Author:
Borrás Teresa,Cowley Dale O.,Asokan Priyadarsini,Pandya Kumar
Abstract
AbstractThe ability to ablate a gene in a given tissue by generating a conditional knockout (cKO) is crucial for determining its function in the targeted tissue. Such tissue-specific ablation is even more critical when the gene’s conventional knockout (KO) is lethal, which precludes studying the consequences of its deletion in other tissues. Therefore, here we describe a successful strategy that generated a Matrix Gla floxed mouse (Mgp.floxed) by the CRISPR/Cas9 system, that subsequently allowed the generation of cKOs by local viral delivery of the Cre-recombinase enzyme. MGP is a well-established inhibitor of calcification gene, highly expressed in arteries’ smooth muscle cells and chondrocytes. MGP is also one of the most abundant genes in the trabecular meshwork, the eye tissue responsible for maintenance of intraocular pressure (IOP) and development of Glaucoma. Our strategy entailed one-step injection of two gRNAs, Cas9 protein and a long-single-stranded-circular DNA donor vector (lsscDNA, 6.7 kb) containing two loxP sitesin cisand 900–700 bp 5′/3′ homology arms. Ocular intracameral injection ofMgp.floxedmice with a Cre-adenovirus, led to anMgp.TMcKO mouse which developed elevated IOP. Our study discovered a new role for theMgpgene as a keeper of physiological IOP in the eye.
Funder
National Institutes of Health
Publisher
Springer Science and Business Media LLC
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