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MgrA 的磷酸化及其对金黄色葡萄球菌 NorA 和 NorB 外排泵表达的影响。

Phosphorylation of MgrA and its effect on expression of the NorA and NorB efflux pumps of Staphylococcus aureus.

机构信息

Division of Infectious Diseases, Massachusetts General Hospital, Harvard Medical School, Boston MA 02114-2696, USA.

出版信息

J Bacteriol. 2010 May;192(10):2525-34. doi: 10.1128/JB.00018-10. Epub 2010 Mar 16.

Abstract

MgrA is a global regulator in Staphylococcus aureus that controls the expression of diverse genes encoding virulence factors and multidrug resistance (MDR) efflux transporters. We identified pknB, which encodes the (Ser/Thr) kinase PknB, in the S. aureus genome. PknB was able to autophosphorylate as well as phosphorylate purified MgrA. We demonstrated that rsbU, which encodes a Ser/Thr phosphatase and is involved in the activation of the SigB regulon, was able to dephosphorylate MgrA-P but not PknB-P. Serines 110 and 113 of MgrA were found to be phosphorylated, and Ala substitutions at these positions resulted in reductions in the level of phosphorylation of MgrA. DNA gel shift binding assays using norA and norB promoters showed that MgrA-P was able to bind the norB promoter but not the norA promoter, a pattern which was the reverse of that for unphosphorylated MgrA. The double mutant MgrA(S110A-S113A) bound to the norA promoter but not the norB promoter. The double mutant led to a 2-fold decrease in norA transcripts and a 2-fold decrease in the MICs of norfloxacin and ciprofloxacin in strain RN6390. Thus, phosphorylation of MgrA results in loss of binding to the norA promoter, but with a gain of the ability to bind the norB promoter. Loss of the ability to phosphorylate MgrA by Ala substitution resulted in increased repression of norA expression and in reductions in susceptibilities to NorA substrates.

摘要

MgrA 是金黄色葡萄球菌中的一种全局调控因子,控制着多种编码毒力因子和多药耐药(MDR)外排转运蛋白的基因的表达。我们在金黄色葡萄球菌基因组中鉴定出编码(Ser/Thr)激酶 PknB 的 pknB。PknB 能够自身磷酸化以及磷酸化纯化的 MgrA。我们证明,编码丝氨酸/苏氨酸磷酸酶并参与 SigB 调控子激活的 rsbU 能够去磷酸化 MgrA-P,但不能去磷酸化 PknB-P。发现 MgrA 的 Ser110 和 Ser113 被磷酸化,并且这些位置的 Ala 取代导致 MgrA 的磷酸化水平降低。使用 norA 和 norB 启动子的 DNA 凝胶迁移结合测定表明,MgrA-P 能够结合 norB 启动子但不能结合 norA 启动子,这种模式与非磷酸化 MgrA 的模式相反。MgrA(S110A-S113A)双突变体结合 norA 启动子但不结合 norB 启动子。双突变体导致 norA 转录物减少 2 倍,并且菌株 RN6390 中诺氟沙星和环丙沙星的 MIC 值降低 2 倍。因此,MgrA 的磷酸化导致与 norA 启动子的结合丧失,但获得与 norB 启动子结合的能力。通过 Ala 取代导致 MgrA 磷酸化能力丧失,导致 norA 表达的抑制增加,并且对 NorA 底物的敏感性降低。

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本文引用的文献

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