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D1-R323、D1-N322、D1-D319、D1-H304 突变对嗜热古菌聚球藻 PSII 功能的影响。

Effects of mutations of D1-R323, D1-N322, D1-D319, D1-H304 on the functioning of photosystem II in Thermosynechococcus vulcanus.

机构信息

Photosynthesis Research Center, Key Laboratory of Photobiology, Institute of Botany, Chinese Academy of Sciences, No. 20, Nanxincun, Xiangshan, Beijing, 100093, China.

University of Chinese Academy of Sciences, Yuquan Rd, Shijingshan District, Beijing, 100049, China.

出版信息

Photosynth Res. 2022 May;152(2):193-206. doi: 10.1007/s11120-022-00920-z. Epub 2022 May 3.

Abstract

Photosystem II (PSII) has a number of hydrogen-bonding networks connecting the manganese cluster with the lumenal bulk solution. The structure of PSII from Thermosynechococcus vulcanus (T. vulcanus) showed that D1-R323, D1-N322, D1-D319 and D1-H304 are involved in one of these hydrogen-bonding networks located in the interfaces between the D1, CP43 and PsbV subunits. In order to investigate the functions of these residues in PSII, we generated seven site-directed mutants D1-R323A, D1-R323E, D1-N322R, D1-D319L, D1-D319R, D1-D319Y and D1-H304D of T. vulcanus and examined the effects of these mutations on the growth and functions of the oxygen-evolving complex. The photoautotrophic growth rates of these mutants were similar to that of the wild type, whereas the oxygen-evolving activities of the mutant cells were decreased differently to 63-91% of that of the wild type at pH 6.5. The mutant cells showed a higher relative activity at higher pH region than the wild type cells, suggesting that higher pH facilitated proton egress in the mutants. In addition, oxygen evolution of thylakoid membranes isolated from these mutants showed an apparent decrease compared to that of the cells. This is due to the loss of PsbU during purification of the thylakoid membranes. Moreover, PsbV was also lost in the PSII core complexes purified from the mutants. Taken together, D1-R323, D1-N322, D1-D319 and D1-H304 are vital for the optimal function of oxygen evolution and functional binding of extrinsic proteins to PSII core, and may be involved in the proton egress pathway mediated by Y.

摘要

光系统 II(PSII)有许多氢键连接锰簇与腔室的整体溶液。来自硫还原球菌(Thermosynechococcus vulcanus,T. vulcanus)的 PSII 结构表明,D1-R323、D1-N322、D1-D319 和 D1-H304 参与了位于 D1、CP43 和 PsbV 亚基之间界面的这些氢键网络之一。为了研究这些残基在 PSII 中的功能,我们生成了七个硫还原球菌的定点突变体 D1-R323A、D1-R323E、D1-N322R、D1-D319L、D1-D319R、D1-D319Y 和 D1-H304D,并研究了这些突变对放氧复合物生长和功能的影响。这些突变体的光自养生长速率与野生型相似,而在 pH 6.5 时,突变细胞的放氧活性降低到野生型的 63-91%。与野生型细胞相比,突变细胞在较高 pH 区域的相对活性更高,表明较高的 pH 促进了突变体中的质子外排。此外,从这些突变体中分离的类囊体膜的氧气释放显示出与细胞相比明显降低。这是由于在类囊体膜的纯化过程中 PsbU 的丢失。此外,在从突变体中纯化的 PSII 核心复合物中也丢失了 PsbV。综上所述,D1-R323、D1-N322、D1-D319 和 D1-H304 对于氧气释放的最佳功能和外在蛋白与 PSII 核心的功能结合至关重要,并且可能参与了由 Y 介导的质子外排途径。

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