Cooperative D1 Degradation in the Photosystem II Repair Mediated by Chloroplastic Proteases in Arabidopsis

被引:138
作者
Kato, Yusuke [1 ]
Sun, Xuwu [2 ]
Zhang, Lixin [2 ]
Sakamoto, Wataru [1 ]
机构
[1] Okayama Univ, Inst Plant Sci & Resources, Kurashiki, Okayama 7100046, Japan
[2] Chinese Acad Sci, Inst Bot, Key Lab Photobiol, Photosynth Res Ctr, Beijing 100093, Peoples R China
基金
日本学术振兴会; 日本科学技术振兴机构;
关键词
SYNECHOCYSTIS SP PCC-6803; DEPENDENT CLP PROTEASE; FTSH PROTEASE; THYLAKOID MEMBRANE; LEAF VARIEGATION; IN-VIVO; YELLOW VARIEGATED2; CRYSTAL-STRUCTURE; MUTANTS LACKING; QUALITY-CONTROL;
D O I
10.1104/pp.112.199042
中图分类号
Q94 [植物学];
学科分类号
071001 ;
摘要
Light energy constantly damages photosynthetic apparatuses, ultimately causing impaired growth. Particularly, the sessile nature of higher plants has allowed chloroplasts to develop unique mechanisms to alleviate the irreversible inactivation of photosynthesis. Photosystem II (PSII) is known as a primary target of photodamage. Photosynthetic organisms have evolved the so-called PSII repair cycle, in which a reaction center protein, D1, is degraded rapidly in a specific manner. Two proteases that perform processive or endopeptidic degradation, FtsH and Deg, respectively, participate in this cycle. To examine the cooperative D1 degradation by these proteases, we engaged Arabidopsis (Arabidopsis thaliana) mutants lacking FtsH2 (yellow variegated2 [var2]) and Deg5/Deg8 (deg5 deg8) in detecting D1 cleaved fragments. We detected several D1 fragments only under the var2 background, using amino-terminal or carboxyl-terminal specific antibodies of D1. The appearance of these D1 fragments was inhibited by a serine protease inhibitor and by deg5 deg8 mutations. Given the localization of Deg5/Deg8 on the luminal side of thylakoid membranes, we inferred that Deg5/Deg8 cleaves D1 at its luminal loop connecting the transmembrane helices C and D and that the cleaved products of D1 are the substrate for FtsH. These D1 fragments detected in var2 were associated with the PSII monomer, dimer, and partial disassembly complex but not with PSII supercomplexes. It is particularly interesting that another processive protease, Clp, was up-regulated and appeared to be recruited from stroma to the thylakoid membrane in var2, suggesting compensation for FtsH deficiency. Together, our data demonstrate in vivo cooperative degradation of D1, in which Deg cleavage assists FtsH processive degradation under photoinhibitory conditions.
引用
收藏
页码:1428 / 1439
页数:12
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