A Simple and Efficient CRISPR Technique for Protein Tagging.

Fanning ZengValerie BeckSven SchuiererIsabelle GarnierCarole MannevilleClaudia AgarinisLapo MorelliLisa QuinnJudith KnehrGuglielmo RomaFrederic BassilanaMark Nash

Published in: Cells (2020)

Genetic knock-in using homology-directed repair is an inefficient process, requiring the selection of few modified cells and hindering its application to primary cells. Here, we describe Homology independent gene Tagging (HiTag), a method to tag a protein of interest by CRISPR in up to 66% of transfected cells with one single electroporation. The technique has proven effective in various cell types and can be used to knock in a fluorescent protein for live cell imaging, to modify the cellular location of a target protein and to monitor the levels of a protein of interest by a luciferase assay in primary cells.

Keyphrases

induced apoptosis
cell cycle arrest
genome wide
protein protein
endoplasmic reticulum stress
amino acid
stem cells
oxidative stress
binding protein
high resolution
mass spectrometry
copy number
high throughput
dna methylation
quantum dots
cell proliferation
transcription factor
fluorescent probe