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P1质粒复制抑制剂决定簇在起始基因内的定位。

Location of a P1 plasmid replication inhibitor determinant within the initiator gene.

作者信息

Muraiso K, Mukhopadhyay G, Chattoraj D K

机构信息

Laboratory of Biochemistry, National Cancer Institute, Bethesda, Maryland 20892.

出版信息

J Bacteriol. 1990 Aug;172(8):4441-7. doi: 10.1128/jb.172.8.4441-4447.1990.

Abstract

The P1 plasmid replication initiator protein, RepA, binds to its own promoter and represses transcription efficiently. There are only about 20 RepA dimers present per repA gene. A possible reason for this highly restrained expression became evident when repA expression was increased by using foreign promoters: with fivefold overexpression, the replication rate was diminished, and with 40-fold overexpression, replication was not detectable. The inhibition was P1 specific: growth of Escherichia coli and replication of pSC101, R6K, and mini-F plasmids were not affected. The activity is apparently not from RepA itself. Excess purified RepA did not inhibit replication in vitro. Mutations of the repA translation initiation codon reduced synthesis of the initiator but not the inhibitory activity. Deletion from either the N- or C-terminal ends of repA (28 and 69 codons, respectively, out of the 286-codon open reading frame) affected the initiator but not the inhibitory activity. Further deletions affected both the activities. These results demonstrate that the integrity of the initiator is not required for inhibition, but involvement of an unstable initiator fragment or of initiator mRNA cannot be ruled out.

摘要

P1质粒复制起始蛋白RepA与其自身启动子结合并有效抑制转录。每个repA基因中仅存在约20个RepA二聚体。当使用外源启动子提高repA表达时,这种高度受限表达的一个可能原因变得明显:过表达五倍时,复制速率降低,而过表达40倍时,无法检测到复制。这种抑制是P1特异性的:大肠杆菌的生长以及pSC101、R6K和mini-F质粒的复制均未受影响。该活性显然并非来自RepA本身。过量纯化的RepA在体外并不抑制复制。repA翻译起始密码子的突变减少了起始蛋白的合成,但不影响抑制活性。从repA的N端或C端分别缺失(在286个密码子的开放阅读框中分别缺失28和69个密码子)影响起始蛋白,但不影响抑制活性。进一步缺失则影响两种活性。这些结果表明,抑制作用并不需要起始蛋白的完整性,但不能排除不稳定的起始蛋白片段或起始蛋白mRNA的参与。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8e44/213273/8fac10ae2656/jbacter00122-0324-a.jpg

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