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  4. Inhibition of HIV-1 multiplication by a modified U7 snRNA inducing Tat and Rev exon skipping
 
research article

Inhibition of HIV-1 multiplication by a modified U7 snRNA inducing Tat and Rev exon skipping

Asparuhova, Maria B.
•
Marti, Gabriela
•
Liu, Songkai
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2007
The journal of gene medicine

The HIV-1 regulatory proteins Tat and Rev are encoded by multiply spliced mRNAs that differ by the use of alternative 3' splice sites at the beginning of the internal exon. If these internal exons are skipped, the expression of these genes, and hence HIV-1 multiplication, should be inhibited. We have previously developed a strategy, based on antisense derivatives of U7 small nuclear RNA, that allows us to induce the skipping of an internal exon in virtually any gene. Here, we have successfully applied this approach to induce a partial skipping of the Tat, Rev (and Nef) internal exons. Three functional U7 constructs were subcloned into a lentiviral vector. Two of them strongly reduced the efficiency of lentiviral particle production compared to vectors carrying either no U7 insert or unrelated U7 cassettes. This defect could be partly or fully compensated by coexpressing Rev from an unspliced mRNA in the producing cell line. Upon stable transduction into CEM-SS or CEM T-lymphocytes, the most efficient of these constructs inhibits HIV-1 multiplication. Although the inhibition is not complete, it is more efficient in combination with another mechanism inhibiting HIV multiplication. Therefore, this new approach targeting HIV-1 regulatory genes at the level of pre-mRNA splicing, in combination with other antiviral strategies, may be a useful new tool in the fight against HIV/AIDS.

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Type
research article
DOI
10.1002/jgm.1027
Web of Science ID

WOS:000247051100001

Author(s)
Asparuhova, Maria B.
Marti, Gabriela
Liu, Songkai
Serhan, Fatima  
Trono, Didier  
Schümperli, Daniel
Date Issued

2007

Publisher

Wiley-Blackwell

Published in
The journal of gene medicine
Volume

9

Issue

5

Start page

323

End page

34

Subjects

Exons

Editorial or Peer reviewed

NON-REVIEWED

Written at

OTHER

EPFL units
LVG  
Available on Infoscience
April 26, 2010
Use this identifier to reference this record
https://infoscience.epfl.ch/handle/20.500.14299/49724
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