Figure 4
Figure 4. MK culture and PPF from fetal liver. (A) Live-cell images of MKs cultured from fetal liver of A+/A+, Agfp/A+, and AgfpR702C/A+ embryos. Phase image is shown for A+/A+ (Ai), fluorescence/DIC overlay image for Agfp/A+ (Aii), and fluorescence z-stack images for Agfp/A+ (Aiii) and AgfpR702C/A+ (Aiv). Arrows indicate proplatelets; arrowheads, platelet buds; green: GFP. Bar, 20μm. (B) Fixed MK cultures stained with anti-CD41 to confirm the identity of the MKs. Note the difference in the length and thickness of the proplatelets (arrows) and the size of the proplatelet buds (arrowheads) between control (Bi-ii) and AgfpR702C/A+ (Biii-iv) MKs. Red indicates CD41; and green, GFP. Bar, 20 μm. (C) Percentage of MKs undergoing PPF in culture (mean ± SD). A+/A+: 30.8% ± 12.6% (n = 5); and AgfpR702C/A+: 7.4% ± 1.9% (n = 9). *P < .001 (t test). (D) Proplatelet bud size in culture. Measurements of the diameters of proplatelet buds are from the confocal microscope images of live Agfp/A+ and AgfpR702C/A+ MKs. Box plot shows median, upper and lower quartiles, and upper and lower 5 percentiles of each group. Agfp/A+: 3.07 ± 1.05 μm (n = 199); and AgfpR702C/A+: 5.84 ± 2.73 μm (n = 107); *P < .001 (t test). (E) In vitro production of platelets from A+/A+ and AgfpR702C/A+ embryonic littermate MKs. DIC imaging shows A+/A+ (Ei) and AgfpR702C/A+ (Eii; GFP signal included) MKs separated from 4-day fetal liver culture by 1.5%-3.0% BSA gradient before PPF; (Eiii-iv) immunofluorescence staining with CD41 Ab to identify platelets after in vitro platelet production by shaking at 150 rpm for 2 hours at 37°. (F) Quantitation of platelet diameter from A+/A+ and AgfpR702C/A+ in vitro platelet production.

MK culture and PPF from fetal liver. (A) Live-cell images of MKs cultured from fetal liver of A+/A+, Agfp/A+, and AgfpR702C/A+ embryos. Phase image is shown for A+/A+ (Ai), fluorescence/DIC overlay image for Agfp/A+ (Aii), and fluorescence z-stack images for Agfp/A+ (Aiii) and AgfpR702C/A+ (Aiv). Arrows indicate proplatelets; arrowheads, platelet buds; green: GFP. Bar, 20μm. (B) Fixed MK cultures stained with anti-CD41 to confirm the identity of the MKs. Note the difference in the length and thickness of the proplatelets (arrows) and the size of the proplatelet buds (arrowheads) between control (Bi-ii) and AgfpR702C/A+ (Biii-iv) MKs. Red indicates CD41; and green, GFP. Bar, 20 μm. (C) Percentage of MKs undergoing PPF in culture (mean ± SD). A+/A+: 30.8% ± 12.6% (n = 5); and AgfpR702C/A+: 7.4% ± 1.9% (n = 9). *P < .001 (t test). (D) Proplatelet bud size in culture. Measurements of the diameters of proplatelet buds are from the confocal microscope images of live Agfp/A+ and AgfpR702C/A+ MKs. Box plot shows median, upper and lower quartiles, and upper and lower 5 percentiles of each group. Agfp/A+: 3.07 ± 1.05 μm (n = 199); and AgfpR702C/A+: 5.84 ± 2.73 μm (n = 107); *P < .001 (t test). (E) In vitro production of platelets from A+/A+ and AgfpR702C/A+ embryonic littermate MKs. DIC imaging shows A+/A+ (Ei) and AgfpR702C/A+ (Eii; GFP signal included) MKs separated from 4-day fetal liver culture by 1.5%-3.0% BSA gradient before PPF; (Eiii-iv) immunofluorescence staining with CD41 Ab to identify platelets after in vitro platelet production by shaking at 150 rpm for 2 hours at 37°. (F) Quantitation of platelet diameter from A+/A+ and AgfpR702C/A+ in vitro platelet production.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal