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  4. Transgene expression in the guinea pig cochlea mediated by a lentivirus-derived gene transfer vector
 
research article

Transgene expression in the guinea pig cochlea mediated by a lentivirus-derived gene transfer vector

Han, J. J.
•
Mhatre, A. N.
•
Wareing, M.
Show more
1999
Human Gene Therapy

The utility of lentivirus as a gene delivery vector in the cochlea was evaluated in vitro and in vivo. Lentivirus transduction was assessed through expression analysis of a reporter gene, green fluorescent protein (GFP), integrated within the viral genome. In vitro characterization of lentivirus-GFP was assessed by infection of explants from cochleas of neonatal rat. The lentiviral vector transduced both spiral ganglion neurons (SGNs) and glial cells. In vivo characterization of lentivirus-GFP was assessed by directly infusing the vector into the guinea pig cochlea via an osmotic minipump. Sections of lentivirus-infused cochlea revealed a highly restricted fluorescence pattern limited to the periphery of the perilymphatic space. Transduction of SGNs and glial cells by lentivirus in vitro but not in vivo suggests limited dissemination of the viral vector from the perilymphatic space. The cellular and tissue architecture of the lentivirus-infused cochlea was intact and free of inflammation. Restricted transduction of cell types confined to the periphery of the perilymphatic space by the lentivirus is ideal for stable production of gene products secreted into the perilymph.

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Type
research article
DOI
10.1089/10430349950017545
Author(s)
Han, J. J.
•
Mhatre, A. N.
•
Wareing, M.
•
Pettis, R.
•
Gao, W. Q.
•
Zufferey, R. N.
•
Trono, Didier  
•
Lalwani, A. K.
Date Issued

1999

Publisher

Mary Ann Liebert

Published in
Human Gene Therapy
Volume

10

Issue

11

Start page

1867

End page

73

Subjects

Gene Transfer Techniques

•

Genetic Vectors

•

Transgenes

Editorial or Peer reviewed

REVIEWED

Written at

EPFL

EPFL units
LVG  
LEN  
Available on Infoscience
September 5, 2005
Use this identifier to reference this record
https://infoscience.epfl.ch/handle/20.500.14299/215845
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