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将腺相关病毒克隆至pBR322:在人细胞中从重组质粒拯救完整病毒。

Cloning of adeno-associated virus into pBR322: rescue of intact virus from the recombinant plasmid in human cells.

作者信息

Samulski R J, Berns K I, Tan M, Muzyczka N

出版信息

Proc Natl Acad Sci U S A. 1982 Mar;79(6):2077-81. doi: 10.1073/pnas.79.6.2077.

Abstract

We have cloned intact duplex adeno-associated virus (AAV) DNA into the bacterial plasmid pBR322. The AAV genome could be rescued from the recombinant plasmid by transfection of the plasmid DNA into human cells with adenovirus 5 as helper. The efficiency of rescue from the plasmid was sufficiently high to produce yields of AAV DNA comparable to those observed after transfection with equal amounts of purified virion DNA. Thus, the recombinant plasmid itself may be a model for studying the rescue of a latent AAV viral infection. In addition, the efficient rescue of viable AAV from the recombinant plasmid should facilitate the genetic analysis of AAV. Finally, the results of an analysis of the DNA from rescued virions indicate that an inversion of the AAV terminal sequences occurred during replication.

摘要

我们已将完整的双链腺相关病毒(AAV)DNA克隆到细菌质粒pBR322中。通过将质粒DNA转染到以腺病毒5作为辅助病毒的人细胞中,可从重组质粒中拯救出AAV基因组。从质粒中拯救的效率足够高,能够产生与用等量纯化病毒粒子DNA转染后观察到的AAV DNA产量相当的产量。因此,重组质粒本身可能是研究潜伏性AAV病毒感染拯救的模型。此外,从重组质粒中高效拯救出有活力的AAV应有助于对AAV进行遗传分析。最后,对拯救出的病毒粒子的DNA分析结果表明,AAV末端序列在复制过程中发生了倒位。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6541/346126/c7c75fef5252/pnas00445-0404-a.jpg

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