Expression and extracellular release of human immunodeficiency virus type 1 Gag precursors by recombinant baculovirus-infected cells.

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J Virol. 1992 May; 66(5): 3230-3235

Expression and extracellular release of human immunodeficiency virus type 1 Gag precursors by recombinant baculovirus-infected cells.

M Royer, S S Hong, B Gay, M Cerutti and P Boulanger

Laboratoire de Virologie et Pathogénèse Moléculaires, Institut de Biologie, Faculté de Médecine, Montpellier, France.

ABSTRACT

The level of synthesis and extracellular release of human immunodeficiencyvirus type 1 Gag by insect cells was analyzed, using eight differentrecombinants of Autographa californica nuclear polyhedrosisvirus harboring various constructs of the gag gene, cloned underthe polyhedrin promoter. The results obtained suggested thatgag expression was mainly regulated at the transcriptional leveland was not significantly influenced by posttranslational events,e.g., Gag self-assembly, nuclear transport, or extracellularrelease. Two different forms of Gag were found in the culturemedium of recombinant-infected cells. One form consisted ofmembrane-enveloped, corelike particles released by budding atthe plasma membrane; the other of nonparticulate, soluble Gagpolyprotein molecules. Both forms coexisted in recombinantsexpressing Gag with an intact N-terminal myristylation signal,whereas recombinants expressing nonmyristylated Gag releasedsolely the soluble form. This suggested that myristylation ofthe N terminus was not a prerequisite for efficient extracellularrelease of Gag by insect cells, which could proceed via twoindependent but simultaneous mechanisms.

J Virol. 1992 May; 66(5): 3230-3235

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