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Monitoring intracellular oxidative events using dynamic spectral unmixing microscopy

机译:使用动态光谱分解显微镜监测细胞内氧化事件

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摘要

There is increasing interest in using live cell imaging to monitor not just individual intracellular endpoints, but to investigate the interplay between multiple molecular events as they unfold in real time within the cell. A major impediment to simultaneous acquisition of fluorescent signals from multiple probes is that emission spectra of many fluorophores overlap, often with maxima that are only a few nanometers apart. Spectral acquisition of mixed fluorescence signals captured within a dedicated scanning range can be used to quantitatively separate signals into component spectra. We report here the development of a novel live cell application of spectral unmixing for the simultaneous monitoring of intracellular events reported by closely-emitting fluorophores responding dynamically to external stimuli. We validate the performance of dynamic spectral unmixing microscopy (DynSUM) using genetically encoded sensors to simultaneously monitor changes in glutathione redox potential (Egsh) and H2O2 production in living cells exposed to oxidizing and reducing agents. We further demonstrate the utility of the DynSUM approach to observe the relationship between the increases in Egsh and H2O2 generation induced in airway epithelial cells exposed to an environmental electrophile.
机译:使用活细胞成像不仅监测单个细胞内终点,而且研究多个分子事件之间的相互作用,这种事件在细胞内实时展开时,人们越来越感兴趣。同时获取来自多个探针的荧光信号的主要障碍是许多荧光团的发射光谱重叠,通常其最大值仅相距几纳米。在专用扫描范围内捕获的混合荧光信号的光谱采集可用于将信号定量分离为组分光谱。我们在这里报告了一种新的活细胞的应用,其光谱解混技术的发展同时监测由动态响应外部刺激的紧密发射荧光团报告的细胞内事件。我们使用遗传编码的传感器来同时监测暴露于氧化剂和还原剂的活细胞中谷胱甘肽氧化还原电势(Egsh)和H2O2产生的变化,验证动态光谱分解显微镜(DynSUM)的性能。我们进一步证明了DynSUM方法的效用,以观察暴露于环境亲电试剂的气道上皮细胞中Egsh的增加与H2O2生成之间的关系。

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