Fig. 2.
Fig. 2. Characterization of the NK cell and DC potential of 2 separate intermediate CD34lo precursors, CD44hi or CD44lo, derived from the earliest intrathymic progenitors. / (A) Representative cell size (forward scatter, FS) and flow cytometry profile (shaded monoparametric histograms) of sorted CD44hi (CD5lo) and CD44lo(CD5+) intermediate CD34lo progenitors (biparametric plots) derived by day 3.5 from CD34hiCD33lo precursors set up in multicytokine-supported cultures. Background fluorescence determined with isotype-matched irrelevant MoAbs is shown (unshaded histograms). Absolute numbers of total viable cells (B), DCs (CD7loCD13+CD1a+) (C), and NK cells (CD7++CD13−CD56+) (D) recovered from either CD44hi (▴) or CD44lo (●) intermediate CD34lo progenitors derived in vitro and sorted as shown in (A), upon reculture in IL-2–supplemented multicytokine-supported conditions. Absolute numbers are referred to 105 input progenitors. Results are presented as the mean of 5 independent experiments.

Characterization of the NK cell and DC potential of 2 separate intermediate CD34lo precursors, CD44hi or CD44lo, derived from the earliest intrathymic progenitors.

(A) Representative cell size (forward scatter, FS) and flow cytometry profile (shaded monoparametric histograms) of sorted CD44hi (CD5lo) and CD44lo(CD5+) intermediate CD34lo progenitors (biparametric plots) derived by day 3.5 from CD34hiCD33lo precursors set up in multicytokine-supported cultures. Background fluorescence determined with isotype-matched irrelevant MoAbs is shown (unshaded histograms). Absolute numbers of total viable cells (B), DCs (CD7loCD13+CD1a+) (C), and NK cells (CD7++CD13CD56+) (D) recovered from either CD44hi (▴) or CD44lo (●) intermediate CD34lo progenitors derived in vitro and sorted as shown in (A), upon reculture in IL-2–supplemented multicytokine-supported conditions. Absolute numbers are referred to 105 input progenitors. Results are presented as the mean of 5 independent experiments.

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