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鼠肝炎病毒nsp1和nsp14诱变对其在细胞培养中复制的影响。

Effects of mutagenesis of murine hepatitis virus nsp1 and nsp14 on replication in culture.

作者信息

Eckerle Lance D, Brockway Sarah M, Sperry Steven M, Lu Xiaotao, Denison Mark R

机构信息

Vanderbilt University Medical Center, Nashville, Tennessee 37232-2581, USA.

出版信息

Adv Exp Med Biol. 2006;581:55-60. doi: 10.1007/978-0-387-33012-9_8.

Abstract

For nsp1, the fact that the carboxy-terminal but not the amino-terminal half of the protein can be deleted suggests that there may be specific and distinct domains within the protein or that the entire protein is dispensable but that the RNA encoding the amino-terminal half of nsp1 cannot be deleted. The identification of specific required residues support the conclusion that it is the portion of the protein that is required for replication. The results of mutagenesis of the nsp14 coding region and flanking cleavage sites also provided important new insights into this protein and its requirements. Our previous study raised the question as to the essential nature of nsp14 in replication. The results of this study show that putative active site residues cannot be substituted without loss of replication in culture. Interestingly, mutagenesis of Tyr414 showed that while this residue can tolerate a number of substitutions, it was intolerant of Lysine or deletion. The results suggest that nsp14 is required for replication. However, whatever functions nsp14 serves appear to be retained by noncleaved or partially processed nsp14, since abolition of either the amino-terminal or carboxy-terminal cleavage site allowed recovery of viable virus.

摘要

对于nsp1而言,该蛋白质的羧基末端而非氨基末端的一半可以被缺失,这一事实表明该蛋白质内部可能存在特定且不同的结构域,或者整个蛋白质是可有可无的,但编码nsp1氨基末端一半的RNA不能被缺失。特定必需残基的鉴定支持了这样的结论,即该蛋白质的这一部分是复制所必需的。nsp14编码区和侧翼切割位点的诱变结果也为该蛋白质及其需求提供了重要的新见解。我们之前的研究提出了关于nsp14在复制中的本质必要性的问题。这项研究的结果表明,假定的活性位点残基在培养中不能被替代而不损失复制能力。有趣的是,对Tyr414的诱变表明,虽然该残基可以耐受多种替代,但它不耐受赖氨酸或缺失。结果表明nsp14是复制所必需的。然而,无论nsp14发挥何种功能,似乎都由未切割或部分加工的nsp14保留,因为氨基末端或羧基末端切割位点的废除都允许恢复有活力的病毒。

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