Figure 1
Figure 1. Selective loss of CD8α+ DCs in Nfil3−/− mice and impaired Flt3-dependent development of CD8α+ DCs in the absence of NFIL3. (A) Nfil3 is highly expressed in DC subsets. Quantitative real-time RT-PCR analysis of Nfil3 mRNA in purified cells (NKs and DCs) or in vitro stimulated cells (B and T cells) was performed. Data show the mean and SD from 3 experiments. (B) Splenocytes from Nfil3+/+ or Nfil3−/− mice were stained for CD11c and PDCA-1 to identify pDCs and cDCs (left) and for CD11c, CD8, CD4, DEC-205, SIRP-α, and CD24 to detect CD8α+ DCs and CD8α − DCs (middle) or to detect CD8α+ DC precursors in CD8α−CD4− DCs (right). Data are representative of 5 experiments with similar results. (C) Thy1.2− thymocytes from Nfil3+/+ or Nfil3−/− mice were stained for CD11c and PDCA-1 to identify pDCs and cDCs (left) and for CD11c, CD8, DEC-205, SIRP-α, and CD24 to detect CD8α+ DCs (right). Data are representative of 5 experiments with similar results. (D) Number of CD8α+DEC-205+ cDCs in spleen and thymus from Nfil3+/+ (○) and Nfil3−/− (●) mice. Cell numbers were calculated on the basis of analyses by flow cytometry (n = 5; *P < .001, **P < .0001). (E) Impaired IL-12 production by splenic DCs in response to polyinosinic:polycytidylic acid [Poly (I:C)] in Nfil3−/− mice. CD11chi cDCs were enriched by a MACS system with anti-Thy1.2 and anti-B220 beads for depletion of T cells, B cells, and pDCs, followed by anti-CD11c beads for isolation of cDCs. Enriched cDCs were unstimulated or stimulated with CpG (0.5 μg/mL), lipopolysaccharide (LPS; 100 μg/mL), or Poly (I:C) (100 μg/mL) for 4 hours. One hour after stimulation, brefeldin A was added to the culture. After stimulation, cells were stained for CD11c and CD45RA, followed by intracellular staining for IL-12. Data are representative of 4 experiments with similar results. (F) Developmental defect of Nfil3−/− BM progenitor cells to CD8α+-equivalent cDCs. BM cells from Nfil3+/+ or Nfil3−/− mice were cultured with FL (50 ng/mL) for 9 days and stained for CD11c, CD45RA, SIRP-α, and CD24. Data are representative of 3 experiments with similar results. (G) FL-DCs from Nfil3+/+ or Nfil3−/− mice were stimulated with Poly (I:C) (100 μg/mL) for 4 hours and stained for IL-12. Data are representative of 3 experiments with similar results. (H) Lack of FL-dependent development of CD8α+ cDC in vivo. Nfil3−/− and Nfil3+/+ mice were injected with B16-FL cells subcutaneously, and spleens were harvested 8 days after injection. Splenocytes were analyzed for CD11c+ (left), and CD8α+ cDCs (right) by flow cytometry. Data are representative of 3 independent experiments. (I) Equal numbers of BM progenitor cells between Nfil3−/− and Nfil3+/+ mice. BM cells from Nfil3−/− and Nfil3+/+ mice were stained for LSK (Lin−c-kithiSca-1+CD127−), CLPs (common lymphoid progenitors; Lin−c-kitintSca-1intCD127+), CMP/GMP/MEPs (myeloid progenitors; Lin−c-kithiSca-1−CD127−), CDPs (common DC progenitors; Lin−Flt3+c-kitloCD127-CD115+), and pre-cDCs (Lin−CD11c+MHCII-Flt3+SIRP-αlo), and cell numbers of each population per 1 × 106 BM cells were calculated. Each dot represents an individual mouse, and gray lines indicate mean cell number. (J) Relative expression of Batf3, Irf8, Id2, Irf4, and Nfil3 genes in Nfil3−/− and Nfil3+/+ BM pre-cDCs was determined by quantitative real-time RT-PCR. Mean expression of RNA in wild-type cells was set as 1. The mean and SD of 2 independent experiments are shown. (K) Rescue of CD8α+-equivalent cDCs by BATF3 and NFIL3 transduction. Nfil3−/− BM cells stimulated with FL were transduced with vector or Batf3- or Nfil3-carrying viruses and cultured for 9 days, then stained for CD11c, CD45RA, SIRP-α, and CD24. Virus-infected cells (green fluorescent protein–positive cells) were analyzed. Data are representative of 3 experiments with similar results.

