Fluorescence-activated droplet sorting (FADS): efficient microfluidic cell sorting based on enzymatic activity

单元格排序 微流控 荧光 生物物理学 分类 化学 介电泳 细胞 纳米技术 生物系统 材料科学 生物化学 生物 计算机科学 物理 量子力学 程序设计语言
作者
Jean‐Christophe Baret,Oliver J. Miller,Valérie Taly,Michaël Ryckelynck,Abdeslam El-Harrak,Lucas Frenz,Christian Rick,Michael L. Samuels,J. Brian Hutchison,Jeremy J. Agresti,Darren R. Link,David A. Weitz,Andrew D. Griffiths
出处
期刊:Lab on a Chip [Royal Society of Chemistry]
卷期号:9 (13): 1850-1850 被引量:945
标识
DOI:10.1039/b902504a
摘要

We describe a highly efficient microfluidic fluorescence-activated droplet sorter (FADS) combining many of the advantages of microtitre-plate screening and traditional fluorescence-activated cell sorting (FACS). Single cells are compartmentalized in emulsion droplets, which can be sorted using dielectrophoresis in a fluorescence-activated manner (as in FACS) at rates up to 2000 droplets s(-1). To validate the system, mixtures of E. coli cells, expressing either the reporter enzyme beta-galactosidase or an inactive variant, were compartmentalized with a fluorogenic substrate and sorted at rates of approximately 300 droplets s(-1). The false positive error rate of the sorter at this throughput was <1 in 10(4) droplets. Analysis of the sorted cells revealed that the primary limit to enrichment was the co-encapsulation of E. coli cells, not sorting errors: a theoretical model based on the Poisson distribution accurately predicted the observed enrichment values using the starting cell density (cells per droplet) and the ratio of active to inactive cells. When the cells were encapsulated at low density ( approximately 1 cell for every 50 droplets), sorting was very efficient and all of the recovered cells were the active strain. In addition, single active droplets were sorted and cells were successfully recovered.
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