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在水裂解反应受到抑制后,光系统II中D1蛋白的光依赖降解加速。

Light-dependent degradation of the D1 protein in photosystem II is accelerated after inhibition of the water splitting reaction.

作者信息

Jegerschöld C, Virgin I, Styring S

机构信息

Department of Biochemistry, University of Stockholm, Sweden.

出版信息

Biochemistry. 1990 Jul 3;29(26):6179-86. doi: 10.1021/bi00478a010.

DOI:10.1021/bi00478a010
PMID:2207066
Abstract

Strong illumination of oxygen-evolving organisms inhibits the electron transport through photosystem II (photoinhibition). In addition the illumination leads to a rapid turnover of the D1 protein in the reaction center of photosystem II. In this study the light-dependent degradation of the D1 reaction center protein and the light-dependent inhibition of electron-transport reactions have been studied in thylakoid membranes in which the oxygen evolution has been reversibly inhibited by Cl- depletion. The results show that Cl(-)-depleted thylakoid membranes are very vulnerable to damage induced by illumination. Both the D1 protein and the inhibition of the oxygen evolution are 15-20 times more sensitive to illumination than in control thylakoid membranes. The presence, during the illumination, of the herbicide 3-(3,4-dichlorophenyl)-1,1-dimethylurea (DCMU) prevented both the light-dependent degradation of the D1 protein and the inhibition of the electron transport. The protection exerted by DCMU is seen only in Cl(-)-depleted thylakoid membranes. These observations lead to the proposal that continuous illumination of Cl(-)-depleted thylakoid membranes generates anomalously long-lived, highly oxidizing radicals on the oxidizing side of photosystem II, which are responsible for the light-induced protein damage and inhibition. The presence of DCMU during the illumination prevents the formation of these radicals, which explains the protective effects of the herbicide. It is also observed that in Cl(-)-depleted thylakoid membranes, oxygen evolution (measured after the readdition of Cl-) is inhibited before electron transfer from diphenylcarbazide to dichlorophenolindophenol.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

对放氧生物的强光照射会抑制通过光系统II的电子传递(光抑制)。此外,光照会导致光系统II反应中心的D1蛋白快速周转。在本研究中,在通过去除Cl-使放氧可逆抑制的类囊体膜中,研究了D1反应中心蛋白的光依赖性降解和电子传递反应的光依赖性抑制。结果表明,去除Cl-的类囊体膜极易受到光照诱导的损伤。D1蛋白和放氧抑制对光照的敏感性比对照类囊体膜高15 - 20倍。在光照期间存在除草剂3-(3,4-二氯苯基)-1,1-二甲基脲(DCMU)可防止D1蛋白的光依赖性降解和电子传递的抑制。DCMU的保护作用仅在去除Cl-的类囊体膜中可见。这些观察结果表明,对去除Cl-的类囊体膜持续光照会在光系统II的氧化侧产生异常长寿命、高氧化性的自由基,这些自由基导致光诱导的蛋白质损伤和抑制。光照期间DCMU的存在可防止这些自由基的形成,这解释了除草剂的保护作用。还观察到,在去除Cl-的类囊体膜中,在电子从二苯卡巴肼转移到二氯酚靛酚之前,放氧(在重新添加Cl-后测量)就受到抑制。(摘要截短于250字)

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