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A Microfluidic Fluorescent Flow Cytometry Capable of Quantifying Cell Sizes and Numbers of Specific Cytosolic Proteins

机译:微流控荧光流式细胞仪能够定量细胞大小和特定胞质蛋白的数量。

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This study presents a microfluidics based cytometry capable of characterizing cell sizes and counting numbers of specific cytosolic proteins where cells were first bound by antibodies labelled with fluorescence and then aspirated into a constriction microchannel in which fluorescent levels were measured. These raw fluorescent pulses were further divided into a rising domain, a stable domain and a declining domain. In addition, antibody solutions with labelled fluorescence were aspirated through the constriction microchannel, yielding curves to translate raw fluorescent levels to protein concentrations. By using key parameters of three domains as well as the calibration curves, cell diameters and the absolute number of β-actins at the single-cell level were quantified as 14.2?±?1.7?μm and 9.62?±?4.29?×?105 (A549, ncell?=?14 242), 13.0?±?2.0?μm and 6.46?±?3.34?×?105 (Hep G2, ncell?=?35 932), 13.8?±?1.9?μm and 1.58?±?0.90?×?106 (MCF 10?A, ncell?=?16 650), and 12.7?±?1.5?μm and 1.09?±?0.49?×?106 (HeLa, ncell?=?26 246). This platform could be further adopted to measure numbers of various cytosolic proteins, providing key insights in proteomics at the single-cell level.
机译:这项研究提出了一种基于微流控的细胞计数法,能够表征细胞大小并计算特定胞质蛋白的数量,其中细胞首先被标记有荧光的抗体结合,然后被吸入收缩的微通道中,在其中测量荧光水平。这些原始荧光脉冲被进一步分为上升域,稳定域和下降域。此外,通过收缩微通道吸出带有标记荧光的抗体溶液,产生将原始荧光水平转化为蛋白质浓度的曲线。通过使用三个域的关键参数以及校准曲线,单细胞水平的细胞直径和β-肌动蛋白的绝对数量被定量为14.2?±?1.7?μm和9.62?±?4.29?×?10 5 (A549,n cell ?=?14 242),13.0?±?2.0?μm和6.46?±?3.34?×?10 5 (Hep G2,n cell ?=?35932),13.8?±?1.9?μm和1.58?±?0.90?×?10 6 (MCF 10 ?A,n cell ?=?16 650)和12.7?±?1.5?μm和1.09?±?0.49?×?10 6 (HeLa,n < sub> cell ?=?26 246)。该平台可进一步用于测量各种胞浆蛋白的数量,从而在单细胞水平上提供蛋白质组学的关键见解。

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