DNA end-resection in highly accessible chromatin produces a toxic break

Berg, Jeroen van den; Joosten, Stacey E. P.; Kim, YongSoo; Manjón, Anna G.; Krenning, Lenno; Koob, Lisa; Feringa, Femke M.; Klompmaker, Rob; Broek, Bram van den; Jalink, Kees; Zwart, Wilbert; Medema, René H.

doi:10.1101/691857

Cited by 13 publications

(18 citation statements)

References 81 publications

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“…Secondly, we find that CDE+ genes are also enriched for genes whose sgRNAs target highly accessible chromatin (methods; hypergeometric P<0.02), consistent with the findings of a recent work that double-stranded breaks induced in highly accessible chromatin regions could induce stronger DNA damage response 16 .…”

supporting

confidence: 90%

Integrated computational and experimental identification of p53, KRAS and VHL mutant selection associated with CRISPR-Cas9 editing

Sinha

Barbosa

Cheng

et al. 2018

Preprint

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Recent studies have reported that CRISPR-Cas9 gene editing induces a p53-dependent DNA damage response in primary cells, which may select for cells with oncogenic p53 mutations 11,12 .It is unclear whether these CRISPR-induced changes are applicable to different cell types, and whether CRISPR gene editing may select for other oncogenic mutations. Addressing these questions, we analyzed genome-wide CRISPR and RNAi screens to systematically chart the mutation selection potential of CRISPR knockouts across the whole exome. Our analysis suggests that CRISPR gene editing can select for mutants of KRAS and VHL, at a level comparable to that reported for p53. These predictions were further validated in a genome-wide manner by analyzing independent CRISPR screens and patients' tumor data. Finally, we performed a new set of pooled and arrayed CRISPR screens to evaluate the competition between CRISPR-edited isogenic p53 WT and mutant cell lines, which further validated our predictions.In summary, our study systematically charts and points to the potential selection of specific cancer driver mutations during CRISPR-Cas9 gene editing.

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supporting

confidence: 90%

Integrated computational and experimental identification of p53, KRAS and VHL mutant selection associated with CRISPR-Cas9 editing

Sinha

Barbosa

Cheng

et al. 2018

Preprint

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“…More importantly, while HR is the preferred pathway that handles DSBs in transcribed chromatin during G2 (Aymard et al, 2014), our data indicate that HR usage is not required to ensure cell viability in this context. This is in agreement with the recent finding that CRISPR/Cas9 induced breaks in DNAse hypersensitive sites (open chromatin) are prone to resection and that inhibiting resection at these DSBs actually improves cell survival (van den Berg et al, 2019). Hence altogether this suggests that DSB in transcribed loci mainly utilizes HR (TAHRR) to ensure accurate repair, but that TAHRR deficiency is not cytotoxic while nevertheless affecting genome stability.…”

Section: Blm and Hencesupporting

confidence: 91%

BLM-dependent Break-Induced Replication handles DSBs in transcribed chromatin upon impaired RNA:DNA hybrids dissolution

Cohen

Guénolé

Marnef

et al. 2020

Preprint

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Transcriptionally active loci are particularly prone to breakage and mounting evidence suggest that DNA Double-Strand Breaks arising in genes are handled by a dedicated repair pathway, Transcription-Coupled DSB Repair (TC-DSBR), that entails R-loops accumulation and dissolution. Here, we uncovered a critical function of the Bloom RecQ DNA helicase (BLM) in TC-DSBR in human cells. BLM is recruited in a transcription dependent-manner at DSBs where it fosters resection, RAD51 binding and accurate Homologous Recombination repair. However, in a R-loop dissolution-deficient background BLM switches from promoting Homologous Recombination to promoting Break-Induced Replication (BIR), which strongly impairs cell viability. Altogether our

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“…For many years the view that a more open chromatin environment of euchromatin is conducive to HDR and that breaks within transcribed genes are repaired more frequently by HDR has persisted (Aymard et al, 2014; Lemaitre et al, 2014). Indeed a recent study using CRISPR-Cas9 to target specific loci found that open-chromatin may recruit insufficient p53 binding protein 1 (53BP1) (van den Berg et al, 2019), required to promote NHEJ and restrict HDR. Additionally, a more nuanced view has recently arisen in which repair choice is actively directed in different chromatin environments.…”

Section: Chromatin Barriers To Resectionmentioning

confidence: 99%

Moving Mountains—The BRCA1 Promotion of DNA Resection

Densham

Morris

2019

Front. Mol. Biosci.

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DNA double-strand breaks (DSBs) occur in our cells in the context of chromatin. This type of lesion is toxic, entirely preventing genome continuity and causing cell death or terminal arrest. Several repair mechanisms can act on DNA surrounding a DSB, only some of which carry a low risk of mutation, so that which repair process is utilized is critical to the stability of genetic material of cells. A key component of repair outcome is the degree of DNA resection directed to either side of the break site. This in turn determines the subsequent forms of repair in which DNA homology plays a part. Here we will focus on chromatin and chromatin-bound complexes which constitute the “mountains” that block resection, with a particular focus on how the breast and ovarian cancer predisposition protein-1 (BRCA1) contributes to repair outcomes through overcoming these blocks.

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DNA end-resection in highly accessible chromatin produces a toxic break

Cited by 13 publications

References 81 publications

Integrated computational and experimental identification of p53, KRAS and VHL mutant selection associated with CRISPR-Cas9 editing

Integrated computational and experimental identification of p53, KRAS and VHL mutant selection associated with CRISPR-Cas9 editing

BLM-dependent Break-Induced Replication handles DSBs in transcribed chromatin upon impaired RNA:DNA hybrids dissolution

Moving Mountains—The BRCA1 Promotion of DNA Resection

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