Literature DB >> 27250209

Detecting Single-Nucleotide Substitutions Induced by Genome Editing.

Yuichiro Miyaoka1, Amanda H Chan1, Bruce R Conklin2.   

Abstract

The detection of genome editing is critical in evaluating genome-editing tools or conditions, but it is not an easy task to detect genome-editing events-especially single-nucleotide substitutions-without a surrogate marker. Here we introduce a procedure that significantly contributes to the advancement of genome-editing technologies. It uses droplet digital polymerase chain reaction (ddPCR) and allele-specific hydrolysis probes to detect single-nucleotide substitutions generated by genome editing (via homology-directed repair, or HDR). HDR events that introduce substitutions using donor DNA are generally infrequent, even with genome-editing tools, and the outcome is only one base pair difference in 3 billion base pairs of the human genome. This task is particularly difficult in induced pluripotent stem (iPS) cells, in which editing events can be very rare. Therefore, the technological advances described here have implications for therapeutic genome editing and experimental approaches to disease modeling with iPS cells.
© 2016 Cold Spring Harbor Laboratory Press.

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Year:  2016        PMID: 27250209     DOI: 10.1101/pdb.top090845

Source DB:  PubMed          Journal:  Cold Spring Harb Protoc        ISSN: 1559-6095


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3.  Rapid, precise quantification of large DNA excisions and inversions by ddPCR.

Authors:  Hannah L Watry; Carissa M Feliciano; Ketrin Gjoni; Gou Takahashi; Yuichiro Miyaoka; Bruce R Conklin; Luke M Judge
Journal:  Sci Rep       Date:  2020-09-10       Impact factor: 4.379

  3 in total

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