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构建在蛋白酶基因中含有特定突变的HIV-1感染性分子克隆。

Construction of infectious molecular clones of HIV-1 containing defined mutations in the protease gene.

作者信息

Winslow D L, Anton E D, Horlick R A, Zagursky R J, Tritch R J, Scarnati H, Ackerman K, Bacheler L T

机构信息

DuPont Merck Pharmaceutical Company, Wilmington, DE 19880-0026.

出版信息

Biochem Biophys Res Commun. 1994 Dec 30;205(3):1651-7. doi: 10.1006/bbrc.1994.2857.

Abstract

A DNA clone of HIV-1 containing the full-length infectious viral sequence was cleaved at a unique Nco I restriction site within the viral genome, and DNA fragments containing the 5' and 3' portions of the HIV genome were subcloned into separate plasmid vectors. The 5' 'half-virus' construct was further modified by incorporating a class IIS restriction site, Esp3I, near the 3' end of the protease gene of HIV. This site, in combination with a natural ApaI site near the 5' end of the protease gene, creates a convenient cassette shuttle vector in which the protease coding region can be easily replaced. Recombinant viruses containing protease genes either altered by site-directed mutagenesis or amplified from clinical or laboratory isolates can be reconstructed. The DNA fragment containing the protease gene is first subcloned into the 5' half-virus shuttle vector plasmid. Infectious recombinant virus is subsequently recovered by cotransfecting 5' and 3' half-virus plasmids linearized at their common Nco I sites into mammalian cells. This method was successfully applied to constructing viruses containing various substitutions in protease.

摘要

一个含有全长感染性病毒序列的HIV-1 DNA克隆在病毒基因组内一个独特的Nco I限制性酶切位点处被切割,含有HIV基因组5'和3'部分的DNA片段被亚克隆到单独的质粒载体中。5'“半病毒”构建体通过在HIV蛋白酶基因3'端附近引入一个IIS类限制性酶切位点Esp3I进行进一步修饰。该位点与蛋白酶基因5'端附近的一个天然ApaI位点相结合,创建了一个方便的盒式穿梭载体,其中蛋白酶编码区可以很容易地被替换。可以重建含有通过定点诱变改变或从临床或实验室分离株扩增的蛋白酶基因的重组病毒。首先将含有蛋白酶基因的DNA片段亚克隆到5'半病毒穿梭载体质粒中。随后通过将在其共同的Nco I位点处线性化的5'和3'半病毒质粒共转染到哺乳动物细胞中来回收感染性重组病毒。该方法已成功应用于构建蛋白酶中含有各种替代物的病毒。

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