Figure 2
NKG2A and KIR expression distinguishes populations of CD56dim NK cells. PBMCs were enriched for NK cells using a negative immunomagnetic bead depletion strategy. A representative example of a 4-color analysis shows gating of (A) CD56bright and CD56dim cells and analysis of the expression of NKG2A and KIR (using a cocktail of EB6, GL183, and DX9 mAbs) on (B) CD56bright and (C) CD56dim cells. Each of the 4 subpopulations shown in panel C was sorted and then analyzed by Q-RT-PCR for the expression of (D) KIR exhibiting variegated expression (vr) (n = 33 reactions), (E) KIR2DL4 (n = 6), (F) NKG2A (n = 7), (G) NKG2D (n = 7), and (H) NKG2E (n = 7). The numbers of NKG2 and KIR2DL4 transcripts in each subpopulation are compared with the positive control of IL-2 activated NK cells to give a relative expression. For comparison of vrKIR expression in the 4 subpopulations, the data for each KIR were normalized to those of the NKG2A+KIR+ (designated by a †). These values were used to calculate a mean relative expression for the activating (KIR2DS1–3, 2DS5, 3DS1) and inhibitory (KIR2DL1–3, 2DL5, 3DL1, 3DL2). When a KIR was not expressed in the NKG2A+KIR+ population, indicating absence of the gene, it was excluded from the calculation of mean relative expression. Error bars indicate SEM.

NKG2A and KIR expression distinguishes populations of CD56dim NK cells. PBMCs were enriched for NK cells using a negative immunomagnetic bead depletion strategy. A representative example of a 4-color analysis shows gating of (A) CD56bright and CD56dim cells and analysis of the expression of NKG2A and KIR (using a cocktail of EB6, GL183, and DX9 mAbs) on (B) CD56bright and (C) CD56dim cells. Each of the 4 subpopulations shown in panel C was sorted and then analyzed by Q-RT-PCR for the expression of (D) KIR exhibiting variegated expression (vr) (n = 33 reactions), (E) KIR2DL4 (n = 6), (F) NKG2A (n = 7), (G) NKG2D (n = 7), and (H) NKG2E (n = 7). The numbers of NKG2 and KIR2DL4 transcripts in each subpopulation are compared with the positive control of IL-2 activated NK cells to give a relative expression. For comparison of vrKIR expression in the 4 subpopulations, the data for each KIR were normalized to those of the NKG2A+KIR+ (designated by a †). These values were used to calculate a mean relative expression for the activating (KIR2DS1–3, 2DS5, 3DS1) and inhibitory (KIR2DL1–3, 2DL5, 3DL1, 3DL2). When a KIR was not expressed in the NKG2A+KIR+ population, indicating absence of the gene, it was excluded from the calculation of mean relative expression. Error bars indicate SEM.

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