Can Designer Indels Be Tailored by Gene Editing?

Trimidal, Sara G.; Benjamin, Ronald; Bae, Ji Eun; Han, Mira V.; Kong, Elizabeth; Singer, Aaron; Williams, Tyler S.; Yang, Bing; Schiller, Martin

doi:10.1002/bies.201900126

Cited by 3 publications

(2 citation statements)

References 100 publications

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“…CRISPR-Cas9 has a repair profile closer to the environmental DSB's one compared to other nucleases with a high frequency of insertions of one nucleotide (Trimidal et al, 2019) and mainly repairs using out-of-frame indels (>70%) and microhomologies (Guo et al, 2018;Taheri-Ghahfarokhi et al, 2018).…”

Section: Repair Pathwaysmentioning

confidence: 99%

Advances in Genome Editing and Application to the Generation of Genetically Modified Rat Models

et al. 2021

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The rat has been extensively used as a small animal model. Many genetically engineered rat models have emerged in the last two decades, and the advent of gene-specific nucleases has accelerated their generation in recent years. This review covers the techniques and advances used to generate genetically engineered rat lines and their application to the development of rat models more broadly, such as conditional knockouts and reporter gene strains. In addition, genome-editing techniques that remain to be explored in the rat are discussed. The review also focuses more particularly on two areas in which extensive work has been done: human genetic diseases and immune system analysis. Models are thoroughly described in these two areas and highlight the competitive advantages of rat models over available corresponding mouse versions. The objective of this review is to provide a comprehensive description of the advantages and potential of rat models for addressing specific scientific questions and to characterize the best genome-engineering tools for developing new projects.

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Section: Repair Pathwaysmentioning

confidence: 99%

Advances in Genome Editing and Application to the Generation of Genetically Modified Rat Models

et al. 2021

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“…Our earlier in silico analysis showed that the gene editing enzymes likely interfere with binding of key components of DNA repair complexes and may alter the preference for C-NHEJ or A-NHEJ 10 . Although XRCC4 and MRE-11 are well studied NHEJ complex proteins, we investigated changes in cellular responses when both C-NHEJ and A-NHEJ are blocked by targeting these proteins.…”

Section: Introductionmentioning

confidence: 99%

Robust Transcriptional Regulatory Response Upon Blocking NHEJ

Benjamin

Banerjee

Guerunk

et al. 2021

Preprint

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Double strand breaks are one of the most lethal forms of DNA lesions that, if left unrepaired can lead to genomic instability, cellular transformation, and cell death. However, cells have two main machineries namely error prone Non homologous end joining repair (NHEJ) or an accurate homology dependent repair to repair the double strand breaks. NHEJ is the preferred mechanism for DNA repair and basically consists of two forms: Canonical (C-NHEJ) and Alternative (A-NHEJ) NHEJ. Our study examined the cellular repair outcome when NHEJ is blocked by targeting two key DNA repair proteins: XRCC4 and MRE-11. We developed an extrachromosomal NHEJ fluorescent reporter assay that uses Transcription activator-like effector nucleases (TALEN) to introduce double strand breaks and detect the NHEJ editing by the presence of GFP fluorescence. We demonstrated the presence of NHEJ editing in the XRCC4(-/-) cells treated with Mirin (a pharmacological inhibitor of MRE-11), albeit with a ~52% efficiency of the normal cells. The transcriptional profiles of the Mirin treated HeLa XRCC4(-/-) cells had 307 uniquely differentially expressed genes that was far greater than HeLa XRCC4(-/-) sample (83 genes) and Mirin treated HeLa cells (30 genes). Pathway analysis unique to the XRCC4(-/-) +Mirin group included differential expression of p53 downstream pathways, and metabolic pathways indicating cell adaptation for energy regulation and stress response. In conclusion, our study showed that the double strand DNA repair can be sustained even in absence of key DNA repair proteins XRCC4 and MRE-11.

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CRISPR–Cas9/CRISPRi tools for cell factory construction in E. coli

Hashemi

2020

World J Microbiol Biotechnol

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Can Designer Indels Be Tailored by Gene Editing?

Cited by 3 publications

References 100 publications

Advances in Genome Editing and Application to the Generation of Genetically Modified Rat Models

Advances in Genome Editing and Application to the Generation of Genetically Modified Rat Models

Robust Transcriptional Regulatory Response Upon Blocking NHEJ

CRISPR–Cas9/CRISPRi tools for cell factory construction in E. coli

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