Journal of General Virology, Vol 78, 273-281, Copyright © 1997 by Society for General Microbiology
Insecticidal activity of a recombinant baculovirus containing an antisense c-myc fragment
SY Lee, X Qu, W Chen, A Poloumienko, N MacAfee, B Morin, C Lucarotti and M Krause
Department of Biology, University of New Brunswick, Fredericton, Canada.
Attempts to develop baculovirus-based insecticides by insertion of genes
encoding enzyme inhibitors, neuropeptides or toxins have met with some
success. However, it is often difficult to ensure correct processing or
secretion of the encoded peptides. Here we tested a simpler strategy by
insertion of an antisense fragment of a host gene to block translation of a
protein essential for larval growth and development. We selected the c-myc
gene for two main reasons: (i) its protein is known to be well conserved in
evolution and to have multiple essential functions during development; and
(ii) c-myc family genes have yet to be characterized in insects, thus
blockage of essential genes by anti-sense transcripts from a strong virus
promoter could provide a sensitive test for the existence of myc-like gene
products. An appropriate fragment of the human c-myc gene was inserted
downstream from the polyhedrin promoter of Autographa californica
nucleopolyhedrovirus and tested in bioassays on Spodoptera frugiperda
larvae. Western blot analysis with a human c-myc antibody revealed an
endogenous protein band which bound specifically to these antibodies. This
band disappeared more rapidly from cells infected with the antisense c-myc
recombinant virus than from those infected with c-myc- negative virus.
Results of bioassays showed that the antisense construct stopped feeding as
soon as the polyhedrin promoter-driven transcripts accumulated, followed
shortly by death of the larvae. These results suggest that c-myc-like
protein(s) exist in insects and that the antisense strategy is an effective
approach to virus insecticide productions.
