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免疫信息学设计的流感 H3N2 病毒神经氨酸酶基因表位肽。

Epitope peptides of influenza H3N2 virus neuraminidase gene designed by immunoinformatics.

机构信息

Key Laboratory for Emergency Pathogen Detection, Guangdong Provincial Center for Disease Control and Prevention, Guangzhou, China.

出版信息

Acta Biochim Biophys Sin (Shanghai). 2012 Feb;44(2):113-8. doi: 10.1093/abbs/gmr101. Epub 2011 Nov 21.

Abstract

The virus surface protein neuraminidase (NA) is a main subtype-specific antigen in influenza type A viruses. Neuraminidase functions as an enzyme to break the bonds between hemagglutinin (HA) and sialic acid to release newly formed viruses from infected cells. In this study, NA genes from the H3N2 subtype virus were sequenced and NA proteins were screened for B-cell epitopes and assessed based on immunoinformatics. Based on this information, three peptides ES8, RR9, and WK7 (covering amino acid residues 221-228, 292-300, and 383-389, respectively) of the NA protein were selected and synthesized artificially. These peptides were used to immunize New Zealand rabbits subcutaneously to raise antisera. Results showed that these three peptides were capable of eliciting antibodies against H3N2 viruses in a specific and sensitive manner, detected in vitro by enzyme-linked immunosorbent assay. Furthermore, hemadsorption anti-releasing effects occurred in three antisera mixtures at a dilution of 1:40. Alignment using database software showed that amino acid residues in these three epitope peptides were substituted at specific sites in all the NAs sequenced in this study. We suggest that these NA epitope peptides might be used in conjunction with HA proteins as vaccine antigens.

摘要

病毒表面蛋白神经氨酸酶(NA)是甲型流感病毒的主要亚型特异性抗原之一。神经氨酸酶作为一种酶,可打破血凝素(HA)与唾液酸之间的键,从而将新形成的病毒从感染细胞中释放出来。在本研究中,对 H3N2 亚型病毒的 NA 基因进行了测序,并对 NA 蛋白进行了 B 细胞表位筛选,并基于免疫信息学进行了评估。基于这些信息,选择并人工合成了神经氨酸酶蛋白的三个肽 ES8、RR9 和 WK7(分别覆盖氨基酸残基 221-228、292-300 和 383-389)。这些肽被用于皮下免疫新西兰兔以产生抗血清。结果表明,这三个肽能够以特异和敏感的方式诱导针对 H3N2 病毒的抗体,通过酶联免疫吸附试验在体外检测到。此外,在三种抗血清混合物中以 1:40 的稀释度发生了血球凝集抗释放作用。使用数据库软件进行比对显示,在本研究中测序的所有 NAs 中,这三个表位肽中的氨基酸残基在特定位点发生了取代。我们建议这些 NA 表位肽可与 HA 蛋白一起用作疫苗抗原。

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