通过大肠杆菌中的同源重组高效生成重组腺病毒载体。
Efficient generation of recombinant adenovirus vectors by homologous recombination in Escherichia coli.
作者信息
Chartier C, Degryse E, Gantzer M, Dieterle A, Pavirani A, Mehtali M
机构信息
Gene Therapy Department, Transgene S.A., Strasbourg, France.
出版信息
J Virol. 1996 Jul;70(7):4805-10. doi: 10.1128/JVI.70.7.4805-4810.1996.
Abstract
Despite recent technical improvements, the construction of recombinant adenovirus vectors remains a time-consuming procedure which requires extensive manipulations of the viral genome in both Escherichia coli and eukaryotic cells. This report describes a novel system based on the cloning and manipulation of the full-length adenovirus genome as a stable plasmid in E. coli, by using the bacterial homologous recombination machinery. The efficiency and flexibility of the method are illustrated by the cloning of the wild-type adenovirus type 5 genome, the insertion of a constitutive promoter upstream from the E3 region, the replacement of the E1 region by an exogenous expression cassette, and the deletion of the E1 region. All recombinant viral DNAS were shown to be fully infectious in permissive cells, and the modified E3 region or the inserted foreign gene was correctly expressed in the infected cells.
摘要
尽管最近技术有所改进,但重组腺病毒载体的构建仍然是一个耗时的过程,需要在大肠杆菌和真核细胞中对病毒基因组进行大量操作。本报告描述了一种新系统,该系统基于利用细菌同源重组机制,将全长腺病毒基因组作为稳定质粒在大肠杆菌中进行克隆和操作。通过克隆野生型5型腺病毒基因组、在E3区域上游插入组成型启动子、用外源表达盒替换E1区域以及删除E1区域,说明了该方法的效率和灵活性。所有重组病毒DNA在允许细胞中均显示出完全感染性,并且修饰后的E3区域或插入的外源基因在感染细胞中正确表达。
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