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在鼠逆转录病毒中鉴定出一种信号,该信号足以将非逆转录病毒RNA包装进病毒粒子。

Identification of a signal in a murine retrovirus that is sufficient for packaging of nonretroviral RNA into virions.

作者信息

Adam M A, Miller A D

机构信息

Fred Hutchinson Cancer Research Center, Seattle, Washington 98104.

出版信息

J Virol. 1988 Oct;62(10):3802-6. doi: 10.1128/JVI.62.10.3802-3806.1988.

Abstract

A region near the 5' end of Moloney murine leukemia virus (MoMLV) is required for packaging of viral RNA into virions. Retroviral vectors based on MoMLV have been constructed that are also efficiently packaged into virions despite removal of most of the interior region of the parental virus. To further localize sequences which are sufficient for packaging, we inserted various fragments from an MoMLV-based retroviral vector into a nonretroviral transcription unit, transfected these constructs into retrovirus-packaging cells, and measured packaging of RNA transcribed from these constructs into virions. Transcripts from some of these constructs were packaged at least as well as those from the parental vector or MoMLV itself. Sequences extending into the gag region, but not the long terminal repeat or tRNA-binding sequences, were required for efficient RNA packaging. RNAs transcribed from constructs which did not contain an insert, or in which the orientation of the insert was reversed, were not packaged at detectable levels. These studies define sequences which are necessary and sufficient for encapsidation of murine leukemia virus RNA into virions.

摘要

莫洛尼鼠白血病病毒(MoMLV)5'端附近的一个区域是病毒RNA包装进病毒粒子所必需的。基于MoMLV构建的逆转录病毒载体,尽管去除了亲本病毒的大部分内部区域,但仍能有效地包装进病毒粒子。为了进一步定位足以实现包装的序列,我们将基于MoMLV的逆转录病毒载体的各种片段插入到非逆转录病毒转录单元中,将这些构建体转染到逆转录病毒包装细胞中,并测量从这些构建体转录的RNA包装进病毒粒子的情况。其中一些构建体的转录本包装效率至少与亲本载体或MoMLV本身的转录本相同。高效RNA包装需要延伸到gag区域的序列,但不需要长末端重复序列或tRNA结合序列。从不含插入片段或插入片段方向相反的构建体转录的RNA,在可检测水平上未被包装。这些研究确定了将鼠白血病病毒RNA包装进病毒粒子所必需且足够的序列。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9a44/253525/9f5763ba5484/jvirol00089-0272-a.jpg

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