Figure 1.
uPA is endocytosed by in vitro–grown MKs and stored in granules. (A) Schematics of the structures of scuPA (top) and uPAT (bottom). Full-length scuPA is composed of (1) an N-terminal growth factor-like domain (GFD, yellow) that binds uPAR; (2) a Kringle domain (K, green) that mediates LRP1-dependent intracellular uptake,36 binding to integrins37,38 and nuclear translocation36; and (3) the protease domain (catalytic domain, gray).39 Site of activation by plasmin is shown in red. uPAT is composed of the protease domain in which 157F158K has been deleted40 to create a thrombin cleavage/activation site (shown in green). (B) Representative WB of lysates of in vitro–grown day-11 MKs in the presence (+) or absence (−) of scuPA (400 nM) added on day 10. WB at the top was with anti-human uPA mouse monoclonal antibody followed by horseradish peroxidase (HRP)-conjugated goat anti-mouse antibody, and bottom shows HPR-conjugated anti–β-actin antibody as a loading control. Size marker is shown to the left of the blot. (C) Dose-dependent uptake of Alexa-568 scuPA by CD34+ MKs. y-axes denote mean fluorescence intensity (MFI) measured by flow cytometry. Mean ± 1 standard deviation (SD) of relative uptake of scuPA compared with the values in its absence. n = 4 independent studies. P values were determined by ordinary 1-way analysis of variance (ANOVA). (D) Same as in panel C but for time course of Alexa-568 scuPA (400 nM) uptake by the CD34+ MKs. (E) Visualization using confocal microscopy of Alexa-568 scuPA (top, red) or Alexa-488 uPAT (bottom, green) endocytosed by day-11 CD34+ MKs for 24 hours starting on day 10 initiation of culture. DAPI (4′,6-diamidino-2-phenylindole; blue) depicts the nuclei. Scale bar is shown.

uPA is endocytosed by in vitrogrown MKs and stored in granules. (A) Schematics of the structures of scuPA (top) and uPAT (bottom). Full-length scuPA is composed of (1) an N-terminal growth factor-like domain (GFD, yellow) that binds uPAR; (2) a Kringle domain (K, green) that mediates LRP1-dependent intracellular uptake,36 binding to integrins37,38 and nuclear translocation36; and (3) the protease domain (catalytic domain, gray).39 Site of activation by plasmin is shown in red. uPAT is composed of the protease domain in which 157F158K has been deleted40 to create a thrombin cleavage/activation site (shown in green). (B) Representative WB of lysates of in vitro–grown day-11 MKs in the presence (+) or absence (−) of scuPA (400 nM) added on day 10. WB at the top was with anti-human uPA mouse monoclonal antibody followed by horseradish peroxidase (HRP)-conjugated goat anti-mouse antibody, and bottom shows HPR-conjugated anti–β-actin antibody as a loading control. Size marker is shown to the left of the blot. (C) Dose-dependent uptake of Alexa-568 scuPA by CD34+ MKs. y-axes denote mean fluorescence intensity (MFI) measured by flow cytometry. Mean ± 1 standard deviation (SD) of relative uptake of scuPA compared with the values in its absence. n = 4 independent studies. P values were determined by ordinary 1-way analysis of variance (ANOVA). (D) Same as in panel C but for time course of Alexa-568 scuPA (400 nM) uptake by the CD34+ MKs. (E) Visualization using confocal microscopy of Alexa-568 scuPA (top, red) or Alexa-488 uPAT (bottom, green) endocytosed by day-11 CD34+ MKs for 24 hours starting on day 10 initiation of culture. DAPI (4′,6-diamidino-2-phenylindole; blue) depicts the nuclei. Scale bar is shown.

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