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Bayesian analysis of fluorescence lifetime imaging data

机译:呼叫荧光寿命成像数据分析

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Fluorescence Lifetime Imaging (FLIM) is an intensity independent and sensitive optical technique for studying the cellular environment but its accuracy is often compromised when low photon counts are available for analysis. We have developed a photon-by-photon Bayesian analysis method targeted at the accurate analysis of low photon count time-domain FLIM data collected using Time Correlated Single Photon Counting (TCSPC). Parameter estimates obtained with our mono-exponential Bayesian analysis compare favorably with those using maximum likelihood, least squares, and phasor analysis, offering robust estimation with greater precision at very low total photon counts, particularly in the presence of significant background levels. Details of the Bayesian implementation are presented alongside results of mono-exponential analysis of both real and synthetic data. We demonstrate that for low photon count data, obtained by imaging human epithelial carcinoma cells expressing cdc42-GFP, Bayesian analysis estimates the green fluorescent protein (GFP) lifetime to a level of accuracy not obtained using maximum likelihood estimation or other techniques. These results are echoed by the analysis of synthetic decay data incorporating a 10% uniform background, with our Bayesian analysis routines yielding lifetime estimates within an accuracy of 20% with about 50 counts. This level of precision is not achieved with maximum likelihood nor phasor analysis techniques with fewer than 100 counts.
机译:荧光寿命成像(FLIM)是一种强度独立和敏感的光学技术,用于研究蜂窝环境,但是当低光子计数可用于分析时,其精度通常受到损害。我们开发了一种逐个光子贝叶斯分析方法,其针对使用时间相关的单光子计数(TCSPC)收集的低光子计数时域flim数据的精确分析。通过我们的单指数贝叶斯分析获得的参数估计与使用最大可能性,最小二乘和分析分析的人相比,提供鲁棒估计,在极低的总光子计数下具有更高的精度,特别是在存在显着的背景水平。贝叶斯实施的细节与实际和合成数据的单通指数分析一起呈现。我们证明,对于通过表达CDC42-GFP的人的上皮癌细胞获得的低光子计数数据,贝叶斯分析估计绿色荧光蛋白(GFP)寿命以使用最大似然估计或其他技术获得的精度水平。这些结果通过分析包含10%均匀背景的合成衰减数据的分析来回应,我们的贝叶斯分析常规产生寿命估计的寿命估计为20%,约50计数。由于最大可能性和相分分析技术,而不是少于100计数的相分析技术,不会实现这种精度。

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