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Virus-like infection induces human β cell dedifferentiation
Masaya Oshima, Klaus-Peter Knoch, Marc Diedisheim, Antje Petzold, Pierre Cattan, Marco Bugliani, Piero Marchetti, Pratik Choudhary, Guo-Cai Huang, Stefan R. Bornstein, Michele Solimena, Olivier Albagli-Curiel, Raphael Scharfmann
Masaya Oshima, Klaus-Peter Knoch, Marc Diedisheim, Antje Petzold, Pierre Cattan, Marco Bugliani, Piero Marchetti, Pratik Choudhary, Guo-Cai Huang, Stefan R. Bornstein, Michele Solimena, Olivier Albagli-Curiel, Raphael Scharfmann
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Research Article Inflammation Virology

Virus-like infection induces human β cell dedifferentiation

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Abstract

Type 1 diabetes (T1D) is a chronic disease characterized by an autoimmune-mediated destruction of insulin-producing pancreatic β cells. Environmental factors such as viruses play an important role in the onset of T1D and interact with predisposing genes. Recent data suggest that viral infection of human islets leads to a decrease in insulin production rather than β cell death, suggesting loss of β cell identity. We undertook this study to examine whether viral infection could induce human β cell dedifferentiation. Using the functional human β cell line EndoC-βH1, we demonstrate that polyinosinic-polycytidylic acid (PolyI:C), a synthetic double-stranded RNA that mimics a byproduct of viral replication, induces a decrease in β cell–specific gene expression. In parallel with this loss, the expression of progenitor-like genes such as SOX9 was activated following PolyI:C treatment or enteroviral infection. SOX9 was induced by the NF-κB pathway and also in a paracrine non–cell-autonomous fashion through the secretion of IFN-α. Lastly, we identified SOX9 targets in human β cells as potentially new markers of dedifferentiation in T1D. These findings reveal that inflammatory signaling has clear implications in human β cell dedifferentiation.

Authors

Masaya Oshima, Klaus-Peter Knoch, Marc Diedisheim, Antje Petzold, Pierre Cattan, Marco Bugliani, Piero Marchetti, Pratik Choudhary, Guo-Cai Huang, Stefan R. Bornstein, Michele Solimena, Olivier Albagli-Curiel, Raphael Scharfmann

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Figure 6

Genes induced in EndoC-βH1 cells by SOX9.

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Genes induced in EndoC-βH1 cells by SOX9.
(A) EndoC-βH1 cells were eithe...
(A) EndoC-βH1 cells were either mock transfected (CTRL) or transfected with PolyI:C and analyzed 24 hours later. Heatmap from global transcriptomic analysis represents previously described SOX9 target genes (n = 3). (B–E) EndoC-βH1 cells were transfected with MCS-ires-GFP, SOX9WT-ires-GFP, VP16-ires-GFP, or VP16-SOX9ΔTAD-ires-GFP plasmid. GFP+ cells were sorted by FACS 48 hours later and RNAs were prepared (n = 2–6). (B and C) RT-qPCR analyses (n = 6). (D and E) Global transcriptomic analyses with Venn diagram and heatmap that represent genes upregulated (>1.5-fold) by SOX9WT-ires-GFP and VP16-SOX9ΔTAD-ires-GFP (n = 2). Data from RT-qPCR represent the mean ± SD. *P < 0.05, **P < 0.01 and ***P < 0.001 relative to control by Student’s t test. ns, not significant.

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