Droplet-based Single-cell Total RNA-seq Reveals Differential Non-Coding Expression and Splicing Patterns during Mouse Development

Author:

Salmen Fredrik,De Jonghe JoachimORCID,Kaminski Tomasz S.ORCID,Alemany AnnaORCID,Parada GuillermoORCID,Verity-Legg Joe,Yanagida AyakaORCID,Kohler Timo N.ORCID,Battich Nicholas,van den Brekel FlorisORCID,Ellermann Anna L.ORCID,Arias Alfonso MartinezORCID,Nichols JenniferORCID,Hemberg MartinORCID,Hollfelder FlorianORCID,van Oudenaarden AlexanderORCID

Abstract

ABSTRACTIn recent years, single-cell transcriptome sequencing has revolutionized biology, allowing for the unbiased characterization of cellular subpopulations. However, most methods amplify the termini of polyadenylated transcripts capturing only a small fraction of the total cellular transcriptome. This precludes the detection of many long non-coding, short non-coding and non-polyadenylated protein-coding transcripts. Additionally, most workflows do not sequence the full transcript hindering the analysis of alternative splicing. We therefore developed VASA-seq to detect the total transcriptome in single cells. VASA-seq is compatible with both plate-based formats and droplet microfluidics. We applied VASA-seq to over 30,000 single cells in the developing mouse embryo during gastrulation and early organogenesis. The dynamics of the total single-cell transcriptome result in the discovery of novel cell type markers many based on non-coding RNA, an in vivo cell cycle analysis and an improved RNA velocity characterization. Moreover, it provides the first comprehensive analysis of alternative splicing during mammalian development.

Publisher

Cold Spring Harbor Laboratory

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