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光系统I的PsaC亚基为快速向铁氧化还原蛋白转移电子提供了一个必需的赖氨酸残基。

The PsaC subunit of photosystem I provides an essential lysine residue for fast electron transfer to ferredoxin.

作者信息

Fischer N, Hippler M, Sétif P, Jacquot J P, Rochaix J D

机构信息

Department of Molecular Biology, University of Geneva, Geneva, Switzerland.

出版信息

EMBO J. 1998 Feb 16;17(4):849-58. doi: 10.1093/emboj/17.4.849.

Abstract

PsaC is the stromal subunit of photosystem I (PSI) which binds the two terminal electron acceptors FA and FB. This subunit resembles 2[4Fe-4S] bacterial ferredoxins but contains two additional sequences: an internal loop and a C-terminal extension. To gain new insights into the function of the internal loop, we used an in vivo degenerate oligonucleotide-directed mutagenesis approach for analysing this region in the green alga Chlamydomonas reinhardtii. Analysis of several psaC mutants affected in PSI function or assembly revealed that K35 is a main interaction site between PsaC and ferredoxin (Fd) and that it plays a key role in the electrostatic interaction between Fd and PSI. This is based upon the observation that the mutations K35T, K35D and K35E drastically affect electron transfer from PSI to Fd, as measured by flash-absorption spectroscopy, whereas the K35R change has no effect on Fd reduction. Chemical cross-linking experiments show that Fd interacts not only with PsaD and PsaE, but also with the PsaC subunit of PSI. Replacement of K35 by T, D, E or R abolishes Fd cross-linking to PsaC, and cross-linking to PsaD and PsaE is reduced in the K35T, K35D and K35E mutants. In contrast, replacement of any other lysine of PsaC does not alter the cross-linking pattern, thus indicating that K35 is an interaction site between PsaC and its redox partner Fd.

摘要

PsaC是光系统I(PSI)的基质亚基,它结合两个末端电子受体FA和FB。该亚基类似于2[4Fe-4S]细菌铁氧化还原蛋白,但包含两个额外的序列:一个内部环和一个C末端延伸。为了深入了解内部环的功能,我们使用体内简并寡核苷酸定向诱变方法分析莱茵衣藻中该区域。对几个在PSI功能或组装上受到影响的psaC突变体的分析表明,K35是PsaC与铁氧化还原蛋白(Fd)之间的主要相互作用位点,并且它在Fd与PSI之间的静电相互作用中起关键作用。这是基于以下观察结果:通过闪光吸收光谱法测量,K35T、K35D和K35E突变极大地影响了从PSI到Fd的电子转移,而K35R变化对Fd还原没有影响。化学交联实验表明,Fd不仅与PsaD和PsaE相互作用,还与PSI的PsaC亚基相互作用。用T、D、E或R取代K35消除了Fd与PsaC的交联,并且在K35T、K35D和K35E突变体中与PsaD和PsaE的交联减少。相反,替换PsaC的任何其他赖氨酸不会改变交联模式,因此表明K35是PsaC与其氧化还原伙伴Fd之间的相互作用位点。

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