Droplet-Based Microfluidics: Formation, Detection and Analytical Characterization

Sammer-Ul Hassan, Xunli Zhang, X. Niu
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引用次数: 2

Abstract

Microfluidics has been a critical technology for over two decades to study and manipulate fluids in microstructures. It has the potential to provide smart microdevices, which can change how modern biology, chemical synthesis, and point-of-care diagnostics are performed [1]. Microfluidics offers many advantages, including minute quantities of samples and reagents, compact ability, low cost, rapid, high resolution and sensitive analyses. Continuous microfluidics typically involves single-phase flow in microchannels, although traditionally liquids with macromolecules, microparticles or cells are also categorized in continuous microfluidics. Due to the small Reynolds number (0.01-100), Re= ULρ/μ, the flow is laminar in microfluidic devices, where U, L, ρ and μ stand for the velocity of the flow, the diameter of the capillary, density and viscosity of fluid flow respectively [2]. Continuous microfluidics suffers from less efficient and slow mixing in microchannels, molecular contamination of loss on the surface of the channels and Taylor dispersion of molecules alongside the microchannels. The Taylor dispersion leads the parabolic velocity movement of liquid inside microchannels, which involves two velocity regimes, i.e. at the walls and in the middle of the microchannel [2,3].
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基于液滴的微流体:形成、检测和分析表征
二十多年来,微流控技术一直是研究和操纵微结构流体的关键技术。它有可能提供智能微型设备,从而改变现代生物学、化学合成和即时诊断的执行方式。微流体提供了许多优点,包括微量的样品和试剂,紧凑性,低成本,快速,高分辨率和敏感的分析。连续微流体通常涉及微通道中的单相流动,尽管传统上带有大分子、微粒或细胞的液体也被归类为连续微流体。由于微流控装置的雷诺数较小(0.01 ~ 100),Re= ULρ/μ,因此微流控装置内的流动为层流,其中U、L、ρ和μ分别代表流动速度、毛细管直径、流体密度和粘度[2]。连续微流体存在微通道中混合效率较低、速度较慢、通道表面损失的分子污染以及微通道旁分子的泰勒分散等问题。泰勒色散导致液体在微通道内的抛物线速度运动,涉及两个速度区,即微通道壁面和微通道中部[2,3]。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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