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对携带TOL质粒pWW0上甲苯降解基因的转座子的遗传分析。

Genetic analysis of a transposon carrying toluene degrading genes on a TOL plasmid pWW0.

作者信息

Tsuda M, Iino T

机构信息

Department of Biology, Faculty of Science, University of Tokyo, Japan.

出版信息

Mol Gen Genet. 1987 Dec;210(2):270-6. doi: 10.1007/BF00325693.

Abstract

Toluene degrading (xyl) genes on a Pseudomonas TOL plasmid pWW0 are located within a 39-kb DNA portion. The 56-kb region including these xyl genes and its 17-kb derivative with a deletion of the internal 39-kb portion transposed to various sites on target replicons such as pACYC184 and R388 in Escherichia coli recA strains. Thus the 56- and 17-kb regions were designated Tn4651 and Tn4652, respectively. Genetic analysis of Tn4652 demonstrated that its transposition occurs by a two-step process, namely, cointegrate formation and its subsequent resolution. The presence in cis of DNA sequences of no more than 150 bp at both ends of Tn4652 was prerequisite for cointegrate formation, and this step was mediated by a trans-acting factor, transposase, which was encoded in a 3.0-kb segment at one end of the transposon. Cointegrate resolution took place site-specifically within a 200-bp fragment, which was situated 10 kb away from the transposase gene. Based on the stability of cointegrates formed by various mini-Tn4652 derivatives, it was shown that the cointegrate resolution requires two trans-acting factors encoded within 1.0- and 1.2-kb fragments that encompass the recombination site involved in the resolution.

摘要

假单胞菌TOL质粒pWW0上的甲苯降解(xyl)基因位于一段39 kb的DNA区域内。包含这些xyl基因的56 kb区域及其缺失内部39 kb部分的17 kb衍生物被转座到大肠杆菌recA菌株中目标复制子(如pACYC184和R388)的不同位点。因此,56 kb和17 kb区域分别被命名为Tn4651和Tn4652。对Tn4652的遗传分析表明,其转座通过两步过程发生,即共整合体形成及其随后的拆分。Tn4652两端不超过150 bp的DNA序列顺式存在是共整合体形成的先决条件,这一步骤由一种反式作用因子转座酶介导,该酶由转座子一端的一个3.0 kb片段编码。共整合体拆分在一个200 bp的片段内位点特异性地发生,该片段位于距转座酶基因10 kb处。基于各种mini-Tn4652衍生物形成的共整合体的稳定性,表明共整合体拆分需要由1.0 kb和1.2 kb片段编码的两种反式作用因子,这两个片段包含参与拆分的重组位点。

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