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叶绿体前体蛋白在导入过程中与Toc159受体的二聚体界面结合。

Chloroplast Preproteins Bind to the Dimer Interface of the Toc159 Receptor during Import.

作者信息

Chang Jun-Shian, Chen Lih-Jen, Yeh Yi-Hung, Hsiao Chwan-Deng, Li Hsou-Min

机构信息

Molecular and Cell Biology, Taiwan International Graduate Program, Academia Sinica and National Defense Medical Center, Taipei 11529, Taiwan (J.-S.C., H.-m.L.); and.

Institute of Molecular Biology, Academia Sinica, Nankang, Taipei 11529, Taiwan (J.-S.C., L.-J.C., Y.-H.Y., C.-D.H., H.-m.L.).

出版信息

Plant Physiol. 2017 Apr;173(4):2148-2162. doi: 10.1104/pp.16.01952. Epub 2017 Mar 1.

Abstract

Most chloroplast proteins are synthesized in the cytosol as higher molecular weight preproteins and imported via the translocons in the outer (TOC) and inner (TIC) envelope membranes of chloroplasts. Toc159 functions as a primary receptor and directly binds preproteins through its dimeric GTPase domain. As a first step toward a molecular understanding of how Toc159 mediates preprotein import, we mapped the preprotein-binding regions on the Toc159 GTPase domain (Toc159G) of pea () using cleavage by bound preproteins conjugated with the artificial protease FeBABE and cysteine-cysteine cross-linking. Our results show that residues at the dimer interface and the switch II region of Toc159G are in close proximity to preproteins. The mature portion of preproteins was observed preferentially at the dimer interface, whereas the transit peptide was found at both regions equally. Chloroplasts from transgenic plants expressing engineered Toc159 with a cysteine placed at the dimer interface showed increased cross-linking to bound preproteins. Our data suggest that, during preprotein import, the Toc159G dimer disengages and the dimer interface contacts translocating preproteins, which is consistent with a model in which conformational changes induced by dimer-monomer conversion in Toc159 play a direct role in facilitating preprotein import.

摘要

大多数叶绿体蛋白在细胞质中作为分子量更大的前体蛋白合成,并通过叶绿体包膜外膜(TOC)和内膜(TIC)中的转运体导入。Toc159作为主要受体,通过其二聚体GTPase结构域直接结合前体蛋白。作为从分子层面理解Toc159如何介导前体蛋白导入的第一步,我们利用与人工蛋白酶FeBABE偶联的结合前体蛋白的切割以及半胱氨酸-半胱氨酸交联,绘制了豌豆()Toc159 GTPase结构域(Toc159G)上的前体蛋白结合区域。我们的结果表明,Toc159G二聚体界面和开关II区域的残基与前体蛋白紧密相邻。在前体蛋白的成熟部分优先在二聚体界面被观察到,而转运肽在两个区域出现的频率相同。来自表达在二聚体界面处放置了一个半胱氨酸的工程化Toc159的转基因植物的叶绿体,显示出与结合的前体蛋白的交联增加。我们的数据表明,在前体蛋白导入过程中,Toc159G二聚体解离,二聚体界面与转运中的前体蛋白接触,这与一个模型一致,即Toc159中二聚体-单体转化诱导的构象变化在促进前体蛋白导入中起直接作用。

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