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莱茵衣藻的磷酸核酮糖激酶:一种受其半胱氨酸残基束缚的卡尔文循环酶。

Phosphoribulokinase from Chlamydomonas reinhardtii: a Benson-Calvin cycle enzyme enslaved to its cysteine residues.

作者信息

Thieulin-Pardo Gabriel, Remy Thérèse, Lignon Sabrina, Lebrun Régine, Gontero Brigitte

机构信息

Aix-Marseille Université, CNRS, UMR 7281 Laboratoire de Bioénergétique et Ingénierie des Protéines, 13402 Marseille Cedex 20, France.

出版信息

Mol Biosyst. 2015 Apr;11(4):1134-45. doi: 10.1039/c5mb00035a.

DOI:10.1039/c5mb00035a
PMID:25688043
Abstract

Phosphoribulokinase (PRK) in the green alga Chlamydomonas reinhardtii is a finely regulated and well-studied enzyme of the Benson-Calvin cycle. PRK can form a complex with glyceraldehyde-3-phosphate dehydrogenase (GAPDH) and the small chloroplast protein CP12. This study aimed to determine the molecular determinants on PRK involved in the complex and the mechanism of action of a recently described novel regulation of PRK that involves glutathionylation. A combination of mass spectrometry, mutagenesis and activity analyses showed that Cys16, besides its role as the binding site of ATP, was also the site for S-glutathionylation. Previous kinetic analysis of the C55S mutant showed that in the oxidized inactive form of PRK, this residue formed a disulfide bridge with the Cys16 residue. This is the only bridge reported for PRK in the literature. Our data show for the first time that a disulfide bridge between Cys243 and Cys249 on PRK is required to form the PRK-GAPDH-CP12 complex. These results uncover a new mechanism for the PRK-GAPDH-CP12 formation involving a thiol disulfide exchange reaction with CP12 and identify Cys16 of PRK as a target of glutathionylation acting against oxidative stress. Although Cys16 is the key residue involved in binding ATP and acting as a defense against oxidative damage, the formation of the algal ternary complex requires the formation of another disulfide bridge on PRK involving Cys243 and Cys249.

摘要

莱茵衣藻中的磷酸核酮糖激酶(PRK)是本森-卡尔文循环中一种受到精细调控且研究充分的酶。PRK可与甘油醛-3-磷酸脱氢酶(GAPDH)和叶绿体小蛋白CP12形成复合物。本研究旨在确定PRK上参与该复合物形成的分子决定因素,以及最近描述的涉及谷胱甘肽化的PRK新调控机制的作用机制。质谱、诱变和活性分析相结合表明,半胱氨酸16除了作为ATP的结合位点外,也是S-谷胱甘肽化的位点。先前对C55S突变体的动力学分析表明,在氧化的无活性形式的PRK中,该残基与半胱氨酸16残基形成了二硫键。这是文献中报道的PRK唯一的二硫键。我们的数据首次表明,PRK上半胱氨酸243和半胱氨酸249之间的二硫键是形成PRK-GAPDH-CP12复合物所必需的。这些结果揭示了一种涉及与CP12进行硫醇-二硫键交换反应的PRK-GAPDH-CP12形成新机制,并确定PRK的半胱氨酸16是对抗氧化应激的谷胱甘肽化靶点。尽管半胱氨酸16是参与结合ATP和抵御氧化损伤的关键残基,但藻类三元复合物的形成需要PRK上另一个涉及半胱氨酸243和半胱氨酸249的二硫键的形成。

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