Figure 3
Figure 3. MIF deficiency leads to reduced numbers of TAMs and increased apoptosis of CLL cells. (A) MIF protein content determined by Western blotting in purified splenic macrophages and B cells and total splenocytes as control from TCL1+/wtMIFwt/wt and TCL1+/wtMIF−/− mice. β-actin as loading control. (B) Absolute numbers of CD68+ TAMs per mm2 in sections of enlarged spleens (top panel) and bone marrow (bottom panel) are higher in TCL1+/wtMIFwt/wt (n = 18) versus TCL1+/wtMIF−/− (n = 14) mice (spleen: P < .0001; bone marrow: P = .066). (C) Representative immunohistochemistry for CD68 in splenic sections of TCL1+/wtMIFwt/wt (top panel) and TCL1+/wtMIF−/− mice (bottom panel). Macrophage agglomerates (red, arrow) are present in spleens of TCL1+/wtMIFwt/wt mice, whereas macrophages are only sparsely distributed in TCL1+/wtMIF−/− mice. Insets represent negative control without primary antibody (10×magnification). Representative CD68/Ki67 double staining of TCL1+/wtMIFwt/wt and TCL1+/wtMIF−/− spleen showing accumulation of proliferating cells (brown) in areas of macrophage agglomeration in TCL1+/wtMIFwt/wt but not in TCL1+/wtMIF−/− spleen. (D) TUNEL-positive cells in splenic sections of TCL1+/wtMIFwt/wt and TCL1+/wtMIF−/− mice (n = 5 per genotype; 62 ± 7 in TCL1+/wtMIFwt/wt mice vs 192 ± 20 in TCL1+/wt MIF−/− mice; P < .0001). (E) Spontaneous and drug-induced rate of apoptosis as detected by flow cytometric positivity for annexin V/7-amino-actinomycin D in cultured nonleukemic splenocytes of TCL1+/wtMIF−/− versus TCL1+/wtMIFwt/wt mice. Cells were treated ex vivo with cytostatic drugs (50μM fludarabine, 61nM vincristine, 1μM prednisolone) for 24 hours. For each group and genotype, n = 5 independent splenocyte preparations were analyzed.

MIF deficiency leads to reduced numbers of TAMs and increased apoptosis of CLL cells. (A) MIF protein content determined by Western blotting in purified splenic macrophages and B cells and total splenocytes as control from TCL1+/wtMIFwt/wt and TCL1+/wtMIF−/− mice. β-actin as loading control. (B) Absolute numbers of CD68+ TAMs per mm2 in sections of enlarged spleens (top panel) and bone marrow (bottom panel) are higher in TCL1+/wtMIFwt/wt (n = 18) versus TCL1+/wtMIF−/− (n = 14) mice (spleen: P < .0001; bone marrow: P = .066). (C) Representative immunohistochemistry for CD68 in splenic sections of TCL1+/wtMIFwt/wt (top panel) and TCL1+/wtMIF−/− mice (bottom panel). Macrophage agglomerates (red, arrow) are present in spleens of TCL1+/wtMIFwt/wt mice, whereas macrophages are only sparsely distributed in TCL1+/wtMIF−/− mice. Insets represent negative control without primary antibody (10×magnification). Representative CD68/Ki67 double staining of TCL1+/wtMIFwt/wt and TCL1+/wtMIF−/− spleen showing accumulation of proliferating cells (brown) in areas of macrophage agglomeration in TCL1+/wtMIFwt/wt but not in TCL1+/wtMIF−/− spleen. (D) TUNEL-positive cells in splenic sections of TCL1+/wtMIFwt/wt and TCL1+/wtMIF−/− mice (n = 5 per genotype; 62 ± 7 in TCL1+/wtMIFwt/wt mice vs 192 ± 20 in TCL1+/wt MIF−/− mice; P < .0001). (E) Spontaneous and drug-induced rate of apoptosis as detected by flow cytometric positivity for annexin V/7-amino-actinomycin D in cultured nonleukemic splenocytes of TCL1+/wtMIF−/− versus TCL1+/wtMIFwt/wt mice. Cells were treated ex vivo with cytostatic drugs (50μM fludarabine, 61nM vincristine, 1μM prednisolone) for 24 hours. For each group and genotype, n = 5 independent splenocyte preparations were analyzed.

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