![Fig. 1. Stages of cell differentiation of murine BM DCs generated in GM-CSF + IL-4. / (A-B) Phenotype of BM DCs analyzed by flow cytometry. Cells were labeled with Cy-Chrome anti-CD11c, PE anti-CD86, and one of the following FITC-labeled mAbs: anti–MHC-I, anti–MHC-II, anti-CD40, anti-CD80, anti-CD11b, anti-CD54, or anti–OX-40L. Flow profiles illustrate the expression of specific markers on CD86− DC (gray profiles) and on CD86+ DC (open profiles, thick line). Isotype controls are represented by open profiles in dashed lines. (C) FITC-dextran and FITC-albumin uptake by CD11c+immunobead-sorted CD86− and CD86+ DC. Only CD86− DCs internalized FITC-dextran and FITC-albumin at 37°C, a phenomenon down-regulated at 0°C. Results are representative of 3 independent experiments. (D) Allostimulatory activity of γ-irradiated, FACS-sorted CD86− (▾), or CD86+ B10 DC (▿), assessed using C3H splenic T cells as responders. B10 (H2b) DC (d 7) were set up at graded concentrations with 2 × 105 responder naive C3H (H2k) T cells, and the cultures were maintained for 72 hours. [3H]TdR was added 18 hours before harvesting. The MLR stimulatory activity of freshly isolated allogeneic (B10 [○]) or syngeneic (C3H [●]) bulk spleen cells is also shown. Results are expressed as mean cpm ± 1 SD and are representative of at least 3 separate experiments.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/98/5/10.1182_blood.v98.5.1512/5/h81711484001.jpeg?Expires=1724240895&Signature=HGZd7u4UnGa~NQ8n70SwtjSet7iK92HdXhijGvl8jBC4x5mEtGofJOnoswwYAqQEkz5f4lVJAUMmO13TiSj9Q3Dt5S~9MsL8nVMwUPibGc47rY8qxaW1GUb0bjDsNWKB9IFp1Cyig-owm35nSdoocY1YsC2DAYz5Mn8dkez5MkWmRTvrvP6qf8sawBg4MB2AuDy8dnIseTxEvUN3kjYy0PRrtquQH-0i3tkRaDC-fzBzcsWVeP4hpz-PgJ~TzHb7NYzh2REuy1GmLJL71XjwIIsMen5Hl1Enomy52VAIJwn9LoQEYBaNaD~QTerCtbDu1GUKmXqXwxBkaDwHfXj4xA__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Stages of cell differentiation of murine BM DCs generated in GM-CSF + IL-4.
(A-B) Phenotype of BM DCs analyzed by flow cytometry. Cells were labeled with Cy-Chrome anti-CD11c, PE anti-CD86, and one of the following FITC-labeled mAbs: anti–MHC-I, anti–MHC-II, anti-CD40, anti-CD80, anti-CD11b, anti-CD54, or anti–OX-40L. Flow profiles illustrate the expression of specific markers on CD86− DC (gray profiles) and on CD86+ DC (open profiles, thick line). Isotype controls are represented by open profiles in dashed lines. (C) FITC-dextran and FITC-albumin uptake by CD11c+immunobead-sorted CD86− and CD86+ DC. Only CD86− DCs internalized FITC-dextran and FITC-albumin at 37°C, a phenomenon down-regulated at 0°C. Results are representative of 3 independent experiments. (D) Allostimulatory activity of γ-irradiated, FACS-sorted CD86− (▾), or CD86+ B10 DC (▿), assessed using C3H splenic T cells as responders. B10 (H2b) DC (d 7) were set up at graded concentrations with 2 × 105 responder naive C3H (H2k) T cells, and the cultures were maintained for 72 hours. [3H]TdR was added 18 hours before harvesting. The MLR stimulatory activity of freshly isolated allogeneic (B10 [○]) or syngeneic (C3H [●]) bulk spleen cells is also shown. Results are expressed as mean cpm ± 1 SD and are representative of at least 3 separate experiments.
