunology ; Encephalitis, Japanese/immunology ; Encephalitis, Japanese/virology ; Epitope Mapping ; Epitopes, B-Lymphocyte/genetics ; Epitopes, B-Lymphocyte/immunology ; Humans ; Molecular Sequence Data ; Sequence Alignment ; West Nile Fever/immunology ; West Nile Fever/virology ; West Nile virus/genetics ; West Nile virus/immunology
References:: J Virol Methods. 2007 May;141(2):133-40. (PMID: 17215048)
J Virol. 2010 Sep;84(18):9227-39. (PMID: 20592088)
Curr Drug Targets. 2004 Jan;5(1):1-15. (PMID: 14738215)
Virus Res. 2008 Aug;135(2):267-72. (PMID: 18485511)
Mol Immunol. 2008 Nov;46(1):125-34. (PMID: 18760481)
J Mol Biol. 2007 Jan 5;365(1):196-210. (PMID: 17059824)
Virology. 1988 Sep;166(1):197-205. (PMID: 3413985)
Blood. 2005 Jun 1;105(11):4337-44. (PMID: 15701713)
Proc Natl Acad Sci U S A. 2004 Mar 9;101(10):3414-9. (PMID: 14993605)
J Virol. 2001 Mar;75(5):2204-12. (PMID: 11160724)
Structure. 2004 Jul;12(7):1157-63. (PMID: 15242592)
Nature. 1975 Aug 7;256(5517):495-7. (PMID: 1172191)
Arch Virol. 2006 Jan;151(1):37-54. (PMID: 16132176)
J Virol. 2009 Apr;83(8):3617-25. (PMID: 19193787)
Biotechnol Annu Rev. 2004;10:151-88. (PMID: 15504706)
J Virol. 1996 Jan;70(1):141-7. (PMID: 8523518)
J Virol. 2001 Oct;75(20):9986-90. (PMID: 11559832)
Emerg Infect Dis. 2002 Jul;8(7):652-6. (PMID: 12095429)
Vet Res. 2004 Jul-Aug;35(4):467-83. (PMID: 15236677)
Arch Virol. 2009;154(8):1211-21. (PMID: 19565324)
J Virol. 2003 Jun;77(12):7143-9. (PMID: 12768036)
Substance Nomenclature:: 0 (Antibodies, Monoclonal)
0 (Capsid Proteins)
0 (Epitopes, B-Lymphocyte)
0 (Peptide Library)
Entry Date(s):: Date Created: 20110308 Date Completed: 20110713 Latest Revision: 20211020
Update Code:: 20240104
PubMed Central ID:: PMC3060845
DOI:: 10.1186/1743-422X-8-100
PMID:: 21375771
: Czasopismo naukowe

Pełny tekst

Background: The West Nile virus (WNV) capsid (C) protein is one of the three viral structural proteins, encapsidates the viral RNA to form the nucleocapsid, and is necessary for nuclear and nucleolar localization. The antigenic sites on C protein that are targeted by humoral immune responses have not been studied thoroughly, and well-defined B-cell epitopes on the WNV C protein have not been reported.
Results: In this study, we generated a WNV C protein-specific monoclonal antibody (mAb) and defined the linear epitope recognized by the mAb by screening a 12-mer peptide library using phage-display technology. The mAb, designated as 6D3, recognized the phages displaying a consensus motif consisting of the amino acid sequence KKPGGPG, which is identical to an amino acid sequence present in WNV C protein. Further fine mapping was conducted using truncated peptides expressed as MBP-fusion proteins. We found that the KKPGGPG motif is the minimal determinant of the linear epitope recognized by the mAb 6D3. Western blot (WB) analysis demonstrated that the KKPGGPG epitope could be recognized by antibodies contained in WNV- and Japanese encephalitis virus (JEV)-positive equine serum, but was not recognized by Dengue virus 1-4 (DENV1-4)-positive mice serum. Furthermore, we found that the epitope recognized by 6D3 is highly conserved among the JEV serocomplex of the Family Flaviviridae.
Conclusion: The KKPGGPG epitope is a JEV serocomplex-specific linear B-cell epitope recognized by the 6D3 mAb generated in this study. The 6D3 mAb may serve as a novel reagent in development of diagnostic tests for JEV serocomplex infection. Further, the identification of the B-cell epitope that is highly conserved among the JEV serocomplex may support the rationale design of vaccines against viruses of the JEV serocomplex.

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