| Literature DB >> 31902667 |
Nataliia Serbyn1, Audrey Noireterre2, Ivona Bagdiul2, Michael Plank3, Agnès H Michel4, Robbie Loewith3, Benoît Kornmann4, Françoise Stutz5.
Abstract
Naturally occurring or drug-induced DNA-protein crosslinks (DPCs) interfere with key DNA transactions if not repaired in a timely manner. The unique family of DPC-specific proteases Wss1/SPRTN targets DPC protein moieties for degradation, including stabilized topoisomerase-1 cleavage complexes (Top1ccs). Here, we describe that the efficient DPC disassembly requires Ddi1, another conserved predicted protease in Saccharomyces cerevisiae. We found Ddi1 in a genetic screen of the tdp1 wss1 mutant defective in Top1cc processing. Ddi1 is recruited to a persistent Top1cc-like DPC lesion in an S phase-dependent manner to assist in the eviction of crosslinked protein from DNA. Loss of Ddi1 or its putative protease activity hypersensitizes cells to DPC trapping agents independently from Wss1 and 26S proteasome, implying its broader role in DPC repair. Among the potential Ddi1 targets, we found the core component of Pol II and show that its genotoxin-induced degradation is impaired in ddi1. We propose that the Ddi1 protease contributes to DPC proteolysis.Entities:
Keywords: 26S proteasome; DNA-protein crosslink; Ddi1; Flp recombinase; RNA polymerase II; Rpb1; Top1; Wss1; protease; yeast
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Year: 2020 PMID: 31902667 DOI: 10.1016/j.molcel.2019.12.007
Source DB: PubMed Journal: Mol Cell ISSN: 1097-2765 Impact factor: 17.970