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Creating a cell line suitable for investigation into the ADAR1 role in hepatitis C virus replication

abstract in conference proceedings
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Author
Roučová, KristinaORCiD Profile - 0000-0001-8081-4538WoS Profile - P-9197-2017
Vopálenský, VáclavORCiD Profile - 0000-0002-4858-4645WoS Profile - Q-6418-2017Scopus Profile - 8575785500
Mašek, TomášORCiD Profile - 0000-0001-8732-0565WoS Profile - Q-4636-2017Scopus Profile - 6603131017
Del Llano, Edgar
Provazník, Jan
Landry, Jonathan J.M.
Azeveda, Nayara
Ehler, Edvard
Kubů, Martin
Beneš, Vladimír
Pospíšek, MartinORCiD Profile - 0000-0002-9490-8911WoS Profile - A-9100-2008Scopus Profile - 6602708932
Šímová, Šárka

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Publication date
2023
Published in
Czech Chemical Society Symposium Series
Volume / Issue
21 (5)
ISBN / ISSN
ISSN: 2336-7202
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  • Faculty of Science
Abstract
Adenosine deaminases acting on RNA (ADAR) perform the adenosine to inosine (A-to-I) type of editing. Out of the three human ADAR proteins, ADAR1 is responsible for the majority of A-to-I editing of dsRNA outside the brain. By introducing I into the RNA sequence, thereby altering the base pairing in the region, or by its sheer dsRNA binding activity, ADAR1 can influence miRNA processing, alternative splicing, nuclear export, degradation or protection of RNA molecules (as reviewed in 1). On top of the variety of effects ADAR1 can have on a particular RNA, ADAR1 editing itself has been shown to be influenced heavily by the cell type. In recent years, studies on particular ADAR1 effects have relied mainly on RNA-seq experiments and knock-down cell line assays.
Keywords
RNA, ADAR1
Permanent link
https://hdl.handle.net/20.500.14178/2062
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Full text of this result is licensed under: Creative Commons Uveďte původ 4.0 International

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