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Phasor approach to fluorescence lifetime microscopy distinguishes different metabolic states of germ cells in a live tissue

机译:荧光寿命显微镜的相量法可区分活组织中生殖细胞的不同代谢状态

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摘要

We describe a label-free imaging method to monitor stem-cell metabolism that discriminates different states of stem cells as they differentiate in living tissues. In this method we use intrinsic fluorescence biomarkers and the phasor approach to fluorescence lifetime imaging microscopy in conjunction with image segmentation, which we use to introduce the concept of the cell phasor. In live tissues we are able to identify intrinsic fluorophores, such as collagen, retinol, retinoic acid, porphyrin, flavins, and free and bound NADH. We have exploited the cell phasor approach to detect a trend in metabolite concentrations along the main axis of the Caenorhabditis elegans germ line. This trend is consistent with known changes in metabolic states during differentiation. The cell phasor approach to lifetime imaging provides a label-free, fit-free, and sensitive method to identify different metabolic states of cells during differentiation, to sense small changes in the redox state of cells, and may identify symmetric and asymmetric divisions and predict cell fate. Our method is a promising noninvasive optical tool for monitoring metabolic pathways during differentiation or disease progression, and for cell sorting in unlabeled tissues.
机译:我们描述了一种无标签的成像方法来监测干细胞代谢,该方法可区分干细胞在活组织中的分化状态。在这种方法中,我们使用固有的荧光生物标记物和相量方法对荧光寿命成像显微镜进行图像分割,并使用图像分割来介绍细胞相量的概念。在活组织中,我们能够鉴定出固有的荧光团,例如胶原蛋白,视黄醇,视黄酸,卟啉,黄素以及游离和结合的NADH。我们已经利用细胞相量方法来检测秀丽隐杆线虫种系主轴上代谢物浓度的趋势。这种趋势与分化过程中代谢状态的已知变化是一致的。用于生命周期成像的细胞相量方法提供了一种无标记,无拟合且敏感的方法,可在分化过程中识别细胞的不同代谢状态,以感知细胞氧化还原状态的细微变化,并可以识别对称和不对称分裂并预测细胞命运。我们的方法是一种有前途的无创光学工具,可用于监测分化或疾病进展过程中的代谢途径以及未标记组织中的细胞分选。

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