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Coupling bimolecular PARylation biosensors with genetic screens to identify PARylation targets
Authors
A Ashworth
J Campbell
+6 more
DB Krastev
CJ Lord
SJ Pettitt
F Song
SS Stoynov
BE Tanos
Publication date
1 May 2018
Publisher
'Springer Science and Business Media LLC'
Doi
Abstract
Copyright © The Author(s) 2018. Poly (ADP-ribose)ylation is a dynamic protein modification that regulates multiple cellular processes. Here, we describe a system for identifying and characterizing PARylation events that exploits the ability of a PBZ (PAR-binding zinc finger) protein domain to bind PAR with high-affinity. By linking PBZ domains to bimolecular fluorescent complementation biosensors, we developed fluorescent PAR biosensors that allow the detection of temporal and spatial PARylation events in live cells. Exploiting transposon-mediated recombination, we integrate the PAR biosensor en masse into thousands of protein coding genes in living cells. Using these PAR-biosensor “tagged” cells in a genetic screen we carry out a large-scale identification of PARylation targets. This identifies CTIF (CBP80/CBP20-dependent translation initiation factor) as a novel PARylation target of the tankyrase enzymes in the centrosomal region of cells, which plays a role in the distribution of the centrosomal satellites.Breast Cancer Now (BBC070X); Cancer Research UK through Program Grants (CRM059X)
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info:doi/10.1038%2Fs41467-018-...
Last time updated on 11/12/2019
Brunel University Research Archive
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oai:bura.brunel.ac.uk:2438/239...
Last time updated on 07/02/2022