Wide-field photon counting fluorescence lifetime imaging microscopy: application to photosynthesizing systems

被引:0
|
作者
Zdeněk Petrášek
Hann-Jörg Eckert
Klaus Kemnitz
机构
[1] Technische Universität Dresden,Biophysics group, Biotechnologisches Zentrum
[2] Technische Universität Berlin,Max
[3] Europhoton GmbH,Volmer
[4] Berlin,Laboratory for Biophysical Chemistry
来源
Photosynthesis Research | 2009年 / 102卷
关键词
Fluorescence lifetime imaging; FLIM; Time-correlated single photon counting; QA detector; Photosynthesis; Chlorophyll;
D O I
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中图分类号
学科分类号
摘要
Fluorescence lifetime imaging microscopy (FLIM) is a technique that visualizes the excited state kinetics of fluorescence molecules with the spatial resolution of a fluorescence microscope. We present a scanningless implementation of FLIM based on a time- and space-correlated single photon counting (TSCSPC) method employing a position-sensitive quadrant anode detector and wide-field illumination. The standard time-correlated photon counting approach leads to picosecond temporal resolution, making it possible to resolve complex fluorescence decays. This allows parallel acquisition of time-resolved images of biological samples under minimally invasive low-excitation conditions (<10mW/cm2). In this way unwanted photochemical reactions induced by high excitation intensities and distorting the decay kinetics are avoided. Comparably low excitation intensities are practically impossible to achieve with a conventional laser scanning microscope, where focusing of the excitation beam into a tight spot is required. Therefore, wide-field FLIM permits to study Photosystem II (PS II) in a way so far not possible with a laser scanning microscope. The potential of the wide-field TSCSPC method is demonstrated by presenting FLIM measurements of the fluorescence dynamics of photosynthetic systems in living cells of the chlorophyll d-containing cyanobacterium Acaryochloris marina.
引用
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页码:157 / 168
页数:11
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