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Efficient and Fast Generation of Relevant Disease Mouse Models by In Vitro and In Vivo Gene Editing of Zygotes

机译:有效和快速的生成相关的疾病小鼠模型的体外和体内基因编辑受精卵的

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摘要

Knockout mice for human disease-causing genes provide valuable models in which new therapeutic approaches can be tested. Electroporation of genome editing tools into zygotes, in vitro or within oviducts, allows for the generation of targeted mutations in a shorter time. We have generated mouse models deficient in genes involved in metabolic rare diseases (Primary Hyperoxaluria Type 1 Pyruvate Kinase Deficiency) or in a tumor suppressor gene (Rasa1). Pairs of guide RNAs were designed to generate controlled deletions that led to the absence of protein. In vitro or in vivo ribonucleoprotein (RNP) electroporation rendered more than 90% and 30% edited newborn animals, respectively. Mice lines with edited alleles were established and disease hallmarks have been verified in the three models that showed a high consistency of results and validating RNP electroporation into zygotes as an efficient technique for disease modeling without the need to outsource to external facilities.
机译:基因敲除小鼠对人类致病基因新的治疗提供有价值的模型方法可以进行测试。基因组编辑工具到受精卵体外或在输卵管内,允许的生成有针对性的突变在更短的时间。生成的小鼠模型缺乏基因(主要参与代谢罕见疾病Hyperoxaluria 1型丙酮酸激酶缺乏症)或肿瘤抑制基因(Rasa1)。指导rna被设计来生成控制删除,导致缺乏蛋白质。体外或体内核糖核蛋白(RNP)电穿孔呈现逾90%和30%分别编辑新生动物。建立与编辑等位基因和疾病在三个模型验证标志显示和高一致性的结果验证RNP电穿孔成受精卵有效的疾病建模技术需要外包给外部设施。

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