首页> 外文期刊>Journal of Photochemistry and Photobiology, B. Biology: Official Journal of the European Society for Photobiology >Photosystem II fluorescence lifetime imaging in avocado leaves: Contributions of the lutein-epoxide and violaxanthin cycles to fluorescence quenching
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Photosystem II fluorescence lifetime imaging in avocado leaves: Contributions of the lutein-epoxide and violaxanthin cycles to fluorescence quenching

机译:鳄梨叶片中的光系统II荧光寿命成像:叶黄素-环氧和紫黄质循环对荧光猝灭的贡献

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Lifetime-resolved imaging measurements of chlorophyll a fluorescence were made on leaves of avocado plants to study whether rapidly reversible ΔpH-dependent (transthylakoid H~+ concentration gradient) thermal energy dissipation (qE) and slowly reversible ApH-independent fluorescence quenching (qI) are modulated by lutein-epoxide and violaxanthin cycles operating in parallel. Under normal conditions (without inhibitors), analysis of the chlorophyll a fluorescence lifetime data revealed two major lifetime pools (1.5 and 0.5 ns) for photosystem II during the ApH build-up under illumination. Formation of the 0.5-ns pool upon illumination was correlated with dark-retention of antheraxanthin and photo-converted lutein in leaves. Interconversion between the 1.5- and 0.5-ns lifetime pools took place during the slow part of the chlorophyll a fluorescence transient: first from 1.5 ns to 0.5 ns in the P-to-S phase, then back from 0.5 ns to 1.5 ns in the S-to-M phase. When linear electron transport and the resulting ApH build-up were inhibited by treatment with 3-(3,4-dichlorophenyl)-1,1-dimethylurea (DCMU), the major fluorescence intensity was due to a 2,2-ns lifetime pool with a minor faster contribution of approximately 0.7 ns. In the presence of DCMU, neither the intensity nor the lifetimes of fluorescence were affected by antheraxanthin and photo-converted lutein. Thus, we conclude that both antheraxanthin and photo-converted lutein are able to enhance ΔpH-dependent qE processes that are associated with the 0.5-ns lifetime pool. However, unlike zeaxanthin, retention of antheraxanthin and photo-converted lutein may not by itself stabilize quenching or cause qI.
机译:在鳄梨植物的叶片上进行终身分辨的叶绿素a荧光成像测量,以研究快速可逆ΔpH依赖性(跨壳类激素H〜+浓度梯度)热能耗散(qE)和缓慢可逆ApH依赖性非荧光猝灭(qI)是否由叶黄素-环氧和紫黄质循环并行调节。在正常条件下(无抑制剂),对叶绿素a荧光寿命数据的分析显示,在光照下ApH积累期间,光系统II的两个主要寿命池(1.5和0.5 ns)。光照后0.5 ns池的形成与花药黄嘌呤的暗度保留和叶中光转化的叶黄素有关。 1.5到0.5 ns寿命池之间的相互转换发生在叶绿素a荧光瞬变的较慢部分:首先在P到S阶段从1.5 ns到0.5 ns,然后在0.5 ns到1.5 ns返回。 S到M阶段。当用3-(3,4-二氯苯基)-1,1-二甲基脲(DCMU)处理抑制线性电子传递和由此产生的ApH积累时,主要的荧光强度归因于2,2-ns的寿命池约0.7 ns的较快贡献。在DCMU存在下,花药黄素和光转化的叶黄素既不会影响荧光的强度,也不会影响其寿命。因此,我们得出的结论是,花药黄素和光转化的叶黄素均能够增强与0.5 ns寿命池相关的ΔpH依赖性qE过程。然而,与玉米黄质不同,保留的是花药黄质和光转化的叶黄素本身不能稳定猝灭或引起qI。

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