Collaborative Action of Brca1 and CtIP in Elimination of Covalent Modifications from Double-Strand Breaks to Facilitate Subsequent Break Repair

Nakamura, Kyoko; Kogame, Toshiaki; Oshiumi, Hiroyuki; Shinohara, Atsushi; Sumitomo, Yoshiki; Agama, Keli; Pommier, ﻿Yves; Tsutsui, Kimiko; Tsutsui, Ken; Hartsuiker, Edgar; Ogi, Tomoo; Takeda, Shunichi; Taniguchi, Yoshihito

doi:10.1371/journal.pgen.1000828

Cited by 139 publications

(184 citation statements)

References 47 publications

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“…The results of the present study clarify the involvement of Tdp1 in resolving Top2cc-mediated DNA damage. Finally, because CtIP (RBBP8) has recently emerged as a critical factor for the repair of topoisomerase-DNA complexes (26,27,50), we generated double mutant DT40 cells for Tdp1 and CtIP and investigated the relative contribution of the Tdp1-and CtIPdependent pathways in the cellular responses to Top1-and Top2-targeting drugs as well as methyl methanesulfonate (MMS).…”

Section: Dna Topoisomerase I (Top1)mentioning

confidence: 99%

“…Recent studies show that CtIP, together with BRCA1, acts in the nuclease-mediated elimination of Top1cc and Top2cc (26,27,50). CtIP S332A/Ϫ/Ϫ DT40 cells, which harbor an alanine substitution at residue Ser-332 of CtIP that abrogates its interaction with BRCA1, are hypersensitive to CPT, etoposide, and MMS but remain proficient in homologous recombination (26). Because this function overlaps with that of Tdp1, we generated double mutant DT40 cells (referred to as CtIP S332A/Ϫ/Ϫ;Tdp1Ϫ/Ϫ) to examine the relationship between Tdp1 and CtIP in different types of DNA repair.…”

Section: Tdp1-mediated Dna Repairmentioning

confidence: 99%

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Tyrosyl-DNA Phosphodiesterase 1 (TDP1) Repairs DNA Damage Induced by Topoisomerases I and II and Base Alkylation in Vertebrate Cells

Murai

Huang

Das

et al. 2012

Journal of Biological Chemistry

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155

207

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Background: Tdp1 is a DNA repair enzyme conserved across eukaryotes. Results: Tdp1 repairs not only 3Ј-tyrosyl-DNA bonds and 3Ј-phosphoglycolates but also 5Ј-tyrosyl-DNA bonds and 3Ј-deoxyribose phosphates. Conclusion:The end processing functions of Tdp1 extend to the repair of Top2-DNA adducts and DNA breaks from base alkylation. Significance: Tdp1 has a broad range of DNA repair activities and is a potential drug target in anticancer therapy.

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Section: Dna Topoisomerase I (Top1)mentioning

confidence: 99%

Section: Tdp1-mediated Dna Repairmentioning

confidence: 99%

Tyrosyl-DNA Phosphodiesterase 1 (TDP1) Repairs DNA Damage Induced by Topoisomerases I and II and Base Alkylation in Vertebrate Cells

Murai

Huang

Das

et al. 2012

Journal of Biological Chemistry

Self Cite

155

207

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“…Moreover, in mammalian cells, CtIP-BRCA1 complex formation facilitates removal of 53BP1 binding protein RIF1 from DSB regions, which otherwise blocks resection (Escribano-Díaz et al, 2013). However, the physiological role of S327 phosphorylation has been questioned by the finding that the chicken CtIP-S332A protein can efficiently promote DSB repair by HR, apparently independently of BRCA1 interaction (Nakamura et al, 2010) and by the fact that that knock-in mice homozygous for CtIP-S326A allele are neither tumor prone or HR deficient . Thus, the biological importance of the BRCA1-CtIP interaction remains unclear.…”

Section: Spontaneous and Parpi-induced Genome Instability In Ctip-defmentioning

confidence: 99%

“…These conclusions were based on the findings that BRCA1-deficient cells exhibit a mild decrease in IR-induced RPA focus formation (Chen et al, 2008;Escribano-Díaz et al, 2013), that BRCA1 and CtIP inhibit RIF1 end-blocking activity in S/G2 (Escribano-Díaz et al, 2013;Zimmermann et al, 2013), and that cells expressing CtIP-327A are defective in HR (Yun and Hiom, 2009). However, subsequent studies in chicken (Nakamura et al, 2010), frog (Peterson et al, 2011), and mouse cells ; analogous to our CtIPnull cells reconstituted with CtIP-S327A), and direct measurements of gene conversion (Chandramouly et al, 2013), argue that the CtIP-BRCA1 interaction is dispensable for HR. Moreover, our finding that restoration of HR in BRCA1-53BP1-deficient cells and increased resection that occurs in the absence of 53BP1 are CtIP dependent, demonstrates that CtIP-mediated resection is BRCA1 independent.…”

