| Literature DB >> 24931605 |
Shin-Heng Chiou1, Caroline Kim-Kiselak2, Viviana I Risca1, Megan K Heimann2, Chen-Hua Chuang1, Aurora A Burds2, William J Greenleaf1, Tyler E Jacks3, David M Feldser4, Monte M Winslow5.
Abstract
Conditional gene deletion in mice has contributed immensely to our understanding of many biological and biomedical processes. Despite an increasing awareness of nonprotein-coding functional elements within protein-coding transcripts, current gene-targeting approaches typically involve simultaneous ablation of noncoding elements within targeted protein-coding genes. The potential for protein-coding genes to have additional noncoding functions necessitates the development of novel genetic tools capable of precisely interrogating individual functional elements. We present a strategy that couples Cre/loxP-mediated conditional gene disruption with faithful GFP reporter expression in mice in which Cre-mediated stable inversion of a splice acceptor-GFP-splice donor cassette concurrently disrupts protein production and creates a GFP fusion product. Importantly, cassette inversion maintains physiologic transcript structure, thereby ensuring proper microRNA-mediated regulation of the GFP reporter, as well as maintaining expression of nonprotein-coding elements. To test this potentially generalizable strategy, we generated and analyzed mice with this conditional knockin reporter targeted to the Hmga2 locus.Entities:
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Year: 2014 PMID: 24931605 PMCID: PMC4113058 DOI: 10.1016/j.celrep.2014.05.031
Source DB: PubMed Journal: Cell Rep Impact factor: 9.423