High-level expression and purification of secreted forms of herpes simplex virus type 1 glycoprotein gD synthesized by baculovirus-infected insect cells.

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J Virol. 1994 February; 68(2): 766-775

High-level expression and purification of secreted forms of herpes simplex virus type 1 glycoprotein gD synthesized by baculovirus-infected insect cells.

W P Sisk, J D Bradley, R J Leipold, A M Stoltzfus, M Ponce de Leon, M Hilf, C Peng, G H Cohen and R J Eisenberg

DuPont Merck Pharmaceutical Company, Wilmington, Delaware 19880-0400.

ABSTRACT

Two forms of herpes simplex virus glycoprotein gD were recombinedinto Autographa californica nuclear polyhedrosis virus (baculovirus)and expressed in infected Spodoptera frugiperda (Sf9) cells.Each protein was truncated at residue 306 of mature gD. Oneform, gD-1(306t), contains the coding sequence of Patton strainherpes simplex virus type 1 gD; the other, gD-1(QAAt), containsthree mutations which eliminate all signals for addition ofN-linked oligosaccharides. Prior to recombination, each genewas cloned into the baculovirus transfer vector pVT-Bac, whichpermits insertion of the gene minus its natural signal peptidein frame with the signal peptide of honeybee melittin. As inthe case with many other baculovirus transfer vectors, pVT-Bacalso contains the promoter for the baculovirus polyhedrin geneand flanking sequences to permit recombination into the polyhedrinsite of baculovirus. Each gD gene was engineered to containcodons for five additional histidine residues following histidineat residue 306, to facilitate purification of the secreted proteinon nickel-containing resins. Both forms of gD-1 were abundantlyexpressed and secreted from infected Sf9 cells, reaching a maximumat 96 h postinfection for gD-1(306t) and 72 h postinfectionfor gD-1(QAAt). Secretion of the latter protein was less efficientthan gD-1(306t), possibly because of the absence of N-linkedoligosaccharides from gD-1(QAAt). Purification of the two proteinsby a combination of immunoaffinity chromatography, nickel-agarosechromatography, and gel filtration yielded products that were> 99% pure, with excellent recovery. We are able to obtain20 mg of purified gD-1(306t) and 1 to 5 mg of purified gD-1(QAAt)per liter of infected insect cells grown in suspension. Bothproteins reacted with monoclonal antibodies to discontinuousepitopes, indicating that they retain native structure. Useof this system for gD expression makes crystallization trialsfeasible.

J Virol. 1994 February; 68(2): 766-775

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