Identification and characterization of the human cytomegalovirus immediate-early region 2 gene that stimulates gene expression from an inducible promoter.

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J Virol. 1987 October; 61(10): 3214-3221

Identification and characterization of the human cytomegalovirus immediate-early region 2 gene that stimulates gene expression from an inducible promoter.

T W Hermiston, C L Malone, P R Witte and M F Stinski

ABSTRACT

The human cytomegalovirus (HCMV) XbaI E cloned DNA fragmentof approximately 20 kilobases can complement an adenovirus mutant(dl312) defective in the E1a viral gene product (D. J. Spectorand M. J. Tevethia, Virology 151:329-338, 1986). This viralDNA fragment contains three immediate-early (IE) genes between0.709 and 0.751 map units (M. F. Stinski, D. R. Thomsen, R.M. Stenberg, and L. C. Goldstein, J. Virol. 46:1-14, 1983).Two of the IE genes, IE1 and IE2, were isolated and tested fora role in regulating viral gene expression. Since HCMV earlyand late promoters require additional characterization, thechloramphenicol acetyl transferase (cat) gene, driven by theadenovirus E2 promoter, was used as an indicator of gene expression.cat expression from this heterologous viral promoter was shownto be stimulated by HCMV at early times after infection. TheIE1 gene product did not function independently in activatingthis promoter. The IE2 gene products could independently stimulatethe expression of a plasmid of a plasmid when the cat gene wasplaced downstream of the inducible E2 promoter (E2CAT). Fiveproteins of different sizes have been predicted to originatefrom IE2, depending on mRNA splicing. The protein products specifiedby the IE2 gene were characterized with an antibody to a syntheticpeptide according to the open reading frame of exon 2. Threeof the five proteins are encoded by exon 2. Three viral proteinsof 82, 54, and 28 kilodaltons (kDa) were detected. The exonscontained in the region designated as IE2a have open readingframes that could code for two of the smaller proteins of 27and 30 kDa. This region, when driven by the HCMV enhancer, couldindependently stimulate gene expression from E2CAT to a highlevel. A plasmid with the HCMV enhancer upstream of exons, thatcould code for the HCMV IE2 proteins of 48 and 51 kDa, as wellas 27- and 30-kDa proteins, also stimulated E2CAT expressionbut at a lower level. The activity of this plasmid was augmentedby the IE1 gene product, despite the fact that the latter geneproduct alone was inactive. It is proposed that the HCMV IEregion 2 gene products are involved in the regulation of viralor host cell promoters either independently or in combinationwith other HCMV IE proteins.

J Virol. 1987 October; 61(10): 3214-3221

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