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Investigating fast enzyme-DNA kinetics using multidimensionalfluorescence imaging and microfluidics

机译:使用多维荧光成像和微流体来研究快速酶-DNA动力学

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We have developed a rapid microfluidic mixing device to image fast kinetics. To verify the performance of the device it was simulated using computational fluid dynamics (CFD) and the results were directly compared to experimental fluorescence lifetime imaging microscopy (FLIM) measurements. The theoretical and measured mixing times of the device were found to be in agreement over a range of flow rates. This mixing device is being developed with the aim of analysing fast enzyme kinetics in the sub-millisecond time domain, which cannot be achieved with conventional macro-stopped flow devices. Here we have studied the binding of a DNA repair enzyme, uracil DNA glycosylase (UDG), to a fluorescently labelled DNA substrate. Bulk phase fluorescence measurements have been used to measure changes on binding: it was found that the fluorescence lifetime increased along with an increase in the polarisation anisotropy and rotational correlation time. Analysis of the same reaction in the microfluidic mixer by CFD enabled us to predict the mixing time of the device to be 46 μs, more than 20 times faster than current stopped-flow techniques. We also demonstrate that it is possible to image UDG-DNA interactions within the micromixer using the signal changes observed from the multidimensional spectrofluorometer.
机译:我们已经开发了一种快速的微流体混合装置,用于图像快速动力学。为了验证使用计算流体动力学(CFD)模拟该设备的性能,结果与实验荧光寿命显微镜(FLIM)测量直接相比。发现该装置的理论和测量混合时间在一系列流速方面是一致的。该混合装置正在开发,目的是分析亚毫秒时域中的快速酶动力学,这不能通过传统的宏观流动装置实现。在这里,我们研究了DNA修复酶,URACIL DNA糖基糖基酶(UDG)的结合,以荧光标记的DNA底物。批量相荧光测量用于测量结合的变化:发现荧光寿命随着偏振各向异性和旋转相关时间的增加而增加。通过CFD分析Microfluidic混合器中的相同反应使我们能够预测装置的混合时间为46μs,比电流停止流动技术快20倍以上。我们还证明,使用从多维光谱荧光计观察到的信号变化,可以使用从多维光谱荧光计观察的信号变化来图像在微混合器内进行图像。

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