A synthetic peptide vector system for optimal gene delivery to corneal endothelium

Background Efficient and non‐toxic gene delivery, preferably with non‐viral DNA vectors readily transferable to clinical practice, is generally regarded as a major limitation for gene therapy. Methods A 31 amino acid, integrin‐targeted bifunctional synthetic peptide (polylysine‐molossin), and two (L...

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Bibliographic Details
Published in:The journal of gene medicine 2004-02, Vol.6 (2), p.185-194
Main Authors: Collins, Louise, Fabre, John W.
Format: Article
Language:English
Subjects:
Animals
Carrier Proteins - metabolism
chloroquine
cornea
Cornea - metabolism
Crotalid Venoms - metabolism
DNA - metabolism
Endothelium - metabolism
fusogenic peptide
Gene therapy
Gene Transfer Techniques
Genes, Reporter
Genetic Vectors
Male
Mitosis - physiology
molossin
non-viral DNA vector
Peptide Fragments - metabolism
Peptides
polylysine
Rabbits
synthetic peptide
Time Factors
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Summary:Background Efficient and non‐toxic gene delivery, preferably with non‐viral DNA vectors readily transferable to clinical practice, is generally regarded as a major limitation for gene therapy. Methods A 31 amino acid, integrin‐targeted bifunctional synthetic peptide (polylysine‐molossin), and two (Lys)16‐containing control peptides, were assessed for ex vivo gene delivery to the rabbit cornea. Critical physical properties of polylysine‐molossin/DNA complexes were evaluated and both chloroquine and a 20 amino acid fusogenic peptide were used to promote endocytic exit. Results Polylysine‐molossin/DNA complexes and (Lys)16/DNA complexes at 10 µg/ml of DNA were much smaller and much more positively charged in non‐ionic isotonic medium (5% dextrose or 5% dextrose buffered to pH 7.4 in 10 mM Tris) when compared with culture medium or phosphate‐buffered saline (PBS). Addition of the fusogenic peptide (net charge −5) reversed the positive charge of complexes in PBS, and reduced the strong positive charge of polylysine‐molossin/DNA complexes in dextrose. Polylysine‐molossin/DNA complexes in 5% dextrose were much more effective for gene delivery to the cornea when compared with complexes in culture medium, and the fusogenic peptide was much more effective than chloroquine for promoting gene delivery. The optimal DNA/polylysine‐molossin/fusogenic peptide w/w ratio was 1 : 3 : 2 at 10 µg/ml of DNA. Essentially 100% of corneal endothelial cells were transfected under these optimal conditions, without any evidence of toxicity. Integrin‐targeting did not contribute significantly to gene delivery in this system. Conclusions This DNA vector system, consisting entirely of synthetic peptides, is ideally suited for clinical applications of gene therapy of the corneal endothelium. Copyright © 2004 John Wiley & Sons, Ltd.
ISSN:1099-498X
1521-2254
DOI:10.1002/jgm.482