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牛乳头瘤病毒1型编码的调节功能对于病毒的短暂复制并非必需,但对于稳定质粒状态的建立却是必需的。

A bovine papillomavirus type 1-encoded modulator function is dispensable for transient viral replication but is required for establishment of the stable plasmid state.

作者信息

Lusky M, Botchan M R

出版信息

J Virol. 1986 Nov;60(2):729-42. doi: 10.1128/JVI.60.2.729-742.1986.

Abstract

A bovine papillomavirus (BPV) type 1-encoded function (M) which is a negative regulator of viral plasmid replication has been described elsewhere (Berg et al. Cell, in press; Roberts and Weintraub, Cell, in press). We report here that expression of M, which is a repressor of transient BPV replication and is not required as a positive factor in these assays, is required for the establishment of the viral genome as a stable nuclear plasmid. This function is encoded in part by the 5' portion of the BPV E1 open reading frame, whereas the 3' part of this open reading frame encodes a positive replication function (R). The R function is required for early replication events. We used transient replication assays to define the phenotypes of mutants in both the R and M genes and complementation tests to show that R and M define two separate genes. We showed that R- and M- mutants could also complement each other in stable assays. In cotransfection experiments, M- mutants had a lethal effect on the growth of G418-resistant colonies, and in addition their morphological transformation efficiencies were reduced. The rare colonies which did appear contained the mutant DNA integrated into the cellular genome. R- mutants transformed with wild-type efficiency, and the mutant DNA was also found integrated. When cotransfected, R- and M- mutants could each be established as unrearranged plasmids.

摘要

1型牛乳头瘤病毒(BPV)编码的一种功能(M)是病毒质粒复制的负调节因子,这在其他地方已有描述(伯格等人,《细胞》,即将发表;罗伯茨和温特劳布,《细胞》,即将发表)。我们在此报告,M的表达是病毒基因组作为稳定核质粒建立所必需的,M是瞬时BPV复制的抑制因子,在这些试验中不是作为正因子所必需的。该功能部分由BPV E1开放阅读框的5'部分编码,而该开放阅读框的3'部分编码正复制功能(R)。R功能是早期复制事件所必需的。我们使用瞬时复制试验来定义R和M基因中突变体的表型,并通过互补试验表明R和M定义了两个独立的基因。我们表明,R突变体和M突变体在稳定试验中也能相互互补。在共转染实验中,M突变体对G418抗性菌落的生长有致死作用,此外它们的形态转化效率降低。确实出现的罕见菌落含有整合到细胞基因组中的突变DNA。R突变体以野生型效率进行转化,并且也发现突变DNA已整合。当共转染时,R突变体和M突变体都可以作为未重排的质粒建立。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4d05/288948/52a3cebf7e46/jvirol00168-0405-a.jpg

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