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副溶血性弧菌中负责热稳定直接溶血素基因(tdh)缺失的功能性插入序列的检测。

Detection of a functional insertion sequence responsible for deletion of the thermostable direct hemolysin gene (tdh) in Vibrio parahaemolyticus.

作者信息

Kamruzzaman Muhammad, Bhoopong Phuangthip, Vuddhakul Varaporn, Nishibuchi Mitsuaki

机构信息

Graduate School of Medicine, Kyoto University, Kyoto 606-8501, Japan.

出版信息

Gene. 2008 Sep 15;421(1-2):67-73. doi: 10.1016/j.gene.2008.06.009. Epub 2008 Jun 12.

Abstract

The thermostable direct hemolysin coded by the tdh gene is a marker of virulent strains of Vibrio parahaemolyticus. The tdh genes are flanked by insertion sequences collectively named as ISVs or their remnants; but the ISVs so far examined have accumulated mutations in the transposase genes and underwent structural arrangements and their transposition activity could not be expected; the tdh gene was thus considered to have been acquired by V. parahaemolyticus through horizontal transfer in the past during evolution. We recently isolated from the same patient tdh+ strains and a tdh(-) strain (PCR examination) that were otherwise indistinguishable. The purpose of this study was to examine the hypothesis that the tdh(-) strain was derived from the tdh+ strain by a deletion of the tdh gene mediated by a functional ISV. Southern blot hybridization showed tdh+ sequences in the tdh(-) strain (PSU-1466). Nucleotide sequence analysis of the tdh and its flanking sequences revealed the tdh gene was split into two parts and they were located 3182-bp apart in PSU-1466. The two tdh sequences were flanked by one of the ISVs, named as ISVpa3, in PSU-1466. This genetic structure could be explained by an ISVpa3-mediated partial tdh deletion from a tdh+ strain followed by transposition of the duplicated ISVpa3 and the deleted tdh sequence into a neighboring location. The ISVpa3 of PSU-1466 coded for a full-length transposase and a DDE motif. We were able to demonstrate transposition activity of the ISVpa3 cloned from PSU-1466 using the replicon fusion assay with the conjugal transfer of a cointegrate from Escherichia coli to V. parahaemolyticus. Our data support ISVpa3-mediated partial tdh deletion resulted in the emergence of the tdh(-) strain.

摘要

由tdh基因编码的耐热直接溶血素是副溶血性弧菌强毒株的一个标志物。tdh基因两侧是统称为ISVs或其残余序列的插入序列;但到目前为止所检测的ISVs在转座酶基因中积累了突变并经历了结构重排,无法预期它们的转座活性;因此tdh基因被认为是副溶血性弧菌在过去进化过程中通过水平转移获得的。我们最近从同一患者中分离出tdh+菌株和一株tdh(-)菌株(PCR检测),除此之外它们无法区分。本研究的目的是检验这样一个假说,即tdh(-)菌株是由tdh+菌株通过功能性ISV介导的tdh基因缺失而产生的。Southern印迹杂交显示tdh(-)菌株(PSU-1466)中有tdh+序列。tdh及其侧翼序列的核苷酸序列分析表明,在PSU-1466中tdh基因被分成两部分,它们相隔3182 bp。这两个tdh序列在PSU-1466中被一个名为ISVpa3的ISVs侧翼包围。这种遗传结构可以解释为ISVpa3介导tdh+菌株的tdh部分缺失,随后重复的ISVpa3和缺失的tdh序列转座到相邻位置。PSU-1466的ISVpa3编码一个全长转座酶和一个DDE基序。我们能够通过复制子融合试验,利用共整合体从大肠杆菌向副溶血性弧菌的接合转移,证明从PSU-1466克隆的ISVpa3的转座活性。我们的数据支持ISVpa3介导的tdh部分缺失导致了tdh(-)菌株的出现。

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