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Efficient generation of adenovirus-based libraries by positive selection of adenoviral recombinants through ectopic expression of the adenovirus protease

机译:通过异位表达腺病毒蛋白酶,通过积极选择腺病毒重组体,有效生成基于腺病毒的文库

摘要

Disclosed is a new system for generating recombinant adenovirus vectors and adenovirus-based expression libraries, by positive selection of recombinants deleted for the endogenous protease gene, which gene is expressibly cloned into another region of the adenoviral genome. In a preferred embodiment, the invention allows positive selection of E1-deleted, protease-deleted recombinant adenovirus vectors comprising an exogenous gene or an expressible piece of exogenous DNA, by providing an expression cassette comprising the protease gene and the exogenous DNA inserted in place of E1 region in a shuttle vector. In vivo recombination of the shuttle vector with a protease-deleted adenoviral genome in suitable non-complementing cells generates viable recombinants only when rescuing the protease cloned in E1 region. Non-recombinant viral genomes are not able to grow due to the deletion of the protease gene, ensuring that only recombinant viral plaques are generated. This positive selection can be used for the generation of a large number of high purity recombinant adenovirus vectors and allows generation of adenovirus-based libraries with diversity exceeding 106 clones.
机译:本发明公开了一种新系统,其用于通过阳性选择缺失内源蛋白酶基因的重组体来产生重组腺病毒载体和基于腺病毒的表达文库,该基因可表达地克隆到腺病毒基因组的另一个区域中。在一个优选的实施方案中,本发明通过提供包含蛋白酶基因和插入的外源DNA的表达盒,可以阳性选择包含外源基因或可表达的外源DNA的E1缺失,蛋白酶缺失的重组腺病毒载体。穿梭向量中的E1区域。仅当挽救克隆在E1区域中的蛋白酶时,穿梭载体与蛋白酶缺失的腺病毒基因组在合适的非互补细胞中的体内重组才产生可行的重组体。由于蛋白酶基因的缺失,非重组病毒基因组无法生长,从而确保仅产生重组病毒噬菌斑。这种积极的选择可以用于生成大量高纯度重组腺病毒载体,并可以生成多样性超过10 6 克隆的基于腺病毒的文库。

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