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鉴定产 albomycin 的链霉菌 sp. 菌株 ATCC 700974 中的两种丝氨酰-tRNA 合成酶。

Characterization of two seryl-tRNA synthetases in albomycin-producing Streptomyces sp. strain ATCC 700974.

机构信息

Molecular and Cellular Biology Program and Department of Biological Sciences, Ohio University, Athens, OH 45701, USA.

出版信息

Antimicrob Agents Chemother. 2009 Nov;53(11):4619-27. doi: 10.1128/AAC.00782-09. Epub 2009 Aug 31.

Abstract

The Trojan horse antibiotic albomycin, produced by Streptomyces sp. strain ATCC 700974, contains a thioribosyl nucleoside moiety linked to a hydroxamate siderophore through a serine residue. The seryl nucleoside structure (SB-217452) is a potent inhibitor of seryl-tRNA synthetase (SerRS) in the pathogenic bacterium Staphylococcus aureus, with a 50% inhibitory concentration (IC(50)) of approximately 8 nM. In the albomycin-producing Streptomyces sp., a bacterial SerRS homolog (Alb10) was found to be encoded in a biosynthetic gene cluster in addition to another serRS gene (serS1) at a different genetic locus. Alb10, named SerRS2 herein, is significantly divergent from SerRS1, which shows high homology to the housekeeping SerRS found in other Streptomyces species. We genetically and biochemically characterized the two genes and the proteins encoded. Both genes were able to complement a temperature-sensitive serS mutant of Escherichia coli and allowed growth at a nonpermissive temperature. serS2 was shown to confer albomycin resistance, with specific amino acid residues in the motif 2 signature sequences of SerRS2 playing key roles. SerRS1 and SerRS2 are comparably efficient in vitro, but the K(m) of serine for SerRS2 measured during tRNA aminoacylation is more than 20-fold higher than that for SerRS1. SB-217452 was also enzymatically generated and purified by two-step chromatography. Its IC(50) against SerRS1 was estimated to be 10-fold lower than that against SerRS2. In contrast, both SerRSs displayed comparable inhibition kinetics for serine hydroxamate, indicating that SerRS2 was specifically resistant to SB-217452. These data suggest that mining Streptomyces genomes for duplicated aminoacyl-tRNA synthetase genes could provide a novel approach for the identification of natural products targeting aminoacyl-tRNA synthetases.

摘要

产阿泊霉素的木马抗生素,由链霉菌属菌株 ATCC 700974 产生,含有通过丝氨酸残基连接到羟肟酸铁载体的硫代核糖核苷部分。丝氨酰核苷结构(SB-217452)是致病细菌金黄色葡萄球菌中丝氨酰-tRNA 合成酶(SerRS)的有效抑制剂,对 50%抑制浓度(IC(50))约为 8 nM。在产阿泊霉素的链霉菌中,除了另一个位于不同遗传位置的 serS1 基因外,还在生物合成基因簇中发现了细菌 SerRS 同源物(Alb10)。Alb10 在此命名为 SerRS2,与其他链霉菌物种中的管家 SerRS 高度同源,与 SerRS1 显著不同。我们从遗传和生化两方面对这两个基因和编码的蛋白质进行了表征。这两个基因都能够互补大肠杆菌的温度敏感型 serS 突变体,并允许在非允许温度下生长。serS2 表现出对阿泊霉素的抗性,SerRS2 特征序列 2 模体中的特定氨基酸残基发挥关键作用。SerRS1 和 SerRS2 在体外的效率相当,但在 tRNA 氨酰化过程中测量的 SerRS2 的丝氨酸 K(m)比 SerRS1 高 20 多倍。SB-217452 也通过两步层析法酶促生成和纯化。其对 SerRS1 的 IC(50)估计比 SerRS2 低 10 倍。相比之下,SerRSs 对丝氨酸羟肟酸均表现出相似的抑制动力学,表明 SerRS2 对 SB-217452 具有特异性抗性。这些数据表明,从链霉菌基因组中挖掘重复的氨酰-tRNA 合成酶基因可能为鉴定靶向氨酰-tRNA 合成酶的天然产物提供一种新方法。

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