The size and symmetry of B capsids of herpes simplex virus type 1 are determined by the gene products of the UL26 open reading frame.

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J Virol. 1994 September; 68(9): 5365-5374

The size and symmetry of B capsids of herpes simplex virus type 1 are determined by the gene products of the UL26 open reading frame.

P Desai, S C Watkins and S Person

Department of Molecular Genetics and Biochemistry, University of Pittsburg Medical School, Pennsylvania 15261.

ABSTRACT

Herpes simplex virus type 1 (HSV-1) B capsids are composed ofseven proteins, designated VP5, VP19C, 21, 22a, VP23, VP24,and VP26 in order of decreasing molecular weight. Three proteins(21, 22a, and VP24) are encoded by a single open reading frame(ORF), UL26, and include a protease whose structure and functionhave been studied extensively by other investigators. The proteaseencoded by this ORF generates VP24 (amino acids 1 to 247), astructural component of the capsid and mature virions, and 21(residues 248 to 635). The protease also cleaves C-terminalresidues 611 to 635 of 21 and 22a, during capsid maturation.Protease activity has been localized to the N-terminal 247 residues.Protein 22a and probably the less abundant protein 21 occupythe internal volume of capsids but are not present in virions;therefore, they may form a scaffold that is used for B capsidassembly. The objective of the present study was to isolateand characterize a mutant virus with a null mutation in UL26.Vero cells were transformed with plasmid DNA that encoded ORFUL25 through UL28 and screened for their ability to supportthe growth of a mutant virus with a null mutation in UL27 (K082).Four of five transformants that supported the growth of theUL27 mutant also supported the growth of a UL27-UL28 doublemutant. One of these transformants (F3) was used to isolatea mutant with a null mutation in UL26. The UL26 null mutationwas constructed by replacement of DNA sequences specifying codons41 through 593 with a lacZ reporter cassette. Permissive cellswere cotransfected with plasmid and wild-type virus DNA, andprogeny viruses were screened for their ability to grow on F3but not Vero cells. A virus with these growth characteristics,designated KUL26 delta Z, that did not express 21, 22a, or VP24during infection of Vero cells was isolated. Radiolabeled nuclearlysates from infected nonpermissive cells were layered ontosucrose gradients and subjected to velocity sedimentation. Apeak of radioactivity for KUL26 delta Z that sedimented morerapidly than B capsids from wild-type-infected cells was observed.Sodium dodecyl sulfate-polyacrylamide gel electrophoresis analysisof the gradient fractions showed that the peak fractions containedVP5, VP19C, VP23, and VP26. Analysis of sectioned cells andof the peak fractions of the gradients by electron microscopyrevealed sheet and spiral structures that appear to be capsidshells.(ABSTRACT TRUNCATED AT 400 WORDS)

J Virol. 1994 September; 68(9): 5365-5374

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