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质粒Rts1的repA C末端区域的定点突变:对复制和自动阻遏功能的多效性影响

Site-directed mutations in the repA C-terminal region of plasmid Rts1: pleiotropic effects on the replication and autorepressor functions.

作者信息

Zeng H, Hayashi T, Terawaki Y

机构信息

Department of Bacteriology, Shinshu University School of Medicine, Matsumoto, Japan.

出版信息

J Bacteriol. 1990 May;172(5):2535-40. doi: 10.1128/jb.172.5.2535-2540.1990.

Abstract

We induced site-directed mutations near the 3' terminus of the gene repA, which encodes the protein of 288 amino acid residues essential for plasmid Rts1 replication, and obtained seven repA mutants. Three of them contained small deletions at the 3' terminus. Mutant repAz delta C4, which encodes a RepA protein that lacks the C-terminal four amino acids, expressed a high-copy-number phenotype and had lost both autorepressor and incompatibility functions. Deletion of one additional amino acid residue to form the RepAz delta C5 protein caused restoration of the wild-type copy number and strong incompatibility. Studies of the remaining four repA mutants, each of which contained a single amino acid substitution near the RepA C terminus, suggested that Lys-268 is involved in both ori(Rts1) activation and autorepressor-incompatibility activities and that Arg-279 contributes to ori(Rts1) activation but not to incompatibility. Lys-268 is part of a dual-lysine sequence with Lys-267 and is located 21 amino acids upstream of the RepA C terminus. A dual-lysine sequence is also found at a similar position in both mini-F RepE and mini-P1 RepA proteins.

摘要

我们在编码质粒Rts1复制所必需的288个氨基酸残基蛋白质的repA基因的3'末端附近诱导了定点突变,并获得了7个repA突变体。其中3个在3'末端含有小的缺失。突变体repAz delta C4编码一种缺少C末端四个氨基酸的RepA蛋白,表现出高拷贝数表型,并且失去了自抑制和不相容性功能。再缺失一个氨基酸残基形成RepAz delta C5蛋白导致野生型拷贝数恢复和强不相容性。对其余四个repA突变体的研究表明,每个突变体在RepA C末端附近都含有一个单一的氨基酸取代,表明Lys-268参与ori(Rts1)激活和自抑制-不相容活性,而Arg-279有助于ori(Rts1)激活但不参与不相容性。Lys-268是与Lys-267形成的双赖氨酸序列的一部分,位于RepA C末端上游21个氨基酸处。在mini-F RepE和mini-P1 RepA蛋白的相似位置也发现了双赖氨酸序列。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2f75/208894/b70015c5346c/jbacter00119-0352-a.jpg

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