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光抑制会影响光系统II中的非血红素铁中心。

Photoinhibition affects the non-heme iron center in photosystem II.

作者信息

Gleiter H M, Nugent J H, Haag E, Renger G

机构信息

Max-Volmer-Institute for Biophysical Chemistry, Technical University Berlin, Germany.

出版信息

FEBS Lett. 1992 Nov 16;313(1):75-9. doi: 10.1016/0014-5793(92)81188-r.

Abstract

Effects on the PS II acceptor side caused by exposure to strong white light (180 W/m2) of PS II membrane fragments (spinach) at pH 6.5 and 0 degrees C were analyzed by measuring low temperature EPR signals and flash-induced transient changes of the fluorescence quantum yield. The following results were obtained: (a) the extent of the light induced g = 1.9 EPR signal as a measure of photochemical Fe2+QA- formation declines with progressing photoinhibition. The half-life of this effect is independent of the absence or presence of an exogenous electron acceptor during the photoinhibitory treatment; (b) in samples photoinhibited in the absence of an electron acceptor and subsequently incubated with K3[Fe(CN)6] in the dark, the extent of the g = 8 EPR signal (reflecting the oxidized Fe3+ form of the endogenous non-heme iron center) and of the flash-induced change of the fluorescence yield (as a measure of fast electron transfer from QA- to Fe3+ after the first flash; [see (1992) Photosynth. Res. 31, 113-126] exhibits the same dependence on photoinhibition time as the g = 1.9 EPR signal; (c) in samples photoinhibited in the presence of an exogenous electron acceptor, the signals reflecting Fe(3+)-formation and fast electron transfer from QA- to Fe3+ decline faster than the g = 1.9 EPR signal. These results provide for the first time direct evidence that the endogenous non-heme iron center located between QA and QB is susceptible to modifications by light stress. The implications of this finding will be discussed.

摘要

通过测量低温EPR信号和闪光诱导的荧光量子产率的瞬态变化,分析了在pH 6.5和0℃条件下,菠菜PS II膜片段暴露于强光(180 W/m²)时对PS II受体侧的影响。得到以下结果:(a)作为光化学Fe²⁺QA⁻形成量度的光诱导g = 1.9 EPR信号的程度随着光抑制的进行而下降。这种效应的半衰期与光抑制处理期间是否存在外源电子受体无关;(b)在无电子受体存在下光抑制的样品,随后在黑暗中与K₃[Fe(CN)₆]孵育,g = 8 EPR信号(反映内源性非血红素铁中心的氧化Fe³⁺形式)的程度以及闪光诱导的荧光产率变化(作为第一次闪光后QA⁻向Fe³⁺快速电子转移的量度;[见(1992年)《光合作用研究》31,113 - 126])与g = 1.9 EPR信号对光抑制时间表现出相同的依赖性;(c)在有外源电子受体存在下光抑制的样品中,反映Fe(3+)形成和QA⁻向Fe³⁺快速电子转移的信号比g = 1.9 EPR信号下降得更快。这些结果首次提供了直接证据,表明位于QA和QB之间的内源性非血红素铁中心易受光胁迫的修饰。将讨论这一发现的意义。

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