Figure 4.
Figure 4. Ligation of Siglec-H does not modulate pDC activation. (A) Bone marrow cells were expanded for 14 days with Flt-3 ligand and labeled with anti-B220 and anti-Ly6c mAbs to identify pDC precursor (left panel). Double-positive cells (top right quadrant, left panel) were sorted and an aliquot stained with either sheep anti–Siglec-H+ (open histogram, right panel) or preimmune immunoglobulin (gray histogram, right panel). (B) FACS-sorted B220+ Ly6c+ cells were cultured with no Ab, MB15 mAb (10 μg/mL), or sheep anti–Siglec-H pAb (10 μg/mL) in the presence or absence of 10 μM CpG 1668 for 18 hours. The concentrations of the indicated cytokines in the cell culture supernatants were determined by flow cytometry.

Ligation of Siglec-H does not modulate pDC activation. (A) Bone marrow cells were expanded for 14 days with Flt-3 ligand and labeled with anti-B220 and anti-Ly6c mAbs to identify pDC precursor (left panel). Double-positive cells (top right quadrant, left panel) were sorted and an aliquot stained with either sheep anti–Siglec-H+ (open histogram, right panel) or preimmune immunoglobulin (gray histogram, right panel). (B) FACS-sorted B220+ Ly6c+ cells were cultured with no Ab, MB15 mAb (10 μg/mL), or sheep anti–Siglec-H pAb (10 μg/mL) in the presence or absence of 10 μM CpG 1668 for 18 hours. The concentrations of the indicated cytokines in the cell culture supernatants were determined by flow cytometry.

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