Using single nuclei for RNA-seq to capture the transcriptome of postmortem neurons

转录组 cDNA文库 生物 核糖核酸 互补DNA 计算生物学 RNA序列 深度测序 基因组文库 基因 分子生物学 基因表达 遗传学 基序列 基因组
作者
Suguna Rani Krishnaswami,Rashel V. Grindberg,Mark Novotny,Pratap Venepally,Benjamin Lacar,Kunal Bhutani,Sara B. Linker,Son Pham,Jennifer A. Erwin,Jeremy A. Miller,Rebecca D. Hodge,James K. McCarthy,Martijn J. E. Kelder,Jamison McCorrison,Brian D. Aevermann,Francisco Díez‐Fuertes,Richard H. Scheuermann,Jun Lee,Ed S. Lein,Nicholas J. Schork
出处
期刊:Nature Protocols [Nature Portfolio]
卷期号:11 (3): 499-524 被引量:486
标识
DOI:10.1038/nprot.2016.015
摘要

A protocol is described for sequencing the transcriptome of a cell nucleus. Nuclei are isolated from specimens and sorted by FACS, cDNA libraries are constructed and RNA-seq is performed, followed by data analysis. Some steps follow published methods (Smart-seq2 for cDNA synthesis and Nextera XT barcoded library preparation) and are not described in detail here. Previous single-cell approaches for RNA-seq from tissues include cell dissociation using protease treatment at 30 °C, which is known to alter the transcriptome. We isolate nuclei at 4 °C from tissue homogenates, which cause minimal damage. Nuclear transcriptomes can be obtained from postmortem human brain tissue stored at -80 °C, making brain archives accessible for RNA-seq from individual neurons. The method also allows investigation of biological features unique to nuclei, such as enrichment of certain transcripts and precursors of some noncoding RNAs. By following this procedure, it takes about 4 d to construct cDNA libraries that are ready for sequencing.
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