Figure 5
Figure 5. Distinctive response of human HSCs and progenitors to oxidative DNA damage. (A) CB Lin−CD34+CD38− cells and Lin−CD34+CD38+ cells were cultured with or without BSO for 2 days. Intracellular ROS concentrations were determined by the intensity of DCF-DA staining using a flow cytometor. The relative ROS level is presented as a fold induction compared with the MFI value detected in cells cultured without BSO. Data from 2 independent experiments are shown (**P < .01). (B) Two days after BSO treatment, cells were pulsed with BrdU and analyzed by flow cytometry. Data from 2 independent experiments are shown (**P < .01). (C) Relative expressions of p16INK4a, p14ARF, and p21CIP1 in Lin−CD34+CD38− cells and Lin−CD34+CD38+ cells cultured with or without BSO were analyzed at the end of 2-day culture by quantitative real-time PCR. Each value was normalized to 18S rRNA expression and is presented as a fold increase compared with the levels detected in cells cultured without BSO (**P < .01). (D) CB Lin−CD34+CD38− cells and Lin−CD34+CD38+ cells cultured with BSO for 2 days were stained with γ-H2AX and p21CIP1 mAbs (γ-H2AX: green; p21CIP1: red; DAPI: blue). Bars represent 5 μm. (E) At 2 days after BSO-treatment, the frequency of apoptotic cells was determined by annexin V/PI staining. Data from 3 independent experiments are shown (**P < .01). (F) The number of γ-H2AX foci per cell in Lin−CD34+CD38− cells and Lin−CD34+CD38+ cells at the indicated time points. Cells cultured with BSO for 2 days were washed, replaced with fresh BSO-free media, and cultured for additional 1, 2, or 3 days (n = 4 in each time point; *P < .05, **P < .01, Lin−CD34+CD38− cells vs Lin−CD34+CD38+ cells).

Distinctive response of human HSCs and progenitors to oxidative DNA damage. (A) CB LinCD34+CD38 cells and LinCD34+CD38+ cells were cultured with or without BSO for 2 days. Intracellular ROS concentrations were determined by the intensity of DCF-DA staining using a flow cytometor. The relative ROS level is presented as a fold induction compared with the MFI value detected in cells cultured without BSO. Data from 2 independent experiments are shown (**P < .01). (B) Two days after BSO treatment, cells were pulsed with BrdU and analyzed by flow cytometry. Data from 2 independent experiments are shown (**P < .01). (C) Relative expressions of p16INK4a, p14ARF, and p21CIP1 in LinCD34+CD38 cells and LinCD34+CD38+ cells cultured with or without BSO were analyzed at the end of 2-day culture by quantitative real-time PCR. Each value was normalized to 18S rRNA expression and is presented as a fold increase compared with the levels detected in cells cultured without BSO (**P < .01). (D) CB LinCD34+CD38 cells and LinCD34+CD38+ cells cultured with BSO for 2 days were stained with γ-H2AX and p21CIP1 mAbs (γ-H2AX: green; p21CIP1: red; DAPI: blue). Bars represent 5 μm. (E) At 2 days after BSO-treatment, the frequency of apoptotic cells was determined by annexin V/PI staining. Data from 3 independent experiments are shown (**P < .01). (F) The number of γ-H2AX foci per cell in LinCD34+CD38 cells and LinCD34+CD38+ cells at the indicated time points. Cells cultured with BSO for 2 days were washed, replaced with fresh BSO-free media, and cultured for additional 1, 2, or 3 days (n = 4 in each time point; *P < .05, **P < .01, LinCD34+CD38 cells vs LinCD34+CD38+ cells).

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