Litcius/Paper detail

CRISPR-Cas12a nucleases function with structurally engineered crRNAs: SynThetic trAcrRNA

Dominika Jędrzejczyk, Line Dahl Poulsen, Marcel Mohr, Nkerorema Djodji Damas, Sanne Schoffelen, Andrea Barghetti, Roland Baumgartner, Brian T. Weinert, Tobias Warnecke, Ryan T. Gill

2022Scientific Reports25 citationsDOIOpen Access PDF

Abstract

CRISPR-Cas12a systems are becoming an attractive genome editing tool for cell engineering due to their broader editing capabilities compared to CRISPR-Cas9 counterparts. As opposed to Cas9, the Cas12a endonucleases are characterized by a lack of trans-activating crRNA (tracrRNA), which reduces the complexity of the editing system and simultaneously makes CRISPR RNA (crRNA) engineering a promising approach toward further improving and modulating editing activity of the CRISPR-Cas12a systems. Here, we design and validate sixteen types of structurally engineered Cas12a crRNAs targeting various immunologically relevant loci in-vitro and in-cellulo. We show that all our structural modifications in the loop region, ranging from engineered breaks (STAR-crRNAs) to large gaps (Gap-crRNAs), as well as nucleotide substitutions, enable gene-cutting in the presence of various Cas12a nucleases. Moreover, we observe similar insertion rates of short HDR templates using the engineered crRNAs compared to the wild-type crRNAs, further demonstrating that the introduced modifications in the loop region led to comparable genome editing efficiencies. In conclusion, we show that Cas12a nucleases can broadly utilize structurally engineered crRNAs with breaks or gaps in the otherwise highly-conserved loop region, which could further facilitate a wide range of genome editing applications.

Topics & Concepts

CRISPRTrans-activating crRNAGenome editingCas9Computational biologyGenome engineeringGuide RNABiologyGeneGeneticsComputer scienceCRISPR and Genetic EngineeringRNA regulation and diseaseRNA and protein synthesis mechanisms