2017
DOI: 10.1038/cr.2017.147
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TDP2, TOP2, and SUMO: what is ZATT about?

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Cited by 21 publications
(14 citation statements)
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“…However, DSB repair was completed in patient cells within 8–24 hours, consistent with the established existence of alternative, nuclease-dependent mechanisms for repair of TOP2-induced DSBs in human cells. 4 , 13 , 14 Similar results were observed in human A549 cells in which TDP2 was mutated by CRISPR/Cas9 gene editing, confirming the importance of TDP2 for repair of TOP2-induced DSBs ( figure 3B ). More importantly, complementation of 850-BR cells with expression construct encoding recombinant human TDP2 restored normal rates of nuclear DSB repair, confirming that the DNA repair defect in the patient fibroblasts was the result of the TDP2 mutation ( figure 3C ).…”
Section: Resultssupporting
confidence: 77%
“…However, DSB repair was completed in patient cells within 8–24 hours, consistent with the established existence of alternative, nuclease-dependent mechanisms for repair of TOP2-induced DSBs in human cells. 4 , 13 , 14 Similar results were observed in human A549 cells in which TDP2 was mutated by CRISPR/Cas9 gene editing, confirming the importance of TDP2 for repair of TOP2-induced DSBs ( figure 3B ). More importantly, complementation of 850-BR cells with expression construct encoding recombinant human TDP2 restored normal rates of nuclear DSB repair, confirming that the DNA repair defect in the patient fibroblasts was the result of the TDP2 mutation ( figure 3C ).…”
Section: Resultssupporting
confidence: 77%
“…In addition to this function, ZNT451/ZATT is able to recruit and activate TDP2. Due to the conformational change of TOP2, TDP2 is subsequently capable to gain access to the crosslink without preceding proteolysis [98,99]. After successful hydrolysis of the crosslink, the resulting DSB can be repaired directly by non homologous end joining [100].…”
Section: Enzymatic Hydrolysis Of a Dpcmentioning
confidence: 99%
“…Abortive TOP2ccs require removal by cellular DNA repair pathways. This involves, at least in part, hydrolytic removal of TOP2 peptide from the DNA break by tyrosyl-DNA phosphodiesterase 2 (TDP2) (Cortes Ledesma et al, 2009;Zagnoli-Vieira and Caldecott, 2017), thereby generating DSBs with 4-base cohesive overhangs that contain ligatable 5 0 -phosphate and 3 0 -hydroxyl termini (Zeng et al, 2011). Since they require no further processing, these protein-free ends are direct substrates for accurate non-homologous end joining (NHEJ) (Gó mez-Herreros et al, 2013).…”
Section: Introductionmentioning
confidence: 99%