Characterization of Mammalian In Vivo Enhancers Using Mouse Transgenesis and CRISPR Genome Editing

增强子 生物 转基因 表观遗传学 基因组 清脆的 转基因 报告基因 计算生物学 遗传学 增强子rna 基因 染色质 功能基因组学 增强剂陷阱 基因组学 基因表达 DNA甲基化 胚胎发生 生殖生物学
作者
Marco Osterwalder,Stella Tran,Riana D. Hunter,Eman M. Meky,Kianna von Maydell,Anne Harrington,Janeth Godoy,Catherine S. Novak,Ingrid Plajzer-Frick,Yiwen Zhu,Jennifer A. Akiyama,Veena Afzal,Evgeny Z. Kvon,L Pennacchio,Diane E. Dickel,Axel Visel
出处
期刊:Methods in molecular biology [Springer Science+Business Media]
卷期号:: 147-186 被引量:32
标识
DOI:10.1007/978-1-0716-1847-9_11
摘要

Embryonic morphogenesis is strictly dependent on tight spatiotemporal control of developmental gene expression, which is typically achieved through the concerted activity of multiple enhancers driving cell type-specific expression of a target gene. Mammalian genomes are organized in topologically associated domains, providing a preferred environment and framework for interactions between transcriptional enhancers and gene promoters. While epigenomic profiling and three-dimensional chromatin conformation capture have significantly increased the accuracy of identifying enhancers, assessment of subregional enhancer activities via transgenic reporter assays in mice remains the gold standard for assigning enhancer activity in vivo. Once this activity is defined, the ideal method to explore the functional necessity of a transcriptional enhancer and its contribution to target gene dosage and morphological or physiological processes is deletion of the enhancer sequence from the mouse genome. Here we present detailed protocols for efficient introduction of enhancer-reporter transgenes and CRISPR-mediated genomic deletions into the mouse genome, including a step-by-step guide for pronuclear microinjection of fertilized mouse eggs. We provide instructions for the assembly and genomic integration of enhancer-reporter cassettes that have been used for validation of thousands of putative enhancer sequences accessible through the VISTA enhancer browser, including a recently published method for robust site-directed transgenesis at the H11 safe-harbor locus. Together, these methods enable rapid and large-scale assessment of enhancer activities and sequence variants in mice, which is essential to understand mammalian genome function and genetic diseases.
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