Figure 2
Figure 2. Subpopulations within pDC preparations. (A) The procedure for isolating pDCs and IKDCs. The initial steps were similar to those used for cDCs (Figure 1) except the immunomagnetic bead depletion mAb cocktail differed. No depletion of cells bearing NK cell markers was used. Rather, the pDCs were isolated by flow cytometric cell sorting (CD45RAhi CD11cint) and segregated into Ly6C+ and Ly6C− subsets, and the IKDCs were segregated as CD49b+ and CD11cint cells, either CD45RAhi or CD45RAint. Full details are in “Materials and methods.” (B) The correlation between Ly6C and Ly49Q expression by pDC preparations. pDCs were isolated as in panel A and gated on sorting as CD11cint CD45RAhi cells.

Subpopulations within pDC preparations. (A) The procedure for isolating pDCs and IKDCs. The initial steps were similar to those used for cDCs (Figure 1) except the immunomagnetic bead depletion mAb cocktail differed. No depletion of cells bearing NK cell markers was used. Rather, the pDCs were isolated by flow cytometric cell sorting (CD45RAhi CD11cint) and segregated into Ly6C+ and Ly6C subsets, and the IKDCs were segregated as CD49b+ and CD11cint cells, either CD45RAhi or CD45RAint. Full details are in “Materials and methods.” (B) The correlation between Ly6C and Ly49Q expression by pDC preparations. pDCs were isolated as in panel A and gated on sorting as CD11cint CD45RAhi cells.

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