Optimized microfluidic formulation and organic excipients for improved lipid nanoparticle mediated genome editing.
Rohan PalankiEmily L HanAmanda M MurrayRohin MagantiSophia TangKelsey L SwingleDongyoon KimHannah YamagataHannah C SaffordKaitlin MrksichWilliam H PeranteauMichael J MitchellPublished in: Lab on a chip (2024)
mRNA-based gene editing platforms have tremendous promise in the treatment of genetic diseases. However, for this potential to be realized in vivo , these nucleic acid cargos must be delivered safely and effectively to cells of interest. Ionizable lipid nanoparticles (LNPs), the most clinically advanced non-viral RNA delivery system, have been well-studied for the delivery of mRNA but have not been systematically optimized for the delivery of mRNA-based CRISPR-Cas9 platforms. In this study, we investigated the effect of microfluidic and lipid excipient parameters on LNP gene editing efficacy. Through in vitro screening in liver cells, we discovered distinct trends in delivery based on phospholipid, cholesterol, and lipid-PEG structure in LNP formulations. Combination of top-performing lipid excipients produced an LNP formulation that resulted in 3-fold greater gene editing in vitro and facilitated 3-fold greater reduction of a therapeutically-relevant protein in vivo relative to the unoptimized LNP formulation. Thus, systematic optimization of LNP formulation parameters revealed a novel LNP formulation that has strong potential for delivery of gene editors to the liver to treat metabolic disease.
Keyphrases
- crispr cas
- genome editing
- drug delivery
- fatty acid
- nucleic acid
- induced apoptosis
- single cell
- cell cycle arrest
- binding protein
- high throughput
- genome wide
- copy number
- circulating tumor cells
- machine learning
- transcription factor
- small molecule
- combination therapy
- signaling pathway
- gene expression
- mass spectrometry
- big data
- water soluble
- walled carbon nanotubes