Cellular gene transfer mediated by influenza virosomes with encapsulated plasmid DNA

Cellular gene transfer mediated by influenza virosomes with encapsulated plasmid DNA

Reconstituted influenza virosomes (virus membrane envelopes) have been used previously to deliver pDNA (plasmid DNA) bound to their external surface to a variety of target cells. Although high transfection efficiencies can be obtained with these complexes in vitro, the virosome-associated DNA is rea...

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Veröffentlicht in:Biochemical journal 2007-07, Vol.405 (1), p.41-49
Hauptverfasser: de Jonge, Jørgen, Leenhouts, Johanna M, Holtrop, Marijke, Schoen, Pieter, Scherrer, Peter, Cullis, Pieter R, Wilschut, Jan, Huckriede, Anke
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Sprache:eng
Schlagworte:
Animals
Cell Line
Gene Transfer Techniques
Influenza virus
Orthomyxoviridae
Plasmids - administration & dosage
Plasmids - genetics
Plasmids - metabolism
Transfection - methods
Virosomes - metabolism
Virosomes - ultrastructure
Virus Internalization
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container_end_page 49
container_issue 1
container_start_page 41
container_title Biochemical journal
container_volume 405
creator de Jonge, Jørgen
Leenhouts, Johanna M
Holtrop, Marijke
Schoen, Pieter
Scherrer, Peter
Cullis, Pieter R
Wilschut, Jan
Huckriede, Anke
description Reconstituted influenza virosomes (virus membrane envelopes) have been used previously to deliver pDNA (plasmid DNA) bound to their external surface to a variety of target cells. Although high transfection efficiencies can be obtained with these complexes in vitro, the virosome-associated DNA is readily accessible to nucleases and could therefore be prone to rapid degradation under in vivo conditions. In the present study, we show a new method for the production of DNA-virosomes resulting in complete protection of the DNA from nucleases. This method relies on the use of the short-chain phospholipid DCPC (dicaproylphosphatidylcholine) for solubilization of the viral membrane. The solubilized viral membrane components are mixed with pDNA and cationic lipid. Reconstitution of the viral envelopes and simultaneous encapsulation of pDNA is achieved by removal of the DCPC from the mixture through dialysis. Analysis by linear sucrose density-gradient centrifugation revealed that protein, phospholipid and pDNA physically associated to particles, which appeared as vesicles with spike proteins inserted in their membranes when analysed by electron microscopy. The DNA-virosomes retained the membrane fusion properties of the native influenza virus. The virosome-associated pDNA was completely protected from degradation by nucleases, providing evidence for the DNA being highly condensed and encapsulated in the lumen of the virosomes. DNA-virosomes, containing reporter gene constructs, transfected a variety of cell lines, with efficiencies approaching 90%. Transfection was completely dependent on the fusogenic properties of the viral spike protein haemagglutinin. Thus, DNA-virosomes prepared by the new procedure are highly efficient vehicles for DNA delivery, offering the advantage of complete DNA protection, which is especially important for future in vivo applications.
doi_str_mv 10.1042/BJ20061756
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source MEDLINE; Elektronische Zeitschriftenbibliothek - Frei zugängliche E-Journals; PubMed Central; Alma/SFX Local Collection
subjects Animals
Cell Line
Gene Transfer Techniques
Influenza virus
Orthomyxoviridae
Plasmids - administration & dosage
Plasmids - genetics
Plasmids - metabolism
Transfection - methods
Virosomes - metabolism
Virosomes - ultrastructure
Virus Internalization
title Cellular gene transfer mediated by influenza virosomes with encapsulated plasmid DNA
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