Human monoclonal ScFv that bind to different functional domains of M2 and inhibit H5N1 influenza virus replication

被引:14
|
作者
Pissawong, Tippawan [1 ]
Maneewatch, Santi [2 ]
Thueng-in, Kanyarat [3 ]
Srimanote, Potjanee [4 ]
Dong-din-on, Fonthip [5 ]
Thanongsaksrikul, Jeeraphong [4 ]
Songserm, Thaweesak [6 ]
Tongtawe, Pongsri [4 ]
Bangphoomi, Kunan [7 ]
Chaicumpa, Wanpen [8 ]
机构
[1] Mahidol Univ, Grad Program Immunol, Dept Immunol, Bangkok 10700, Thailand
[2] Mahidol Univ, Dept Mol Trop Med & Genet, Bangkok 10400, Thailand
[3] Kasetsart Univ, Dept Microbiol & Immunol, Bangkok 10900, Thailand
[4] Thammasat Univ, Grad Program Biomed Sci, Pathum Thani 12120, Thailand
[5] Kasetsart Univ, Ctr Agr Biotechnol, Dept Biochem, Bangkok 10900, Thailand
[6] Kasetsart Univ, Dept Vet Pathol, Nakhopathom 73140, Thailand
[7] Kasetsart Univ, Dept Biochem, Bangkok 10900, Thailand
[8] Mahidol Univ, Lab Res & Technol Dev, Dept Parasitol, Bangkok 10700, Thailand
关键词
Influenza virus; H5N1; M2; protein; Human ScFv; Phage display; Virus neutralization; Quantitative real-time RT-PCR; Mimotope; Molecular docking; SINGLE-CHAIN ANTIBODIES; PROTON CHANNEL; MECHANISM; AMANTADINE;
D O I
10.1186/1743-422X-10-148
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
Background: Novel effective anti-influenza agent that tolerates influenza virus antigenic variation is needed. Highly conserved influenza virus M2 protein has multiple pivotal functions including ion channel activity for vRNP uncoating, anti-autophagy and virus assembly, morphogenesis and release. Thus, M2 is an attractive target of anti-influenza agents including small molecular drugs and specific antibodies. Methods: Fully human monoclonal single chain antibodies (HuScFv) specific to recombinant and native M2 proteins of A/H5N1 virus were produced from huscfv-phagemid transformed E. coli clones selected from a HuScFv phage display library using recombinant M2 of clade 1 A/H5N1 as panning antigen. The HuScFv were tested for their ability to inhibit replication of A/H5N1 of both homologous and heterologous clades. M2 domains bound by HuScFv of individual E. coli clones were identified by phage mimotope searching and computerized molecular docking. Results: HuScFv derived from four huscfv-phagemid transformed E. coli clones (no. 2, 19, 23 and 27) showed different amino acid sequences particularly at the CDRs. Cells infected with A/H5N1 influenza viruses (both adamantane sensitive and resistant) that had been exposed to the HuScFv had reduced virus release and intracellular virus. Phage peptide mimotope search and multiple alignments revealed that conformational epitopes of HuScFv2 located at the residues important for ion channel activity, anti-autophagy and M1 binding; epitopic residues of HuScFv19 located at the M2 amphipathic helix and cytoplasmic tail important for anti-autophagy, virus assembly, morphogenesis and release; epitope of HuScFv23 involved residues important for the M2 activities similar to HuScFv2 and also amphipathic helix residues for viral budding and release while HuScFv27 epitope spanned ectodomain, ion channel and anti-autophagy residues. Results of computerized homology modelling and molecular docking conformed to the epitope identification by phages. Conclusions: HuScFv that bound to highly conserved epitopes across influenza A subtypes and human pathogenic H5N1clades located on different functional domains of M2 were produced. The HuScFv reduced viral release and intracellular virus of infected cells. While the molecular mechanisms of the HuScFv await experimental validation, the small human antibody fragments have high potential for developing further as a safe, novel and mutation tolerable anti-influenza agent especially against drug resistant variants.
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页数:14
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