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来自嗜热栖热菌 HB8 的 TetR 家族转录调节因子 SbtR 的结构与功能。

Structure and function of a TetR family transcriptional regulator, SbtR, from thermus thermophilus HB8.

机构信息

RIKEN SPring-8 Center, RIKEN Harima Institute, 1-1-1 Kouto, Sayo, Hyogo 679-5148, Japan.

出版信息

Proteins. 2013 Jul;81(7):1166-78. doi: 10.1002/prot.24266. Epub 2013 Apr 10.

DOI:10.1002/prot.24266
PMID:23408580
Abstract

SbtR is one of the four TetR family transcriptional regulators present in the extremely thermophilic bacterium, Thermus thermophilus HB8. We identified 10 genes controlled by four promoters with negative regulation by SbtR in vitro. The SbtR-regulated gene products include probable transporters, probable enzymes for sugar or amino acid metabolism, and nucleic acid-related enzymes. SbtR binds pseudopalindromic sequences, with the consensus sequence of 5'-TGACCCNNKGGTCA-3' surrounding the promoters, and has a proposed 1:1 dimer binding stoichiometry. The X-ray crystal structure analysis revealed that SbtR comprises either nine or 10 α-helices and forms a dimer, as in the typical TetR family proteins. Similar to many characterized TetR family regulators, SbtR has a predicted ligand-binding pocket at the center of each monomer. Interestingly, the SbtR dimer contains an intermolecular disulfide bridge, formed between the Cys164 residues at the entrance of the pocket. The Cys164Ser and Cys164Ala mutant SbtR proteins formed homodimers similar to that of the wild type, but their thermal stabilities were lower by about 8°C, indicating that the disulfide bridge contributes to the thermal stability of the protein. However, altered repression activity of the mutants was not observed in vitro. From these results, we propose that ligand-binding is essential for SbtR to disengage from DNA, in a similar manner to the other characterized TetR family regulators. The formation and reduction of the disulfide bond might function in controlling the ligand-binding affinity of this transcriptional regulator.

摘要

SbtR 是嗜热菌 Thermus thermophilus HB8 中存在的四个 TetR 家族转录调节因子之一。我们在体外鉴定了 10 个受 SbtR 负调控的基因,这些基因受四个启动子控制。SbtR 调节的基因产物包括可能的转运蛋白、可能的糖或氨基酸代谢酶以及与核酸相关的酶。SbtR 结合假回文序列,启动子周围的共有序列为 5'-TGACCCNNKGGTCA-3',并具有拟议的 1:1 二聚体结合比例。X 射线晶体结构分析表明,SbtR 由 9 个或 10 个α-螺旋组成,形成二聚体,与典型的 TetR 家族蛋白相似。与许多已鉴定的 TetR 家族调节剂相似,SbtR 在每个单体的中心具有预测的配体结合口袋。有趣的是,SbtR 二聚体包含一个分子间二硫键,该键在口袋入口处的 Cys164 残基之间形成。Cys164Ser 和 Cys164Ala 突变 SbtR 蛋白形成类似于野生型的同源二聚体,但它们的热稳定性降低了约 8°C,表明二硫键有助于蛋白质的热稳定性。然而,在体外未观察到突变体的抑制活性改变。根据这些结果,我们提出配体结合对于 SbtR 从 DNA 上脱离是必不可少的,这与其他已鉴定的 TetR 家族调节剂类似。二硫键的形成和还原可能在控制该转录调节剂的配体结合亲和力方面发挥作用。

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