Generation of Human Isogenic Induced Pluripotent Stem Cell Lines with CRISPR Prime Editing.
Lori L BonnycastleAmy J SwiftErin C MansellAngela LeeElizabeth WinnickiElizabeth S LiCatherine C RobertsonVictoria A ParsonsTrung HuynhChad KrilowKaren L MohlkeMichael R ErdosNarisu NarisuFrancis S CollinsPublished in: The CRISPR journal (2024)
We developed an efficient CRISPR prime editing protocol and generated isogenic-induced pluripotent stem cell (iPSC) lines carrying heterozygous or homozygous alleles for putatively causal single nucleotide variants at six type 2 diabetes loci ( ABCC8 , MTNR1B , TCF7L2 , HNF4A , CAMK1D , and GCK ). Our two-step sequence-based approach to first identify transfected cell pools with the highest fraction of edited cells significantly reduced the downstream efforts to isolate single clones of edited cells. We found that prime editing can make targeted genetic changes in iPSC and optimization of system components and guide RNA designs that were critical to achieve acceptable efficiency. Systems utilizing PEmax, epegRNA modifications, and MLH1dn provided significant benefit, producing editing efficiencies of 36-73%. Editing success and pegRNA design optimization required for each variant differed depending on the sequence at the target site. With attention to design, prime editing is a promising approach to generate isogenic iPSC lines, enabling the study of specific genetic changes in a common genetic background.
Keyphrases
- crispr cas
- genome editing
- genome wide
- type diabetes
- induced apoptosis
- stem cells
- induced pluripotent stem cells
- copy number
- high glucose
- cell cycle arrest
- diabetic rats
- endothelial cells
- randomized controlled trial
- oxidative stress
- dna methylation
- cell death
- insulin resistance
- signaling pathway
- single cell
- quality improvement
- immune response
- weight loss
- cell proliferation
- metabolic syndrome
- toll like receptor
- amino acid
- stress induced
- bone marrow