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Human monoclonal antibodies to West Nile virus identify epitopes on the prM protein.

机译:针对西尼罗河病毒的人类单克隆抗体可识别prM蛋白上的表位。

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摘要

Hybridoma cell lines (2E8, 8G8 and 5G12) producing fully human monoclonal antibodies (hMAbs) specific for the pre-membrane (prM) protein of West Nile virus (WNV) were prepared using a human fusion partner cell line, MFP-2, and human peripheral blood lymphocytes from a blood donor diagnosed with WNV fever in 2004. Using site-directed mutagenesis of a WNV-like particle (VLP) we identified 4 amino acid residues in the prM protein unique to WNV and important in the binding of these hMAbs to the VLP. Residues V19 and L33 are important epitopes for the binding of all three hMAbs. Mutations at residue, T20 and T24 affected the binding of hMAbs, 8G8 and 5G12 only. These hMAbs did not significantly protect AG129 interferon-deficient mice or Swiss Webster outbred mice from WNV infection.
机译:使用人融合伴侣细胞系MFP-2和MFP-2,制备产生对西尼罗河病毒(WNV)的膜前(prM)蛋白具有特异性的完全人单克隆抗体(hMAb)的杂交瘤细胞系(2E8、8G8和5G12)。来自2004年诊断为WNV发热的献血者的人外周血淋巴细胞。使用WNV样颗粒(VLP)的定点诱变,我们在prM蛋白中鉴定了WNV独特的4个氨基酸残基,并且对这些hMAb的结合很重要到VLP。残基V19和L33是所有三种hMAb结合的重要表位。残基,T20和T24处的突变仅影响hMAb,8G8和5G12的结合。这些hMAb不能显着保护AG129干扰素缺陷小鼠或Swiss Webster近交小鼠免受WNV感染。

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