首页> 美国卫生研究院文献>Journal of Bacteriology >In vitro binding of the Salmonella dublin virulence plasmid regulatory protein SpvR to the promoter regions of spvA and spvR.
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In vitro binding of the Salmonella dublin virulence plasmid regulatory protein SpvR to the promoter regions of spvA and spvR.

机译:沙门氏菌都柏林毒力质粒调节蛋白SpvR与spvA和spvR启动子区域的体外结合。

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摘要

The spv regulon of Salmonella dublin is essential for virulence in mice. SpvR, a LysR-type regulator, induces the expression of the spvABCD operon and its own expression in the stationary phase of bacterial growth and in macrophages. We constructed fusion proteins to the maltose-binding protein (MBP) and a His tag peptide (His) to overcome the insolubility and to facilitate purification of SpvR. We demonstrated that both fusion proteins, MBP-SpvR and His-SpvR, were able to induce spvA expression in vivo. MBP-SpvR was produced as soluble protein, whereas His-SpvR was only marginally present in the soluble cell fraction. Affinity chromatography resulted in at least 95% pure MBP-SpvR protein and in an enrichment of His-SpvR. Gel mobility shift assay revealed that the SpvR fusion proteins were able to bind to 125-and 147-bp DNA fragments of the spvA and spvR promoter regions, respectively. DNase I footprint experiments showed that the fusion proteins protected DNA regions of 54 and 50 bp within the spvA and spvR promoter regions, respectively.
机译:沙门氏菌都柏林的spv regulon对小鼠的毒性至关重要。 SpvR,一种LysR型调节剂,在细菌生长的稳定期和巨噬细胞中诱导spvABCD操纵子的表达及其自身表达。我们构建了麦芽糖结合蛋白(MBP)和His标签肽(His)的融合蛋白,以克服不溶性并促进SpvR的纯化。我们证明这两种融合蛋白,MBP-SpvR和His-SpvR,都能够在体内诱导spvA表达。 MBP-SpvR生产为可溶性蛋白,而His-SpvR仅少量存在于可溶性细胞级分中。亲和色谱法产生至少95%的纯MBP-SpvR蛋白和丰富的His-SpvR。凝胶迁移率迁移分析表明,SpvR融合蛋白能够分别与spvA和spvR启动子区域的125和147 bp DNA片段结合。 DNase I足迹实验表明,融合蛋白分别保护了spvA和spvR启动子区域内54 bp和50 bp的DNA区域。

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