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首页> 外文期刊>Journal of bacteriology >In the Staphylococcus aureus Two-Component System sae, the Response Regulator SaeR Binds to a Direct Repeat Sequence and DNA Binding Requires Phosphorylation by the Sensor Kinase SaeS
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In the Staphylococcus aureus Two-Component System sae, the Response Regulator SaeR Binds to a Direct Repeat Sequence and DNA Binding Requires Phosphorylation by the Sensor Kinase SaeS

机译:在金黄色葡萄球菌两组分系统sae中,响应调节剂SaeR绑定到直接重复序列,DNA结合需要通过传感器激酶SaeS进行磷酸化。

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Staphylococcus aureus uses the SaeRS two-component system to control the expression of many virulence factors such as alpha-hemolysin and coagulase; however, the molecular mechanism of this signaling has not yet been elucidated. Here, using the P1 promoter of the sae operon as a model target DNA, we demonstrated that the unphosphorylated response regulator SaeR does not bind to the P1 promoter DNA, while its C-terminal DNA binding domain alone does. The DNA binding activity of full-length SaeR could be restored by sensor kinase SaeS-induced phosphorylation. Phosphorylated SaeR is more resistant to digestion by trypsin, suggesting conformational changes. DNase I footprinting assays revealed that the SaeR protection region in the P1 promoter contains a direct repeat sequence (GTTAAN6GTTAA [where N is any nucleotide]). This sequence is critical to the binding of phosphorylated SaeR. Mutational changes in the repeat sequence greatly reduced both the in vitro binding of SaeR and the in vivo function of the P1 promoter. From these results, we concluded that SaeR recognizes the direct repeat sequence as a binding site and that binding requires phosphorylation by SaeS.
机译:金黄色葡萄球菌使用SaeRS两组分系统控制许多毒力因子的表达,例如α-溶血素和凝固酶。然而,该信号传导的分子机制尚未阐明。在这里,我们使用 sae 操纵子的P1启动子作为模型目标DNA,我们证明了未磷酸化的应答调节因子SaeR不会与P1启动子DNA结合,而仅其C端DNA结合域可以。全长SaeR的DNA结合活性可以通过传感器激酶SaeS诱导的磷酸化来恢复。磷酸化的SaeR对胰蛋白酶的消化更有抵抗力,表明其构象变化。 DNase I足迹分析表明,P1启动子中的SaeR保护区含有一个直接重复序列(GTTAAN 6 GTTAA [其中N是任何核苷酸])。此序列对于磷酸化SaeR的结合至关重要。重复序列的突变改变大大降低了SaeR的体外结合和P1启动子的体内功能。根据这些结果,我们得出结论,SaeR将直接重复序列识别为结合位点,并且结合需要SaeS进行磷酸化。

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