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体内光合系统的皮秒荧光

Picosecond fluorescence from photosynthetic systems in vivo.

作者信息

Searle G F, Tredwell C J

出版信息

Ciba Found Symp. 1978(61):257-81. doi: 10.1002/9780470720431.ch14.

Abstract

Picosecond time-resolved fluorescence emission from the pigments of intact photosynthetic systems and isolated pigment-protein fractions has been used to probe the mechanism of energy transfer and the organization of the pigments. The fluorescence kinetics of chlorophyll and the phycobilins of the red alga, Porphyridium cruentum, are governed by time-dependent kinetics, but the observed time dependence of the chlorophyll a fluorescence decay from dark-adapted Chlorella pyrenoidosa and spinach sub-chloroplast fractions is still open to conjecture. In contrast to the green plants containing only chlorophyll and carotenoids, Porphyridium shows distinct emission bands for each the pigments in the transfer sequence. The rate of energy transfer in vivo has the empirical form: dS/dt = -1/2S At-1/2, where S is the excited-state population of the donor pigment and A is the overall rate of energy transfer to the acceptor pigment. The kinetic analysis can describe closely the observed fluorescence risetimes and lifetimes of the photosynthetic pigments of Porphyridium. The extremely rapid rates of energy transfer, determined by this treatment, imply that exciton migration within each pigment bed of the phycobilisome is less extensive than in the chlorophyll-antenna systems. Changes in the fluorescence yield and decay kinetics of chlorophyll a and allophycocyanin in vivo can be induced at high excitation intensities by exciton-exciton annihilation.

摘要

利用完整光合系统和分离的色素 - 蛋白质组分中色素的皮秒时间分辨荧光发射来探究能量转移机制和色素的组织方式。红球藻(Porphyridium cruentum)中叶绿素和藻胆素的荧光动力学受时间依赖性动力学支配,但对于黑暗适应的小球藻(Chlorella pyrenoidosa)和菠菜亚叶绿体组分中叶绿素a荧光衰减的时间依赖性观察结果仍有待推测。与仅含有叶绿素和类胡萝卜素的绿色植物不同,红球藻在能量转移序列中的每种色素都显示出明显的发射带。体内能量转移速率具有经验公式:dS/dt = -1/2S At-1/2,其中S是供体色素的激发态群体,A是向受体色素的总能量转移速率。动力学分析可以紧密描述观察到的红球藻光合色素的荧光上升时间和寿命。通过这种处理确定的极快能量转移速率意味着藻胆体每个色素层内的激子迁移比叶绿素天线系统中的激子迁移范围更小。在高激发强度下,激子 - 激子湮灭可诱导体内叶绿素a和别藻蓝蛋白的荧光产率和衰减动力学发生变化。

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