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来自集胞藻PCC 6803野生型及光系统II突变体的析氧光系统II制剂。

Oxygen-evolving photosystem II preparation from wild type and photosystem II mutants of Synechocystis sp. PCC 6803.

作者信息

Kirilovsky D L, Boussac A G, van Mieghem F J, Ducruet J M, Sétif P R, Yu J J, Vermaas W F, Rutherford A W

机构信息

Département de Biologie, URA CNRS 1290, Gif-sur-Yvette, France.

出版信息

Biochemistry. 1992 Feb 25;31(7):2099-107. doi: 10.1021/bi00122a030.

DOI:10.1021/bi00122a030
PMID:1311205
Abstract

We present here a simple and rapid method which allows relatively large quantities of oxygen-evolving photosystem II- (PS-II-) enriched particles to be obtained from wild-type and mutants of the cyanobacterium Synechocystis 6803. This method is based on that of Burnap et al. [Burnap, R., Koike, H., Sotiropoulou, G., Sherman, L. A., & Inoue, Y. (1989) Photosynth. Res. 22, 123-130] but is modified so that the whole preparation, from cells to PS-II particles, is achieved in 10 h and involves only one purification step. The purified preparation exhibits a 5-6-fold increase of O2-evolution activity on a chlorophyll basis over the thylakoids. The ratio of PS-I to PS-II is about 0.14:1 in the preparation. The secondary quinone electron acceptor, QB, is present in this preparation as demonstrated by thermoluminescence studies. These PS-II particles are well-suited to spectroscopic studies as demonstrated by the range of EPR signals arising from components of PS-II that are easily detectable. Among the EPR signals presented are those from a formal S3-state, attributed to an oxidized amino acid interacting magnetically with the Mn complex in Ca(2+)-deficient PS-II particles, and from S2 modified by the replacement of Ca2+ by Sr2+. Neither of these signals has been previously reported in cyanobacteria. Their detection under these conditions indicates a similar lesion caused by Ca2+ depletion in both plants and cyanobacteria. The protocol has also been applied to mutants which have site-specific changes in PS-II. Data are presented on mutants having changes on the electron donor (Y160F) and electron acceptor (G215W) side of the D2 polypeptide.

摘要

我们在此展示一种简单快速的方法,该方法能从集胞藻6803蓝细菌的野生型和突变体中获得相对大量的富含放氧光系统II(PS-II)的颗粒。此方法基于Burnap等人的方法[Burnap, R., Koike, H., Sotiropoulou, G., Sherman, L. A., & Inoue, Y. (1989) Photosynth. Res. 22, 123 - 130],但经过改进,使得从细胞到PS-II颗粒的整个制备过程能在10小时内完成,并且只涉及一步纯化。纯化后的制剂在叶绿素基础上的放氧活性比类囊体提高了5 - 6倍。制剂中PS-I与PS-II的比例约为0.14:1。热发光研究表明,二级醌电子受体QB存在于该制剂中。这些PS-II颗粒非常适合进行光谱研究,这一点从PS-II各组分产生的一系列易于检测的电子顺磁共振(EPR)信号中得到了证明。所呈现的EPR信号包括来自形式上的S3态的信号,该信号归因于在缺钙的PS-II颗粒中一个氧化的氨基酸与锰复合物发生磁相互作用;以及来自用Sr2+取代Ca2+而修饰的S2的信号。这两种信号此前在蓝细菌中均未被报道过。在这些条件下对它们的检测表明,植物和蓝细菌中因Ca2+耗竭而导致的损伤相似。该方案也已应用于PS-II发生位点特异性变化的突变体。文中给出了关于D2多肽电子供体(Y160F)和电子受体(G215W)侧发生变化的突变体的数据。

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