Figure 5.
Figure 5. Sustained DRAQ5 positivity, decreased hemoglobinization, and altered cytomorphology of maturing EpoR-HM erythroblasts. (A) Bone marrow–derived erythroid progenitor cells were expanded in SP34-EX medium and subsequently were cultured in differentiation medium for 40 hours. Frequencies of DRAQ5negTer119pos erythroblasts then were determined. (B) In parallel, cultures were analyzed for hemoglobinization (benzidine-positive colonies). (C) Hemoglobin levels in maturing wt-EpoR, EpoR-HM, and EpoR-H erythroblasts were also assayed using diaminofluorene (DAF) and by visualization of pelleted cells. For EpoR-HM erythroblasts, apparently immature morphologies were observed in cytospin preparations (right panel). Micrograph images were visualized using an Olympus IX70 microscope equipped with a 100×/1.3 oil-immersion objective lens (Olympus, Melville, NY). Immersion oil no. 16212 from Cargille Labs (Cedar Grove, NJ) was used with the lens. A Zeiss Axiocam 412312 camera and Axio-vision 4.1 software (Zeiss, Thornwood, NY) were used to capture and process images. In dotplots, the numbers in quadrants (clockwise from bottom left) indicate the percentage of Ter119negDraq5neg, Ter119highDraq5neg, Ter119highDraq5high, and Ter119negDraq5pos cells among total live-gated cells. In the bar graphs, plotted values are mean values plus or minus SE; n = 4 wt-EpoR, EpoR-HM, and EpoR-H mice.

Sustained DRAQ5 positivity, decreased hemoglobinization, and altered cytomorphology of maturing EpoR-HM erythroblasts. (A) Bone marrow–derived erythroid progenitor cells were expanded in SP34-EX medium and subsequently were cultured in differentiation medium for 40 hours. Frequencies of DRAQ5negTer119pos erythroblasts then were determined. (B) In parallel, cultures were analyzed for hemoglobinization (benzidine-positive colonies). (C) Hemoglobin levels in maturing wt-EpoR, EpoR-HM, and EpoR-H erythroblasts were also assayed using diaminofluorene (DAF) and by visualization of pelleted cells. For EpoR-HM erythroblasts, apparently immature morphologies were observed in cytospin preparations (right panel). Micrograph images were visualized using an Olympus IX70 microscope equipped with a 100×/1.3 oil-immersion objective lens (Olympus, Melville, NY). Immersion oil no. 16212 from Cargille Labs (Cedar Grove, NJ) was used with the lens. A Zeiss Axiocam 412312 camera and Axio-vision 4.1 software (Zeiss, Thornwood, NY) were used to capture and process images. In dotplots, the numbers in quadrants (clockwise from bottom left) indicate the percentage of Ter119negDraq5neg, Ter119highDraq5neg, Ter119highDraq5high, and Ter119negDraq5pos cells among total live-gated cells. In the bar graphs, plotted values are mean values plus or minus SE; n = 4 wt-EpoR, EpoR-HM, and EpoR-H mice.

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