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Regulation of ETAA1-mediated ATR activation couples DNA replication fidelity and genome stability

J Cell Biol. 2019; 
Achuthankutty D#, Thakur RS#, Haahr P#, Hoffmann S, Drainas AP, Bizard AH, Weischenfeldt J, Hickson ID, Mailand N,
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Peptide Synthesis Antibodies used in this study included mouse monoclonals to actin (MAB1501; Millipore), cyclin A (611268; BD Biosciences), cyclin B (610220; BD Biosciences), GFP (11814460001; Roche), γ-H2AX (2577, Cell Signaling; and 05-636, Millipore), PICH (04- 1540; Millipore), and vinculin (V9131; Sigma-Aldrich); rabbit polyclonals to Aurora B pT232 (600-401-677; Rockland), Chk1 pS317 (2344; Cell Signaling), FANCD2 (NB100-182; Novus Biologicals), GFP (sc-8334; Santa Cruz), histone H3-pS10 (06-570; Millipore), MCM10 (12251-1-AP; Proteintech Europe), phospho- (Ser) CDK substrate (pSP; 2324; Cell Signaling), and phosphoATM/ATR substrate (pSQ; 9607; Cell Signaling). Polyclonal phospho-specific antibodies to S95 and S111 in human ETAA1 were produced in rabbit (GenScript) using internal ETAA1 peptides as antigens. Get A Quote

摘要

The ATR kinase is a master regulator of the cellular response to DNA replication stress. Activation of ATR relies on dual pathways involving the TopBP1 and ETAA1 proteins, both of which harbor ATR-activating domains (AADs). However, the exact contribution of the recently discovered ETAA1 pathway to ATR signaling in different contexts remains poorly understood. Here, using an unbiased CRISPR-Cas9-based genome-scale screen, we show that the ATR-stimulating function of ETAA1 becomes indispensable for cell fitness and chromosome stability when the fidelity of DNA replication is compromised. We demonstrate that the ATR-activating potential of ETAA1 is controlled by cell cycle- and replication stress-dependent phosph... More

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