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In vivo kinetics and nonradioactive imaging of rapidly proliferating cells in graft-versus-host disease
Nataliya P. Buxbaum, … , Remy J. Bosselut, Ronald E. Gress
Nataliya P. Buxbaum, … , Remy J. Bosselut, Ronald E. Gress
Published June 15, 2017
Citation Information: JCI Insight. 2017;2(12):e92851. https://doi.org/10.1172/jci.insight.92851.
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Resource and Technical Advance Immunology Transplantation

In vivo kinetics and nonradioactive imaging of rapidly proliferating cells in graft-versus-host disease

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Abstract

Hematopoietic stem cell transplantation (HSCT) offers a cure for cancers that are refractory to chemotherapy and radiation. Most HSCT recipients develop chronic graft-versus-host disease (cGVHD), a systemic alloimmune attack on host organs. Diagnosis is based on clinical signs and symptoms, as biopsies are risky. T cells are central to the biology of cGVHD. We found that a low Treg/CD4+ T effector memory (Tem) ratio in circulation, lymphoid, and target organs identified early and established mouse cGVHD. Using deuterated water labeling to measure multicompartment in vivo kinetics of these subsets, we show robust Tem and Treg proliferation in lymphoid and target organs, while Tregs undergo apoptosis in target organs. Since deuterium enrichment into DNA serves as a proxy for cell proliferation, we developed a whole-body clinically relevant deuterium MRI approach to nonradioactively detect cGVHD and potentially allow imaging of other diseases characterized by rapidly proliferating cells.

Authors

Nataliya P. Buxbaum, Donald E. Farthing, Natella Maglakelidze, Martin Lizak, Hellmut Merkle, Andrea C. Carpenter, Brittany U. Oliver, Veena Kapoor, Ehydel Castro, Gregory A. Swan, Liliane M. dos Santos, Nicolas J. Bouladoux, Catherine V. Bare, Francis A. Flomerfelt, Michael A. Eckhaus, William G. Telford, Yasmine Belkaid, Remy J. Bosselut, Ronald E. Gress

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Figure 4

Label loss kinetics for Tregs in the liver in allogeneic (allo) hematopoietic stem cell transplant recipients (HSCT) are driven by increased propensity for apoptosis rather than trafficking.

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Label loss kinetics for Tregs in the liver in allogeneic (allo) hematopo...
(A) Label loss kinetics for allogeneic liver–derived Treg and Tem cells. Data are representative of 3 independent experiments for day +14 and +28 (n = 5–8 mice per experiment per cohort). (B) Caspase 3 staining for CD4+ Treg and Tem subsets extracted from the spleen and liver at day +14 (n = 5 mice per cohort). (C) The mean total CD4+ T cell number measured in the peripheral blood of each experimental cohort at day +14 and +28. (D) The mean total Tem cell number measured in the peripheral blood of each experimental cohort at day +14 and +28. Data are representative of 4 independent experiments (n = 2–6 mice per experiment per cohort). For panels C and D, **P < 0.01, ***P < 0.001; Tukey’s test with 2-way ANOVA.

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