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高通量液滴数字 PCR。

High-throughput droplet PCR.

机构信息

School of Chemical Engineering and Analytical Sciences, Manchester Interdisciplinary Biocentre, University of Manchester, UK.

出版信息

Methods. 2010 Apr;50(4):277-81. doi: 10.1016/j.ymeth.2010.01.030. Epub 2010 Feb 2.

Abstract

The polymerase chain reaction has facilitated the ready analysis of nucleic acids. A next challenge requires the development of means to unravel the complexity of heterogeneous tissues. This has presented the task of producing massively parallelized quantitative nucleic acid data from the cellular constituents of tissues. The production of aqueous droplets in a two phase flow is shown to be readily and routinely facilitated by miniaturized fluidic devices. Droplets serve as ideal means to package a future generation of PCR, offering an enhanced handling potential by virtue of reactant containment, to concurrently eliminate both contamination and sample loss. This containment also enables the measurement of nucleic acids from populations of cells, or molecules by means of high throughput, single cell analysis. Details are provided for the production of a prototype micro-fluidic device which shows the production and stable flow of droplets which we suggest will be suitable for droplet-based continuous flow micro-fluidic PCR. Suggestions are also made as to the optimal fabrication techniques and the importance of device calibration.

摘要

聚合酶链反应使得核酸的分析变得轻而易举。下一个挑战是需要开发手段来揭示异质组织的复杂性。这就提出了从组织的细胞成分中生成大规模并行化定量核酸数据的任务。两相流中的水滴的产生很容易通过微型化的流体装置来实现。水滴作为包装下一代 PCR 的理想手段,通过反应物的容纳提供了增强的处理潜力,从而同时消除污染和样品损失。这种容纳还使得能够通过高通量单细胞分析对细胞群体或分子中的核酸进行测量。提供了用于生产原型微流控设备的详细信息,该设备显示了水滴的生产和稳定流动,我们建议该水滴适合基于液滴的连续流微流控 PCR。还提出了关于最佳制造技术和设备校准重要性的建议。

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