Section: Model For Functions Of Brca1 and Ctip In Dsb Resectionmentioning

confidence: 99%

CtIP-mediated resection is essential for viability and can operate independently of BRCA1

Polato¹,

Bunting²,

Wong³

et al. 2014

J Cell Biol

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“…Alternatively, trapped TOP1 can be removed nucleolytically (21,22). For repair of the 5′-phosphotyrosyl-linked TOP2 adducts, only nucleolytic mechanisms were considered (23,24) until a protein known as "TRAF and TNF receptor-associated protein" (TTRAP) or "ETS1-associated protein II" (EAPII) (25) was found to have such an activity (26); that protein has been renamed "TDP2" (Fig. 2B).…”

mentioning

confidence: 99%

Involvement of the host DNA-repair enzyme TDP2 in formation of the covalently closed circular DNA persistence reservoir of hepatitis B viruses

Königer

Wingert

Marsmann

et al. 2014

Proc. Natl. Acad. Sci. U.S.A.

206

193

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Hepatitis B virus (HBV), the causative agent of chronic hepatitis B and prototypic hepadnavirus, is a small DNA virus that replicates by protein-primed reverse transcription. The product is a 3-kb relaxed circular DNA (RC-DNA) in which one strand is linked to the viral polymerase (P protein) through a tyrosyl-DNA phosphodiester bond. Upon infection, the incoming RC-DNA is converted into covalently closed circular (ccc) DNA, which serves as a viral persistence reservoir that is refractory to current anti-HBV treatments. The mechanism of cccDNA formation is unknown, but the release of P protein is one mandatory step. Structural similarities between RC-DNA and cellular topoisomerase-DNA adducts and their known repair by tyrosyl-DNA-phosphodiesterase (TDP) 1 or TDP2 suggested that HBV may usurp these enzymes for its own purpose. Here we demonstrate that human and chicken TDP2, but only the yeast ortholog of TDP1, can specifically cleave the Tyr-DNA bond in virus-adapted model substrates and release P protein from authentic HBV and duck HBV (DHBV) RC-DNA in vitro, without prior proteolysis of the large P proteins. Consistent with TPD2's having a physiological role in cccDNA formation, RNAi-mediated TDP2 depletion in human cells significantly slowed the conversion of RC-DNA to cccDNA. Ectopic TDP2 expression in the same cells restored faster conversion kinetics. These data strongly suggest that TDP2 is a first, although likely not the only, host DNA-repair factor involved in HBV cccDNA biogenesis. In addition to establishing a functional link between hepadnaviruses and DNA repair, our results open new prospects for directly targeting HBV persistence.hepatitis B virus persistence | TDP substrate specificity | virus-DNA repair interface M ore than 250 million people worldwide are chronically infected with hepatitis B virus (HBV) (1) and are at a highly increased risk for developing end-stage liver disease (2). Current treatments with IFN-α or nucleos(t)ide analogs (NAs) are only partially effective (3, 4). Importantly, they do not directly target the viral persistence reservoir, an episomal covalently closed circular (ccc) DNA form of the viral genome that serves as template for all viral transcripts; hence a few cccDNA molecules present in the liver can reactivate full viral replication. Eliminating infection thus will require the elimination of cccDNA. cccDNA is generated, upon infection, from the viral polymerase (P protein)-linked relaxed circular (RC) DNA present in incoming virions (Fig. 1A). The mechanism by which RC-DNA is converted to cccDNA is poorly understood, but it must involve multiple steps (see below). Because the ∼3-kb genomes of HBV and the other hepadnaviruses [e.g., from ducks (DHBV)] are too small to encode all the activities required for this conversion, these activities must be provided by the host cell.RC-DNA from all hepadnaviruses bears several molecular peculiarities that result from its generation by protein-primed reverse transcription (for reviews, see refs. 5 and 6). The pregenomic RNA (p...

show abstract

Collaborative Action of Brca1 and CtIP in Elimination of Covalent Modifications from Double-Strand Breaks to Facilitate Subsequent Break Repair

Cited by 139 publications

References 47 publications

Tyrosyl-DNA Phosphodiesterase 1 (TDP1) Repairs DNA Damage Induced by Topoisomerases I and II and Base Alkylation in Vertebrate Cells

Tyrosyl-DNA Phosphodiesterase 1 (TDP1) Repairs DNA Damage Induced by Topoisomerases I and II and Base Alkylation in Vertebrate Cells

CtIP-mediated resection is essential for viability and can operate independently of BRCA1

Involvement of the host DNA-repair enzyme TDP2 in formation of the covalently closed circular DNA persistence reservoir of hepatitis B viruses

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