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五日热巴尔通体gyrB基因突变赋予对香豆霉素A1的抗性。

Mutations in Bartonella bacilliformis gyrB confer resistance to coumermycin A1.

作者信息

Battisti J M, Smitherman L S, Samuels D S, Minnick M F

机构信息

Division of Biological Sciences, The University of Montana, Missoula, Montana 59812-1002, USA.

出版信息

Antimicrob Agents Chemother. 1998 Nov;42(11):2906-13. doi: 10.1128/AAC.42.11.2906.

Abstract

This study describes the first isolation and characterization of spontaneous mutants conferring natural resistance to an antibiotic for any Bartonella species. The Bartonella bacilliformis gyrB gene, which encodes the B subunit of DNA gyrase, was cloned and sequenced. The gyrB open reading frame (ORF) is 2,079 bp and encodes a deduced amino acid sequence of 692 residues, corresponding to a predicted protein of approximately 77.5 kDa. Sequence alignment indicates that B. bacilliformis GyrB is most similar to the GyrB protein from Bacillus subtilis (40.1% amino acid sequence identity) and that it contains the longest N-terminal tail (52 residues) of any GyrB characterized to date. The cloned B. bacilliformis gyrB was expressed in an Escherichia coli S30 cell extract and was able to functionally complement a temperature-sensitive E. coli Cour gyrB mutant (strain N4177). We isolated and characterized spontaneous mutants of B. bacilliformis resistant to coumermycin A1, an antibiotic that targets GyrB. Sequence analysis of gyrB from 12 Cour mutants of B. bacilliformis identified single nucleotide transitions at three separate loci in the ORF. The predicted amino acid substitutions resulting from these transitions are Gly to Ser at position 124 (Gly124-->Ser), Arg184-->Gln, and Thr214-->Ala or Thr214-->Ile, which are analogous to mutated residues found in previously characterized resistant gyrB genes from Borrelia burgdorferi, E. coli, Staphylococcus aureus, and Haloferax sp. The Cour mutants are three to five times more resistant to coumermycin A1 than the wild-type parental strain.

摘要

本研究描述了首次分离和鉴定出对任何巴尔通体属物种的抗生素具有天然抗性的自发突变体。编码DNA促旋酶B亚基的巴尔通体杆菌gyrB基因被克隆并测序。gyrB开放阅读框(ORF)为2079 bp,编码一个由692个残基组成的推导氨基酸序列,对应于一个预测分子量约为77.5 kDa的蛋白质。序列比对表明,巴尔通体杆菌GyrB与枯草芽孢杆菌的GyrB蛋白最相似(氨基酸序列同一性为40.1%),并且它含有迄今为止所鉴定的任何GyrB中最长的N端尾巴(52个残基)。克隆的巴尔通体杆菌gyrB在大肠杆菌S30细胞提取物中表达,并能够在功能上互补温度敏感型大肠杆菌Cour gyrB突变体(菌株N4177)。我们分离并鉴定了对香豆霉素A1具有抗性的巴尔通体杆菌自发突变体,香豆霉素A1是一种靶向GyrB的抗生素。对来自12个巴尔通体杆菌Cour突变体的gyrB进行序列分析,在ORF的三个不同位点鉴定出单核苷酸转换。这些转换导致的预测氨基酸取代分别为第124位的甘氨酸到丝氨酸(Gly124→Ser)、Arg184→Gln以及Thr214→Ala或Thr214→Ile,这些与先前在伯氏疏螺旋体、大肠杆菌、金黄色葡萄球菌和嗜盐菌属中鉴定的抗性gyrB基因中的突变残基类似。Cour突变体对香豆霉素A1的抗性比野生型亲本菌株高3至5倍。

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Adv Pediatr Infect Dis. 1996;11:1-27.
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