A stable but reversible integrated surrogate reporter for assaying CRISPR/Cas9-stimulated homology-directed repair

Yahong Wen; Grace Liao; Thomas Pritchard; Ting-Ting Zhao; Jon P Connelly; Shondra M Pruett-Miller; Valerie Blanc; Nicholas O Davidson; Blair B Madison

doi:10.1074/jbc.M117.777722

A stable but reversible integrated surrogate reporter for assaying CRISPR/Cas9-stimulated homology-directed repair

J Biol Chem. 2017 Apr 14;292(15):6148-6162. doi: 10.1074/jbc.M117.777722. Epub 2017 Feb 22.

Authors

Yahong Wen¹, Grace Liao¹, Thomas Pritchard¹, Ting-Ting Zhao², Jon P Connelly³, Shondra M Pruett-Miller³, Valerie Blanc¹, Nicholas O Davidson¹, Blair B Madison⁴

Affiliations

¹ From the Division of Gastroenterology, Washington University School of Medicine, Saint Louis, Missouri 63110.
² First Hospital of China Medical University, Department of Breast Surgery, Shenyang, China 110001.
³ Genome Engineering and iPSC Center (GEiC), Department of Genetics, Washington University, Saint Louis, Missouri 63110, and.
⁴ From the Division of Gastroenterology, Washington University School of Medicine, Saint Louis, Missouri 63110, bmadison@wustl.edu.

Abstract

The discovery and application of CRISPR/Cas9 technology for genome editing has greatly accelerated targeted mutagenesis in a variety of organisms. CRISPR/Cas9-mediated site-specific cleavage is typically exploited for the generation of insertions or deletions (indels) after aberrant dsDNA repair via the endogenous non-homology end-joining (NHEJ) pathway or, alternatively, for enhancing homology-directed repair to facilitate the generation of a specific mutation (or "knock-in"). However, there is a need for efficient cellular assays that can measure Cas9/guide RNA activity. Reliable methods for enriching and identifying desired mutants are also lacking. Here we describe a method using the Piggybac transposon for stable genomic integration of an H2B-GFP reporter or a hygromycin resistance gene for assaying Cas9 target cleavage and homology-directed repair. The H2B-GFP fusion protein provides increased stability and an obvious pattern of nuclear localization. This method, called SRIRACCHA (i.e. a stable, but reversible, integrated reporter for assaying CRISPR/Cas-stimulated HDR activity), enables the enrichment of mutants via selection of GFP-positive or hygromycin-resistant mammalian cells (immortalized or non-immortalized) as a surrogate for the modification of the endogenous target site. Currently available hyperactive Piggybac transposase mutants allow both delivery and removal of the surrogate reporters, with minimal risk of generating undesirable mutations. This assay permits rapid screening for efficient guide RNAs and the accelerated identification of mutant clones and is applicable to many cell types. We foresee the utility of this approach in contexts in which the maintenance of genomic integrity is essential, for example, when engineering cells for therapeutic purposes.

Keywords: CRISPR/Cas; DNA endonuclease; HDR; Piggybac; gene knockout; genome editing; homologous recombination; surrogate reporter; transposable element (TE).

Publication types

Research Support, Non-U.S. Gov't
Research Support, N.I.H., Extramural

MeSH terms

Animals
CRISPR-Cas Systems*
Cell Line, Tumor
Gene Deletion*
Gene Targeting / methods*
Genetic Vectors / genetics*
Mice

Abstract

Publication types

MeSH terms

Grants and funding