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CRISPR-Cas12a-mediated DNA clamping triggers target-strand cleavage
BiologyNature Chemical Biology

CRISPR-Cas12a-mediated DNA clamping triggers target-strand cleavage

M. M. Naqvi, L. Lee, et al.

Dive into the fascinating world of CRISPR-Cas12a with this study by Mohsin M. Naqvi, Laura Lee, Oscar E. Torres Montaguth, Fiona M. Diffin, and Mark D. Szczelkun. Discover how target strand cleavage follows non-target strand cleavage, revealing intricate mechanisms of DNA unwinding and Cas12a-DNA interactions. This research uncovers critical insights into CRISPR's operation that could reshape genetic engineering.... show more
Abstract
Clustered regularly interspaced short palindromic repeats (CRISPR)-Cas12a is widely used for genome editing and diagnostics, so it is important to understand how RNA-guided DNA recognition activates the cleavage of the target strand (TS) following non-target-strand (NTS) cleavage. Here we used single-molecule magnetic tweezers, gel-based assays and nanopore sequencing to explore DNA unwinding and cleavage. In addition to dynamic and heterogeneous R-loop formation, we also directly observed transient double-stranded DNA unwinding downstream of the 20-bp heteroduplex and, following NTS cleavage, formation of a hyperstable ‘clamped’ Cas12a-DNA intermediate necessary for TS cleavage. Annealing of a 4-nucleotide 3’ CRISPR RNA overhang to the unwound TS downstream of the heteroduplex inhibited clamping and slowed TS cleavage by ~16-fold. Alanine substitution of a conserved aromatic amino acid in the REC2 subdomain that normally caps the R-loop relieved this inhibition but favoured stabilisation of unwound states, suggesting that the REC2 subdomain regulates access of the 3’ CRISPR RNA to downstream DNA.
Publisher
Nature Chemical Biology
Published On
Jul 14, 2022
Authors
Mohsin M. Naqvi, Laura Lee, Oscar E. Torres Montaguth, Fiona M. Diffin, Mark D. Szczelkun
Tags
CRISPR-Cas12aDNA cleavagesingle-molecule magnetic tweezersnanopore sequencingNTS cleavagehyperstableCRISPR RNA
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