Microfluidic single-cell whole-transcriptome sequencing

Aaron M. Streets; Xiannian Zhang; Chen Cao; Yuhong Pang; Xinglong Wu; Liang Xiong; Lu Yang; Yusi Fu; Liang Zhao; Fuchou Tang; Yanyi Huang

doi:10.1073/pnas.1402030111

Edited by Stephen R. Quake, Stanford University, Stanford, CA, and approved April 2, 2014 (received for review February 3, 2014)

Significance

RNA sequencing of single cells enables measurement of biological variation in heterogeneous cellular populations and dissection of transcriptome complexity that is masked in ensemble measurements of gene expression. The low quantity of RNA in a single cell, however, hinders efficient and consistent reverse transcription and amplification of cDNA, limiting accuracy and obscuring biological variation with high technical noise. We developed a microfluidic approach to prepare cDNA from single cells for high-throughput transcriptome sequencing. The microfluidic platform facilitates single-cell manipulation, minimizes contamination, and furthermore, provides improved detection sensitivity and measurement precision, which is necessary for differentiating biological variability from technical noise.

Abstract

Single-cell whole-transcriptome analysis is a powerful tool for quantifying gene expression heterogeneity in populations of cells. Many techniques have, thus, been recently developed to perform transcriptome sequencing (RNA-Seq) on individual cells. To probe subtle biological variation between samples with limiting amounts of RNA, more precise and sensitive methods are still required. We adapted a previously developed strategy for single-cell RNA-Seq that has shown promise for superior sensitivity and implemented the chemistry in a microfluidic platform for single-cell whole-transcriptome analysis. In this approach, single cells are captured and lysed in a microfluidic device, where mRNAs with poly(A) tails are reverse-transcribed into cDNA. Double-stranded cDNA is then collected and sequenced using a next generation sequencing platform. We prepared 94 libraries consisting of single mouse embryonic cells and technical replicates of extracted RNA and thoroughly characterized the performance of this technology. Microfluidic implementation increased mRNA detection sensitivity as well as improved measurement precision compared with tube-based protocols. With 0.2 M reads per cell, we were able to reconstruct a majority of the bulk transcriptome with 10 single cells. We also quantified variation between and within different types of mouse embryonic cells and found that enhanced measurement precision, detection sensitivity, and experimental throughput aided the distinction between biological variability and technical noise. With this work, we validated the advantages of an early approach to single-cell RNA-Seq and showed that the benefits of combining microfluidic technology with high-throughput sequencing will be valuable for large-scale efforts in single-cell transcriptome analysis.

Footnotes

↵¹A.M.S. and X.Z. contributed equally to this work.
↵²Present address: Research Center for Bioengineering and Sensing Technology, University of Science and Technology Beijing, Beijing 100083, China.
↵³To whom correspondence may be addressed. E-mail: zhaoliang2013{at}ustb.edu.cn, tangfuchou{at}pku.edu.cn, or yanyi{at}pku.edu.cn.

Author contributions: A.M.S., L.Z., F.T., and Y.H. designed research; A.M.S., X.Z., C.C., and L.Z. performed research; C.C., Y.P., X.W., L.X., L.Y., Y.F., and F.T. contributed new reagents/analytic tools; A.M.S., X.Z., C.C., L.Z., and Y.H. analyzed data; and A.M.S., X.Z., L.Z., F.T., and Y.H. wrote the paper.
This article is a PNAS Direct Submission.
Data deposition: The data reported in this paper have been deposited in the Gene Expression Omnibus (GEO) database, www.ncbi.nlm.nih.gov/geo (accession no. GSE47835).
This article contains supporting information online at www.pnas.org/lookup/suppl/doi:10.1073/pnas.1402030111/-/DCSupplemental.