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Systematic Method for the Kinetic Modeling of Temporally Resolved Hyperspectral Microscope Images of Fluorescently Labeled Cells

机译:荧光标记细胞的暂时分辨高光谱显微镜图像动力学建模的系统方法

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摘要

In this paper we report the application of a novel method for fitting kinetic models to temporally resolved hyperspectral images of fluorescently labeled cells to mathematically resolve pure-component spatial images, pure-component spectra, and pure-component reaction profiles. The method is demonstrated on one simulated image and two experimental cell images, including human embryonic kidney cells (HEK 293) and human A549 pulmonary type II epithelial cells. In both cell images, inhibitor kappa B kinase alpha (IKKalpha) and mitochondrial antiviral signaling protein (MAVS) were labeled with green and yellow fluorescent protein, respectively. Kinetic modeling was performed on the compressed images by using a separable least squares method. A combination of several first-order decays were needed to adequately model the photobleaching processes for each fluorophore observed in these images, consistent with the hypothesis that each fluorophore was found in several different environments within the cells. Numerous plausible mechanisms for kinetic modeling of the photobleaching processes in these images were tested and a method for selecting the most parsimonious and statistically sufficient model was used to prepare spatial maps of each fluorophore.
机译:在本文中,我们报告了一种新颖的动力学模型拟合方法的应用,该模型适用于荧光标记细胞的时间分辨高光谱图像,以数学方式解析纯组分的空间图像,纯组分的光谱和纯组分的反应曲线。该方法在一张模拟图像和两张实验细胞图像上得到了证明,其中包括人类胚胎肾细胞(HEK 293)和人类A549肺II型上皮细胞。在两个细胞图像中,分别用绿色和黄色荧光蛋白标记抑制剂κB激酶α(IKK alpha )和线粒体抗病毒信号蛋白(MAVS)。通过使用可分离的最小二乘法对压缩图像进行动力学建模。需要几个一级衰减的组合来充分模拟在这些图像中观察到的每个荧光团的光致漂白过程,这与在细胞内的几种不同环境中发现每个荧光团的假设相一致。测试了这些图像中光漂白过程动力学建模的许多合理机制,并使用了一种选择最简约和统计学上足够的模型的方法来准备每个荧光团的空间图。

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    《Applied Spectroscopy》 |2009年第3期|261-270|共10页
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