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锌外排系统的基因组分析和特性研究,一株耐高锌细菌,Comamonas testosteroni S44。

Genome analysis and characterization of zinc efflux systems of a highly zinc-resistant bacterium, Comamonas testosteroni S44.

机构信息

State Key Laboratory of Agricultural Microbiology, College of Life Science and Technology, Huazhong Agricultural University, Wuhan 430070, China.

出版信息

Res Microbiol. 2011 Sep;162(7):671-9. doi: 10.1016/j.resmic.2011.06.002. Epub 2011 Jun 13.

Abstract

A novel and multiple metal(loid)-resistant strain Comamonas testosteroni S44 with a high Zn(2+) resistance level (10 mM) was isolated. To understand the molecular basis for the high zinc resistance, whole genome sequencing was performed and revealed a large number of genes encoding putative metal(loid) resistance proteins, mobile genetic elements (MGEs) and horizontal gene transfer (HGT) events that may have occurred to adapt to a metal(loid)-contaminated environment. In particular, 9 putative Zn(2+) transporters [4 znt operons encoding putative Zn(2+)-translocating P-type ATPases and 5 czc operons encoding putative RND-driven (resistance, nodulation, cell division protein family)] tripartite protein complexes were identified. Real-time RT-PCR analysis revealed that the four zntA-like genes were all induced by Zn(2+), while czcA genes were either Zn(2+)-induced or downregulated by Zn(2+). Furthermore, a zntR1A1 operon encoding a ZntR-type regulator and a P-type ATPase was studied in detail. The zntR1 deletion strain (S44ΔzntR1) displayed intermediate resistance to Zn(2+) (6 mM) and accumulated more intracellular Zn(2+). Reporter gene expression assays indicated that ZntR1 responded to Zn(2+), Cd(2+) and Pb(2+), with Zn(2+) being the best inducer. Gene transcription analysis indicated that ZntR1 was a regulator for transcription of zntA1, while other putative ZntR-type regulators may also regulate the transcription expression of zntA1.

摘要

一株具有高锌(2+)抗性水平(10 mM)的新型、多重金属(类)抗性菌株 Comamonas testosteroni S44 被分离出来。为了了解高锌抗性的分子基础,进行了全基因组测序,结果显示了大量编码潜在金属(类)抗性蛋白、移动遗传元件(MGEs)和水平基因转移(HGT)事件的基因,这些基因可能发生了以适应受金属(类)污染的环境。特别是,鉴定出了 9 个潜在的 Zn(2+)转运体[4 个 znt 操纵子编码潜在的 Zn(2+)转运 P 型 ATPase 和 5 个 czc 操纵子编码潜在的 RND 驱动(抗性、结节、细胞分裂蛋白家族)]三组分蛋白复合物。实时 RT-PCR 分析显示,四个 zntA 样基因均受 Zn(2+)诱导,而 czcA 基因则受 Zn(2+)诱导或下调。此外,详细研究了一个编码 ZntR 型调节剂和 P 型 ATPase 的 zntR1A1 操纵子。zntR1 缺失株(S44ΔzntR1)对 Zn(2+)(6 mM)表现出中等抗性,并积累了更多的细胞内 Zn(2+)。报告基因表达分析表明,ZntR1 对 Zn(2+)、Cd(2+)和 Pb(2+)有反应,其中 Zn(2+)是最好的诱导剂。基因转录分析表明,ZntR1 是 zntA1 转录的调节剂,而其他潜在的 ZntR 型调节剂也可能调节 zntA1 的转录表达。

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