Exonuclease-enhanced prime editors

Author:

Truong Dong-Jiunn JefferyORCID,Geilenkeuser JulianORCID,Wendel Stephanie VictoriaORCID,Wilming Julius Clemens HeinrichORCID,Armbrust NiklasORCID,Binder Eva Maria HildegardORCID,Santl Tobias Heinrich,Siebenhaar AnnikaORCID,Gruber Christoph,Phlairaharn TeeradonORCID,Živanić MilicaORCID,Westmeyer Gil GregorORCID

Abstract

AbstractPrime editing (PE) is a powerful gene-editing technique based on targeted gRNA-templated reverse transcription and integration of the de novo synthesized single-stranded DNA. To circumvent one of the main bottlenecks of the method, the competition of the reverse-transcribed 3′ flap with the original 5′ flap DNA, we generated an enhanced fluorescence-activated cell sorting reporter cell line to develop an exonuclease-enhanced PE strategy (‘Exo-PE’) composed of an improved PE complex and an aptamer-recruited DNA-exonuclease to remove the 5′ original DNA flap. Exo-PE achieved better overall editing efficacy than the reference PE2 strategy for insertions ≥30 base pairs in several endogenous loci and cell lines while maintaining the high editing precision of PE2. By enabling the precise incorporation of larger insertions, Exo-PE complements the growing palette of different PE tools and spurs additional refinements of the PE machinery.

Publisher

Springer Science and Business Media LLC

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