4.6 Article

CASB: a concanavalin A-based sample barcoding strategy for single-cell sequencing

期刊

MOLECULAR SYSTEMS BIOLOGY
卷 17, 期 4, 页码 -

出版社

WILEY
DOI: 10.15252/msb.202010060

关键词

CASB; combinatorial sample indexing; sample multiplexing; single‐ cell RNA sequencing; single‐ nucleus ATAC sequencing

资金

  1. Shenzhen Key Laboratory of Gene Regulation and Systems Biology, Shenzhen-Hong Kong Institute of Brain Science-Shenzhen Fundamental Research Institutions [2021SHIBS0002]
  2. Shenzhen Science and Technology Program [KQTD20180411143432337, JCYJ20190809154407564]
  3. National Natural Science Foundation of China [31970601, 31701237, 31900431]

向作者/读者索取更多资源

A Concanavalin A-based sample barcoding strategy (CASB) for single-cell sequencing was reported, showing high efficiency, accuracy in sample assignment, and sensitivity in detecting artifacts. The method demonstrated advantages in tracking transcriptomic dynamics, revealing epigenomic and transcriptomic changes, and scalability.
Sample multiplexing facilitates single-cell sequencing by reducing costs, revealing subtle difference between similar samples, and identifying artifacts such as cell doublets. However, universal and cost-effective strategies are rather limited. Here, we reported a concanavalin A-based sample barcoding strategy (CASB), which could be followed by both single-cell mRNA and ATAC (assay for transposase-accessible chromatin) sequencing techniques. The method involves minimal sample processing, thereby preserving intact transcriptomic or epigenomic patterns. We demonstrated its high labeling efficiency, high accuracy in assigning cells/nuclei to samples regardless of cell type and genetic background, and high sensitivity in detecting doublets by three applications: 1) CASB followed by scRNA-seq to track the transcriptomic dynamics of a cancer cell line perturbed by multiple drugs, which revealed compound-specific heterogeneous response; 2) CASB together with both snATAC-seq and scRNA-seq to illustrate the IFN-gamma-mediated dynamic changes on epigenome and transcriptome profile, which identified the transcription factor underlying heterogeneous IFN-gamma response; and 3) combinatorial indexing by CASB, which demonstrated its high scalability.

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