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鉴定参与拟南芥光驯化的光系统 II 磷酸酶。

Identification of a photosystem II phosphatase involved in light acclimation in Arabidopsis.

机构信息

Department of Botany and Plant Biology, University of Geneva, 30 quai Ernest Ansermet, 1211 Geneva 4, Switzerland.

出版信息

Plant Cell. 2012 Jun;24(6):2596-609. doi: 10.1105/tpc.112.095703. Epub 2012 Jun 15.

Abstract

Reversible protein phosphorylation plays a major role in the acclimation of the photosynthetic apparatus to changes in light. Two paralogous kinases phosphorylate subsets of thylakoid membrane proteins. STATE TRANSITION7 (STN7) phosphorylates LHCII, the light-harvesting antenna of photosystem II (PSII), to balance the activity of the two photosystems through state transitions. STN8, which is mainly involved in phosphorylation of PSII core subunits, influences folding of the thylakoid membranes and repair of PSII after photodamage. The rapid reversibility of these acclimatory responses requires the action of protein phosphatases. In a reverse genetic screen, we identified the chloroplast PP2C phosphatase, PHOTOSYSTEM II CORE PHOSPHATASE (PBCP), which is required for efficient dephosphorylation of PSII proteins. Its targets, identified by immunoblotting and mass spectrometry, largely coincide with those of the kinase STN8. The recombinant phosphatase is active in vitro on a synthetic substrate or on isolated thylakoids. Thylakoid folding is affected in the absence of PBCP, while its overexpression alters the kinetics of state transitions. PBCP and STN8 form an antagonistic kinase and phosphatase pair whose substrate specificity and physiological functions are distinct from those of STN7 and the counteracting phosphatase PROTEIN PHOSPHATASE1/THYLAKOID-ASSOCIATED PHOSPHATASE38, but their activities may overlap to some degree.

摘要

可逆蛋白质磷酸化在光合作用器官对光变化的适应中起着主要作用。两个类似的激酶磷酸化类囊体膜蛋白的亚群。状态转换 7(STN7)磷酸化 LHCII,即光系统 II(PSII)的光捕获天线,通过状态转换来平衡两个光系统的活性。STN8 主要参与 PSII 核心亚基的磷酸化,影响类囊体膜的折叠和 PSII 在光损伤后的修复。这些适应性反应的快速可逆性需要蛋白质磷酸酶的作用。在反向遗传筛选中,我们鉴定了叶绿体 PP2C 磷酸酶 PHOTOSYSTEM II CORE PHOSPHATASE(PBCP),它是 PSII 蛋白有效去磷酸化所必需的。通过免疫印迹和质谱鉴定的其靶标,在很大程度上与激酶 STN8 的靶标重合。重组磷酸酶在体外合成底物或分离的类囊体上具有活性。在缺乏 PBCP 的情况下,类囊体折叠受到影响,而其过表达改变了状态转换的动力学。PBCP 和 STN8 形成一个拮抗的激酶和磷酸酶对,其底物特异性和生理功能与 STN7 和拮抗磷酸酶 PROTEIN PHOSPHATASE1/THYLAKOID-ASSOCIATED PHOSPHATASE38 不同,但它们的活性可能在一定程度上重叠。

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