Type I IFN response associated with mTOR activation in the TAFRO subtype of idiopathic multicentric Castleman disease
Ruth-Anne Langan Pai, Alberto Sada Japp, Michael Gonzalez, Rozena F. Rasheed, Mariko Okumura, Daniel Arenas, Sheila K. Pierson, Victoria Powers, Awo Akosua Kesewa Layman, Charlly Kao, Hakon Hakonarson, Frits van Rhee, Michael R. Betts, Taku Kambayashi, David C. Fajgenbaum
Ruth-Anne Langan Pai, Alberto Sada Japp, Michael Gonzalez, Rozena F. Rasheed, Mariko Okumura, Daniel Arenas, Sheila K. Pierson, Victoria Powers, Awo Akosua Kesewa Layman, Charlly Kao, Hakon Hakonarson, Frits van Rhee, Michael R. Betts, Taku Kambayashi, David C. Fajgenbaum
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Research Article Hematology Immunology

Type I IFN response associated with mTOR activation in the TAFRO subtype of idiopathic multicentric Castleman disease

Abstract

The TAFRO clinical subtype of idiopathic multicentric Castleman disease (iMCD-TAFRO) is a rare hematologic illness involving episodic disease flares of thrombocytopenia, anasarca, fever, reticulin myelofibrosis, renal dysfunction, and organomegaly (TAFRO) and progressive multiple organ dysfunction. We previously showed that the mTOR signaling pathway is elevated in lymph nodes of iMCD-TAFRO patients and that an mTOR inhibitor is effective in a small cohort of patients. However, the upstream mechanisms, cell types, and mediators involved in disease pathogenesis remain unknown. Here, we developed a targeted approach to identify candidate cellular drivers and mechanisms in iMCD-TAFRO through cellular and transcriptomic studies. Using paired iMCD-TAFRO PBMC samples collected during flare and remission, we identified T cell activation and alterations in NK cell and monocyte subset frequencies during iMCD-TAFRO flare. These changes were associated with increased Type I IFN (IFN-I) response gene signatures across CD8+ T cells, NK cells, and monocytes. Finally, we found that IFN-β stimulation of monocytes and T cells from iMCD-TAFRO patient remission samples induced increased mTOR activation compared with healthy donors, and this was abrogated with either mTORC1 or JAK1/2 inhibition. The data presented here support a potentially novel role for IFN-I signaling as a driver of increased mTOR signaling in iMCD-TAFRO.

Authors

Ruth-Anne Langan Pai, Alberto Sada Japp, Michael Gonzalez, Rozena F. Rasheed, Mariko Okumura, Daniel Arenas, Sheila K. Pierson, Victoria Powers, Awo Akosua Kesewa Layman, Charlly Kao, Hakon Hakonarson, Frits van Rhee, Michael R. Betts, Taku Kambayashi, David C. Fajgenbaum

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Figure 7

Induction of mTOR signaling downstream of IFN-β in iMCD-TAFRO.

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Induction of mTOR signaling downstream of IFN-β in iMCD-TAFRO. (A) Schem...
(A) Schematic detailing Type I IFN proximal signaling to JAK, downstream activation of mTOR to phosphorylate ribosomal protein S6, and parallel engagement of p38 and pSTAT1/pSTAT2 leading to expression of IFN-stimulated genes (ISGs). Created with www.BioRender.com (B–D) Percent of healthy donor (black) cells (n = 8) and iMCD-TAFRO remission (blue) cells (n = 8) expressing phosphorylated ribosomal protein S6 (S235/S236) upon stimulation with 100 ng/mL IFN-β for 0, 30, 60, or 120 minutes within CD14+ classical monocytes (B), CD4+ T cells (C), and CD8+ T cells (D). (E–G) Percent of iMCD-TAFRO remission cells (n = 8) expressing phosphorylated ribosomal protein S6 (S235/S236) upon stimulation with 100 ng/mL IFN-β for 0 or 120 minutes within CD14+ classical monocytes (E), CD4+ T cells (F), and CD8+ T cells (G). (H–J) Comparison of the change in the percentage of cells compared with untreated samples expressing phosphorylated ribosomal protein S6 (S235/S236) following treatment with either 100 ng/mL IFN-β alone or both IFN-β and 1 μM JAKi within CD14+ classical monocytes (H), CD4+ T cells (I), and CD8+ T cells (J) from iMCD-TAFRO samples from remission. Data are mean ± SEM. For time-dependent comparisons, P values are based on 2-way ANOVA with Bonferroni’s correction for multiple comparisons. P values are based on 1-tailed, paired t tests between samples treated with IFN-β and IFN-β and JAKi.