A Simple and Efficient CRISPR Technique for Protein Tagging

Fanning Zeng,Valerie Beck,Sven Schuierer, Isabelle Garnier,Carole Manneville,Claudia Agarinis,Lapo Morelli,Lisa Quinn,Judith Knehr,Guglielmo Roma,Frederic Bassilana,Mark Nash

CELLS（2020）

Novartis Inst Biomed Res

Cited 5|Views36

Abstract

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.

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Key words

CRISPR knock in,non-homologous end-joining (NHEJ),protein tagging

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