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人轮状病毒亚基蛋白VP8上连续中和表位的精细定位

Fine mapping of sequential neutralization epitopes on the subunit protein VP8 of human rotavirus.

作者信息

Kovacs-Nolan Jennifer, Yoo Dongwan, Mine Yoshinori

机构信息

Department of Food Science, University of Guelph, Guelph, ON, Canada N1G 2W1.

出版信息

Biochem J. 2003 Nov 15;376(Pt 1):269-75. doi: 10.1042/BJ20021969.

Abstract

The epitopes of the HRV (human rotavirus), especially those involved in virus neutralization, have not been determined in their entirety, and would have significant implications for HRV vaccine development. In the present study, we report on the epitope mapping and identification of sequential neutralization epitopes, on the Wa strain HRV subunit protein VP8, using synthetic overlapping peptides. Polyclonal antibodies against recombinant Wa VP8 were produced previously in chicken, and purified from egg yolk, which showed neutralizing activity against HRV in vitro. Overlapping VP8 peptide fragments were synthesized and probed with the anti-VP8 antibodies, revealing five sequential epitopes on VP8. Further analysis suggested that three of the five epitopes detected, M1-L10, I55-D66 and L223-P234, were involved in virus neutralization, indicating that sequential epitopes may also be important for the HRV neutralization. The interactions of the antibodies with the five epitopes were characterized by an examination of the critical amino acids involved in antibody binding. Epitopes comprised primarily of hydrophobic amino acid residues, followed by polar and charged residues. The more critical amino acids appeared to be located near the centre of the epitopes, with proline, isoleucine, serine, glutamine and arginine playing an important role in the binding of antibody to the VP8 epitopes.

摘要

人轮状病毒(HRV)的表位,尤其是那些参与病毒中和的表位,尚未完全确定,这对HRV疫苗的开发具有重要意义。在本研究中,我们报告了使用合成重叠肽对HRV Wa株亚基蛋白VP8上的表位图谱绘制及连续中和表位的鉴定。先前已在鸡体内产生了针对重组Wa VP8的多克隆抗体,并从蛋黄中纯化,该抗体在体外显示出对HRV的中和活性。合成了重叠的VP8肽片段并用抗VP8抗体进行检测,揭示了VP8上的五个连续表位。进一步分析表明,检测到的五个表位中的三个,即M1-L10、I55-D66和L223-P234,参与了病毒中和,这表明连续表位对HRV中和也可能很重要。通过检查参与抗体结合的关键氨基酸来表征抗体与这五个表位的相互作用。表位主要由疏水氨基酸残基组成,其次是极性和带电荷的残基。更关键的氨基酸似乎位于表位的中心附近,脯氨酸、异亮氨酸、丝氨酸、谷氨酰胺和精氨酸在抗体与VP8表位的结合中起重要作用。

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