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一种在pol基因中有一个错义密码子的突变型鼠白血病病毒在影响整合的功能方面存在缺陷。

A mutant murine leukemia virus with a single missense codon in pol is defective in a function affecting integration.

作者信息

Donehower L A, Varmus H E

出版信息

Proc Natl Acad Sci U S A. 1984 Oct;81(20):6461-5. doi: 10.1073/pnas.81.20.6461.

Abstract

We have used site-directed mutagenesis of cloned Moloney murine leukemia virus (MuLV) DNA to define a function encoded in the 3' region of the viral pol gene and required for efficient integration of viral DNA. One mutant, MuLV-SF1, contained a single base substitution (C to T at base 4950) that resulted in an arginine to cysteine change in a region highly conserved among retroviruses. Mutant DNA, introduced into rat cells by cotransfection with a herpes simplex virus thymidine kinase gene (HSV tk), directed production of virus particles with reverse transcriptase activity. Infection of cells with these particles led to synthesis of full-length linear and circular forms of unintegrated viral DNA; however, integrated viral DNA was decreased at least by a factor of 10 when examined by DNA hybridization, and the mutant particles were less efficient then wild-type virus at establishing an infection by a factor of at least 300. Pseudotypes formed with the proteins of MuLV-SF1 and the genome of a replication defective marker MuLV, carrying the HSV tk gene, were less effective by at least a factor of 100 in producing tk+ colonies than pseudotypes formed with proteins encoded by wild-type virus. When the MuLV-SF1 pseudotypes did produce tk+ cells, most of the proviruses were integrated aberrantly. We conclude that the MuLV-SF1 pol gene is defective for a function that is required for normal integrative recombination and dissociable from DNA synthesis.

摘要

我们利用克隆的莫洛尼鼠白血病病毒(MuLV)DNA的定点诱变来确定病毒pol基因3'区域编码的一种功能,该功能是病毒DNA高效整合所必需的。一个突变体MuLV-SF1包含一个单碱基替换(第4950位碱基由C变为T),导致逆转录病毒中高度保守区域的一个精氨酸变为半胱氨酸。通过与单纯疱疹病毒胸苷激酶基因(HSV tk)共转染将突变DNA导入大鼠细胞,可指导产生具有逆转录酶活性的病毒颗粒。用这些颗粒感染细胞会导致全长线性和环状形式的未整合病毒DNA的合成;然而,通过DNA杂交检测时,整合的病毒DNA至少减少了10倍,并且与野生型病毒相比,突变颗粒在建立感染方面的效率至少低300倍。由MuLV-SF1的蛋白质和携带HSV tk基因的复制缺陷标记MuLV的基因组形成的假型,在产生tk+菌落方面比由野生型病毒编码的蛋白质形成的假型效率至少低100倍。当MuLV-SF1假型确实产生tk+细胞时,大多数前病毒的整合都是异常的。我们得出结论,MuLV-SF1 pol基因在正常整合重组所需的功能方面存在缺陷,并且与DNA合成可分离。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8ab7/391944/09dc688aed9e/pnas00621-0208-a.jpg

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