Inhibition of expression of differentiation markers hemoglobin and glycophorin A and impaired disappearance of CD34 in erythroid cells cocultivated with HZ or treated with HNE. (A-C) Erythroid cells were cocultivated with HZ (25μM HZ-heme), treated with HNE (7μM), or kept as untreated controls (CTRL) in liquid culture. (A) Cellular hemoglobin was quantified by the Drabkin method and expressed as micrograms per 10⁶ cells. (B) The surface expression of CD34 and (C) glycophorin A was quantified by flow cytometry after immune staining and expressed as MFI. (D) CD34 expression was monitored in erythroid cells cocultivated with unfed (Mo), HZ-fed (Mo + HZ) (25μM HZ-heme, corresponding to 12 RBCs/monocyte in terms of heme content), or RBC-fed (Mo + RBC) monocytes (50 RBCs/monocyte). Means ± SE of 3 independent experiments. The significance of differences (P < .05) between untreated and HZ- (*) or HNE-treated (§) cells (A-C), or between erythroid cells cocultivated with HZ-fed monocytes and unfed (*) or RBC-fed monocytes (§; D) are indicated. (E-F) GlycophorinA and CD34 measured by flow cytometry in erythroid cells at days 15 and 1 of coincubation with HZ (solid line filled space) and HNE (dotted line unfilled space) and in control erythroid cells (solid line, unfilled space). Background is plotted as dashed line.