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拟南芥PsbO2蛋白调节光系统II反应中心D1蛋白的去磷酸化和周转。

The Arabidopsis PsbO2 protein regulates dephosphorylation and turnover of the photosystem II reaction centre D1 protein.

作者信息

Lundin Björn, Hansson Maria, Schoefs Benoît, Vener Alexander V, Spetea Cornelia

机构信息

Division of Cell Biology, Linköping University, SE-581 85 Linköping, Sweden.

出版信息

Plant J. 2007 Feb;49(3):528-39. doi: 10.1111/j.1365-313X.2006.02976.x. Epub 2007 Jan 8.

DOI:10.1111/j.1365-313X.2006.02976.x
PMID:17217465
Abstract

The extrinsic photosystem II (PSII) protein of 33 kDa (PsbO), which stabilizes the water-oxidizing complex, is represented in Arabidopsis thaliana (Arabidopsis) by two isoforms. Two T-DNA insertion mutant lines deficient in either the PsbO1 or the PsbO2 protein were retarded in growth in comparison with the wild type, while differing from each other phenotypically. Both PsbO proteins were able to support the oxygen evolution activity of PSII, although PsbO2 was less efficient than PsbO1 under photoinhibitory conditions. Prolonged high light stress led to reduced growth and fitness of the mutant lacking PsbO2 as compared with the wild type and the mutant lacking PsbO1. During a short period of treatment of detached leaves or isolated thylakoids at high light levels, inactivation of PSII electron transport in the PsbO2-deficient mutant was slowed down, and the subsequent degradation of the D1 protein was totally inhibited. The steady-state levels of in vivo phosphorylation of the PSII reaction centre proteins D1 and D2 were specifically reduced in the mutant containing only PsbO2, in comparison with the mutant containing only PsbO1 or with wild-type plants. Phosphorylation of PSII proteins in vitro proceeded similarly in thylakoid membranes from both mutants and wild-type plants. However, dephosphorylation of the D1 protein occurred much faster in the thylakoids containing only PsbO2. We conclude that the function of PsbO1 in Arabidopsis is mostly in support of PSII activity, whereas the interaction of PsbO2 with PSII regulates the turnover of the D1 protein, increasing its accessibility to the phosphatases and proteases involved in its degradation.

摘要

稳定水氧化复合物的33 kDa外在光系统II(PSII)蛋白(PsbO)在拟南芥中有两种同工型。与野生型相比,缺乏PsbO1或PsbO2蛋白的两个T-DNA插入突变株系生长受阻,且表型不同。尽管在光抑制条件下PsbO2的效率低于PsbO1,但两种PsbO蛋白都能够支持PSII的放氧活性。与野生型和缺乏PsbO1的突变体相比,长期高光胁迫导致缺乏PsbO2的突变体生长和适应性降低。在高光水平下对离体叶片或分离的类囊体进行短时间处理期间,缺乏PsbO2的突变体中PSII电子传递的失活减缓,随后D1蛋白的降解被完全抑制。与仅含有PsbO1的突变体或野生型植物相比,仅含有PsbO2的突变体中PSII反应中心蛋白D1和D2的体内磷酸化稳态水平特异性降低。在来自两种突变体和野生型植物的类囊体膜中,PSII蛋白的体外磷酸化过程相似。然而,仅含有PsbO2的类囊体中D1蛋白的去磷酸化发生得更快。我们得出结论,拟南芥中PsbO1的功能主要是支持PSII活性,而PsbO2与PSII的相互作用调节D1蛋白的周转,增加其对参与其降解的磷酸酶和蛋白酶的可及性。

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