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Directed evolution expands CRISPR–Cas12a genome-editing capacity

Enbo Ma, Kai Chen, Honglue Shi, Kevin Wasko, Isabel Esain-Garcia, Marena Trinidad, Kaihong Zhou, Jinjuan Ye, Jennifer A. Doudna

2025Nucleic Acids Research15 citationsDOIOpen Access PDF

Abstract

CRISPR-Cas12a enzymes are versatile RNA-guided genome-editing tools with applications encompassing viral diagnosis, agriculture, and human therapeutics. However, their dependence on a 5'-TTTV-3' protospacer adjacent motif (PAM) next to DNA target sequences restricts Cas12a's gene targeting capability to only ∼1% of a typical genome. To mitigate this constraint, we used a bacterial-based directed evolution assay combined with rational engineering to identify variants of Lachnospiraceae bacterium Cas12a with expanded PAM recognition. The resulting Cas12a variants use a range of noncanonical PAMs while retaining recognition of the canonical 5'-TTTV-3' PAM. In particular, biochemical and cell-based assays show that the variant Flex-Cas12a utilizes 5'-NYHV-3' PAMs that expand DNA recognition sites to ∼25% of the human genome. With enhanced targeting versatility, Flex-Cas12a unlocks access to previously inaccessible genomic loci, providing new opportunities for both therapeutic and agricultural genome engineering.

Topics & Concepts

BiologyCRISPRGenome editingGenome engineeringGenomeComputational biologyGeneticsGeneHuman genomeDNACas9CRISPR and Genetic EngineeringRNA and protein synthesis mechanismsInsect symbiosis and bacterial influences
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