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厚层样品中的光抑制:光衰减对基于叶绿素荧光的参数的影响。

Photoinhibition in optically thick samples: Effects of light attenuation on chlorophyll fluorescence-based parameters.

机构信息

Department of Biology and CESAM - Centre for Environmental and Marine Studies, University of Aveiro, Campus de Santiago, 3810-193 Aveiro, Portugal.

Department of Biology, Mount Allison University, Sackville, Canada NB E4L 3G7, Canada.

出版信息

J Theor Biol. 2021 Mar 21;513:110580. doi: 10.1016/j.jtbi.2021.110580. Epub 2021 Jan 12.

Abstract

Oxygenic photoautotrophs are, paradoxically, subject to photoinhibition of their photosynthetic apparatus, in particular one of its major components, the Photosystem II (PSII). Photoinhibition is generalized across species, light conditions and habitats, imposing substantial metabolic costs that lower photosynthetic productivity and constrain the niches of photoautotrophy. As a process driven by light reaching PSII, light attenuation in optically thick samples influences both the actual extent, and the detection, of photoinhibition. Chlorophyll fluorescence is widely used to measure photoinhibition, but fluorescence-based parameters are affected by light attenuation of both downwelling incident radiation traversing the sample to reach PSII, and emitted fluorescence upwelling through the sample. We used modelling, experimental manipulation of within-sample light attenuation, and meta-analysis of published data, to show substantial, differential effects of light attenuation and depth-integration of emitted fluorescence upon measurements of photoinhibition. Numerical simulations and experimental manipulation of light attenuation indicated that PSII photoinactivation tracked using chlorophyll fluorescence can appear to be over three times lower than the inherent cellular susceptibility to photoinactivation, in optically-dense samples such as leaves or biofilms. The meta-analysis of published data showed that this general trend was unknowingly present in the literature, revealing an overall difference of more than five times between optically thick leaves and optically thin cell suspensions. Although fluorescence-based parameters may provide ecophysiologically relevant information for characterizing the sample as a whole, light attenuation and depth integration can vary between samples independently of their intrinsic physiology. They should be used with caution when aiming to quantify in absolute terms inherent photoinhibition-related parameters in optically thick samples.

摘要

好氧光合自养生物具有矛盾性,其光合作用器官,尤其是其中一个主要组件 PSII(Photosystem II)会受到光抑制。光抑制在物种、光照条件和生境中普遍存在,会造成大量代谢成本,降低光合作用生产力,并限制自养生物的生态位。作为由 PSII 接收的光驱动的过程,在光学厚样品中光衰减会影响光抑制的实际程度和检测。叶绿素荧光广泛用于测量光抑制,但基于荧光的参数会受到穿过样品到达 PSII 的下向入射辐射的光衰减以及通过样品上涌的发射荧光的光衰减的影响。我们使用建模、对样品内光衰减的实验操作以及对已发表数据的荟萃分析,表明在测量光抑制时,光衰减和发射荧光的深度积分对测量结果有很大的、不同的影响。数值模拟和光衰减的实验操作表明,使用叶绿素荧光跟踪的 PSII 光失活似乎比在光学密集样品(如叶片或生物膜)中细胞对光失活的固有敏感性低三倍以上。对已发表数据的荟萃分析表明,这种一般趋势在文献中未被察觉,揭示了在光学厚叶片和光学薄细胞悬浮液之间存在超过五倍的总体差异。尽管基于荧光的参数可以为整体特征化提供具有生态生理学意义的信息,但在不考虑其内在生理学的情况下,光衰减和深度积分在不同样品之间可能会有所不同。当试图用绝对术语量化光学厚样品中固有光抑制相关参数时,应谨慎使用它们。

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