Figure 2
Figure 2. Jak2FF/FF leads to partial IFN-γ signaling in primary macrophages and MEFs. (A) Jak2+/+, Jak2FF/FF, and Jak2−/− embryos (upper panel) and embryonic livers (lower panel) derived at E12.5. (B) Embryonic liver cells from Jak2+/+, Jak2+/FF, and Jak2FF/FF embryos were prepared at E12.5 and stimulated for 1 hour with Epo or left untreated. Cellular lysates were prepared and analyzed by immunoblotting using the indicated antibodies. (C) Fetal liver cells from Jak2+/+, Jak2FF/FF, and Jak2−/− embryos were prepared at E12.5 and were incubated with macrophage colony-stimulating factor for 6 days. FLDM were then stimulated with IFN-γ for 48 hours or left untreated. Cells were stained for F4/80 as a marker for mature macrophages. F4/80-positive cells were analyzed for MHC-I (H-2Kb) surface expression as a marker for IFN-γ signaling. One representative of 3 independent experiments run in triplicate is shown. The MHC-I expression of each genotype without stimulation was set as 100%. The standard deviation was below 3.7% of the detected values. ***P < .001. (D) MEFs from Jak2+/+, Jak2FF/FF, and Jak2−/− mice were stimulated in vitro with IFN-γ for the indicated time points. Subsequently, cellular lysates were prepared and analyzed by immunoblotting for expression of phospho-Stat1 (Y701), Stat1, and Jak2. β-actin served as a loading control. Results shown are representative of 3 independent experiments.

Jak2FF/FFleads to partial IFN-γ signaling in primary macrophages and MEFs. (A) Jak2+/+, Jak2FF/FF, and Jak2−/− embryos (upper panel) and embryonic livers (lower panel) derived at E12.5. (B) Embryonic liver cells from Jak2+/+, Jak2+/FF, and Jak2FF/FF embryos were prepared at E12.5 and stimulated for 1 hour with Epo or left untreated. Cellular lysates were prepared and analyzed by immunoblotting using the indicated antibodies. (C) Fetal liver cells from Jak2+/+, Jak2FF/FF, and Jak2−/− embryos were prepared at E12.5 and were incubated with macrophage colony-stimulating factor for 6 days. FLDM were then stimulated with IFN-γ for 48 hours or left untreated. Cells were stained for F4/80 as a marker for mature macrophages. F4/80-positive cells were analyzed for MHC-I (H-2Kb) surface expression as a marker for IFN-γ signaling. One representative of 3 independent experiments run in triplicate is shown. The MHC-I expression of each genotype without stimulation was set as 100%. The standard deviation was below 3.7% of the detected values. ***P < .001. (D) MEFs from Jak2+/+, Jak2FF/FF, and Jak2−/− mice were stimulated in vitro with IFN-γ for the indicated time points. Subsequently, cellular lysates were prepared and analyzed by immunoblotting for expression of phospho-Stat1 (Y701), Stat1, and Jak2. β-actin served as a loading control. Results shown are representative of 3 independent experiments.

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