Journal of General Virology, Vol 78, 953-963, Copyright © 1997 by Society for General Microbiology
Baculovirus-mediated trans-epithelial transport of proteins in infected caterpillars
M Sarvari, P Zavodszky, K Molnar, P Low and M Sass
Institute of Enzymology, Hungarian Academy of Sciences, Budapest, Hungary.
Baculovirus-mediated abnormal protein trafficking was studied in infected
caterpillars by using heterologous proteins. The gene for human complement
C1r was expressed in larvae of Mamestra brassicae by a recombinant
Autographa californica nuclear polyhedrosis virus (AcMNPV) vector. By
following the time-course of recombinant C1r distribution among various
tissues, cell types and cell organelles, we concluded that the dominant
site of recombinant protein synthesis was the fat body, although some
production in the haemocytes and midgut was also observed. Only about 4% of
the cells of the infected organs expressed recombinant C1r, which was then
secreted into the haemolymph. The tracheal and integumental cuticle was
rich in recombinant protein from the fourth day after infection although
epidermal cells did not synthesize recombinant C1r. The morphological
picture suggested that the accumulation was a consequence of a
trans-epithelial transport. This transport process was checked by following
the fate of the 49 kDa haemolymph protein and injected ovalbumin in
AcMNPV-infected Mamestra brassicae and in Lymantria dispar nuclear
polyhedrosis virus-infected Lymantria dispar larvae. Both proteins were
able to pass the basal membrane of the epidermis and accumulated in the
cuticle, while in control larvae neither was transported. The observed
trans-epithelial transport points to the role of baculoviruses in directing
recombinant, endo- and exo-genous proteins to cuticulated tissues. Based on
these results we conclude that the permeability of basal membranes
undergoes a characteristic change during the course of baculovirus
infection.
