Issue 47, 2019, Issue in Progress
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RSC Advances

Model Affitin and PEG modifications onto siRNA lipid nanocapsules: cell uptake and in vivo biodistribution improvements

Pauline Resnier,a   Elise Lepeltier, ORCID logo a   Anthea Lucrezia Emina,a   Natacha Galopin,b   Jérôme Bejaud,a   Stephanie David,c   Caroline Ballet,d   Thierry Benvegnu,d   Frédéric Pecorari,e   Igor Chourpa, ORCID logo c   Jean-Pierre Benoita  and  Catherine Passirani ORCID logo *a  

* Corresponding authors

a MINT, UNIV Angers, INSERM 1066, CNRS 6021, Université Bretagne Loire, Angers, France
E-mail: catherine.passirani@univ-angers.fr

b CRCINA, INSERM, Université d'Angers, Université de Nantes, Nantes, France

c EA6295 – Nanomédicaments et Nanosondes, Université François-Rabelais de Tours, UFR de Pharmacie, 31 avenue Monge, F-37200 Tours, France

d Univ Rennes, Ecole Nationale Supérieure de Chimie de Rennes, CNRS, ISCR-UMR 6226, F-35000 Rennes, France

e UMR CNRS 6299 – INSERM U892, CRCNA, F-44007 Nantes, France

Abstract

Malignant melanoma is an aggressive tumor, associated with the presence of local and/or distant metastases. The development of gene therapy by the use of small interfering RNA (siRNA) represents a promising new treatment. However, the protection of this biomolecule is necessary in order for it to be intravenously administrated, for example via its incorporation into nanomedicines. In parallel to the passive targeting usually obtained by pegylation, various studies have aimed at developing “smart” nanomedicines to efficiently deliver the drug to tumor sites. In this work, siRNA loaded lipid nanocapsules (LNCs) were modified with DSPE-polyethylene glycol (DSPE-PEG), tetraether-PEG (TE-PEG) and/or with an Affitin model, to assay multiple targeting strategies. The uptake of fluorescently labelled LNCs, nanocarrier integrity and siRNA release into human SK-Mel28 melanoma cells were studied by flow cytometry, conventional confocal microscopy and by confocal spectral imaging in a Förster Resonance Energy Transfer (FRET) mode. Surface modified siRNA LNCs were followed after human plasma incubation and after intravenous injection, in order to compare the stealth properties. Finally, the biodistribution of the different siRNA LNCs in healthy and melanoma tumor bearing mice models was assessed by in vivo biofluorescence imaging (BFI), to evaluate the potential tumor targeting ability. The post-insertion of DSPE-PEG induced a strong decrease of the internalization into melanoma cells compared to TE-PEG modification. Both PEG polymer decorations induced a great plasma protection of siRNA but only DSPE-PEG led to stealth properties, even at low concentration (5 mM). The Affitin grafting by thiolation of DSPE-PEG was validated on siRNA LNCs. DSPE-PEG-Affitin LNCs were not detected in this melanoma tumor model but did not show unspecific accumulation in organs. DSPE-PEG and TE-PEG LNCs induced a significant intratumoral accumulation of modified LNCs.

Graphical abstract: Model Affitin and PEG modifications onto siRNA lipid nanocapsules: cell uptake and in vivo biodistribution improvements

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Article information

DOI
https://doi.org/10.1039/C9RA03668G
Article type
Paper
Submitted
15 May 2019
Accepted
06 Aug 2019
First published
30 Aug 2019
This article is Open Access
Creative Commons BY-NC license

RSC Adv., 2019,9, 27264-27278

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Model Affitin and PEG modifications onto siRNA lipid nanocapsules: cell uptake and in vivo biodistribution improvements

P. Resnier, E. Lepeltier, A. L. Emina, N. Galopin, J. Bejaud, S. David, C. Ballet, T. Benvegnu, F. Pecorari, I. Chourpa, J. Benoit and C. Passirani, RSC Adv., 2019, 9, 27264 DOI: 10.1039/C9RA03668G

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