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来自蓝细菌的光系统I反应中心中的能量转移与捕获

Energy transfer and trapping in photosystem I reaction centers from cyanobacteria.

作者信息

DiMagno L, Chan C K, Jia Y, Lang M J, Newman J R, Mets L, Fleming G R, Haselkorn R

机构信息

Department of Chemistry, University of Chicago, IL 60637, USA.

出版信息

Proc Natl Acad Sci U S A. 1995 Mar 28;92(7):2715-9. doi: 10.1073/pnas.92.7.2715.

DOI:10.1073/pnas.92.7.2715
PMID:7708712
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC42289/
Abstract

A mutant strain of the cyanobacterium Synechocystis 6803, TolE4B, was constructed by genetic deletion of the protein that links phycobilisomes to thylakoid membranes and of the CP43 and CP47 proteins of photosystem II (PSII), leaving the photosystem I (PSI) center as the sole chromophore in the photosynthetic membranes. Both intact membrane and detergent-isolated samples of PSI were characterized by time-resolved and steady-state fluorescence methods. A decay component of approximately 25 ps dominates (99% of the amplitude) the fluorescence of the membrane sample. This result indicates that an intermediate lifetime is not associated with the intact membrane preparation and the charge separation in PSI is irreversible. The decay time of the detergent-isolated sample is similar. The 600-nm excited steady-state fluorescence spectrum displays a red fluorescence peak at approximately 703 nm at room temperature. The 450-nm excited steady-state fluorescence spectrum is dominated by a single peak around 700 nm without 680-nm "bulk" fluorescence. The experimental results were compared with several computer simulations. Assuming an antenna size of 130 chlorophyll molecules, an apparent charge separation time of approximately 1 ps is estimated. Alternatively, the kinetics could be modeled on the basis of a two-domain antenna for PSI, consistent with the available structural data, each containing approximately 65 chlorophyll a molecules. If excitation can migrate freely within each domain and communication between domains occurs only close to the reaction center, a charge separation time of 3-4 ps is obtained instead.

摘要

通过基因敲除连接藻胆体与类囊体膜的蛋白质以及光系统II(PSII)的CP43和CP47蛋白质,构建了蓝藻集胞藻6803的突变株TolE4B,使得光合膜中光系统I(PSI)中心成为唯一的发色团。完整膜和去污剂分离的PSI样品均采用时间分辨和稳态荧光方法进行表征。膜样品的荧光主要由一个约25皮秒的衰减成分主导(占幅度的99%)。这一结果表明,完整膜制备过程中不存在中间寿命,并且PSI中的电荷分离是不可逆的。去污剂分离样品的衰减时间与之相似。600纳米激发的稳态荧光光谱在室温下于约703纳米处显示一个红色荧光峰。450纳米激发的稳态荧光光谱由一个约700纳米处的单峰主导,没有680纳米的“整体”荧光。实验结果与几种计算机模拟进行了比较。假设天线大小为130个叶绿素分子,则估计表观电荷分离时间约为1皮秒。或者,动力学可以基于PSI的双域天线进行建模,这与现有的结构数据一致,每个域包含约65个叶绿素a分子。如果激发能在每个域内自由迁移,且域间通信仅在靠近反应中心处发生,则得到的电荷分离时间为3 - 4皮秒。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a82d/42289/893139fc13f8/pnas01485-0310-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a82d/42289/893139fc13f8/pnas01485-0310-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a82d/42289/893139fc13f8/pnas01485-0310-a.jpg

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