Megan E Pearce et al 2008 Nanotechnology 19 175103 doi:10.1088/0957-4484/19/17/175103
Megan E Pearce1, Hoang Q Mai1, Namhoon Lee2, Sarah C Larsen2,3 and Aliasger K Salem1,3
Show affiliationsHere, we report on a new zeolite-based silicalite nanoparticle that can enhance the transfection efficiencies generated by poly ethylene imine–plasmid DNA (PEI–pDNA) complexes via a sedimentation mechanism and can enhance the transfection efficiencies of pDNA alone when surface functionalized with amine groups. The silicalite nanoparticles have a mean size of 55 nm. Functionalizing the silicalite nanoparticles with amine groups results in a clear transition in zeta potential from −25.9 ± 2.3 mV (pH 7.4) for unfunctionalized silicalite nanoparticles to 4.9 ± 0.7 mV (pH 7.4) for amine functionalized silicalite nanoparticles. We identify that silicalite nanoparticles used to promote non-viral vector acceleration to the cell surface are found in acidic vesicles or the cytoplasm but not the nucleus. An MTT (3-[4,5-dimethylthiazol-2-yl]-2,5-diphenyl tetrazolium bromide) assay showed that the silicalite nanoparticles were non-toxic at the concentrations tested for transfection. We show that surface functionalization of silicalite nanoparticles with amine groups results in a significant (230%) increase in transfection efficiency of pDNA when compared to unfunctionalized silicalite nanoparticles. Silicalite nanoparticles enhanced pDNA–PEI induced transfection of human embryonic kidney (HEK-293) cells by over 150%.
87.85.Qr Nanotechnologies-design
Issue 17 (30 April 2008)
Received 22 January 2008, in final form 26 February 2008
Published 25 March 2008
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