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Phasor-based single-molecule fluorescence lifetime imaging using a wide-field photon-counting detector

机译:使用广域光子计数探测器的基于相量的单分子荧光寿命成像

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Fluorescence lifetime imaging (FLIM) is a powerful approach to studying the immediate environment of molecules. For example, it is used in biology to study changes in the chemical environment, or to study binding processes, aggregation, and conformational changes by measuring Forster resonance energy transfer (FRET) between donor and acceptor fluorophores. FLIM can be acquired by time-domain measurements (time-correlated single-photon counting) or frequency-domain measurements (with PMT modulation or digital frequency domain acquisition) in a confocal setup, or with wide-field systems (using time-gated cameras). In the best cases, the resulting data is analyzed in terms of multicomponent fluorescence lifetime decays with demanding requirements in terms of signal level (and therefore limited frame rate). Recently, the phasor approach has been proposed as a powerful alternative for fluorescence lifetime analysis of FLIM, ensemble, and single-molecule experiments. Here we discuss the advantages of combining phasor analysis with a new type of FLIM acquisition hardware presented previously, consisting of a high temporal and spatial resolution wide-field single-photon counting device (the H33D detector). Experimental data with live cells and quantum dots will be presented as an illustration of this new approach.
机译:荧光寿命成像(FLIM)是研究分子周围环境的有效方法。例如,它用于生物学研究化学环境的变化,或通过测量供体和受体荧光团之间的Forster共振能量转移(FRET)研究结合过程,聚集和构象变化。可以在共聚焦设置中通过时域测量(与时间相关的单光子计数)或频域测量(与PMT调制或数字频域获取)来获取FLIM,也可以通过广域系统(使用时控相机)来获取FLIM。 )。在最佳情况下,将根据多组分荧光寿命衰减对结果数据进行分析,并根据信号水平(并因此限制帧速率)对要求进行苛刻的分析。近来,相量方法已被提出作为FLIM,集成和单分子实验的荧光寿命分析的有力替代方法。在这里,我们讨论将相量分析与先前介绍的新型FLIM采集硬件相结合的优点,该硬件包括高时间和空间分辨率的宽视场单光子计数设备(H33D检测器)。带有活细胞和量子点的实验数据将作为这种新方法的说明。

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