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Simultaneous targeting of linked loci in mouse embryos using base editing.


ABSTRACT: A particular challenge in genome engineering has been the simultaneous introduction of mutations into linked (located on the same chromosome) loci. Although CRISPR/Cas9 has been widely used to mutate individual sites, its application in simultaneously targeting of linked loci is limited as multiple nearby double-stranded DNA breaks created by Cas9 routinely result in the deletion of sequences between the cleavage sites. Base editing is a newer form of genome editing that directly converts C?G-to-T?A, or A?T-to-G?C, base pairs without introducing double-stranded breaks, thus opening the possibility to generate linked mutations without disrupting the entire locus. Through the co-injection of two base editors and two sgRNAs into mouse zygotes, we introduced C?G-to-T?A transitions into two cytokine-sensing transcription factor binding sites separated by 9?kb. We determined that one enhancer activates the two flanking genes in mammary tissue during pregnancy and lactation. The ability to introduce linked mutations simultaneously in one step into the mammalian germline has implications for a wide range of applications, including the functional analysis of linked cis-elements creating disease models and correcting pathogenic mutations.

SUBMITTER: Lee HK 

PROVIDER: S-EPMC6367434 | biostudies-literature | 2019 Feb

REPOSITORIES: biostudies-literature

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Simultaneous targeting of linked loci in mouse embryos using base editing.

Lee Hye Kyung HK   Willi Michaela M   Smith Harold E HE   Miller Shannon M SM   Liu David R DR   Liu Chengyu C   Hennighausen Lothar L  

Scientific reports 20190207 1


A particular challenge in genome engineering has been the simultaneous introduction of mutations into linked (located on the same chromosome) loci. Although CRISPR/Cas9 has been widely used to mutate individual sites, its application in simultaneously targeting of linked loci is limited as multiple nearby double-stranded DNA breaks created by Cas9 routinely result in the deletion of sequences between the cleavage sites. Base editing is a newer form of genome editing that directly converts C∙G-to  ...[more]

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