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F质粒TraI的全面诱变揭示了其在接合调控中的作用。

General mutagenesis of F plasmid TraI reveals its role in conjugative regulation.

作者信息

Haft Rembrandt J F, Palacios Gilberto, Nguyen Tran, Mally Manuela, Gachelet Eliora G, Zechner Ellen L, Traxler Beth

机构信息

Department of Microbiology, University of Washington, Seattle, WA 98195-7242, USA.

出版信息

J Bacteriol. 2006 Sep;188(17):6346-53. doi: 10.1128/JB.00462-06.

Abstract

Bacteria commonly exchange genetic information by the horizontal transfer of conjugative plasmids. In gram-negative conjugation, a relaxase enzyme is absolutely required to prepare plasmid DNA for transit into the recipient via a type IV secretion system. Here we report a mutagenesis of the F plasmid relaxase gene traI using in-frame, 31-codon insertions. Phenotypic analysis of our mutant library revealed that several mutant proteins are functional in conjugation, highlighting regions of TraI that can tolerate insertions of a moderate size. We also demonstrate that wild-type TraI, when overexpressed, plays a dominant-negative regulatory role in conjugation, repressing plasmid transfer frequencies approximately 100-fold. Mutant TraI proteins with insertions in a region of approximately 400 residues between the consensus relaxase and helicase sequences did not cause conjugative repression. These unrestrictive TraI variants have normal relaxase activity in vivo, and several have wild-type conjugative functions when expressed at normal levels. We postulate that TraI negatively regulates conjugation by interacting with and sequestering some component of the conjugative apparatus. Our data indicate that the domain responsible for conjugative repression resides in the central region of TraI between the protein's catalytic domains.

摘要

细菌通常通过接合质粒的水平转移来交换遗传信息。在革兰氏阴性菌的接合过程中,一种松弛酶对于通过IV型分泌系统将质粒DNA转运到受体细胞中是绝对必需的。在此,我们报道了利用框内31密码子插入对F质粒松弛酶基因traI进行的诱变。对我们的突变体文库进行的表型分析表明,几种突变蛋白在接合过程中具有功能,突出了TraI中能够耐受中等大小插入的区域。我们还证明,野生型TraI在过表达时,在接合过程中发挥显性负调控作用,将质粒转移频率抑制约100倍。在共有松弛酶序列和解旋酶序列之间约400个残基的区域中插入突变的TraI蛋白不会导致接合抑制。这些不受限制的TraI变体在体内具有正常的松弛酶活性,并且其中几种在正常水平表达时具有野生型接合功能。我们推测TraI通过与接合装置的某些成分相互作用并使其隔离来负调控接合。我们的数据表明,负责接合抑制的结构域位于TraI蛋白催化结构域之间的中央区域。

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