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光系统II的逐步光抑制。对集胞藻属PCC 6803中反应中心多肽D1的D-E环经修饰的突变体的研究。

Stepwise photoinhibition of photosystem II. Studies with Synechocystis species PCC 6803 mutants with a modified D-E loop of the reaction center polypeptide D1.

作者信息

Mulo P, Laakso S, Mäenpää P, Aro E M

机构信息

Department of Biology, University of Turku, FIN-20014 Turku, Finland.

出版信息

Plant Physiol. 1998 Jun;117(2):483-90. doi: 10.1104/pp.117.2.483.

Abstract

Several mutant strains of Synechocystis sp. PCC 6803 with large deletions in the D-E loop of the photosystem II (PSII) reaction center polypeptide D1 were subjected to high light to investigate the role of this hydrophilic loop in the photoinhibition cascade of PSII. The tolerance of PSII to photoinhibition in the autotrophic mutant DeltaR225-F239 (PD), when oxygen evolution was monitored with 2,6-dichloro-p-benzoquinone and the equal susceptibility compared with control when monitored with bicarbonate, suggested an inactivation of the QB-binding niche as the first event in the photoinhibition cascade in vivo. This step in PD was largely reversible at low light without the need for protein synthesis. Only the next event, inactivation of QA reduction, was irreversible and gave a signal for D1 polypeptide degradation. The heterotrophic deletion mutants DeltaG240-V249 and DeltaR225-V249 had severely modified QB pockets, yet exhibited high rates of 2,6-dichloro-p-benzoquinone-mediated oxygen evolution and less tolerance to photoinhibition than PD. Moreover, the protein-synthesis-dependent recovery of PSII from photoinhibition was impaired in the DeltaG240-V249 and DeltaR225-V249 mutants because of the effects of the mutations on the expression of the psbA-2 gene. No specific sequences in the D-E loop were found to be essential for high rates of D1 polypeptide degradation.

摘要

对集胞藻6803(Synechocystis sp. PCC 6803)的几个突变菌株进行了研究,这些菌株的光系统II(PSII)反应中心多肽D1的D-E环存在大片段缺失,通过高光处理来探究这个亲水性环在PSII光抑制级联反应中的作用。当用2,6-二氯对苯醌监测放氧时,自养突变体DeltaR225-F239(PD)中PSII对光抑制的耐受性,以及用碳酸氢盐监测时与对照相比的同等敏感性,表明QB结合位点的失活是体内光抑制级联反应中的首个事件。在低光条件下,PD中的这一步在很大程度上是可逆的,无需蛋白质合成。只有下一个事件,即QA还原的失活是不可逆的,并发出了D1多肽降解的信号。异养缺失突变体DeltaG240-V249和DeltaR225-V249的QB口袋有严重改变,但2,6-二氯对苯醌介导的放氧速率很高,且对光抑制的耐受性比PD低。此外,由于突变对psbA-2基因表达的影响,DeltaG240-V249和DeltaR225-V249突变体中PSII从光抑制中依赖蛋白质合成的恢复受到损害。在D-E环中未发现对D1多肽高降解速率至关重要的特定序列。

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