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一种选择和回收重组腺病毒载体的高效方法。

An efficient procedure to select and recover recombinant adenovirus vectors.

作者信息

Imler J L, Chartier C, Dieterlé A, Dreyer D, Mehtali M, Pavirani A

机构信息

Department of Gene Therapy Research, Transgène SA, Strasbourg, France.

出版信息

Gene Ther. 1995 Jun;2(4):263-8.

PMID:7552986
Abstract

Adenoviruses are efficient gene transfer vectors for a variety of cell types. To date, the most widely used methods to construct recombinant adenoviruses involve either in vitro ligation or recombination between one-half of the virus genome, previously cloned in a plasmid vector and engineered to contain the desired expression cassette, and the other half of the virus genome prepared from virions. Although quite effective, these approaches produce viral progeny containing a mixture of recombinant and parental background virus. Thus the recovery of the recombinant virus can be difficult, especially when it grows more slowly than the parental virus. To improve selection and recovery of recombinant adenoviruses, we have constructed an adenovirus vector, AdTG6553, in which the E1 region has been replaced by the thymidine kinase (tk) gene of herpes simplex virus type 1. We show that infection of cells with AdTG6553 in the presence of the nucleoside analog ganciclovir (GCV) prevents viral replication. The conditional lethal phenotype introduced in AdTG6553 makes it a valuable tool to counter-select parental background virus in the presence of GCV and isolate replication-deficient recombinant adenoviruses in which the tk expression cassette has been replaced by a new gene.

摘要

腺病毒是适用于多种细胞类型的高效基因转移载体。迄今为止,构建重组腺病毒最广泛使用的方法涉及体外连接,或在先前克隆于质粒载体并经改造以包含所需表达盒的病毒基因组的一半与从病毒粒子制备的病毒基因组的另一半之间进行重组。尽管这些方法相当有效,但会产生含有重组背景病毒和亲本背景病毒混合物的病毒后代。因此,重组病毒的回收可能很困难,尤其是当它比亲本病毒生长得更慢时。为了改进重组腺病毒的筛选和回收,我们构建了一种腺病毒载体AdTG6553,其中E1区域已被单纯疱疹病毒1型的胸苷激酶(tk)基因取代。我们表明,在核苷类似物更昔洛韦(GCV)存在的情况下,用AdTG6553感染细胞可阻止病毒复制。AdTG6553中引入的条件致死表型使其成为在GCV存在下反选亲本背景病毒并分离其中tk表达盒已被新基因取代的复制缺陷型重组腺病毒的有价值工具。

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