Figure 1.
Figure 1. Effects of hyperoxic-hypoxic-hyperoxic treatment on expansion of WT and Fancc–/–BM lin– cells. (A) Growth of WT and Fancc–/– BM lin– cells over 10 days. Cells were incubated in hyperoxia (21% O2; Con: control) only or first subjected to 2 cycles of hypoxia (1% O2) for 4 hours then hyperoxia for 1 hour (Reoxy: reoxygenation). The cells were then incubated in hyperoxia for 10 days. The NAC cultures were the same as the reoxygenated cells except that the medium contained N-acetyl-L-cysteine (NAC) at a concentration of 1 mM. Data represent the mean ± SD of 3 independent experiments. *P < .05 between reoxygenated Fancc–/– cells and untreated Fancc–/– or WT NAC or Fancc–/– NAC samples; **P < .05 between reoxygenated Fancc–/– cells and any one of all other groups. (B) Expansion of BM cells enriched for HSCs and progenitor cells. The inserted panel shows the initial numbers of the Sca-1+ c-kit+ and Sca-1– c-kit+ subpopulations in the BM Lin– cells. WT and Fancc–/– BM lin– cells (1 × 105/mL) were treated as described in panel A. At day 5, the cells were counted and then stained with Sca-1–PE and c-kit–APC antibodies and analyzed by flow cytometry. The cell numbers were calculated by multiplication of the total numbers of cells harvested with the percentage of each phenotype of Lin– cells determined by flow cytometric analysis. The mean ± SD of 3 independent experiments is shown. *Statistical significance between WT and Fancc–/– samples at P < .01. (C) WT and Fancc–/– BM lin– cells described in panel B were counted on day 0 and day 5 after hyperoxic-hypoxic-hyperoxic treatment, stained with Sca-1–PE and c-kit–APC antibodies, and then with annexin V–FITC. Percentages of apoptosis in the 2 subpopulations were analyzed by flow cytometry. Data represent the mean ± SD of 3 independent experiments. (D) Apoptosis in WT and Fancc–/– BM lin– cells described in panel D except that analysis was conducted at 0, 4, 8, 16, 24, and 48 hours after hyperoxic-hypoxic-hyperoxic treatment. Data represent the mean ± SD of 3 independent experiments. *P < .05 between reoxygenated Fancc–/– cells and untreated Fancc–/– cells. **P < .01 between reoxygenated Fancc–/– and reoxygenated WT cells. (E) Effect of reoxygenation on BM progenitor activity. The colony-forming cell (CFC) activity of WT and Fancc–/– BM lin– cells was evaluated after hyperoxia (Con) only or 2 cycles of hyperoxic-hypoxic-hyperoxic treatments (Reoxy). Data shown represent the number (mean ± SD) of CFU-GMs, BFU-Es, and total number of colonies from 3 independent experiments. *Statistical significance between WT and Fancc–/– samples at P < .05.

Effects of hyperoxic-hypoxic-hyperoxic treatment on expansion of WT and Fancc/BM lin cells. (A) Growth of WT and Fancc/ BM lin cells over 10 days. Cells were incubated in hyperoxia (21% O2; Con: control) only or first subjected to 2 cycles of hypoxia (1% O2) for 4 hours then hyperoxia for 1 hour (Reoxy: reoxygenation). The cells were then incubated in hyperoxia for 10 days. The NAC cultures were the same as the reoxygenated cells except that the medium contained N-acetyl-L-cysteine (NAC) at a concentration of 1 mM. Data represent the mean ± SD of 3 independent experiments. *P < .05 between reoxygenated Fancc/ cells and untreated Fancc/ or WT NAC or Fancc/ NAC samples; **P < .05 between reoxygenated Fancc/ cells and any one of all other groups. (B) Expansion of BM cells enriched for HSCs and progenitor cells. The inserted panel shows the initial numbers of the Sca-1+ c-kit+ and Sca-1 c-kit+ subpopulations in the BM Lin cells. WT and Fancc/ BM lin cells (1 × 105/mL) were treated as described in panel A. At day 5, the cells were counted and then stained with Sca-1–PE and c-kit–APC antibodies and analyzed by flow cytometry. The cell numbers were calculated by multiplication of the total numbers of cells harvested with the percentage of each phenotype of Lin cells determined by flow cytometric analysis. The mean ± SD of 3 independent experiments is shown. *Statistical significance between WT and Fancc/ samples at P < .01. (C) WT and Fancc/ BM lin cells described in panel B were counted on day 0 and day 5 after hyperoxic-hypoxic-hyperoxic treatment, stained with Sca-1–PE and c-kit–APC antibodies, and then with annexin V–FITC. Percentages of apoptosis in the 2 subpopulations were analyzed by flow cytometry. Data represent the mean ± SD of 3 independent experiments. (D) Apoptosis in WT and Fancc/ BM lin cells described in panel D except that analysis was conducted at 0, 4, 8, 16, 24, and 48 hours after hyperoxic-hypoxic-hyperoxic treatment. Data represent the mean ± SD of 3 independent experiments. *P < .05 between reoxygenated Fancc/ cells and untreated Fancc/ cells. **P < .01 between reoxygenated Fancc/ and reoxygenated WT cells. (E) Effect of reoxygenation on BM progenitor activity. The colony-forming cell (CFC) activity of WT and Fancc/ BM lin cells was evaluated after hyperoxia (Con) only or 2 cycles of hyperoxic-hypoxic-hyperoxic treatments (Reoxy). Data shown represent the number (mean ± SD) of CFU-GMs, BFU-Es, and total number of colonies from 3 independent experiments. *Statistical significance between WT and Fancc/ samples at P < .05.

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