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从恶臭假单胞菌PPN的Tn5染色体突变体中分离高频重组供体并重新校准遗传图谱。

Isolation of high frequency of recombination donors from Tn5 chromosomal mutants of Pseudomonas putida PPN and recalibration of the genetic map.

作者信息

Strom A D, Hirst R, Petering J, Morgan A

机构信息

Department of Genetics and Developmental Biology, Monash University, Clayton, Victoria, Australia.

出版信息

Genetics. 1990 Nov;126(3):497-503. doi: 10.1093/genetics/126.3.497.

Abstract

A Tn5 loaded derivative of the IncP-10 plasmid R91-5 (pMO75) was used as a suicide vector to generate random chromosomal insertion mutations in Pseudomonas putida PPN. Reintroduction of pMO75 into such mutants resulted in integration of the plasmid at the site of Tn5 insertion, giving rise to two classes of high frequency of donors recombination (Hfr) donors, transferring chromosome at high frequency (greater than 10(-1) per donor cell) in opposite directions. Consequently, Tn5 induced auxotrophic mutations could be equated with or distinguished from previously mapped mutations, and closely linked markers ordered, on the basis of marker recovery using the two classes of Hfr donor. The isolation of many new transfer origins allowed more accurate time-of-entry analysis than previously possible and resulted in the reduction of the genetic map from 103 min to 88 min.

摘要

IncP-10 质粒 R91-5(pMO75)的一个携带 Tn5 的衍生物被用作自杀载体,以在恶臭假单胞菌 PPN 中产生随机染色体插入突变。将 pMO75 重新导入此类突变体导致质粒在 Tn5 插入位点整合,产生了两类高频供体重组(Hfr)供体,它们以相反方向高频(每个供体细胞大于 10^(-1))转移染色体。因此,基于使用这两类 Hfr 供体的标记回收,Tn5 诱导的营养缺陷型突变可以与先前定位的突变等同或区分开来,并对紧密连锁的标记进行排序。许多新转移起点的分离使得比以前更准确的进入时间分析成为可能,并导致遗传图谱从 103 分钟减少到 88 分钟。

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