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A One-Step PCR-Based Assay to Evaluate the Efficiency and Precision of Genomic DNA-Editing Tools.

Authors :
Germini D
Bou Saada Y
Tsfasman T
Osina K
Robin C
Lomov N
Rubtsov M
Sjakste N
Lipinski M
Vassetzky Y
Source :
Molecular therapy. Methods & clinical development [Mol Ther Methods Clin Dev] 2017 Mar 08; Vol. 5, pp. 43-50. Date of Electronic Publication: 2017 Mar 08 (Print Publication: 2017).
Publication Year :
2017

Abstract

Despite rapid progress, many problems and limitations persist and limit the applicability of gene-editing techniques. Making use of meganucleases, TALENs, or CRISPR/Cas9-based tools requires an initial step of pre-screening to determine the efficiency and specificity of the designed tools. This step remains time consuming and material consuming. Here we propose a simple, cheap, reliable, time-saving, and highly sensitive method to evaluate a given gene-editing tool based on its capacity to induce chromosomal translocations when combined with a reference engineered nuclease. In the proposed technique, designated engineered nuclease-induced translocations (ENIT), a plasmid coding for the DNA-editing tool to be tested is co-transfected into carefully chosen target cells along with that for an engineered nuclease of known specificity and efficiency. If the new enzyme efficiently cuts within the desired region, then specific chromosomal translocations will be generated between the two targeted genomic regions and be readily detectable by a one-step PCR or qPCR assay. The PCR product thus obtained can be directly sequenced, thereby determining the exact position of the double-strand breaks induced by the gene-editing tools. As a proof of concept, ENIT was successfully tested in different cell types and with different meganucleases, TALENs, and CRISPR/Cas9-based editing tools.

Details

Language :
English
ISSN :
2329-0501
Volume :
5
Database :
MEDLINE
Journal :
Molecular therapy. Methods & clinical development
Publication Type :
Academic Journal
Accession number :
28480303
Full Text :
https://doi.org/10.1016/j.omtm.2017.03.001