Rescue of vector-expressed fowl plague virus hemagglutinin in biologically active form by acidotropic agents and coexpressed M2 protein.

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J Virol. 1994 February; 68(2): 920-926

Rescue of vector-expressed fowl plague virus hemagglutinin in biologically active form by acidotropic agents and coexpressed M2 protein.

M Ohuchi, A Cramer, M Vey, R Ohuchi, W Garten and H D Klenk

Institut für Virologie, Philipps-Universität Marburg, Germany.

ABSTRACT

The hemagglutinin of the Rostock strain of fowl plague viruswas expressed in CV-1 cells by a simian virus 40 vector, andits stability in the exocytotic transport process was examinedby a fusion assay. A 50-fold increase in the fusion activityof the hemagglutinin was observed when expression occurred inthe presence of ammonium chloride, Tris-HCl, or high doses ofamantadine. When chloroquine, another acidotropic agent, wasused, the hemagglutinin exposed at the cell surface had to beactivated by trypsin, because intracellular cleavage was inhibitedby this compound. Hemagglutinin mutants resistant to intracellularcleavage did not require acidotropic agents for full expressionof fusion activity, when treated with trypsin after arrivalat the cell surface. These results indicate that fowl plaguevirus hemagglutinin expressed by a simian virus 40 vector isdenatured in the acidic milieu of the exocytotic pathway andthat cleavage is a major factor responsible for the pH instability.Coexpression with the M2 protein also markedly enhanced thefusion activity of the hemagglutinin, and this effect was inhibitedby low doses of amantadine. These results support the conceptthat M2, known to have ion channel function, protects the hemagglutininfrom denaturation by raising the pH in the exocytotic transportsystem. The data also stress the importance of acidotropic agentsor coexpressed M2 for the structural and functional integrityof vector-expressed hemagglutinin.

J Virol. 1994 February; 68(2): 920-926

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