Cellular Repressor Inhibits Human Cytomegalovirus Transcription from the UL127 Promoter

doi:10.1128/JVI.78.10.5113-5123.2004

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Journal of Virology, May 2004, p. 5113-5123, Vol. 78, No. 10
0022-538X/04/$08.00+0 DOI: 10.1128/JVI.78.10.5113-5123.2004
Copyright © 2004, American Society for Microbiology. All Rights Reserved.

Cellular Repressor Inhibits Human Cytomegalovirus Transcription from the UL127 Promoter

Philip E. Lashmit,¹ Christopher A. Lundquist, Jeffery L. Meier,²^,3 and Mark F. Stinski¹^*

Department of Microbiology,¹ Department of Internal Medicine, Carver College of Medicine, University of Iowa,² Veterans Administration Medical Center, Iowa City, Iowa 52242³

Received 2 January 2004/ Accepted 28 January 2004

The region of the human cytomegalovirus (HCMV) genome betweenthe UL127 promoter and the major immediate-early (MIE) enhanceris referred to as the unique region. The role of this regionduring a viral infection is not known. In wild-type HCMV-infectedpermissive fibroblasts, there is no transcription from the UL127promoter at any time during productive infection. Our investigatorspreviously reported that the region upstream of the UL127 TATAbox repressed expression from the UL127 promoter (C. A. Lundquistet al., J. Virol. 73:9039-9052, 1999). The region was reportedto contain functional NF1 DNA binding sites (L. Hennighausenand B. Fleckenstein, EMBO J. 5:1367-1371, 1986). Sequence analysisof this region detected additional consensus binding sites forthree transcriptional regulatory proteins, FoxA (HNF-3), suppressorof Hairy wing, and CAAT displacement protein. The cis-actingelements in the unique region prevented activation of the earlyUL127 promoter by the HCMV MIE proteins. In contrast, deletionof the region permitted very high activation of the UL127 promoterby the viral MIE proteins. Mutation of the NF1 sites had noeffect on the basal activity of the promoter. To determine therole of the other sites in the context of the viral genome,recombinant viruses were generated in which each putative repressorsite was mutated and the effect on the UL127 promoter was analyzed.Mutation of the putative Fox-like site resulted in a significantincrease in expression from the viral early UL127 promoter.Insertion of wild-type Fox-like sites between the HCMV immediate-early(IE) US3 TATA box and the upstream NF- ${kappa}$ B-responsive enhancer(R2) also significantly decreased gene expression, but mutatedFox-like sites did not. The wild-type Fox-like site inhibitsactivation of a viral IE enhancer-containing promoter. Cellularprotein, which is present in uninfected or infected permissivecell nuclear extracts, binds to the wild-type Fox-like sitebut not to mutated sites. Reasons for repression of UL127 genetranscription during productive infection are discussed.

* Corresponding author. Mailing address: Department of Microbiology, 3-772 BSB, University of Iowa, Iowa City, IA 52242-1109. Phone: (319) 335-7792. Fax: (319) 335-9006. E-mail: mark-stinski{at}uiowa.edu.

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