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Understanding the diversity of genetic outcomes from CRISPR-Cas generated homology-directed repair

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As CRISPR-Cas systems advance toward clinical application, it is essential to identify all the outcomes of gene-editing activity in human cells. Reports highlighting the remarkable success of homology-directed repair (HDR)… Click to show full abstract

As CRISPR-Cas systems advance toward clinical application, it is essential to identify all the outcomes of gene-editing activity in human cells. Reports highlighting the remarkable success of homology-directed repair (HDR) in the treatment of inherited diseases may inadvertently underreport the collateral activity of this remarkable technology. We are utilizing an in vitro gene-editing system in which a CRISPR-Cas complex provides the double-stranded cleavage and a mammalian cell-free extract provides the enzymatic activity to promote non-homologous end joining, micro-homology mediated end joining, and homology-directed repair. Here, we detail the broad spectrum of gene-editing reaction outcomes utilizing Cas9 and Cas12a in combination with single-stranded donor templates of the sense and nonsense polarity. This system offers the opportunity to see the range of outcomes of gene-editing reactions in an unbiased fashion, detailing the distribution of DNA repair outcomes as a function of a set of genetic tools.Brett Sansbury et al. show that a CRISPR-Cas complex that provides double-stranded cleavage combined with a mammalian cell-free extract can enhance non-homologous end joining and homology-directed repair. They use the system to show the range of genetic outcomes of gene-editing.

Keywords: directed repair; crispr cas; homology directed; homology; repair

Journal Title: Communications Biology
Year Published: 2019

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