Figure 4
Figure 4. CD48−/− BM microenvironment displays a dysregulation of cytokines. (A) BM supernatant was isolated from 8- to 12-week-old CD48−/− and WT mice, and using cytokine bead arrays we found a severe decrease in IFNγ and Cxcl9. Other cytokines showed a trend of lower levels in the CD48−/− BM (supplemental Figure 3). (B) Intracellular IFNγ was examined by flow cytometry in hematopoietic progenitors (KLS). A small but consistent population of IFNγ+ progenitors was observed, and the CD48−/− mice exhibited a smaller population of IFNγ+ cells in comparison to WT. (C) CD244 expression was examined in short-term progenitors (SPneg KLS) with TaqMan real-time PCR. CD244 was found to be 5-fold higher in the CD48−/− short-term progenitors. SYBR green real-time PCR was used to analyze the CD244 isoforms present in the short-term progenitors (SPneg KLS) and GAPDH was used as an external control. (D) The Itgb2-Vav-Pak-Erk pathway was examined by flow cytometry to determine whether it was up-regulated in the CD48−/− hematopoietic progenitors (KLS). The number of Itgb2+ cells was slightly increased in the CD48−/− KLS cells, moreover CD48−/− cells expressing Itgb2 did so at a higher level. (E) In addition, activation of Pak and Erk, as measured by phosphorylation, was significantly increased in the CD48−/− KLS cells (2-way ANOVA, P < .05).

CD48−/− BM microenvironment displays a dysregulation of cytokines. (A) BM supernatant was isolated from 8- to 12-week-old CD48−/− and WT mice, and using cytokine bead arrays we found a severe decrease in IFNγ and Cxcl9. Other cytokines showed a trend of lower levels in the CD48−/− BM (supplemental Figure 3). (B) Intracellular IFNγ was examined by flow cytometry in hematopoietic progenitors (KLS). A small but consistent population of IFNγ+ progenitors was observed, and the CD48−/− mice exhibited a smaller population of IFNγ+ cells in comparison to WT. (C) CD244 expression was examined in short-term progenitors (SPneg KLS) with TaqMan real-time PCR. CD244 was found to be 5-fold higher in the CD48−/− short-term progenitors. SYBR green real-time PCR was used to analyze the CD244 isoforms present in the short-term progenitors (SPneg KLS) and GAPDH was used as an external control. (D) The Itgb2-Vav-Pak-Erk pathway was examined by flow cytometry to determine whether it was up-regulated in the CD48−/− hematopoietic progenitors (KLS). The number of Itgb2+ cells was slightly increased in the CD48−/− KLS cells, moreover CD48−/− cells expressing Itgb2 did so at a higher level. (E) In addition, activation of Pak and Erk, as measured by phosphorylation, was significantly increased in the CD48−/− KLS cells (2-way ANOVA, P < .05).

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