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The IFI16 restriction factor cooperates with HCMV pUL83 to down-regulate UL54 gene expression and viral DNA synthesis

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23 July 2021

AperTO - Archivio Istituzionale Open Access dell'Università di Torino

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The IFI16 restriction factor cooperates with HCMV pUL83 to down-regulate UL54 gene expression and viral DNA synthesis

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DOI:10.1016/j.cyto.2015.08.067 Terms of use:

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The IFI16 restriction factor cooperates with HCMV pUL83 to down-regulate UL54 gene expression and viral DNA synthesis

Matteo Biolatti1, Sara Pautasso1, Valentina Dell’Oste1, Marco De Andrea1,2, Jens von Einem3, Bodo Plachter4, Manfred Marschall5, Marisa Gariglio2, Santo Landolfo1

1

University of Turin, Turin, Italy; 2University of Piemonte Orientale “A. Avogadro”, Novara, Italy;

3

University Hospital Ulm, Ulm, Germany; 4University Medical Center of the Johannes Gutenberg, Mainz, Germany; 5University of Erlangen-Nürnberg, Erlangen, Germany

During the early phase of human cytomegalovirus (HCMV) infection, the Interferon-γ -Inducible factor 16 (IFI16) behaves as a pattern recognition receptor (PRR) sensing viral DNA and triggering antiviral cytokine release. Later on, it restricts virus replication by down-regulating expression of viral genes committed to DNA synthesis including UL54 and UL44. These activities are modulated by viral proteins including pUL83, a tegument protein involved in viral evasion. Here, we demonstrate that pUL83 interacts with IFI16 relieving its inhibitory activity on UL54 gene transcription. We also establish that, starting from 48 h post-infection, IFI16 is stabilized and protected from degradation by pUL83 as observed infecting human foreskin fibroblasts with the wild type HCMV strain (v65Rev) or the v65Stop lacking pUL83 expression. Upon infection with an HCMV mutant virus (RV-VM1) expressing a pUL83 lacking the nuclear egression signal (NES), IFI16 is retained in the nucleus and does not migrate into the cytoplasm. Interestingly, accumulation of nuclear pUL83 preventes the formation of discrete puncta and dissipates aggregation of IFI16 filaments. We observe that IFI16 shows an half-life of less than 1 h in the absence of pUL83 compared with 2 h in the presence of pUL83 demonstrating that IFI16 is less stable in the absence of pUL83. Consistent with this, we observe restoration of IFI16 protein in v65Stop-infected cells compared to v65Rev-infected cells in presence of the proteasome inhibitor MG132. Our results demonstrate a novel role for the pUL83 protein that stabilizes and protects IFI16 from proteasome degradation during HCMV infection and modulates suppression of UL54 gene activity

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