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通过 FLIM 对癌细胞中自体荧光 NAD(P)H、FAD 和色氨酸的氧化还原状态进行分段细胞分析。

Segmented cell analyses to measure redox states of autofluorescent NAD(P)H, FAD & Trp in cancer cells by FLIM.

机构信息

The W.M. Keck Center for Cellular Imaging, University of Virginia, Charlottesville, VA, USA.

Departments of Biology, University of Virginia, Charlottesville, VA, USA.

出版信息

Sci Rep. 2018 Jan 8;8(1):79. doi: 10.1038/s41598-017-18634-x.

Abstract

Multiphoton FLIM microscopy offers many opportunities to investigate processes in live cells, tissue and animal model systems. For redox measurements, FLIM data is mostly published by cell mean values and intensity-based redox ratios. Our method is based entirely on FLIM parameters generated by 3-detector time domain microscopy capturing autofluorescent signals of NAD(P)H, FAD and novel FLIM-FRET application of Tryptophan and NAD(P)H-a2%/FAD-a1% redox ratio. Furthermore, image data is analyzed in segmented cells thresholded by 2 × 2 pixel Regions of Interest (ROIs) to separate mitochondrial oxidative phosphorylation from cytosolic glycolysis in a prostate cancer cell line. Hundreds of data points allow demonstration of heterogeneity in response to intervention, identity of cell responders to treatment, creating thereby different sub-populations. Histograms and bar charts visualize differences between cells, analyzing whole cell versus mitochondrial morphology data, all based on discrete ROIs. This assay method allows to detect subtle differences in cellular and tissue responses, suggesting an advancement over means-based analyses.

摘要

多光子 FLIM 显微镜为研究活细胞、组织和动物模型系统中的过程提供了许多机会。对于氧化还原测量,FLIM 数据主要由细胞平均值和基于强度的氧化还原比发布。我们的方法完全基于通过 3 探测器时域显微镜生成的 FLIM 参数,该显微镜捕获 NAD(P)H、FAD 和色氨酸和 NAD(P)H-a2%/FAD-a1% 氧化还原比的新型 FLIM-FRET 应用的自发荧光信号。此外,图像数据在通过 2x2 像素感兴趣区域 (ROI) 进行分段的细胞中进行分析,以将前列腺癌细胞系中的线粒体氧化磷酸化与细胞质糖酵解分开。数百个数据点允许证明对干预的异质性、对治疗有反应的细胞的身份,从而创建不同的亚群。直方图和条形图可视化细胞之间的差异,分析整个细胞与线粒体形态数据,所有这些都基于离散的 ROI。该测定方法允许检测细胞和组织反应中的细微差异,表明该方法优于基于均值的分析。

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