Regulation of Transcriptional Activity of Merkel Cell Polyomavirus Large T-Antigen by PKA-Mediated Phosphorylation

Mar Falquet; Carla Prezioso; Maria Ludvigsen; Jack-Ansgar Bruun; Sara Passerini; Baldur Sveinbjørnsson; Valeria Pietropaolo; Ugo Moens

doi:10.3390/ijms24010895

Regulation of Transcriptional Activity of Merkel Cell Polyomavirus Large T-Antigen by PKA-Mediated Phosphorylation

Int J Mol Sci. 2023 Jan 3;24(1):895. doi: 10.3390/ijms24010895.

Authors

Mar Falquet¹, Carla Prezioso^{2

3}, Maria Ludvigsen¹, Jack-Ansgar Bruun⁴, Sara Passerini³, Baldur Sveinbjørnsson^{1

5}, Valeria Pietropaolo³, Ugo Moens²

Affiliations

¹ Molecular Inflammation Research Group, Department of Medical Biology, University of Tromsø-The Arctic University of Norway, 9037 Tromsø, Norway.
² Microbiology of Chronic Neuro-Degenerative Pathologies, IRCSS San Raffaele, 00163 Rome, Italy.
³ Department of Public Health and Infectious Diseases, Sapienza University of Rome, 00185 Rome, Italy.
⁴ Department of Medical Biology, Proteomics Platform, University of Tromsø-The Arctic University of Norway, 9037 Tromsø, Norway.
⁵ Childhood Cancer Research Unit, Department of Women's and Children's Health, Karolinska Institute, 17177 Stockholm, Sweden.

Abstract

Merkel cell polyomavirus (MCPyV) is the major cause of Merkel cell carcinoma (MCC), an aggressive skin cancer. MCPyV large T-antigen (LTag) and small T-antigen (sTag) are the main oncoproteins involved in MCPyV-induced MCC. A hallmark of MCPyV-positive MCC cells is the expression of a C-terminal truncated LTag. Protein kinase A (PKA) plays a fundamental role in a variety of biological processes, including transcription by phosphorylating and thereby regulating the activity of transcription factors. As MCPyV LTag has been shown to be phosphorylated and acts as a transcription factor for the viral early and late promoter, we investigated whether LTag can be phosphorylayted by PKA, and whether this affects the transcript activity of LTag. Using a phosphorylation prediction algorithm, serine 191, 203, and 265 were identified as putative phosphorylation sites for PKA. Mass spectrometry of in vitro PKA-phosphorylated peptides confirmed phosphorylation of S203 and S265, but not S191. Full-length LTag inhibited early and late promoter activity of MCPyV, whereas the truncated MKL2 LTag variant stimulated both promoters. Single non-phosphorylable, as well as phosphomimicking mutations did not alter the inhibitory effect of full-length LTag. However, the non-phosphorylable mutations abrogated transactivation of the MCPyV promoters by MKL2 LTag, whereas phosphomimicking substitutions restored the ability of MKL2 LTag to activate the promoters. Triple LTag and MKL2 LTag mutants had the same effect as the single mutants. Activation of the PKA signaling pathway did not enhance MCPyV promoter activity, nor did it affect LTag expression levels in MCPyV-positive Merkel cell carcinoma (MCC) cells. Our results show that phosphorylation of truncated LTag stimulates viral promoter activity, which may contribute to higher levels of the viral oncoproteins LTag and sTag. Interfering with PKA-induced LTag phosphorylation/activity may be a therapeutic strategy to treat MCPyV-positive MCC patients.

Keywords: Merkel cell carcinoma; Merkel cell polyomavirus; PKA; forskolin; large T-antigen; phosphorylation.

MeSH terms

Antigens, Polyomavirus Transforming* / metabolism
Carcinoma, Merkel Cell* / metabolism
Carcinoma, Merkel Cell* / virology
Cyclic AMP-Dependent Protein Kinases / genetics
Cyclic AMP-Dependent Protein Kinases / metabolism
Humans
Merkel cell polyomavirus* / metabolism
Phosphorylation
Polyomavirus Infections* / metabolism
Polyomavirus Infections* / virology
Skin Neoplasms* / metabolism
Skin Neoplasms* / virology
Transcription, Genetic
Tumor Virus Infections* / metabolism
Tumor Virus Infections* / virology

Substances

Cyclic AMP-Dependent Protein Kinases
Antigens, Polyomavirus Transforming

Abstract

MeSH terms

Substances

Grants and funding