A Notch/IL-21 signaling axis primes bone marrow T cell progenitor expansion
Kilian Sottoriva, Na Yoon Paik, Zachary White, Thilinie Bandara, Lijian Shao, Teruyuki Sano, Kostandin V. Pajcini
Kilian Sottoriva, Na Yoon Paik, Zachary White, Thilinie Bandara, Lijian Shao, Teruyuki Sano, Kostandin V. Pajcini
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Research Article Hematology Transplantation

A Notch/IL-21 signaling axis primes bone marrow T cell progenitor expansion

Abstract

Long-term impairment in T cell–mediated adaptive immunity is a major clinical obstacle following treatment of blood disorders with hematopoietic stem cell transplantation. Although T cell development in the thymus has been extensively characterized, there are significant gaps in our understanding of prethymic processes that influence early T cell potential. We have uncovered a Notch/IL-21 signaling axis in bone marrow common lymphoid progenitor (CLP) cells. IL-21 receptor expression was driven by Notch activation in CLPs, and in vivo treatment with IL-21 induced Notch-dependent CLP proliferation. Taking advantage of this potentially novel signaling axis, we generated T cell progenitors ex vivo, which improved repopulation of the thymus and peripheral lymphoid organs of mice in an allogeneic transplant model. Importantly, Notch and IL-21 activation were equally effective in the priming and expansion of human cord blood cells toward the T cell fate, confirming the translational potential of the combined treatment.

Authors

Kilian Sottoriva, Na Yoon Paik, Zachary White, Thilinie Bandara, Lijian Shao, Teruyuki Sano, Kostandin V. Pajcini

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Figure 2

IL21r is a BM-specific Notch target.

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IL21r is a BM-specific Notch target. (A) Representative histogram for IL...
(A) Representative histogram for IL21r staining on BM CLP and thymic DN1, DN2, DN3, and CD8+ populations. (B) IL21r MFI normalized to isotype control for BM CLP and thymic DN1, DN2, DN3, and CD8+ populations (n = 3). (C) Expression of IL21r relative to GAPDH normalized to CLP determined by qRT-PCR of mRNA isolated from BM CLP and thymic DN3 and CD8+ cells from WT (n = 3) mice. (D) (Left) Representative flow plot of hematopoietic progenitor LinSca1+cKit+ (LSK) cells cultured on OP9-DL1 cells for 4 days, gated on live cells. (Right) Expression of Deptor and IL21r relative to GAPDH normalized to DMSO determined by qRT-PCR of mRNA isolated from DMSO and GSI-treated LSK 4-day cultures (n = 3). GSI added for final 24 hours. (E) (Left) Representative flow plot of LSK cells cultured on OP9-DL1 cells for 10 days, gated on live cells. (Right) Expression of Deptor and IL21r relative to GAPDH and normalized to DMSO determined by qRT-PCR of mRNA isolated from DMSO and GSI-treated 10-day LSK cultures on OP9-DL1 (n = 3). GSI added for final 24 hours. (F) Expression of Deptor, IL21r, and Hes1 relative to EF1α normalized to WT determined by qRT-PCR of mRNA isolated from sorted WT or Notch1+/ΔTAD thymic DN3 cells (n = 3). (G) (Left) Representative histograms for intracellular ICN1 of thymic DP, DN3, and BM CLP populations stained with anti-rabbit–Alexa Fluor 647 secondary antibody. Gray/filled = no primary antibody control, black/empty = ICN1. (Right) MFI of ICN1 normalized to secondary antibody control (n = 4). *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001. Statistical analysis performed using Student’s 2-tailed t test (DF) and 1-way ANOVA (B, C, and G).