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Multiplexing Fluorescence Anisotropy Using Frequency Encoding

机译:频率编码复用荧光各向异性

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In this report, a method to multiplex fluorescence anisotropy measurements is described using frequency encoding. As a demonstration of the method, simultaneous competitive immunoassays for insulin and glucagon were performed by measuring the ratio of bound and free Cy5-insulin and FITC-glucagon in the presence,of their respective antibodies. A vertically polarized 635 nm laser was pulsed at 73 Hz and used to excite CyS-insulin, while a vertically polarized 488 nm laser pulsed at 137 Hz excited FITC-glucagon. The total emission was split into parallel and perpendicular polarizations and collected onto separate photomultiplier tubes. The signals from each channel were demodulated using a fast Fourier transform, resolving the contributions from each fluorophore. Anisotropy calculations were carried out using the magnitude of the peaks in the frequency domain. The method produced the expected shape of the calibration curves with limits of detection of 0.6 and S nM for insulin and glucagon, respectively. This methodology could readily be expanded to other biological systems and further multiplexed to monitor increased numbers of analytes.
机译:在此报告中,描述了使用频率编码复用荧光各向异性测量的方法。作为该方法的证明,在存在各自抗体的情况下,通过测量结合的和游离的Cy5-胰岛素和FITC-胰高血糖素的比率,对胰岛素和胰高血糖素进行同时竞争性免疫测定。垂直偏振的635 nm激光以73 Hz的脉冲脉冲被用来激发CyS胰岛素,而垂直偏振的488 nm激光以137 Hz的脉冲激发FITC-胰高血糖素。总发射分为平行和垂直极化,并收集到单独的光电倍增管上。使用快速傅立叶变换对来自每个通道的信号进行解调,以解析每个荧光团的贡献。使用频域中峰值的大小进行各向异性计算。该方法产生了预期的校准曲线形状,胰岛素和胰高血糖素的检出限分别为0.6和S nM。这种方法可以很容易地扩展到其他生物系统,并且可以进一步复用以监视增加数量的分析物。

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