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四个志贺氏菌亚群中鞭毛主操纵子的检测与特性分析。

Detection and characterization of the flagellar master operon in the four Shigella subgroups.

作者信息

Al Mamun A A, Tominaga A, Enomoto M

机构信息

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

出版信息

J Bacteriol. 1996 Jul;178(13):3722-6. doi: 10.1128/jb.178.13.3722-3726.1996.

DOI:10.1128/jb.178.13.3722-3726.1996
PMID:8682772
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC232628/
Abstract

Strains in the genus Shigella are nonmotile, but they retain some cryptic flagellar operons whether functional or defective (A.Tominaga, M. A.-H. Mahmoud, T. Mukaihara, and M. Enomoto, Mol. Microbiol. 12:277-285, 1994). To disclose the cause of motility loss in shigellae, the presence or defectiveness of the flhD and flhC genes, composing the master operon whose mutation causes inactivation of the entire flagellar regulon, was examined in the four Shigella subgroups. The flhD operon cloned from Shigella boydii and Shigella sonnei can activate, though insufficiently, the regulon in the Escherichia coli flhD or flhC mutant background. The clone from Shigella dysenteriae has a functional flhD gene and nonfunctional flhC gene, and its inactivation has been caused by the IS1 element inserted in its 5' end. The operon of Shigella flexneri is nonfunctional and has suffered an IS1-insertion mutation at the 5' end of the flhD gene. Comparison of restriction maps indicates that only the central 1.8-kb region, including part of the flhC gene and its adjacent mot operon, is conserved among the four Shigella subgroups as well as in E. coli, but in Salmonella typhimurium the whole map is quite different from the others. Motility loss in shigellae is not attributable to genetic damage in the master operon of a common ancestor, but it occurs separately in respective ancestors of the four subgroups, and in both S. dysenteriae and S.flexneri IS1 insertion in the master operon might be the primary cause of motility loss.

摘要

志贺氏菌属的菌株无运动性,但无论功能正常与否,它们都保留了一些隐蔽的鞭毛操纵子(A. 富永、M. A.-H. 马哈茂德、T. 向原和M. 榎本,《分子微生物学》12:277 - 285,1994年)。为了揭示志贺氏菌运动性丧失的原因,研究了构成主操纵子的flhD和flhC基因的存在或缺陷情况,该主操纵子的突变会导致整个鞭毛调节子失活,研究对象为四个志贺氏菌亚群。从鲍氏志贺氏菌和宋内志贺氏菌克隆的flhD操纵子,虽激活作用不足,但能在大肠杆菌flhD或flhC突变背景下激活调节子。从痢疾志贺氏菌克隆的片段有一个功能性flhD基因和一个无功能的flhC基因,其失活是由插入其5'端的IS1元件导致的。福氏志贺氏菌的操纵子无功能,且在flhD基因的5'端发生了IS1插入突变。限制性酶切图谱比较表明,仅包括flhC基因部分及其相邻的mot操纵子的中央1.8 kb区域,在四个志贺氏菌亚群以及大肠杆菌中是保守的,但在鼠伤寒沙门氏菌中,整个图谱与其他物种有很大不同。志贺氏菌运动性丧失并非归因于共同祖先主操纵子的基因损伤,而是在四个亚群各自的祖先中分别发生的,并且在痢疾志贺氏菌和福氏志贺氏菌中,主操纵子中的IS1插入可能是运动性丧失的主要原因。

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