| Literature DB >> 32003222 |
Yuhang Jiang1, Qiao Lu2, Yongheng Wang1, Emily Xu1, Alison Ho1, Priya Singh1, Yifei Wang1, Zhaozhong Jiang1, Fan Yang1, Gregory T Tietjen1,3, Peter Cresswell2, W Mark Saltzman1,4,5.
Abstract
Endosomal escape is a key step for intracellular drug delivery of nucleic acids, but reliable and sensitive methods for its quantitation remain an unmet need. In order to rationally optimize the mRNA transfection efficiency of a library of polymeric materials, we designed a deactivated Renilla luciferase-derived molecular probe whose activity can be restored only in the cytosol. This probe can be coencapsulated with mRNA in the same delivery vehicle, thereby accurately measuring its endosomal escape efficiency. We examined a library of poly(amine-co-ester) (PACE) polymers with different end groups using this probe and observed a strong correlation between endosomal escape and transfection efficiency (R2 = 0.9334). In addition, we found that mRNA encapsulation efficiency and endosomal escape, but not uptake, were determinant factors for transfection efficiency. The polymers with high endosomal escape/transfection efficiency in vitro also showed good transfection efficiency in vivo, and mRNA expression was primarily observed in spleens after intravenous delivery. Together, our study suggests that the luciferase probe can be used as an effective tool to quantitate endosomal escape, which is essential for rational optimization of intracellular drug delivery systems.Entities:
Keywords: Endosomal escape; PACE; ddRLuc-Fc; mRNA delivery; nanoparticles
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Year: 2020 PMID: 32003222 PMCID: PMC7195212 DOI: 10.1021/acs.nanolett.9b04426
Source DB: PubMed Journal: Nano Lett ISSN: 1530-6984 Impact factor: 12.262