Targeting specific DNA G-quadruplexes with CRISPR-guided G-quadruplex-binding proteins and ligands.
Geng QinZhenqi LiuJie YangXiaofeng LiaoChuanqi ZhaoJinsong RenXiaogang QuPublished in: Nature cell biology (2024)
Despite the demonstrated importance of DNA G-quadruplexes (G4s) in health and disease, technologies to readily manipulate specific G4 folding for functional analysis and therapeutic purposes are lacking. Here we employ G4-stabilizing protein/ligand in conjunction with CRISPR to selectively facilitate single or multiple targeted G4 folding within specific genomic loci. We demonstrate that fusion of nucleolin with a catalytically inactive Cas9 can specifically stabilize G4s in the promoter of oncogene MYC and muscle-associated gene Itga7 as well as telomere G4s, leading to cell proliferation arrest, inhibition of myoblast differentiation and cell senescence, respectively. Furthermore, CRISPR can confer intra-G4 selectivity to G4-binding compounds pyridodicarboxamide and pyridostatin. Compared with traditional G4 ligands, CRISPR-guided biotin-conjugated pyridodicarboxamide enables a more precise investigation into the biological functionality of de novo G4s. Our study provides insights that will enhance understanding of G4 functions and therapeutic interventions.
Keyphrases
- genome wide
- genome editing
- crispr cas
- dna methylation
- single molecule
- copy number
- cell proliferation
- circulating tumor
- public health
- healthcare
- cancer therapy
- cell free
- cell cycle
- molecular dynamics simulations
- transcription factor
- dna damage
- gene expression
- binding protein
- single cell
- skeletal muscle
- cell therapy
- photodynamic therapy
- social media
- nucleic acid
- signaling pathway
- protein protein
- dna binding
- mesenchymal stem cells