Cloning-free CRISPR/Cas system facilitates functional cassette knock-in in mice

Authors
Aida T1, Chiyo K2, Usami T3, Ishikubo H4, Imahashi R5, Wada Y6, Tanaka KF7, Sakuma T8, Yamamoto T9, Tanaka K10,11,12.
08-12-2015
12:00pm
PST
Categories
Chemical Biology of RNA
Abstract
Although the CRISPR/Cas system has enabled one-step generation of knockout mice, low success rates of cassette knock-in limit its application range. Here we show that cloning-free, direct nuclear delivery of Cas9 protein complex with chemically synthesized dual RNAs enables highly efficient target digestion, leading to generation of knock-in mice carrying a functional cassette with up to 50% efficiency, compared with just 10% by a commonly used method consisting of Cas9 mRNA and single guide RNA. Our cloning-free CRISPR/Cas system facilitates rapid one-step generation of cassette knock-in mice, accelerating functional genomic research by providing various in vivo genetic tools.