Generation of gene-edited rats by delivery of CRISPR/Cas9 protein and donor DNA into intact zygotes using electroporation

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作者
Séverine Remy
Vanessa Chenouard
Laurent Tesson
Claire Usal
Séverine Ménoret
Lucas Brusselle
Jean-Marie Heslan
Tuan Huan Nguyen
Jeremy Bellien
Jean Merot
Anne De Cian
Carine Giovannangeli
Jean-Paul Concordet
Ignacio Anegon
机构
[1] Centre de Recherche en Transplantation et Immunologie UMR1064,
[2] INSERM,undefined
[3] Université de Nantes,undefined
[4] Institut de Transplantation Urologie Néphrologie (ITUN),undefined
[5] CHU Nantes,undefined
[6] Platform Transgenic Rats and ImmunoPhenomics,undefined
[7] INSERM UMR 1064-CRTI,undefined
[8] Platform GenoCellEdit,undefined
[9] INSERM UMR 1064-CRTI,undefined
[10] INSERM U1096,undefined
[11] Institut du thorax,undefined
[12] INSERM UMR 1087,undefined
[13] CNRS UMR 6291,undefined
[14] INSERM U565,undefined
[15] CNRS UMR7196,undefined
[16] Museum National d’Histoire Naturelle,undefined
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摘要
The generation of gene-edited animals using the CRISPRs/Cas9 system is based on microinjection into zygotes which is inefficient, time consuming and demands high technical skills. We report the optimization of an electroporation method for intact rat zygotes using sgRNAs and Cas9 protein in combination or not with ssODNs (~100 nt). This resulted in high frequency of knockouts, between 15 and 50% of analyzed animals. Importantly, using ssODNs as donor template resulted in precise knock-in mutations in 25–100% of analyzed animals, comparable to microinjection. Electroporation of long ssDNA or dsDNA donors successfully used in microinjection in the past did not allow generation of genome-edited animals despite dsDNA visualization within zygotes. Thus, simultaneous electroporation of a large number of intact rat zygotes is a rapid, simple, and efficient method for the generation of a variety of genome-edited rats.
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