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Flavodiiron Protein Flv2/Flv4-Related Photoprotective Mechanism Dissipates Excitation Pressure of PSII in Cooperation with Phycobilisomes in Cyanobacteria

机译:Flavodiiron蛋白Flv2 / Flv4相关的光保护机制与蓝藻中的藻胆体协同消散PSII的激发压力。

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摘要

Oxygenic photosynthesis evolved with cyanobacteria, the ancestors of plant chloroplasts. The highly oxidizing chemistry of water splitting required concomitant evolution of efficient photoprotection mechanisms to safeguard the photosynthetic machinery. The role of flavodiiron proteins (FDPs), originally called A-type flavoproteins or Flvs, in this context has only recently been appreciated. Cyanobacterial FDPs constitute a specific protein group that evolved to protect oxygenic photosynthesis. There are four FDPs in Synechocystis sp. PCC 6803 (Flv1 to Flv4). Two of them, Flv2 and Flv4, are encoded by an operon together with a Sll0218 protein. Their expression, tightly regulated by CO2 levels, is also influenced by changes in light intensity. Here we describe the overexpression of the flv4-2 operon in Synechocystis sp. PCC 6803 and demonstrate that it results in improved photochemistry of PSII. The flv4-2/OE mutant is more resistant to photoinhibition of PSII and exhibits a more oxidized state of the plastoquinone pool and reduced production of singlet oxygen compared with control strains. Results of biophysical measurements indicate that the flv4-2 operon functions in an alternative electron transfer pathway from PSII, and thus alleviates PSII excitation pressure by channeling up to 30% of PSII-originated electrons. Furthermore, intact phycobilisomes are required for stable expression of the flv4-2 operon genes and for the Flv2/Flv4 heterodimer-mediated electron transfer mechanism. The latter operates in photoprotection in a complementary way with the orange carotenoid protein-related nonphotochemical quenching. Expression of the flv4-2 operon and exchange of the D1 forms in PSII centers upon light stress, on the contrary, are mutually exclusive photoprotection strategies among cyanobacteria.
机译:氧合光合作用随着蓝细菌的发展而发展,蓝细菌是植物叶绿体的祖先。水分解的高度氧化化学需要伴随着有效的光保护机制的发展,以保护光合作用机制。在这种情况下,最初被称为A型黄素蛋白或Flvs的黄素二铁蛋白(FDP)的作用直到最近才被人们所认识。蓝藻FDP构成了一个特定的蛋白质基团,可以进化为保护氧的光合作用。蓝藻属中有四个FDP。 PCC 6803(Flv1至Flv4)。 Flv2和Flv4这两个是由操纵子与Sll0218蛋白一起编码的。它们的表达受到二氧化碳水平的严格控制,也受到光强度变化的影响。在这里,我们描述了Synechocystis sp。中flv4-2操纵子的过表达。 PCC 6803并证明它可改善PSII的光化学性能。与对照菌株相比,flv4-2 / OE突变体对PSII的光抑制具有更强的抵抗力,并且质体醌库的氧化态更强,单线态氧的产生减少。生物物理测量结果表明,flv4-2操纵子在PSII的另一种电子转移途径中起作用,并因此通过引导多达30%的PSII起源的电子来缓解PSII激发压力。此外,完整的藻胆体对于flv4-2操纵子基因的稳定表达和Flv2 / Flv4异二聚体介导的电子转移机制是必需的。后者以与橙色类胡萝卜素蛋白相关的非光化学淬灭的互补方式在光保护中起作用。相反,flv4-2操纵子的表达和PSII中D1形式的交换以光应力为中心,这是蓝细菌之间相互排斥的光保护策略。

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