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DNA腺嘌呤甲基化对P1 oriR和宿主oriC复制起点进行两级控制的证据。

Evidence of two levels of control of P1 oriR and host oriC replication origins by DNA adenine methylation.

作者信息

Abeles A, Brendler T, Austin S

机构信息

Laboratory of Chromosome Biology, National Cancer Institute-Frederick Cancer Research and Development Center, Maryland 21701-1201.

出版信息

J Bacteriol. 1993 Dec;175(24):7801-7. doi: 10.1128/jb.175.24.7801-7807.1993.

Abstract

A mutant mini-P1 plasmid with increased copy number can be established in Dam- strains of Escherichia coli, where mini-P1 plasmid replication is normally blocked. Comparison of this plasmid and a plasmid driven by the host oriC replication origin showed that both origins are subject to control by methylation at two different levels. First, both origins appear to be subject to negative regulation acting at the level of hemimethylation. This probably involves the sequestration of the hemimethylated DNA produced by replication, as has been previously described for oriC. Second, both origins show a positive requirement for adenine methylation for efficient function in vivo. This conclusion is supported by the behavior of the P1 origin in an improved in vitro replication system. In vitro, where sequestration of hemimethylated DNA is not expected to occur, the hemimethylated P1 origin DNA was fully functional as a template. However, the activity of fully unmethylated DNA was severely restricted in comparison with that of either of the methylated forms. This in vitro uncoupling of the two effects of origin methylation suggests that two separate mechanisms are involved.

摘要

一种拷贝数增加的突变型微型P1质粒可在大肠杆菌的Dam-菌株中构建,而在该菌株中微型P1质粒的复制通常受阻。将此质粒与由宿主oriC复制起点驱动的质粒进行比较,结果表明这两个起点都受到两个不同水平甲基化的调控。首先,两个起点似乎都受到在半甲基化水平起作用的负调控。这可能涉及对复制产生的半甲基化DNA的隔离,正如之前对oriC所描述的那样。其次,两个起点在体内高效发挥功能时都对腺嘌呤甲基化有正向需求。这一结论得到了P1起点在改进的体外复制系统中的行为的支持。在体外,预计不会发生半甲基化DNA的隔离,半甲基化的P1起点DNA作为模板具有完全功能。然而,与任何一种甲基化形式相比,完全未甲基化DNA的活性受到严重限制。起点甲基化这两种效应在体外的解偶联表明涉及两种不同的机制。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f12b/206955/610e4e9fbc63/jbacter00066-0065-a.jpg

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