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一种有效的扰动方法,用于预测谷氨酰胺结合蛋白的功能关键位点。

An efficient perturbation method to predict the functionally key sites of glutamine binding protein.

机构信息

College of Life Science and Bioengineering, Beijing University of Technology, Beijing 100124, China.

College of Life Science and Bioengineering, Beijing University of Technology, Beijing 100124, China.

出版信息

Comput Biol Chem. 2017 Apr;67:62-68. doi: 10.1016/j.compbiolchem.2016.12.003. Epub 2016 Dec 29.

Abstract

Glutamine-Binding Protein (GlnBP) of Escherichia coli, an important member of the periplasmic binding protein family, is responsible for the first step in the active transport of glutamine across the cytoplasmic membrane. In this work, the functionally key regulation sites of GlnBP were identified by utilizing a perturbation method proposed by our group, in which the residues whose perturbations markedly change the binding free energy between GlnBP and glutamine are considered to be functionally key residues. The results show that besides the substrate binding sites, some other residues distant from the binding pocket, including the ones in the hinge regions between the two domains, the front- and back- door channels and the exposed region, are important for the function of glutamine binding and transport. The predicted results are well consistent with the theoretical and experimental data, which indicates that our method is an effective approach to identify the key residues important for both ligand binding and long-range allosteric signal transmission. This work can provide some insights into the function performance of GlnBP and the physical mechanism of its allosteric regulation.

摘要

大肠杆菌的谷氨酰胺结合蛋白(GlnBP)是周质结合蛋白家族的重要成员,负责谷氨酰胺穿过细胞质膜的主动转运的第一步。在这项工作中,利用我们小组提出的一种扰动方法鉴定了 GlnBP 的功能关键调节位点,其中那些扰动明显改变 GlnBP 和谷氨酰胺之间结合自由能的残基被认为是功能关键残基。结果表明,除了底物结合位点外,一些其他的残基,包括两个结构域之间的铰链区域、前后门通道和暴露区域中的残基,对谷氨酰胺结合和转运的功能也很重要。预测结果与理论和实验数据非常吻合,这表明我们的方法是一种有效的方法,可以识别对配体结合和长程变构信号传递都很重要的关键残基。这项工作可以为 GlnBP 的功能表现和变构调节的物理机制提供一些见解。

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