Vaccinia virus expression vector: coexpression of beta-galactosidase provides visual screening of recombinant virus plaques.

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Mol Cell Biol. 1985 December; 5(12): 3403-3409

Vaccinia virus expression vector: coexpression of beta-galactosidase provides visual screening of recombinant virus plaques.

S Chakrabarti, K Brechling and B Moss

ABSTRACT

We constructed a plasmid coexpression vector that directs theinsertion of a foreign gene of interest together with the Escherichiacoli beta-galactosidase (beta gal) gene into the thymidine kinase(TK) locus of the vaccinia virus genome. Tissue culture cellsthat had been infected with vaccinia virus were transfectedwith a plasmid vector containing a foreign gene. TK- recombinantscould be selected by a plaque assay on TK- cells in the presenceof 5-bromodeoxyuridine and distinguished from spontaneous TK-mutants by the addition of a beta-gal indicator to the agaroseoverlay. Plaques that expressed beta-gal stained dark blue withinseveral hours at 37 degrees C. Alternatively, TK- selectioncould be eliminated, and recombinant plaques could be readilyidentified solely by their blue color. The reverse procedure,in which the starting virus expresses beta-gal (i.e., formsblue plaques) and the desired recombinant has deleted the entirebeta-gal gene (i.e., forms white plaques), is another alternative.Each protocol was tested by constructing vaccinia virus recombinantsthat express hepatitis B virus surface antigen.

Mol Cell Biol. 1985 December; 5(12): 3403-3409

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