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dc.contributor.authorBerrios, Christianen_US
dc.contributor.authorPadi, Meghaen_US
dc.contributor.authorKeibler, Mark A.en_US
dc.contributor.authorPark, Donglim Estheren_US
dc.contributor.authorMolla, Vadimen_US
dc.contributor.authorCheng, Jingweien_US
dc.contributor.authorLee, Soo Mien_US
dc.contributor.authorStephanopoulos, Gregoryen_US
dc.contributor.authorQuackenbush, Johnen_US
dc.contributor.authorDeCaprio, James A.en_US
dc.date.accessioned2017-01-03T23:50:19Z
dc.date.issued2016en_US
dc.identifier.citationBerrios, Christian, Megha Padi, Mark A. Keibler, Donglim Esther Park, Vadim Molla, Jingwei Cheng, Soo Mi Lee, Gregory Stephanopoulos, John Quackenbush, and James A. DeCaprio. 2016. “Merkel Cell Polyomavirus Small T Antigen Promotes Pro-Glycolytic Metabolic Perturbations Required for Transformation.” PLoS Pathogens 12 (11): e1006020. doi:10.1371/journal.ppat.1006020. http://dx.doi.org/10.1371/journal.ppat.1006020.en
dc.identifier.issn1553-7366en
dc.identifier.urihttp://nrs.harvard.edu/urn-3:HUL.InstRepos:29739150
dc.description.abstractMerkel cell polyomavirus (MCPyV) is an etiological agent of Merkel cell carcinoma (MCC), a highly aggressive skin cancer. The MCPyV small tumor antigen (ST) is required for maintenance of MCC and can transform normal cells. To gain insight into cellular perturbations induced by MCPyV ST, we performed transcriptome analysis of normal human fibroblasts with inducible expression of ST. MCPyV ST dynamically alters the cellular transcriptome with increased levels of glycolytic genes, including the monocarboxylate lactate transporter SLC16A1 (MCT1). Extracellular flux analysis revealed increased lactate export reflecting elevated aerobic glycolysis in ST expressing cells. Inhibition of MCT1 activity suppressed the growth of MCC cell lines and impaired MCPyV-dependent transformation of IMR90 cells. Both NF-κB and MYC have been shown to regulate MCT1 expression. While MYC was required for MCT1 induction, MCPyV-induced MCT1 levels decreased following knockdown of the NF-κB subunit RelA, supporting a synergistic activity between MCPyV and MYC in regulating MCT1 levels. Several MCC lines had high levels of MYCL and MYCN but not MYC. Increased levels of MYCL was more effective than MYC or MYCN in increasing extracellular acidification in MCC cells. Our results demonstrate the effects of MCPyV ST on the cellular transcriptome and reveal that transformation is dependent, at least in part, on elevated aerobic glycolysis.en
dc.language.isoen_USen
dc.publisherPublic Library of Scienceen
dc.relation.isversionofdoi:10.1371/journal.ppat.1006020en
dc.relation.hasversionhttp://www.ncbi.nlm.nih.gov/pmc/articles/PMC5120958/pdf/en
dash.licenseLAAen_US
dc.subjectBiology and Life Sciencesen
dc.subjectBiochemistryen
dc.subjectMetabolismen
dc.subjectMetabolic Processesen
dc.subjectGlycolysisen
dc.subjectGeneticsen
dc.subjectGene Expressionen
dc.subjectCell Biologyen
dc.subjectCell Physiologyen
dc.subjectCell Metabolismen
dc.subjectComputational Biologyen
dc.subjectGenome Analysisen
dc.subjectTranscriptome Analysisen
dc.subjectGenomicsen
dc.subjectGene Regulationen
dc.subjectMetabolic Pathwaysen
dc.subjectPhysical Sciencesen
dc.subjectChemistryen
dc.subjectChemical Compoundsen
dc.subjectOrganic Compoundsen
dc.subjectCarbohydratesen
dc.subjectMonosaccharidesen
dc.subjectGlucoseen
dc.subjectOrganic Chemistryen
dc.subjectBiology and life sciencesen
dc.subjectGene expressionen
dc.subjectGene regulationen
dc.subjectSmall interfering RNAsen
dc.subjectNucleic acidsen
dc.subjectRNAen
dc.subjectNon-coding RNAen
dc.titleMerkel Cell Polyomavirus Small T Antigen Promotes Pro-Glycolytic Metabolic Perturbations Required for Transformationen
dc.typeJournal Articleen_US
dc.description.versionVersion of Recorden
dc.relation.journalPLoS Pathogensen
dash.depositing.authorPadi, Meghaen_US
dc.date.available2017-01-03T23:50:19Z
dc.identifier.doi10.1371/journal.ppat.1006020*
dash.contributor.affiliatedPark, Donglim
dash.contributor.affiliatedCheng, Jingwei
dash.contributor.affiliatedPadi, Megha
dash.contributor.affiliatedDeCaprio, James
dash.contributor.affiliatedQuackenbush, John
dc.identifier.orcid0000-0002-2702-5879


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