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色氨酸合酶α亚基中的远程相互作用有助于协调配体结合、催化和底物运输。

Long-range interactions in the α subunit of tryptophan synthase help to coordinate ligand binding, catalysis, and substrate channeling.

机构信息

Department of Chemistry, Pennsylvania State University, 240 Chemistry Building, University Park, PA 16802, USA.

出版信息

J Mol Biol. 2013 May 13;425(9):1527-45. doi: 10.1016/j.jmb.2013.01.030. Epub 2013 Jan 30.

DOI:10.1016/j.jmb.2013.01.030
PMID:23376097
Abstract

The α-subunit of tryptophan synthase (αTS) catalyzes the conversion of indole-3-glycerol phosphate to d-glyceraldehyde-3-phosphate and indole. We propose that allosteric networks intrinsic to αTS are modulated by the binding of the β-subunit to regulate αTS function. Understanding these long-range amino acid networks in αTS thus gives insight into the coordination of the two active sites within TS. In this study, we have used Ala residues as probes for structural and dynamic changes of αTS throughout its catalytic cycle, in the absence of the β-subunit. Projection analysis of the chemical shift changes by site-specific amino acid substitutions and ligand titrations indicates that αTS has three important conformational states: ligand-free, glyceraldehyde-3-phosphate-bound(like), and the active states. The amino acid networks within these conformations are different, as suggested by chemical shift correlation analysis. In particular, there are long-range connections, only in the active state, between Ala47, which reports on structural and dynamic changes associated with the general acid/base Glu49, and residues within the β2α2 loop, which contains the catalytically important Asp60 residue. These long-range interactions are likely important for coordinating chemical catalysis. In the free state, but not in the active state, there are connections between the β2α2 and β6α6 loops that likely help to coordinate substrate binding. Changes in the allosteric networks are also accompanied by protein dynamic changes. During catalytic turnover, the protein becomes more rigid on the millisecond timescale and the active-site dynamics are driven to a faster nanosecond timescale.

摘要

色氨酸合酶的α 亚基(αTS)催化吲哚-3-甘油磷酸转化为 d-甘油醛-3-磷酸和吲哚。我们提出,β 亚基与 αTS 的结合调节别构网络,从而调节 αTS 的功能。因此,了解 αTS 中的这些长程氨基酸网络可以深入了解 TS 内两个活性位点的协调。在这项研究中,我们使用 Ala 残基作为探针,在没有 β 亚基的情况下,研究 αTS 在整个催化循环中的结构和动态变化。通过对特定氨基酸取代和配体滴定的化学位移变化进行投影分析,表明 αTS 有三个重要的构象状态:无配体、甘油醛-3-磷酸结合(类似)和活性状态。如化学位移相关分析所示,这些构象中的氨基酸网络是不同的。特别是,在活性状态下,Ala47 与 Glu49 之间存在长程连接,Ala47 报告与 Glu49 相关的结构和动力学变化,而 Glu49 是一种通用酸/碱残基;Ala47 与β2α2 环内的残基之间存在长程连接,β2α2 环包含催化上重要的 Asp60 残基。这些长程相互作用可能对协调化学催化很重要。在自由状态下,但不在活性状态下,β2α2 和β6α6 环之间存在连接,这可能有助于协调底物结合。变构网络的变化伴随着蛋白质动态变化。在催化周转期间,蛋白质在毫秒时间尺度上变得更加刚性,并且活性位点的动力学被驱动到更快的纳秒时间尺度。

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