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光诱导的从光系统I到NADP(+)的电子转移:体内环境的表征与初步模拟

Photo-induced electron transfer from photosystem I to NADP(+): characterization and tentative simulation of the in vivo environment.

作者信息

Moal Gwenaëlle, Lagoutte Bernard

机构信息

Service de Bioenergetique, Biologie Structurale et Mecanismes, Gif sur Yvette, France.

出版信息

Biochim Biophys Acta. 2012 Sep;1817(9):1635-45. doi: 10.1016/j.bbabio.2012.05.015. Epub 2012 Jun 6.

DOI:10.1016/j.bbabio.2012.05.015
PMID:22683536
Abstract

The photoproduction of NADPH in photosynthetic organisms requires the successive or concomitant interaction of at least three proteins: photosystem I (PSI), ferredoxin (Fd) and ferredoxin:NADP(+) oxidoreductase (FNR). These proteins and their surrounding medium have been carefully analysed in the cyanobacterium Synechocystis sp. PCC 6803. A high value of 550mg/ml was determined for the overall solute content of the cell soluble compartment. PSI and Fd are present at similar concentrations, around 500μM, whereas the FNR associated to phycobilisome is about 4 fold less concentrated. Membrane densities of FNR and trimeric PSI have been estimated to 2000 and 2550 per μm(2), respectively. An artificial confinement of Fd to PSI was designed using fused constructs between Fd and PsaE, a peripheral and stroma located PSI subunit. The best covalent system in terms of photocatalysed NADPH synthesis can be equivalent to the free system in a dilute medium. In a macrosolute crowded medium (375mg/ml), this optimized PSI/Fd covalent complex exhibited a huge superiority compared to the free system. This is a likely consequence of restrained diffusion constraints due to the vicinity of two out of the three protein partners. In vivo, Fd is the free partner, but the constant proximity between PSI and the phycobilisome associated FNR creates a similar situation, with two closely associated partners. This organization seems well adapted for an efficient in vivo production of the stable and fast diffusing NADPH.

摘要

光合生物中NADPH的光生合成需要至少三种蛋白质的相继或同时相互作用:光系统I(PSI)、铁氧化还原蛋白(Fd)和铁氧化还原蛋白:NADP(+)氧化还原酶(FNR)。这些蛋白质及其周围介质已在集胞藻属蓝细菌PCC 6803中得到仔细分析。细胞可溶性部分的总溶质含量测定值高达550mg/ml。PSI和Fd的浓度相似,约为500μM,而与藻胆体相关的FNR浓度约低4倍。FNR和三聚体PSI的膜密度估计分别为每μm² 2000和2550。利用Fd与PsaE(一种位于外周和基质的PSI亚基)之间的融合构建体设计了一种将Fd人工限制在PSI上的方法。就光催化NADPH合成而言,最佳的共价系统在稀介质中可等同于游离系统。在大分子溶质拥挤的介质(375mg/ml)中,这种优化的PSI/Fd共价复合物与游离系统相比表现出巨大优势。这可能是由于三个蛋白质伙伴中的两个靠得很近,限制了扩散约束的结果。在体内,Fd是游离伙伴,但PSI与藻胆体相关的FNR之间的持续接近创造了类似的情况,即有两个紧密相关的伙伴。这种组织似乎非常适合在体内高效产生稳定且扩散迅速的NADPH。

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