Fig. 4.
Fig. 4. Plasminogen activators in QPD platelets. / Plasminogen activators were analyzed on casein substrate gels containing plasminogen. (A, D) Samples tested after 10% nonreduced SDS-PAGE. (B, C) Samples spotted directly onto substrate gels. (A) QPD releasate (QR, 6 μL; QR*, 10 μL) contained plasminogen activators that comigrated with tcu-PA (tcuPA, 8.8 ng) and LMW u-PA (LMWuPA, 3.2 ng), but not with purified plasmin (10 ng) or t-PA (tPA, 1 IU). (B) Unlike t-PA (0.5 IU), tcu-PA (5 ng) and the plasminogen activators in 1 μL QR and QL (QPD lysate) were inhibited on gels with added (+) 1 mM amiloride. (C) Large amounts of recombinant PAI-1 (final concentrations shown) were required to fully neutralize the plasminogen activators in pooled QR. (D) Zymograms indicated that the 100-, 50-, and 33-kd proteases in QR (5 μL/lane) were removed by rabbit antibodies to human u-PA (depl), but not by normal rabbit IgG (sham). The 33-kd protease in lanes sham and QR was evident on the original gel.

Plasminogen activators in QPD platelets.

Plasminogen activators were analyzed on casein substrate gels containing plasminogen. (A, D) Samples tested after 10% nonreduced SDS-PAGE. (B, C) Samples spotted directly onto substrate gels. (A) QPD releasate (QR, 6 μL; QR*, 10 μL) contained plasminogen activators that comigrated with tcu-PA (tcuPA, 8.8 ng) and LMW u-PA (LMWuPA, 3.2 ng), but not with purified plasmin (10 ng) or t-PA (tPA, 1 IU). (B) Unlike t-PA (0.5 IU), tcu-PA (5 ng) and the plasminogen activators in 1 μL QR and QL (QPD lysate) were inhibited on gels with added (+) 1 mM amiloride. (C) Large amounts of recombinant PAI-1 (final concentrations shown) were required to fully neutralize the plasminogen activators in pooled QR. (D) Zymograms indicated that the 100-, 50-, and 33-kd proteases in QR (5 μL/lane) were removed by rabbit antibodies to human u-PA (depl), but not by normal rabbit IgG (sham). The 33-kd protease in lanes sham and QR was evident on the original gel.

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