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  NASC-seq monitors RNA synthesis in single cells.

Hendriks, G. J., Jung, L. A., Larsson, A. J. M., Lidschreiber, M., Forsman, O. A., Lidschreiber, K., et al. (2019). NASC-seq monitors RNA synthesis in single cells. Nature Communications, 10(1): 3138. doi:10.1038/s41467-019-11028-9.

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 Creators:
Hendriks, G. J., Author
Jung, L. A., Author
Larsson, A. J. M., Author
Lidschreiber, M.1, Author           
Forsman, O. A., Author
Lidschreiber, K.1, Author           
Cramer, P.1, Author           
Sandberg, R., Author
Affiliations:
1Department of Molecular Biology, MPI for Biophysical Chemistry, Max Planck Society, ou_1863498              

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 Abstract: Sequencing of newly synthesised RNA can monitor transcriptional dynamics with great sensitivity and high temporal resolution, but is currently restricted to populations of cells. Here, we develop new transcriptome alkylation-dependent single-cell RNA sequencing (NASC-seq), to monitor newly synthesised and pre-existing RNA simultaneously in single cells. We validate the method on pre-labelled RNA, and by demonstrating that more newly synthesised RNA was detected for genes with known high mRNA turnover. Monitoring RNA synthesis during Jurkat T-cell activation with NASC-seq reveals both rapidly up- and down-regulated genes, and that induced genes are almost exclusively detected as newly transcribed. Moreover, the newly synthesised and pre-existing transcriptomes after T-cell activation are distinct, confirming that NASC-seq simultaneously measures gene expression corresponding to two time points in single cells. Altogether, NASC-seq enables precise temporal monitoring of RNA synthesis at single-cell resolution during homoeostasis, perturbation responses and cellular differentiation.

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Language(s): eng - English
 Dates: 2019-07-17
 Publication Status: Published online
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 Rev. Type: Peer
 Identifiers: DOI: 10.1038/s41467-019-11028-9
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Title: Nature Communications
Source Genre: Journal
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Pages: 9 Volume / Issue: 10 (1) Sequence Number: 3138 Start / End Page: - Identifier: -