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Rapid and continuous magnetic separation in droplet microfluidic devices

机译:液滴微流控设备中的快速连续磁分离

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We present a droplet microfluidic method to extract molecules of interest from a droplet in a rapid and continuous fashion. We accomplish this by first marginalizing functionalized super-paramagnetic beads within the droplet using a magnetic field, and then splitting the droplet into one droplet containing the majority of magnetic beads and one droplet containing the minority fraction. We quantitatively analysed the factors which affect the efficiency of marginalization and droplet splitting to optimize the enrichment of magnetic beads. We first characterized the interplay between the droplet velocity and the strength of the magnetic field and its effect on marginalization. We found that marginalization is optimal at the midline of the magnet and that marginalization is a good predictor of bead enrichment through splitting at low to moderate droplet velocities. Finally, we focused our efforts on manipulating the splitting profile to improve the enrichment provided by asymmetric splitting. We designed asymmetric splitting forks that employ capillary effects to preferentially extract the bead-rich regions of the droplets. Our strategy represents a framework to optimize magnetic bead enrichment methods tailored to the requirements of specific droplet-based applications. We anticipate that our separation technology is well suited for applications in single-cell genomics and proteomics. In particular, our method could be used to separate mRNA bound to poly-dT functionalized magnetic microparticles from single cell lysates to prepare single-cell cDNA libraries.
机译:我们提出了一种液滴微流体方法,以快速连续的方式从液滴中提取目标分子。为此,我们首先使用磁场将液滴中的功能化超顺磁性微珠边缘化,然后将其分成包含大部分磁珠的一个液滴和包含少数磁珠的一个液滴。我们定量分析了影响边缘化和液滴分裂效率的因素,以优化磁珠的富集。我们首先描述了液滴速度与磁场强度之间的相互作用及其对边缘化的影响。我们发现边缘化在磁体的中线是最佳的,边缘化是通过以低至中等的液滴速度分裂产生的磁珠富集的良好预测指标。最后,我们集中精力处理分裂剖面,以改善非对称分裂提供的富集作用。我们设计了采用毛细管效应的非对称分裂叉,以优先提取液滴的富珠区域。我们的策略代表了一个框架,可以优化磁珠富集方法,以适合基于特定液滴的应用需求。我们期望我们的分离技术非常适合单细胞基因组学和蛋白质组学的应用。特别地,我们的方法可用于从单细胞裂解物中分离结合到聚dT功能化磁性微粒的mRNA,从而制备单细胞cDNA文库。

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