Promoter-specific trans activation and repression by human cytomegalovirus immediate-early proteins involves common and unique protein domains.

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J Virol. 1990 April; 64(4): 1556-1565

Promoter-specific trans activation and repression by human cytomegalovirus immediate-early proteins involves common and unique protein domains.

R M Stenberg, J Fortney, S W Barlow, B P Magrane, J A Nelson and P Ghazal

Department of Microbiology and Immunology, Eastern Virginia Medical School, Norfolk 23501.

ABSTRACT

trans activation of promoters by viral regulatory proteins providesa useful tool to study coordinate control of gene expression.Immediate-early (IE) regions 1 and 2 of human cytomegalovirus(CMV) code for a series of proteins that originate from differentiallyspliced mRNAs. These IE proteins are proposed to regulate thetemporal expression of the viral genome. To examine the structureand function of the IE proteins, we used linker insertion mutagenesisof the IE gene region as well as cDNA expression vector cloningof the abundant IE mRNAs. We showed that IE1 and IE2 proteinsof CMV exhibit promoter-specific differences in their modesof action by either trans activating early and IE promotersor repressing the major IE promoter (MIEP). Transient cotransfectionexperiments with permissive human cells revealed a synergisticinteraction between the 72- and the 86-kilodalton (kDa) IE proteinsin trans activating an early promoter. In addition, transfectionstudies revealed that the 72-kDa protein was capable of transactivating the MIEP. In contrast, the 86-kDa protein specificallyrepressed the MIEP and this repression was suppressed by the72-kDa protein. Furthermore, observations based on the primarysequence structure revealed a modular arrangement of putativeregulatory motifs that could either potentiate or repress geneexpression. These modular domains are either shared or uniqueamong the IE proteins. From these data, we propose a model forIE protein function in the coordinate control of CMV gene expression.

J Virol. 1990 April; 64(4): 1556-1565

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