Issue 6, 2011
From the journal:

Molecular BioSystems

1,4-Butanediol diglycidyl ether (BDE)-crosslinked PEI-g-imidazolenanoparticles as nucleic acid-carriers in vitro and in vivo

Ritu Goyal,a   Ruby Bansal,a   Shilpa Tyagi,b   Yogeshwer Shukla,b   Pradeep Kumara  and  Kailash Chand Gupta*ab  

* Corresponding authors

a Institute of Genomics and Integrative Biology (CSIR), Mall Road, Delhi University Campus, Delhi-110 007, India

b Indian Institute of Toxicology Research (CSIR), Mahatma Gandhi Marg, Lucknow-226 001, Uttar Pradesh, India
E-mail: kcgupta@iitr.res.in
Tel: +91-522-2621856

Abstract

Previously reported 1,4-butanediol diglycidyl ether (BDE) crosslinked PEI (branched polyethylenimine, 25 k) nanoparticles (A. Swami, R. Kurupati, A. Pathak, Y. Singh, P. Kumar and K. C. Gupta, A unique and highly efficient non-viral DNA/siRNA delivery system based on PEI-bisepoxide nanoparticles, Biochem. Biophys. Res. Commun., 2007, 362, 835–841) (PN NPs) were reacted with varying proportions of a novel linker, 2-(N-1-tritylimidazol-4-yl)-N-(6-glycidyloxyhexyl)-acetamide (IGA linker, 3), to yield PN-g-imidazolyl nanoparticles (PNIm) with improved transfection efficiency. Here, the IGA linker (3) reacted through an epoxy ring to partially convert the residual 1° and 2° amines present in PN NPs to 2° and 3°, respectively, without altering the total number of amines and additionally incorporating the delocalized positive charge of the imidazolyl moiety. The resulting particles were characterized for their size, zeta potential and DNA complexing ability. PNIm/DNA nanoplexes, in the size range of 120–400 nm, were evaluated for transfection efficiency in HeLa, HEK293 and CHO cell lines, which was found to be ∼11, ∼2–3 and ∼2–17 folds higher than PEI, PN-2 (the best working sample of the PN series) (A. Swami, R. Kurupati, A. Pathak, Y. Singh, P. Kumar and K. C. Gupta, A unique and highly efficient non-viral DNA/siRNA delivery system based on PEI-bisepoxide nanoparticles, Biochem. Biophys. Res. Commun., 2007, 362, 835–841) and commercial transfection reagents tested in this study, respectively. Also, flow cytometric analysis showed ∼78% (ca. ∼43% in PN-2) cells transfected with the PNIm 10(6)/DNA complex (the best working sample of the PNIm series) in HEK293 cells. Transfection of GFP specific siRNA in HEK293 cells suppressed the gene expression by ∼90% (ca. ∼70% in PN-2). All the cell lines treated with PNIm/DNA nanoplexes showed >90% viability. In vivo gene expression of luciferase enzyme in Balb/c mice showed highest expression in spleen after seven days.

Graphical abstract: 1,4-Butanediol diglycidyl ether (BDE)-crosslinked PEI-g-imidazole nanoparticles as nucleic acid-carriers in vitro and in vivo

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Article information

DOI
https://doi.org/10.1039/C1MB05049D
Article type
Paper
Submitted
07 Feb 2011
Accepted
23 Mar 2011
First published
19 Apr 2011

Mol. BioSyst., 2011,7, 2055-2065

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1,4-Butanediol diglycidyl ether (BDE)-crosslinked PEI-g-imidazole nanoparticles as nucleic acid-carriers in vitro and in vivo

R. Goyal, R. Bansal, S. Tyagi, Y. Shukla, P. Kumar and K. C. Gupta, Mol. BioSyst., 2011, 7, 2055 DOI: 10.1039/C1MB05049D

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