1. Efficient cytokine-induced IL-13 production by mast cells requires both IL-33 and IL-3 
Ilkka S. Junttila, MD, PhD, Cynthia Watson, BSc, Laura Kummola, MSc, Xi Chen, MD, Jane Hu-Li, BSc, Liying Guo, PhD, Ryoji Yagi, PhD, William E. Paul, MD 
Journal of Allergy and Clinical Immunology 
Volume 132, Issue 3, Pages e10 (September 2013)
DOI: /j.jaci
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2. Fig 1
Generation and characterization of IL-13 DsRed reporter mice. A, Strategy and transgenic construct used to generate IL-13 DsRed mice. B, Southern blot analysis identifying DsRed+ pups. C, Correlation of IL-13 protein production with DsRed intensity. D, Correlation of IL-13 and DsRed mRNA expression in purified BMMCs.
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3. Fig 2
Peritoneal cavity mast cell IL-33−mediated IL-13 production requires an IL-3−STAT5 signal. A, DsRed expression in c-Kit+/FcεRI+ cells from peritoneal cavities of WT and DsRed mice on cytokine stimulation. B, DsRed expression in response to various STAT5 activators among c-Kit+/FcεRI+ cells. C, STAT5 activation in response to different cytokines in c-Kit+/FcεRI+ cells of the B6 peritoneal cavity. The red line indicates the basal level of STAT5 phosphorylation in unstimulated cells. TSLP, Thymic stromal lymphopoietin.
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4. Fig 3
BMMCs and bone marrow−derived basophils respond to exogenous IL-18 and IL-33. A, DsRed expression in BMMCs from DsRed transgenic mice on cytokine stimulation. B, DsRed expression in bone marrow−derived basophils from DsRed transgenic mice on cytokine stimulation. C, DsRed background in bone marrow cultures is located in basophils and mast cells. D, T1-ST2 mAb decreases DsRed expression in BMMCs. SSC, Side scatter.
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5. Fig 4
MyDd88 expression coupled with strong STAT5 phosphorylation is required for optimal IL-13 expression from BMMCs in response to IL-33. A, MyD88−/− BMMCs do not express IL-13 in response to IL-33. B, IL-3 replacement with IL-4 decreases STAT5 phosphorylation of BMMC STAT5. C, IL-3 replacement with IL-4 decreases IL-33−induced DsRed expression. D, STAT5 phosphorylation is not affected by deletion of MyD88.
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6. Fig 5
Expression of T1-ST2 in mast cells. A, T1-ST2 surface staining is specific because TH2 cells express high levels of T1-ST2. B, Effect of cytokines on T1-ST2 expression in peritoneal cavity mast cells (PCMCs) and BMMCs. C, Quantitation of T1-ST2 expression in BMMCs and PCMCs. D, IL-3 replacement with IL-4 does not affect T1-ST2 expression in BMMCs. E, MyD88 does not regulate T1-ST2 expression.
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7. Fig 6
IL-18 and IL-33 receptor expression in BMMCs and bone marrow−derived basophils. A, IL-18Rα expression in bone marrow−derived basophils and BMMCs. B, T1-ST2 expression in bone marrow−derived basophils and BMMCs. C, Quantitation of IL-18Rα and T1-ST2 expression in bone marrow−derived basophils and BMMCs from 4 independent experiments.
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8. Fig E1
TH2-differentiated CD4 T cells from different DsRed transgenic mice indicate good correlation between the proportion of DsRed+ cells and the frequency of IL-4−producing cells. The founders of the mice used in experiments described in this report were K-1.
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9. Fig E2
Identifying mast cells in mouse peritoneal exudate. Live cell gate indicates a small consistent c-Kit/FcεRI−positive population in peritoneal cavities of both B6 and DsRed transgenic (Tg) mice.
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10. Fig E3
DsRed production in response to IL-1 family members and IL-3 in bone marrow−derived mast cells cultured for 40 days in IL-3. To quantitate the data, the induction of DsRed in 3 experiments on day 12 and day 40 BMMCs is shown with means and SEMs of DsRed+ cells.
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11. Fig E4
Splenocytes from 1 WT mouse (upper panel) and 2 DsRed transgenic mice (middle and lower panels) were stimulated as indicated for 4 hours. Subsequently, DsRed expression of FcεRI+/B220− cells was measured (x-axis). Numbers indicate the percentage of DsRed+ FcεRI+/B220− cells.
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12. Fig E5
IL-6 production by WT BMMCs. Cells were stimulated as indicated for 4 hours in the presence of brefeldin A and stained for FcεRI, c-Kit, and IL-6. Cells shown here are FcεRI+/c-Kit+. The lower panel shows means and SEMs from 3 independent experiments.
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13. Fig E6
IL-13 production by WT and Myd88−/− bone marrow–derived basophils. Cells were stimulated as indicated for 5 hours and stained for FcεRI, c-Kit, and IL-13. Cells shown here are FcεRI+/c-Kit−.
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14. Fig E7
DsRed production in response to IL-3 and IL-33 by bone marrow–derived mast cells cultured for 40 days in IL-3, followed by a 2-day culture in IL-3 or SCF. Data from 3 experiments shows means and SEMs. STAT5 phosphorylation in BMMCs cultured in SCF or IL-3 is shown, as well as quantitation of the data from 3 experiments. Means and SEMs of specific STAT5 phosphorylation retracted by isotype controls are shown.
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15. Fig E8
STAT5 phosphorylation in WT and MyD88−/− bone marrow–derived basophils. FcεRI+/c-Kit− cells from 10-day IL-3 culture were stained for phospho-STAT5 before the cells were stimulated with IL-33 or IL-3 plus IL-33 (as in Fig 4, D).
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16. Fig E9
Expression of the receptor for IL-33 in peritoneal cavity mast cells. Cells from peritoneal cavity flushes were stained immediately after flushing for c-Kit and FcεRI. Simultaneously, cells were stained for T1-ST2 (blue histogram) or isotype control (red histogram). c-Kit/FcεRI double-positive cells that had neither T1-ST2 nor isotype control staining overlapped completely with isotype control staining.
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17. Fig E10
IL-18R expression by splenic basophils. Splenocytes from WT B6 mice were stained with B220/FcεRI and either IL-18Rα mAb or unstained control. The upper right panel shows IL-18Rα expression on B cells (B220+/FcεRI−). The lower right panel shows IL-18Rα expression on basophils (FcεRI+/B220−). Splenic basophil IL-18Rα expression is higher than bone marrow–derived basophil IL-18Rα expression (see Fig 6, A).
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