Novel dextran - Spermine conjugates as transfecting agents: Comparing water-soluble and micellar polymers

H. Eliyahu, A. Makovitzki, T. Azzam, A. Zlotkin, A. Joseph, D. Gazit, Y. Barenholz, A. J. Domb

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Abstract

Recently, a novel cationic polymer, dextran-spermine (D-SPM) was developed for gene delivery. An efficient transfection was obtained using this polycation for a variety of genes and cell lines in serum-free or serum-poor medium. However, transfection using the water-soluble D-SPM-based polyplexes decreased with increasing serum concentration in cell culture in a concentration-dependent manner, reaching 95% inhibition at 50% serum in the cell growth medium. In order to overcome this obstacle, oleyl derivatives of D-SPM (which form micelles in aqueous phase) were synthesized at 1, 10, and 20 mol% of oleyl moiety to polymer E-NH2 to form N-oleyl-D-SPM (ODS). Polyplexes based on ODS transfected well in medium containing 50% serum. Comparison with polyplexes based on well-established polymers (branched and linear polyethyleneimine) and with DOTAP/Cholesterol lipoplexes showed that regarding β-galactosidase transgene expression level and cytotoxicity in tissue culture, the D-SPM and ODS compare well with the above polyplexes and lipoplexes. Intracellular trafficking using FITC-labeled ODS and Rhodamine-labeled pGeneGrip plasmid cloned with hBMP2 monitored by confocal microscopy revealed that during the transfection process the fluorescent-labeled polymer concentrates in the Golgi apparatus and around the nucleus, while the cell cytoplasm was free of fluorescent particles, suggesting that the polyplexes move in the cell toward the nucleus by vesicular transport through the cytoplasm and not by a random diffusion. We found that the plasmids penetrate the cell nucleus without the polymer. Preliminary results in zebra fish and mice demonstrate the potential of ODS to serve as an efficient nonviral vector for in vivo transfection.

Original languageEnglish
Pages (from-to)494-503
Number of pages10
JournalGene Therapy
Volume12
Issue number6
DOIs
StatePublished - Mar 2005
Externally publishedYes

Bibliographical note

Funding Information:
This study was partially supported by the AFIRST, French–Israel Cooperation on Gene Therapy, and by the US–Israel Binational Fund (BSF) to AD, and by the Barenholz Fund and the Israel Science Foundation (ISF) to YB. We would like to thank Dr M Tarshish and Dr Y Zilberman for technical assistance and Mr S Geller for editing this manuscript.

Funding

This study was partially supported by the AFIRST, French–Israel Cooperation on Gene Therapy, and by the US–Israel Binational Fund (BSF) to AD, and by the Barenholz Fund and the Israel Science Foundation (ISF) to YB. We would like to thank Dr M Tarshish and Dr Y Zilberman for technical assistance and Mr S Geller for editing this manuscript.

FundersFunder number
AFIRST
Barenholz Fund
French–Israel Cooperation on Gene Therapy
US–Israel Binational Fund
United States-Israel Binational Science Foundation
Israel Science Foundation

    Keywords

    • Gene delivery
    • Intracellular trafficking
    • Oleyl
    • Serum

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