Human Cytomegalovirus UL84 Oligomerization and Heterodimerization Domains Act as Transdominant Inhibitors of oriLyt-Dependent DNA Replication: Evidence that IE2-UL84 and UL84-UL84 Interactions Are Required for Lytic DNA Replication

doi:10.1128/JVI.78.17.9203-9214.2004

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Journal of Virology, September 2004, p. 9203-9214, Vol. 78, No. 17
0022-538X/04/$08.00+0 DOI: 10.1128/JVI.78.17.9203-9214.2004
Copyright © 2004, American Society for Microbiology. All Rights Reserved.

Human Cytomegalovirus UL84 Oligomerization and Heterodimerization Domains Act as Transdominant Inhibitors of oriLyt-Dependent DNA Replication: Evidence that IE2-UL84 and UL84-UL84 Interactions Are Required for Lytic DNA Replication

Kelly S. Colletti, Yiyang Xu, Sylvia A. Cei, Margaret Tarrant, and Gregory S. Pari^*

Department of Microbiology and Immunology and the Cell and Molecular Biology Program, University of Nevada-Reno, Reno, Nevada

Received 20 February 2004/ Accepted 19 April 2004

Human cytomegalovirus (HCMV) UL84 encodes a 75-kDa protein requiredfor oriLyt-dependent DNA replication and interacts with IE2in infected and transfected cells. UL84 localizes to the nucleusof transfected and infected cells and is found in viral replicationcompartments. In transient assays it was shown that UL84 caninterfere with the IE2-mediated transactivation of the UL112/113promoter of HCMV. To determine whether UL84 protein-proteininteractions are necessary for lytic DNA synthesis, we purifiedUL84 and used this protein to generate a monoclonal antibody.Using this antibody, we now show that UL84 forms a stable interactionwith itself in vivo. The point of self-interaction maps to aregion of the protein between amino acids 151 and 200, a domainthat contains a series of highly charged amino acid residues.Coimmunoprecipitation assays determined that UL84 interactswith a protein domain present within the first 215 amino acidsof IE2. We also show that an intact leucine zipper domain ofUL84 is required for a stable interaction with IE2 and UL84leucine zipper mutants fail to complement oriLyt-dependent DNAreplication. UL84 leucine zipper mutants no longer interferewith IE2-mediated transactivation of the UL112/113 promoter,confirming that the leucine zipper is essential for a functionalinteraction with IE2. In addition, we demonstrate that boththe leucine zipper and oligomerization domains of UL84 can actas transdominant-negative inhibitors of lytic replication inthe transient assay, strongly suggesting that both an IE2-UL84and a UL84-UL84 interaction are required for DNA synthesis.

* Corresponding author. Mailing address: University of Nevada-Reno, Department of Microbiology, School of Medicine, Howard Bldg., Reno, NV 89557. Phone: (775) 784-4824. Fax: (775) 327-2332. E-mail: gpari{at}med.unr.edu.

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