Figure 3
Figure 3. High purity of leukocyte fractions was achieved by immunologic cell separations. The purity of all cell fractions was assessed by flow cytometry using side-forward scatter and antigenic characteristics. The fraction of granulocytes in the preisolation reference control whole blood was 72% (A). SSC indicates side scatter channel. (B) Shown is the enrichment of monocytes from 18% to 98% in the Lymphoprep MNC fraction by removal of cells positive for CD3, CD7, CD16, CD19, CD56, CD123, and CD235A. Monocytes were depleted down to 0.08% in the Lymphoprep RBC pellet (C). The purity of granulocyte fraction was 98% after removal of CD14-positive cells from the lower Polymorphprep layer, and the monocyte contamination of granulocyte preparation was only 0.3% (D). Flow cytometric histograms and the plotted mean percentage of analyzed cells are presented.

High purity of leukocyte fractions was achieved by immunologic cell separations. The purity of all cell fractions was assessed by flow cytometry using side-forward scatter and antigenic characteristics. The fraction of granulocytes in the preisolation reference control whole blood was 72% (A). SSC indicates side scatter channel. (B) Shown is the enrichment of monocytes from 18% to 98% in the Lymphoprep MNC fraction by removal of cells positive for CD3, CD7, CD16, CD19, CD56, CD123, and CD235A. Monocytes were depleted down to 0.08% in the Lymphoprep RBC pellet (C). The purity of granulocyte fraction was 98% after removal of CD14-positive cells from the lower Polymorphprep layer, and the monocyte contamination of granulocyte preparation was only 0.3% (D). Flow cytometric histograms and the plotted mean percentage of analyzed cells are presented.

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