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肺炎链球菌色氨酸合酶α亚基 TIM 桶中的 3D 结构域交换。

3D domain swapping in the TIM barrel of the α subunit of Streptococcus pneumoniae tryptophan synthase.

机构信息

Midwest Center for Structural Genomics, X-ray Science Division, Argonne National Laboratory, Argonne, IL 60439, USA.

Center for Biocrystallographic Research, Institute of Bioorganic Chemistry, Polish Academy of Sciences, Poznan, Poland.

出版信息

Acta Crystallogr D Struct Biol. 2020 Feb 1;76(Pt 2):166-175. doi: 10.1107/S2059798320000212. Epub 2020 Jan 31.

DOI:10.1107/S2059798320000212
PMID:32038047
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7008512/
Abstract

Tryptophan synthase catalyzes the last two steps of tryptophan biosynthesis in plants, fungi and bacteria. It consists of two protein chains, designated α and β, encoded by trpA and trpB genes, that function as an αββα complex. Structural and functional features of tryptophan synthase have been extensively studied, explaining the roles of individual residues in the two active sites in catalysis and allosteric regulation. TrpA serves as a model for protein-folding studies. In 1969, Jackson and Yanofsky observed that the typically monomeric TrpA forms a small population of dimers. Dimerization was postulated to take place through an exchange of structural elements of the monomeric chains, a phenomenon later termed 3D domain swapping. The structural details of the TrpA dimer have remained unknown. Here, the crystal structure of the Streptococcus pneumoniae TrpA homodimer is reported, demonstrating 3D domain swapping in a TIM-barrel fold for the first time. The N-terminal domain comprising the H0-S1-H1-S2 elements is exchanged, while the hinge region corresponds to loop L2 linking strand S2 to helix H2'. The structural elements S2 and L2 carry the catalytic residues Glu52 and Asp63. As the S2 element is part of the swapped domain, the architecture of the catalytic apparatus in the dimer is recreated from two protein chains. The homodimer interface overlaps with the α-β interface of the tryptophan synthase αββα heterotetramer, suggesting that the 3D domain-swapped dimer cannot form a complex with the β subunit. In the crystal, the dimers assemble into a decamer comprising two pentameric rings.

摘要

色氨酸合酶催化植物、真菌和细菌中色氨酸生物合成的最后两个步骤。它由两条蛋白质链组成,分别命名为α和β,由 trpA 和 trpB 基因编码,作为一个 αββα 复合物发挥作用。色氨酸合酶的结构和功能特征已得到广泛研究,解释了两个活性部位中单个残基在催化和变构调节中的作用。TrpA 是蛋白质折叠研究的模型。1969 年,Jackson 和 Yanofsky 观察到通常单体的 TrpA 形成一小部分二聚体。二聚化被假设通过单体链的结构元件的交换发生,后来称为 3D 结构域交换。TrpA 二聚体的结构细节仍然未知。本文报道了肺炎链球菌 TrpA 同源二聚体的晶体结构,首次证明了 TIM 桶折叠中的 3D 结构域交换。包含 H0-S1-H1-S2 元件的 N 端结构域被交换,而铰链区对应于连接 S2 链和 H2'螺旋的 L2 环。S2 和 L2 结构元件携带催化残基 Glu52 和 Asp63。由于 S2 元件是交换结构域的一部分,因此二聚体中催化装置的结构是由两条蛋白质链重建的。同源二聚体界面与色氨酸合酶 αββα 杂四聚体的 α-β 界面重叠,表明 3D 结构域交换的二聚体不能与β亚基形成复合物。在晶体中,二聚体组装成包含两个五聚体环的十聚体。

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