Highly Multiplexed, Efficient, and Automated Single‐Cell MicroRNA Sequencing with Digital Microfluidics.

微流控 小RNA 多路复用 吞吐量 计算机科学 计算生物学 单细胞测序 计算机硬件 纳米技术 生物 材料科学 基因 遗传学 无线 突变 电信 外显子组测序
作者
Yingwen Chen,Xuanqun Wang,Na Xing,Yingkun Zhang,Zan Li,Xiaohong Chen,Linfeng Cai,Jia Song,Ren Xu,Chaoyong Yang
出处
期刊:Small methods [Wiley]
卷期号:8 (3) 被引量:3
标识
DOI:10.1002/smtd.202301250
摘要

Abstract Single‐cell microRNA (miRNA) sequencing has allowed for comprehensively studying the abundance and complex networks of miRNAs, which provides insights beyond single‐cell heterogeneity into the dynamic regulation of cellular events. Current benchtop‐based technologies for single‐cell miRNA sequencing are low throughput, limited reaction efficiency, tedious manual operations, and high reagent costs. Here, a highly multiplexed, efficient, integrated, and automated sample preparation platform is introduced for single‐cell miRNA sequencing based on digital microfluidics (DMF), named Hiper‐seq. The platform integrates major steps and automates the iterative operations of miRNA sequencing library construction by digital control of addressable droplets on the DMF chip. Based on the design of hydrophilic micro‐structures and the capability of handling droplets of DMF, multiple single cells can be selectively isolated and subject to sample processing in a highly parallel way, thus increasing the throughput and efficiency for single‐cell miRNA measurement. The nanoliter reaction volume of this platform enables a much higher miRNA detection ability and lower reagent cost compared to benchtop methods. It is further applied Hiper‐seq to explore miRNAs involved in the ossification of mouse skeletal stem cells after bone fracture and discovered unreported miRNAs that regulate bone repairing.
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