Editing the Genome Without Double-Stranded DNA Breaks.
Alexis C KomorAhmed H BadranDavid R LiuPublished in: ACS chemical biology (2017)
Genome editing methods have commonly relied on the initial introduction of double-stranded DNA breaks (DSBs), resulting in stochastic insertions, deletions, and translocations at the target genomic locus. To achieve gene correction, these methods typically require the introduction of exogenous DNA repair templates and low-efficiency homologous recombination processes. In this review, we describe alternative, mechanistically motivated strategies to perform chemistry on the genome of unmodified cells without introducing DSBs. One such strategy, base editing, uses chemical and biological insights to directly and permanently convert one target base pair to another. Despite its recent introduction, base editing has already enabled a number of new capabilities and applications in the genome editing community. We summarize these advances here and discuss the new possibilities that this method has unveiled, concluding with a brief analysis of future prospects for genome and transcriptome editing without double-stranded DNA cleavage.
Keyphrases
- crispr cas
- genome editing
- dna repair
- genome wide
- circulating tumor
- dna damage
- nucleic acid
- cell free
- single molecule
- binding protein
- copy number
- dna damage response
- induced apoptosis
- current status
- dna methylation
- healthcare
- mental health
- circulating tumor cells
- single cell
- oxidative stress
- cell cycle arrest
- rna seq
- transcription factor
- pi k akt