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Signal Discrimination Between Fluorescent Proteins in Live Cells by Long-wavelength Optical Modulation

机译:通过长波长光学调制在活细胞中荧光蛋白之间的信号辨别

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摘要

Fluorescent proteins (FPs) have revolutionized molecular and cellular biology; yet, discrimination over cellular autofluorescence, spectral deconvolution, or detection at low concentrations remain challenging problems in many biological applications. By optically depopulating a photoinduced dark state with orange secondary laser co-excitation, the higher-energy green AcGFP fluorescence is dynamically increased. Modulating this secondary laser then modulates the higher-energy, collected fluorescence; enabling its selective detection by removing heterogeneous background from other FPs. Order-of-magnitude reduction in obscuring fluorophore background emission has been achieved in both fixed and live cells. This longwavelength modulation expands the dimensionality to discriminate FP emitters based on dark state lifetimes and enables signal of interest to be recovered by removing heterogeneous background emitter signals. Thus, AcGFP is not only useful for extracting weak signals from systems plagued by high background, but it is a springboard for further FP optimization and utilization for improving sensitivity and selectivity in biological fluorescence imaging.
机译:荧光蛋白(FP)彻底改变了分子和细胞生物学。然而,在许多生物学应用中,对细胞自发荧光,光谱去卷积或低浓度检测的区分仍然是具有挑战性的问题。通过用橙色二次激光共激发使光诱导的暗态减光,可以动态增加高能绿色AcGFP荧光。调制此次级激光,然后调制更高能量的收集到的荧光;通过从其他FP去除异质背景来进行选择性检测。在固定细胞和活细胞中都可以实现使荧光团背景模糊的数量级降低。这种长波长调制扩展了维数,可根据暗态寿命来区分FP发射器,并通过去除异质背景发射器信号来恢复感兴趣的信号。因此,AcGFP不仅可用于从高背景困扰的系统中提取微弱的信号,而且是进一步进行FP优化和利用以改善生物荧光成像灵敏度和选择性的跳板。

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