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莱茵衣藻的荧光寿命成像显微镜:非光化学猝灭突变体及光合抑制剂对叶绿素荧光慢速瞬态的影响

Fluorescence lifetime imaging microscopy of Chlamydomonas reinhardtii: non-photochemical quenching mutants and the effect of photosynthetic inhibitors on the slow chlorophyll fluorescence transient.

作者信息

Holub O, Seufferheld M J, Gohlke C, Heiss G J, Clegg R M

机构信息

Department of Physics, University of Illinois at Urbana-Champaign, 1110 West Green St., Urbana, IL 61801, USA.

出版信息

J Microsc. 2007 May;226(Pt 2):90-120. doi: 10.1111/j.1365-2818.2007.01763.x.

Abstract

Fluorescence lifetime-resolved images of chlorophyll fluorescence were acquired at the maximum P-level and during the slower transient (up to 250 s, including P-S-M-T) in the green photosynthetic alga Chlamydomonas reinhardtii. At the P-level, wild type and the violaxanthin-accumulating mutant npq1 show similar fluorescence intensity and fluorescence lifetime-resolved images. The zeaxanthin-accumulating mutant npq2 displays reduced fluorescence intensity at the P-level (about 25-35% less) and corresponding lifetime-resolved frequency domain phase and modulation values compared to wild type/npq1. A two-component analysis of possible lifetime compositions shows that the reduction of the fluorescence intensity can be interpreted as an increase in the fraction of a short lifetime component. This supports the important photoprotection function of zeaxanthin in photosynthetic samples, and is consistent with the notion of a 'dimmer switch'. Similar, but quantitatively different, behaviour was observed in the intensity and fluorescence lifetime-resolved imaging measurements for cells that were treated with the electron transport inhibitor 3-(3,4-dichlorophenyl)-1,1-dimethyl urea, the efficient PSI electron acceptor methyl viologen and the protonophore nigericin and. Lower fluorescence intensities and lifetimes were observed for all npq2 mutant samples at the P-level and during the slow fluorescence transient, compared to wild type and the npq1 mutant. The fluorescence lifetime-resolved measurements during the slow fluorescence changes after the P level up to 250 s for the wild type and the two mutants, in the presence and absence of the above inhibitors, were analyzed with a graphical procedure (polar plots) to determine lifetime compositions. At higher illumination intensity, wild type and npq1 cells show a rise in fluorescence intensity and corresponding rise in the species concentration of the slow lifetime component after the initial decrease following the P level. This reversal is absent in the npq2 mutant, and for all samples in the presence of the inhibitors. Lifetime heterogeneities were observed in experiments averaged over multiple cells as well as within single cells, and these were followed over time. Cells in the resting state (induced by several hours of darkness), instead of the normal swimming state, show shortened lifetimes. The above results are discussed in terms of a superposition of effects on electron transfer and protonation rates, on the so-called 'State Transitions', and on non-photochemical quenching. Our data indicate two major populations of chlorophyll a molecules, defined by two 'lifetime pools' centred on slower and faster fluorescence lifetimes.

摘要

在绿色光合藻类莱茵衣藻中,于最大P水平以及较慢瞬态过程(长达250秒,包括P - S - M - T)期间采集了叶绿素荧光的荧光寿命分辨图像。在P水平时,野生型和积累紫黄质的突变体npq1显示出相似的荧光强度和荧光寿命分辨图像。与野生型/npq1相比,积累玉米黄质的突变体npq2在P水平时荧光强度降低(约低25 - 35%),且相应的寿命分辨频域相位和调制值也降低。对可能的寿命组成进行的双组分分析表明,荧光强度的降低可解释为短寿命组分比例的增加。这支持了玉米黄质在光合样品中的重要光保护功能,并且与“调光开关”的概念一致。在用电子传递抑制剂3 - (3,4 - 二氯苯基)-1,1 - 二甲基脲、高效PSI电子受体甲基紫精和质子载体尼日利亚菌素处理的细胞的强度和荧光寿命分辨成像测量中,观察到了类似但在数量上不同的行为。与野生型和npq1突变体相比,在P水平以及慢荧光瞬态期间,所有npq2突变体样品的荧光强度和寿命都较低。对于野生型和两个突变体,在存在和不存在上述抑制剂的情况下,在P水平后长达250秒的慢荧光变化期间进行的荧光寿命分辨测量,采用图形程序(极坐标图)进行分析以确定寿命组成。在较高光照强度下,野生型和npq1细胞在P水平后的初始下降之后,荧光强度上升,且慢寿命组分的物种浓度相应上升。这种反转在npq2突变体中不存在,并且在存在抑制剂的情况下所有样品中也不存在。在对多个细胞平均以及单个细胞内进行的实验中都观察到了寿命异质性,并且对其随时间进行了跟踪。处于静止状态(由数小时黑暗诱导)而非正常游动状态的细胞显示出较短的寿命。根据对电子转移和质子化速率、所谓的“状态转换”以及非光化学猝灭的叠加效应来讨论上述结果。我们的数据表明叶绿素a分子存在两个主要群体,由以较慢和较快荧光寿命为中心的两个“寿命池”定义。

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