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merG基因产物与假单胞菌K-62菌株对苯基汞的抗性有关。

The merG gene product is involved in phenylmercury resistance in Pseudomonas strain K-62.

作者信息

Kiyono M, Pan-Hou H

机构信息

Faculty of Pharmaceutical Sciences, Setsunan University, Hirakata, Osaka 573-0101, Japan.

出版信息

J Bacteriol. 1999 Feb;181(3):726-30. doi: 10.1128/JB.181.3.726-730.1999.

Abstract

The physiological function of a new gene, hereby designated merG, located between merA and merB on the broad-spectrum mer operon of Pseudomonas strain K-62 plasmid pMR26 was investigated. The 654-bp merG gene encodes a protein with a canonical leader sequence at its N terminus. The processing of the signal peptide of this protein was dose-dependently inhibited by sodium azide, a potent inhibitor of protein export. These results suggest that the mature MerG protein (ca. 20 kDa) may be located in the periplasm. Deletion of the merG gene from the broad-spectrum mer operon of pMR26 had no effect on the inorganic mercury resistance phenotype, but rendered the bacterium more sensitive to phenylmercury than its isogenic wild-type strain. Escherichia coli cells bearing pMU29, which carries a deletion of the merG gene, took up significantly more phenylmercury than the bacteria with the intact plasmid pMRA17. When the merG gene in a compatible plasmid was transformed into the E. coli strain carrying pMU29, the high uptake of and high sensitivity to phenylmercury were almost completely restored to their original levels. These results demonstrate that the merG gene is involved in phenylmercury resistance, presumably by reducing in-cell permeability to phenylmercury.

摘要

对位于假单胞菌K - 62菌株质粒pMR26的广谱汞操纵子上merA和merB之间的一个新基因(在此命名为merG)的生理功能进行了研究。654碱基对的merG基因在其N端编码一个具有典型前导序列的蛋白质。该蛋白质信号肽的加工受到叠氮化钠(一种蛋白质输出的有效抑制剂)的剂量依赖性抑制。这些结果表明,成熟的MerG蛋白(约20 kDa)可能位于周质中。从pMR26的广谱汞操纵子中删除merG基因对无机汞抗性表型没有影响,但使该细菌对苯基汞比其同基因野生型菌株更敏感。携带缺失merG基因的pMU29的大肠杆菌细胞比携带完整质粒pMRA17的细菌摄取显著更多的苯基汞。当将兼容质粒中的merG基因转化到携带pMU29的大肠杆菌菌株中时,对苯基汞的高摄取和高敏感性几乎完全恢复到原始水平。这些结果表明,merG基因参与苯基汞抗性,可能是通过降低细胞对苯基汞的通透性。

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