Selective loss of CD8α+ DCs in Nfil3−/− mice and impaired Flt3-dependent development of CD8α+ DCs in the absence of NFIL3. (A) Nfil3 is highly expressed in DC subsets. Quantitative real-time RT-PCR analysis of Nfil3 mRNA in purified cells (NKs and DCs) or in vitro stimulated cells (B and T cells) was performed. Data show the mean and SD from 3 experiments. (B) Splenocytes from Nfil3+/+ or Nfil3−/− mice were stained for CD11c and PDCA-1 to identify pDCs and cDCs (left) and for CD11c, CD8, CD4, DEC-205, SIRP-α, and CD24 to detect CD8α+ DCs and CD8α DCs (middle) or to detect CD8α+ DC precursors in CD8αCD4 DCs (right). Data are representative of 5 experiments with similar results. (C) Thy1.2 thymocytes from Nfil3+/+ or Nfil3−/− mice were stained for CD11c and PDCA-1 to identify pDCs and cDCs (left) and for CD11c, CD8, DEC-205, SIRP-α, and CD24 to detect CD8α+ DCs (right). Data are representative of 5 experiments with similar results. (D) Number of CD8α+DEC-205+ cDCs in spleen and thymus from Nfil3+/+ (○) and Nfil3−/− (●) mice. Cell numbers were calculated on the basis of analyses by flow cytometry (n = 5; *P < .001, **P < .0001). (E) Impaired IL-12 production by splenic DCs in response to polyinosinic:polycytidylic acid [Poly (I:C)] in Nfil3−/− mice. CD11chi cDCs were enriched by a MACS system with anti-Thy1.2 and anti-B220 beads for depletion of T cells, B cells, and pDCs, followed by anti-CD11c beads for isolation of cDCs. Enriched cDCs were unstimulated or stimulated with CpG (0.5 μg/mL), lipopolysaccharide (LPS; 100 μg/mL), or Poly (I:C) (100 μg/mL) for 4 hours. One hour after stimulation, brefeldin A was added to the culture. After stimulation, cells were stained for CD11c and CD45RA, followed by intracellular staining for IL-12. Data are representative of 4 experiments with similar results. (F) Developmental defect of Nfil3−/− BM progenitor cells to CD8α+-equivalent cDCs. BM cells from Nfil3+/+ or Nfil3−/− mice were cultured with FL (50 ng/mL) for 9 days and stained for CD11c, CD45RA, SIRP-α, and CD24. Data are representative of 3 experiments with similar results. (G) FL-DCs from Nfil3+/+ or Nfil3−/− mice were stimulated with Poly (I:C) (100 μg/mL) for 4 hours and stained for IL-12. Data are representative of 3 experiments with similar results. (H) Lack of FL-dependent development of CD8α+ cDC in vivo. Nfil3−/− and Nfil3+/+ mice were injected with B16-FL cells subcutaneously, and spleens were harvested 8 days after injection. Splenocytes were analyzed for CD11c+ (left), and CD8α+ cDCs (right) by flow cytometry. Data are representative of 3 independent experiments. (I) Equal numbers of BM progenitor cells between Nfil3−/− and Nfil3+/+ mice. BM cells from Nfil3−/− and Nfil3+/+ mice were stained for LSK (Linc-kithiSca-1+CD127), CLPs (common lymphoid progenitors; Linc-kitintSca-1intCD127+), CMP/GMP/MEPs (myeloid progenitors; Linc-kithiSca-1CD127), CDPs (common DC progenitors; LinFlt3+c-kitloCD127-CD115+), and pre-cDCs (LinCD11c+MHCII-Flt3+SIRP-αlo), and cell numbers of each population per 1 × 106 BM cells were calculated. Each dot represents an individual mouse, and gray lines indicate mean cell number. (J) Relative expression of Batf3, Irf8, Id2, Irf4, and Nfil3 genes in Nfil3−/− and Nfil3+/+ BM pre-cDCs was determined by quantitative real-time RT-PCR. Mean expression of RNA in wild-type cells was set as 1. The mean and SD of 2 independent experiments are shown. (K) Rescue of CD8α+-equivalent cDCs by BATF3 and NFIL3 transduction. Nfil3−/− BM cells stimulated with FL were transduced with vector or Batf3- or Nfil3-carrying viruses and cultured for 9 days, then stained for CD11c, CD45RA, SIRP-α, and CD24. Virus-infected cells (green fluorescent protein–positive cells) were analyzed. Data are representative of 3 experiments with similar results.

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