Figure 6
Figure 6. Tumor stage-specific macrophage repolarization in the myeloma niche in the absence of Tpl2. Macrophage polarization was assessed using flow cytometric analysis of C11b+/F4/80+ macrophages from BMs of age-matched (8-month old) and “tumor matched” wild-type (Vκ*MYC/Tpl2+/+) and Vκ*MYC/Tpl2−/− animals. Representative results from 3 animals in each group are shown. The C11b+/F4/80+ gate is shown to the left. The dot plots represent the frequency of the M1-like fraction (CD68int/Ly6Cint) and M2-like fraction (CD68hi/Ly6Chi) in the total C11b+/F4/80+ gate in each genotype. M1 polarization has been shown to result in downregulation of CD68 in macrophages.76 On the right panels, histograms depict the relative frequency of iNOS+ and Arginase-1+ cells in each subpopulation, depicted in RED (M1-like) and BLUE (M2-like). APC, allophycocyanin; FITC, fluorescein isothiocyanate; PE, phycoerythrin.

Tumor stage-specific macrophage repolarization in the myeloma niche in the absence of Tpl2. Macrophage polarization was assessed using flow cytometric analysis of C11b+/F4/80+ macrophages from BMs of age-matched (8-month old) and “tumor matched” wild-type (Vκ*MYC/Tpl2+/+) and Vκ*MYC/Tpl2−/− animals. Representative results from 3 animals in each group are shown. The C11b+/F4/80+ gate is shown to the left. The dot plots represent the frequency of the M1-like fraction (CD68int/Ly6Cint) and M2-like fraction (CD68hi/Ly6Chi) in the total C11b+/F4/80+ gate in each genotype. M1 polarization has been shown to result in downregulation of CD68 in macrophages.76  On the right panels, histograms depict the relative frequency of iNOS+ and Arginase-1+ cells in each subpopulation, depicted in RED (M1-like) and BLUE (M2-like). APC, allophycocyanin; FITC, fluorescein isothiocyanate; PE, phycoerythrin.

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