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一种用于逆转录病毒RNA与细胞RNA之间非同源重组的模型系统。

A model system for nonhomologous recombination between retroviral and cellular RNA.

作者信息

Hajjar A M, Linial M L

机构信息

Division of Basic Sciences, Fred Hutchinson Cancer Research Center, Seattle, Washington 98104.

出版信息

J Virol. 1993 Jul;67(7):3845-53. doi: 10.1128/JVI.67.7.3845-3853.1993.

Abstract

A current model for the generation of transforming retroviruses proposes that read-through RNAs, containing both viral and cellular sequences, are copackaged with viral genomic RNA. It is, however, possible that a cellular mRNA is occasionally encapsidated into a retroviral particle, even though viral packaging sequences are absent. We have generated recombinant proviruses following copackaging of an avian leukosis viral genomic RNA and a neo-containing RNA completely devoid of retroviral sequences. In these studies, we used the packaging cell line SE21Q1b, which has the unique ability to randomly package cellular mRNA into retroviral particles. We describe 10 recombinants obtained following copackaging of nonhomologous RNAs. Our data show that recombination is not occurring at the DNA level in the parental SE21Q1b cells but is occurring at the RNA level, during reverse transcription. These data further suggest that reverse transcriptase can preferentially jump between templates at short stretches of homology in otherwise unrelated RNAs. We conclude that retroviral sequences are not required for packaged mRNA to be reverse transcribed and to be included in integrated proviruses.

摘要

一种关于转化逆转录病毒产生的当前模型提出,包含病毒和细胞序列的通读RNA与病毒基因组RNA一起被共包装。然而,即使没有病毒包装序列,细胞mRNA偶尔也有可能被包裹进逆转录病毒颗粒中。我们通过将禽白血病病毒基因组RNA和完全不含逆转录病毒序列的含新霉素RNA共包装,产生了重组前病毒。在这些研究中,我们使用了包装细胞系SE21Q1b,它具有将细胞mRNA随机包装进逆转录病毒颗粒的独特能力。我们描述了在非同源RNA共包装后获得的10个重组体。我们的数据表明,在亲本SE21Q1b细胞中,重组不是发生在DNA水平,而是发生在逆转录过程中的RNA水平。这些数据进一步表明,逆转录酶可以在其他不相关RNA的短同源片段处优先在模板之间跳跃。我们得出结论,包装的mRNA进行逆转录并被纳入整合的前病毒不需要逆转录病毒序列。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/beaa/237749/629bb5bdb4b9/jvirol00028-0162-a.jpg

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