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Classical swine fever virus virulence determinant and a novel classical swine fever vaccine

机译:古典猪瘟病毒毒力决定因素和新型古典猪瘟疫苗

摘要

Transposon linker insertion mutagenesis of a full-length infectious clone of the highly pathogenic classical swine fever virus (CSFV) isolate Brescia (pBIC) was used to identify genetic determinants of CSFV virulence and host range. A virus mutant, RB-C22 (RB-C22v), possessing a 19-residue tag insertion at the carboxyl end of E1 was constructed. RB-C22v and the parental virus pBIC (pBICv) exhibited similar growth characteristics on primary porcine macrophage cell cultures although RB-C22v produced significantly smaller plaques on SK6 cell cultures. In vivo, RB-C22v was markedly attenuated in swine. In contrast with pBIC infection, where mortality was 100%, all RB-C22v-infected pigs survived infection remaining clinically normal. Additionally, chimeras of the Brescia strain and the attenuated vaccine strain CS were constructed and evaluated for viral virulence in swine. Chimeras 138.8v and 337.14v, chimeras containing the E2 glycoprotein of CS and chimeric virus 319.1v, which contained only the CS E2 glycoprotein in the Brescia background, were attenuated in swine. Chimeras encoding all Brescia structural proteins in a CS genetic background remained attenuated, indicating that additional mutations outside the structural region are important for CS vaccine virus attenuation. The combined results indicate a significant role for E1 glycoprotein and E2 glycoprotein in swine virulence.
机译:高致病性经典猪瘟病毒(CSFV)分离株布雷西亚(pBIC)的全长传染性克隆的转座子接头插入诱变用于鉴定CSFV毒力和宿主范围的遗传决定因素。构建了病毒突变体RB-C22(RB-C22v),其在E1的羧基末端具有19个残基的标签插入。 RB-C22v和亲代病毒pBIC(pBICv)在原代猪巨噬细胞细胞培养物中表现出相似的生长特征,尽管RB-C22v在SK6细胞培养物中产生的噬菌斑明显较小。在体内,RB-C22v在猪中显着减毒。与死亡率为100%的pBIC感染相反,所有被RB-C22v感染的猪在感染后仍存活,临床上保持正常。另外,构建了布雷西亚菌株和减毒疫苗菌株CS的嵌合体,并评价了猪中的病毒毒力。猪中的嵌合体138.8v和337.14v,含有CS E2糖蛋白的嵌合体和嵌合病毒319.1v(在布雷西亚背景中仅含有CS E2糖蛋白)被减毒。在CS遗传背景下编码所有布雷西亚结构蛋白的嵌合体仍保持弱化状态,这表明结构区域外的其他突变对于CS疫苗病毒的弱化很重要。结合的结果表明E1糖蛋白和E2糖蛋白在猪毒力中具有重要作用。

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