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首页> 外文期刊>Virology >Proteolytic processing in infectious bursal disease virus: identification of the polyprotein cleavage sites by site-directed mutagenesis.
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Proteolytic processing in infectious bursal disease virus: identification of the polyprotein cleavage sites by site-directed mutagenesis.

机译:传染性法氏囊病病毒的蛋白水解过程:通过定点诱变鉴定多蛋白切割位点。

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摘要

The infectious bursal disease virus (IBDV), a member of the Birnaviridae family, is the causative agent of an immune depressive disease that affects domesticated and wild avian species. The expression strategy of IBDV includes the synthesis of a 110-kDa polyprotein containing the capsid precursor polypeptides. The polyprotein is autocatalitically processed rendering three polypeptides: NH2-VPX-VP4-VP3-COOH. We have carried out a systematic analysis, using a series of plasmids encoding polyproteins containing either deletions or single amino acid substitutions, to identify the processing sites. The results obtained showed the existence of two sites, 511LAA513 and 754MAA756, that are essential for the processing of the VPX-VP4 and VP4-VP3 precursors, respectively. These sequences are highly conserved among IBDV strains form serotypes 1 and 2. A secondary VPX-VP4 processing site was detected in a 19-amino acid stretch located upstream of the 511LAA513 site. Analyses using versions of the 754MAA756 VP4-VP3 processing site containing conservative and nonconservative amino acid substitutions demonstrated that the specificity of the cleavage is dictated by the conserved AA dipeptide. Copyright 1999 Academic Press.
机译:传染性法氏囊病病毒(IBDV)是Birnaviridae家族的成员,是影响家养和野生禽类的免疫抑制性疾病的病原体。 IBDV的表达策略包括合成包含衣壳前体多肽的110kDa多蛋白。多蛋白经过自动催化处理,生成了三个多肽:NH2-VPX-VP4-VP3-COOH。我们使用编码含有缺失或单个氨基酸取代的多蛋白的一系列质粒进行了系统的分析,以鉴定加工位点。获得的结果表明存在两个位点511LAA513和754MAA756,它们分别对VPX-VP4和VP4-VP3前体的加工至关重要。这些序列在血清型1和2的IBDV菌株之间高度保守。在位于511LAA513位点上游的19个氨基酸序列中检测到第二个VPX-VP4加工位点。使用包含保守和非保守氨基酸取代的754MAA756 VP4-VP3加工位点版本进行的分析表明,切割的特异性由保守的AA二肽决定。版权所有1999,学术出版社。

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