Figure 3
Stroma and HDC induce NK differentiation in the CD34+ HPC subset that could not differentiate into NK cells with cytokines alone. (A) Semi-log plot showing the fraction of negative wells (wells containing no NK precursors) as a function of input cells per well. Three subsets of CD34+ cells were tested in limiting dilution culture with only cytokines (IL-15, IL-7, SCF, FLT-3L, and IL-3): CD34+CD38−NKlin− (□, dashed line), CD34+CD38+NKlin− (◇, dotted line), and CD34+NKlin+ (▴, solid line). No positive wells were observed for NKlin− subsets cultured with cytokines alone, and the plot therefore shows a flat slope for these conditions. In contrast, CD34+NKlin+ subset showed a measurable fraction of positive wells in culture with cytokines alone, thus creating a steeper slope of the regression line. A representative donor (n = 4) is shown. (B) Calculated NKp frequencies for the 3 CD34+ HPC subsets cultured with the above-mentioned cytokines (n = 4 donors), expressed as number of NKp/106 cells. (C) Semi-log plot of the fraction of negative wells as a function of input cells per well for the CD34+CD38+NKlin− fraction cultured with cytokines alone (◇, long-dashed line), cytokines and HDC (■, gray line), cytokines and stroma (▴, black line), and cytokines and HDC and stroma (○, short-dashed line). A representative donor (n = 4) is shown. (D) Calculated NKp/106 cells for CD34+CD38+NKlin− fraction cultured in different conditions (n = 4 donors tested). (E) Semi-log plot of the fraction of negative wells as a function of input cells per well for the CD34+CD38−NKlin− fraction cultured with cytokines alone (◇, long-dashed line), with cytokines and HDC (■, gray line), with cytokines and stroma (▴, black line), and with cytokines and HDC and stroma (○, short-dashed line). A representative donor (n = 4) is shown. (F) NKp frequency per 106 cells in the CD34+CD38−NKlin− population cultured in different conditions; n = 4 donors tested. Groups showing significant differences are indicated by asterisks (***P < .001, **P = .001-.01, and *P = .01-.05), 1-way analysis of variance on log-transformed values with Bonferroni posttest. (G) Fold change in mRNA levels coding for T-cell factor/lymphoid enhancer factor (TCF/LEF) transcription factors and their downstream targets (WISP and CyclinD1) induced in NKlin−CD34+ HPCs after 14 days of culture of with (1) cytokines, stromal cells, and HDC versus (2) cytokines only. (H) Effect of Dickkopf-1 (DKK-1) on the generation of NK cells from CD34+ HPCs in the culture with cytokines, stroma, and HDC. Shown are the average number of CD56+ cells/well after 21 days of culture ± SEM. The difference between no addition of DKK-1 and addition at 10 ng/mL is statistically significant (P = .012). Results are the mean of 6 wells for each condition and are representative of independent 2 donors.

Stroma and HDC induce NK differentiation in the CD34+ HPC subset that could not differentiate into NK cells with cytokines alone. (A) Semi-log plot showing the fraction of negative wells (wells containing no NK precursors) as a function of input cells per well. Three subsets of CD34+ cells were tested in limiting dilution culture with only cytokines (IL-15, IL-7, SCF, FLT-3L, and IL-3): CD34+CD38NKlin (□, dashed line), CD34+CD38+NKlin (◇, dotted line), and CD34+NKlin+ (▴, solid line). No positive wells were observed for NKlin subsets cultured with cytokines alone, and the plot therefore shows a flat slope for these conditions. In contrast, CD34+NKlin+ subset showed a measurable fraction of positive wells in culture with cytokines alone, thus creating a steeper slope of the regression line. A representative donor (n = 4) is shown. (B) Calculated NKp frequencies for the 3 CD34+ HPC subsets cultured with the above-mentioned cytokines (n = 4 donors), expressed as number of NKp/106 cells. (C) Semi-log plot of the fraction of negative wells as a function of input cells per well for the CD34+CD38+NKlin fraction cultured with cytokines alone (◇, long-dashed line), cytokines and HDC (■, gray line), cytokines and stroma (▴, black line), and cytokines and HDC and stroma (○, short-dashed line). A representative donor (n = 4) is shown. (D) Calculated NKp/106 cells for CD34+CD38+NKlin fraction cultured in different conditions (n = 4 donors tested). (E) Semi-log plot of the fraction of negative wells as a function of input cells per well for the CD34+CD38NKlin fraction cultured with cytokines alone (◇, long-dashed line), with cytokines and HDC (■, gray line), with cytokines and stroma (▴, black line), and with cytokines and HDC and stroma (○, short-dashed line). A representative donor (n = 4) is shown. (F) NKp frequency per 106 cells in the CD34+CD38NKlin population cultured in different conditions; n = 4 donors tested. Groups showing significant differences are indicated by asterisks (***P < .001, **P = .001-.01, and *P = .01-.05), 1-way analysis of variance on log-transformed values with Bonferroni posttest. (G) Fold change in mRNA levels coding for T-cell factor/lymphoid enhancer factor (TCF/LEF) transcription factors and their downstream targets (WISP and CyclinD1) induced in NKlinCD34+ HPCs after 14 days of culture of with (1) cytokines, stromal cells, and HDC versus (2) cytokines only. (H) Effect of Dickkopf-1 (DKK-1) on the generation of NK cells from CD34+ HPCs in the culture with cytokines, stroma, and HDC. Shown are the average number of CD56+ cells/well after 21 days of culture ± SEM. The difference between no addition of DKK-1 and addition at 10 ng/mL is statistically significant (P = .012). Results are the mean of 6 wells for each condition and are representative of independent 2 donors.

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