Figure 2
Figure 2. MKs derived from ES cells deficient in WAVE2. (A) Immunoblots of WAVE2, WAVE1, Abi1, and tubulin from lysates of day-5 embryoid bodies (EBs). To avoid contamination with mouse feeder fibroblasts, day-0 ES cells, were sorted with c-Kit+ cells, applied to EB media,33 and cultured for 5 days. (B) Flow cytometric dotplots of side and forward scatter profiles of 10 000 live cells on day 8, and expression profiles of αIIb and GPIbα stained cells (day 8), as described previously.28,29 On day 12, all cells collected from a 6-well culture plate were stained with anti-αIIb, anti-GPIbα, and propidium iodide and were mixed with True Count Beads. WAVE2+/+, WAVE2+/−, or WAVE2−/− cells and beads were then subjected to flow cytometry. Representative dot plots show all viable cells from WAVE2+/+ and WAVE2−/− plates. Quantification for GPIbα+ cells in an arbitrary gate was performed as described in “Materials and methods.” The graph on the right shows means (± SD; n = 3). (C) On day 8 or day 12, weakly adherent or floating cells28,29 were subjected to cytospin preparation and to staining by Wright-Giemsa technique. WAVE2−/− MKs showed decreased number of large sized cells. (D) On day 12, live cells were fixed following cytospin preparation. Cells were permeabilized, stained with anti-VWF followed by rabbit Alexa 488 (green), and anti-αIIb followed by mouse Alexa 568 (red) with nuclei marked by 4,6-diamino-2-phenylindole (DAPI) staining (blue). WAVE2−/− MK retained VWF expression (diffuse but decreased) in cytoplasm while VWF expression in WAVE2+/+ MK was distributed clearly along the plasma membrane in peripheral cytoplasm (◀). (E) On day 11 (i) or day 12 (ii), proplatelet-exhibiting MKs derived from normal ES cells were fixed and plated on poly-L-lysine–coated cover glasses. Cells were permeabilized and were stained with rhodamine-conjugated phalloidin to mark F-actin (red) and with anti-WAVE2 antibody followed by Alexa 488 (green). Arrowheads indicate swellings. See “Image acquisition for platelet and MK spreading” for complete image acquisition information. (F) The left figure shows means (± SD; n = 3) of total number of proplatelets in a 6-well plate on day 12. The right figure shows means (± SD; n = 3) of number of αIIb+ particles within the same flow cytometry gate as that used for murine platelets. Quantification was performed using True Count Beads as described in “Quantification of mature MKs and platelets.”

MKs derived from ES cells deficient in WAVE2. (A) Immunoblots of WAVE2, WAVE1, Abi1, and tubulin from lysates of day-5 embryoid bodies (EBs). To avoid contamination with mouse feeder fibroblasts, day-0 ES cells, were sorted with c-Kit+ cells, applied to EB media,33  and cultured for 5 days. (B) Flow cytometric dotplots of side and forward scatter profiles of 10 000 live cells on day 8, and expression profiles of αIIb and GPIbα stained cells (day 8), as described previously.28,29  On day 12, all cells collected from a 6-well culture plate were stained with anti-αIIb, anti-GPIbα, and propidium iodide and were mixed with True Count Beads. WAVE2+/+, WAVE2+/−, or WAVE2−/− cells and beads were then subjected to flow cytometry. Representative dot plots show all viable cells from WAVE2+/+ and WAVE2−/− plates. Quantification for GPIbα+ cells in an arbitrary gate was performed as described in “Materials and methods.” The graph on the right shows means (± SD; n = 3). (C) On day 8 or day 12, weakly adherent or floating cells28,29  were subjected to cytospin preparation and to staining by Wright-Giemsa technique. WAVE2−/− MKs showed decreased number of large sized cells. (D) On day 12, live cells were fixed following cytospin preparation. Cells were permeabilized, stained with anti-VWF followed by rabbit Alexa 488 (green), and anti-αIIb followed by mouse Alexa 568 (red) with nuclei marked by 4,6-diamino-2-phenylindole (DAPI) staining (blue). WAVE2−/− MK retained VWF expression (diffuse but decreased) in cytoplasm while VWF expression in WAVE2+/+ MK was distributed clearly along the plasma membrane in peripheral cytoplasm (◀). (E) On day 11 (i) or day 12 (ii), proplatelet-exhibiting MKs derived from normal ES cells were fixed and plated on poly-L-lysine–coated cover glasses. Cells were permeabilized and were stained with rhodamine-conjugated phalloidin to mark F-actin (red) and with anti-WAVE2 antibody followed by Alexa 488 (green). Arrowheads indicate swellings. See “Image acquisition for platelet and MK spreading” for complete image acquisition information. (F) The left figure shows means (± SD; n = 3) of total number of proplatelets in a 6-well plate on day 12. The right figure shows means (± SD; n = 3) of number of αIIb+ particles within the same flow cytometry gate as that used for murine platelets. Quantification was performed using True Count Beads as described in “Quantification of mature MKs and platelets.”

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