Nucleic Acids Research, Vol 25, Issue 16 3199-3203, Copyright © 1997 by Oxford University Press
S Joshi, SF Ding and SE Liem
A Moloney murine leukemia virus (MoMuLV)-derived packaging retroviral
vector, pUCMoTN-PR3, was previously developed in which the packaging (psi)
signal was cloned within the 5'-long terminal repeat (LTR) U3-r and U5
sequences. The MoTN-PR3 vector particles released from a transfected
packaging cell line contain RNAs with r-psi-U5 sequences at the 5'-end and
U3-r sequences at the 3'-end. Upon infection, these vector particles can
efficiently transduce the neomycin phosphotransferase (neo) gene to the
target cells. The structure of the proviral DNA synthesized in these cells
was shown to contain modified 5'- and 3'-LTRs with U3-r-psi-U5 sequences,
indicating that this vector can undergo reverse transcription and
integration. Analysis of psi signal-containing RNAs revealed that in
addition to vector RNA transcribed from the MoMuLV 5'-LTR promoter,
readthrough neo RNA transcribed from the internal herpes simplex virus
(HSV) thymidine kinase (tk) promoter and cellular RNAs transcribed from the
MoMuLV 3'- LTR promoter are produced. Of these, the downstream cellular
RNAs are also packaged within the vector particles. These vector particles
containing the vector and non-vector RNAs carrying the MoMuLV psi signal
are non-infectious. It is proposed that intracellular expression of
packageable non-viral RNAs may represent an effective strategy for
inhibiting animal and plant virus replication.
ARTICLES
Co-packaging of non-vector RNAs generates replication-defective retroviral vector particles: a novel approach for blocking retrovirus replication
Department of Medical Genetics and Microbiology, Faculty of Medicine, University of Toronto, Toronto, Ontario M5S 3E2, Canada. sadhna.joshi.sukhwal@utoronto.ca
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