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Resolving the contribution of the uncoupled phycobilisomes to cyanobacterial pulse-amplitude modulated (PAM) fluorometry signals

机译:解决未偶联的藻胆体对蓝细菌脉冲幅度调制(PAM)荧光检测信号的影响

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摘要

Pulse-amplitude modulated (PAM) fluorometry is extensively used to characterize photosynthetic organisms on the slow time-scale (1–1000 s). The saturation pulse method allows determination of the quantum yields of maximal (FM) and minimal fluorescence (F0), parameters related to the activity of the photosynthetic apparatus. Also, when the sample undergoes a certain light treatment during the measurement, the fluorescence quantum yields of the unquenched and the quenched states can be determined. In the case of cyanobacteria, however, the recorded fluorescence does not exclusively stem from the chlorophyll a in photosystem II (PSII). The phycobilins, the pigments of the cyanobacterial light-harvesting complexes, the phycobilisomes (PB), also contribute to the PAM signal, and therefore, F0 and FM are no longer related to PSII only. We present a functional model that takes into account the presence of several fluorescent species whose concentrations can be resolved provided their fluorescence quantum yields are known. Data analysis of PAM measurements on in vivo cells of our model organism Synechocystis PCC6803 is discussed. Three different components are found necessary to fit the data: uncoupled PB (PBfree), PB–PSII complexes, and free PSI. The free PSII contribution was negligible. The PBfree contribution substantially increased in the mutants that lack the core terminal emitter subunits allophycocyanin D or allophycocyanin F. A positive correlation was found between the amount of PBfree and the rate constants describing the binding of the activated orange carotenoid protein to PB, responsible for non-photochemical quenching.Electronic supplementary materialThe online version of this article (doi:10.1007/s11120-015-0141-x) contains supplementary material, which is available to authorized users.
机译:脉冲幅度调制(PAM)荧光测定法已广泛用于在较慢的时间尺度(1–1000 s)上表征光合生物。饱和脉冲法可以确定最大光量子(FM)和最小荧光光(F0)的量子产率,这是与光合作用装置的活性有关的参数。同样,当样品在测量过程中经过一定的光处理时,可以确定未淬灭态和淬灭态的荧光量子产率。但是,对于蓝细菌而言,记录的荧光并不仅仅来自光系统II(PSII)中的叶绿素a。藻胆素是蓝细菌光捕获复合物的色素,藻胆体(PB)也有助于PAM信号,因此F0和FM不再仅与PSII相关。我们提出了一种功能模型,该模型考虑了几种荧光物质的存在,只要已知其荧光量子产率,即可解决其浓度问题。讨论了对我们模型有机体集胞藻PCC6803的体内细胞进行PAM测量的数据分析。发现需要三种不同的成分来拟合数据:未耦合的PB(PBfree),PB-PSII复合体和游离的PSI。 PSII的免费捐款微不足道。在缺乏核心末端发射子亚基别藻蓝蛋白D或别藻蓝蛋白F的突变体中,PBfree的贡献显着增加。发现PBfree的量与描述活化的橙色类胡萝卜素蛋白与PB结合的速率常数之间呈正相关,这与非-光化学淬灭电子补充材料本文的在线版本(doi:10.1007 / s11120-015-0141-x)包含补充材料,授权用户可以使用。

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