首页> 外文会议>Advanced Photon Counting Techniques; Proceedings of SPIE-The International Society for Optical Engineering; vol.6372 >Application of novel low-intensity non-scanning fluorescence lifetime imaging microscopy for monitoring excited state dynamics in individual chloroplasts and living cells of photosynthetic organisms
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Application of novel low-intensity non-scanning fluorescence lifetime imaging microscopy for monitoring excited state dynamics in individual chloroplasts and living cells of photosynthetic organisms

机译:新型低强度非扫描荧光寿命成像显微镜在监测光合生物单个叶绿体和活细胞中激发态动态中的应用

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摘要

Picosecond fluorescence lifetime imaging microscopy (FLIM) provides a most valuable tool to analyze the primary processes of photosynthesis in individual cells and chloroplasts of living cells. In order to obtain correct lifetimes of the excited states, the peak intensity of the exciting laser pulses as well as the average intensity has to be sufficiently low to avoid distortions of the kinetics by processes such as singlet-singlet annihilation, closing of the reaction centers or photoinhibition. In the present study this requirement is achieved by non-scanning wide-field FLIM based on time- and space-correlated single-photon counting (TSCSPC) using a novel microchannel plate photomultiplier with quadrant anode (QA-MCP) that allows parallel acquisition of time-resolved images under minimally invasive low-excitation conditions. The potential of the wide-field TSCSPC method is demonstrated by presenting results obtained from measurements of the fluorescence dynamics in individual chloroplasts of moss leaves and living cells of the chlorophyll d-containing cyanobacterium Acaryochloris marina.
机译:皮秒荧光寿命成像显微镜(FLIM)提供了最有价值的工具,用于分析单个细胞和活细胞的叶绿体中光合作用的主要过程。为了获得正确的激发态寿命,激发激光脉冲的峰值强度以及平均强度必须足够低,以避免诸如单重态单an灭,关闭反应中心之类的过程造成动力学失真。或光抑制。在本研究中,这一要求是通过使用具有象限阳极的新型微通道平板光电倍增管(QA-MCP),基于时间和空间相关的单光子计数(TSCSPC),通过对时间和空间相关的单光子计数的非扫描宽视野FLIM来实现的,微创低激发条件下的时间分辨图像。通过呈现从对苔藓叶片的单个叶绿体和含叶绿素d的蓝藻滨海蓝藻的活细胞中的荧光动力学进行测量获得的结果,证明了宽域TSCSPC方法的潜力。

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