CRISPR C-to-G base editors for inducing targeted DNA transversions in human cells
Author: ["Ibrahim C. Kurt","Ronghao Zhou","Sowmya Iyer","Sara P. Garcia","Bret R. Miller","Lukas M. Langner","Julian Grünewald","J. Keith Joung"]
Publication: Nature Biotechnology
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Abstract
CRISPR-guided DNA cytosine and adenine base editors are widely used for many applications1–4 but primarily create DNA base transitions (that is, pyrimidine-to-pyrimidine or purine-to-purine). Here we describe the engineering of two base editor architectures that can efficiently induce targeted C-to-G base transversions, with reduced levels of unwanted C-to-W (W = A or T) and indel mutations. One of these C-to-G base editors (CGBE1), consists of an RNA-guided Cas9 nickase, an Escherichia coli–derived uracil DNA N-glycosylase (eUNG) and a rat APOBEC1 cytidine deaminase variant (R33A) previously shown to have reduced off-target RNA and DNA editing activities5,6. We show that CGBE1 can efficiently induce C-to-G edits, particularly in AT-rich sequence contexts in human cells. We also removed the eUNG domain to yield miniCGBE1, which reduced indel frequencies but only modestly decreased editing efficiency. CGBE1 and miniCGBE1 enable C-to-G edits and will serve as a basis for optimizing C-to-G base editors for research and therapeutic applications. A new base editor enables the creation of C-to-G base changes in human cells.
Cite this article
Kurt, I.C., Zhou, R., Iyer, S. et al. CRISPR C-to-G base editors for inducing targeted DNA transversions in human cells. Nat Biotechnol 39, 41–46 (2021). https://doi.org/10.1038/s41587-020-0609-x
