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High-Throughput Microfluidic Labyrinth for the Label-free Isolation of Circulating Tumor Cells.高通量微流控迷宫用于无标记循环肿瘤细胞的分离。
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Multicolor Fluorescence Detection-Based Microfluidic Device for Single-Cell Metabolomics: Simultaneous Quantitation of Multiple Small Molecules in Primary Liver Cells.基于多色荧光检测的单细胞代谢组学微流控装置:在原代肝细胞中同时定量多种小分子。
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利用微流控热凝胶电泳中的焦耳加热来创建用于细胞富集的可逆屏障。

Harnessing Joule heating in microfluidic thermal gel electrophoresis to create reversible barriers for cell enrichment.

机构信息

Department of Chemistry, Wayne State University, Detroit, Michigan, USA.

出版信息

Electrophoresis. 2021 Jun;42(11):1238-1246. doi: 10.1002/elps.202000379. Epub 2021 Feb 26.

DOI:10.1002/elps.202000379
PMID:33570796
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC8178196/
Abstract

Gel electrophoresis is a ubiquitous bioanalytical technique used to characterize the components of cell lysates. However, analyses of bulk lysates sacrifice detection sensitivity because intracellular biomolecules become diluted, and the liberation of proteases and nucleases can degrade target analytes. This report describes a method to enrich cells directly within a microfluidic gel as a first step toward online measurement of trace intracellular biomolecules with minimal dilution and degradation. Thermal gels were employed as the gel matrix because they can be reversibly converted between liquid and solid phases as a function of temperature. Rather than fabricate costly heating elements into devices to control temperature-and thus the phase of the gel-Joule heating was used instead. Adjoining regions of liquid-phase and solid-phase gel were formed within microfluidic channels by selectively inducing localized Joule heat. Cells migrated through the liquid gel but could not enter the solid gel-accumulating at the liquid-solid gel boundary-whereas small molecule contaminants passed through to waste. Barriers were then liquified on-demand by removing Joule heat to collect the purified, non-lysed cells for downstream analyses. Using voltage-controlled Joule heating to regulate the phase of thermal gels is an innovative approach to facilitate in-gel cell enrichment in low-cost microfluidic devices.

摘要

凝胶电泳是一种普遍使用的生物分析技术,用于分析细胞裂解物的成分。然而,对大量裂解物的分析会牺牲检测灵敏度,因为细胞内生物分子被稀释,而且蛋白酶和核酸酶的释放会降解目标分析物。本报告描述了一种在微流控凝胶中直接富集细胞的方法,作为在线测量痕量细胞内生物分子的第一步,该方法最小化了稀释和降解。热凝胶被用作凝胶基质,因为它们可以根据温度在液相和固相之间可逆转换。为了控制温度并由此控制凝胶的相,没有将昂贵的加热元件制造到设备中,而是使用了焦耳加热。通过有选择地诱导局部焦耳热,在微流道中形成液相和固相凝胶相邻区域。细胞通过液相凝胶迁移,但不能进入固相凝胶——而是聚集在固液凝胶边界处——而小分子污染物则通过进入废物。然后通过去除焦耳热按需使屏障液化,以收集纯化的、未裂解的细胞进行下游分析。使用电压控制的焦耳加热来调节热凝胶的相是一种创新的方法,可以在低成本微流控设备中促进凝胶内细胞富集。