Application of long single-stranded DNA donors in genome editing: generation and validation of mouse mutants

Codner, Gemma; Mianné, Joffrey; Caulder, Adam; Loeffler, Jorik; Fell, Rachel; King, Ruairidh; Allan, Alasdair; Mackenzie, Matthew; Pike, Fran J.; McCabe, Christopher V.; Christou, Skevoulla; Joynson, Sam; Hutchison, Marie; Stewart, Michelle; Kumar, Saumya; Simon, Michelle; Agius, Loranne; Anstee, Quentin M.; Volynski, Kirill E.; Kullmann, Dimitri M.; Wells, Sara; Teboul, Lydia

doi:10.1186/s12915-018-0530-7

Cited by 78 publications

(88 citation statements)

References 30 publications

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“…Clrn2 clarinet /+ carrier mice were subsequently backcrossed to C57BL/6J for ten generations until congenic. The Clrn2 del629 mutant line was generated on a C57BL/6N background by the Molecular and Cellular Biology group at the Mary Lyon Centre (MLC), MRC Harwell Institute using CRISPR‐Cas9 genome editing (Mianne et al , ; Codner et al , ) (). Within the MLC, all mice were housed and maintained under specific pathogen‐free conditions in individually ventilated cages, with environmental conditions as outlined in the Home Office Code of Practice.…”

Section: Methodsmentioning

confidence: 99%

Clarin‐2 is essential for hearing by maintaining stereocilia integrity and function

et al. 2019

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Hearing relies on mechanically gated ion channels present in the actin‐rich stereocilia bundles at the apical surface of cochlear hair cells. Our knowledge of the mechanisms underlying the formation and maintenance of the sound‐receptive structure is limited. Utilizing a large‐scale forward genetic screen in mice, genome mapping and gene complementation tests, we identified Clrn2 as a new deafness gene. The Clrn2clarinet/clarinet mice (p.Trp4* mutation) exhibit a progressive, early‐onset hearing loss, with no overt retinal deficits. Utilizing data from the UK Biobank study, we could show that CLRN2 is involved in human non‐syndromic progressive hearing loss. Our in‐depth morphological, molecular and functional investigations establish that while it is not required for initial formation of cochlear sensory hair cell stereocilia bundles, clarin‐2 is critical for maintaining normal bundle integrity and functioning. In the differentiating hair bundles, lack of clarin‐2 leads to loss of mechano‐electrical transduction, followed by selective progressive loss of the transducing stereocilia. Together, our findings demonstrate a key role for clarin‐2 in mammalian hearing, providing insights into the interplay between mechano‐electrical transduction and stereocilia maintenance.

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Section: Methodsmentioning

confidence: 99%

Clarin‐2 is essential for hearing by maintaining stereocilia integrity and function

et al. 2019

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“…Here we injected lssDNA, not dsDNA, and we do not know how lssDNA behaves in injected Xenopus embryos as opposed to injected dsDNA that can persist (at least somatically) in adults and often exists as tandem head‐to‐tail concatemers integrated in the genome (Etkin & Pearman, 1987 and references therein). In mice, it has been shown that random insertions of injected lssDNA into the genome could also occur (Codner et al, 2018). Because of these results, we tested whether any evidence of germline transmission of randomly integrated lssDNA can be observed in albino embryos obtained from the F0 “Female 1” crossed with an albino male.…”

Section: Resultsmentioning

confidence: 99%

Simple embryo injection of long single‐stranded donor templates with the CRISPR/Cas9 system leads to homology‐directed repair in Xenopus tropicalis and Xenopus laevis

Nakayama

Grainger

Cha

2020

Genesis

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Summary We report model experiments in which simple microinjection of fertilized eggs has been used to effectively perform homology‐directed repair (HDR)‐mediated gene editing in the two Xenopus species used most frequently for research: X. tropicalis and X. laevis. We have used long single‐stranded DNAs having phosphorothioate modifications as donor templates for HDR at targeted genomic sites using the Clustered Regularly Interspaced Short Palindromic Repeats/CRISPR‐associated protein 9 (CRISPR/Cas9) system. First, X. tropicalis tyr mutant (i.e., albino) embryos were successfully rescued: partially pigmented tadpoles were seen in up to 35% of injected embryos, demonstrating the potential for efficient insertion of targeted point mutations. Second, in order to demonstrate the ability to tag genes with fluorescent proteins (FPs), we targeted the melanocyte‐specific gene slc45a2.L of X. laevis to label it with the Superfolder green FP (sfGFP), seeing mosaic expression of sfGFP in melanophores in up to 20% of injected tadpoles. Tadpoles generated by these two approaches were raised to sexual maturity, and shown to successfully transmit HDR constructs through the germline with precise targeting and seamless recombination. F1 embryos showed rescue of the tyr mutation (X. tropicalis) and tagging in the appropriate pigment cell‐specific manner of slc45a2.L with sfGFP (X. laevis).

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“…The first thing to take into account after an experiment involving CRISPR-Cas9 tools is the genetic noise (variability) produced by the endogenous repairing systems, particularly the non-homologous end joining pathway. No matter what you do, or what tricks you implement, you are going to be dealing with mosaic founder mice, whose complexity can vary enormously (Codner et al, 2018;Seruggia, Fernández, Cantero, Pelczar, & Montoliu, 2015). The CRISPR-Cas9 reagents, deposited (microinjected or electroporated) in mouse fertilized oocytes, will remain active for several cell divisions.…”

Section: Methods 1: Genotyping Genome-edited Mice To Detect Your Allelmentioning

confidence: 99%

Simple Protocol for Generating and Genotyping Genome‐Edited Mice With CRISPR‐Cas9 Reagents

et al. 2020

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The simple protocol described in this article aims to provide all required information, as a comprehensive, easy‐to‐follow step‐by‐step method, to ensure the generation of the expected genome‐edited mice. Here, we provide protocols for the preparation of CRISPR‐Cas9 reagents for microinjection and electroporation into one‐cell mouse embryos to create knockout or knock‐in mouse models, and for genotyping the resulting offspring with the latest innovative next‐generation sequencing methods. © 2020 by John Wiley & Sons, Inc. Basic Protocol 1: Designing the best RNA guide for your gene disruption/editing strategy Basic Protocol 2: Preparing and validating CRISPR‐Cas9 reagents Basic Protocol 3: Preparing and injecting CRISPR‐Cas9 compounds into fertilized mouse oocytes Basic Protocol 4: Genotyping genome‐edited mice Support Protocol: Genotyping for CRISPR‐generated “indel” mutations

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Application of long single-stranded DNA donors in genome editing: generation and validation of mouse mutants

Cited by 78 publications

References 30 publications

Clarin‐2 is essential for hearing by maintaining stereocilia integrity and function

Clarin‐2 is essential for hearing by maintaining stereocilia integrity and function

Simple embryo injection of long single‐stranded donor templates with the CRISPR/Cas9 system leads to homology‐directed repair in Xenopus tropicalis and Xenopus laevis

Simple Protocol for Generating and Genotyping Genome‐Edited Mice With CRISPR‐Cas9 Reagents

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