Plasminogen Depletion during Streptokinase Treatment or Two-Chain Urokinase Incubation Correlates with Decreased Clot Lysability Ex Vivo and In Vitro

Páll T Önundarson; H Magnús Haraldsson; Lena Bergmann; Charles W Francis; Victor J Marder

doi:10.1055/s-0038-1649714

Thrombosis and Haemostasis, Inhaltsverzeichnis

Thromb Haemost 1993; 70(06): 0998-1004
DOI: 10.1055/s-0038-1649714

Original Article

Fibrinolysis

Schattauer GmbH Stuttgart

Plasminogen Depletion during Streptokinase Treatment or Two-Chain Urokinase Incubation Correlates with Decreased Clot Lysability Ex Vivo and In Vitro

Páll T Önundarson

¹The Department of Hematology, Landspítalinn University Hospital, Reykjavik, Iceland

,

H Magnús Haraldsson

¹The Department of Hematology, Landspítalinn University Hospital, Reykjavik, Iceland

,

Lena Bergmann

¹The Department of Hematology, Landspítalinn University Hospital, Reykjavik, Iceland

,

Charles W Francis

²The Hematology Unit, Department of Medicine, University of Rochester, School of Medicine and Dentistry, Rochester, New York, USA

,

Victor J Marder

²The Hematology Unit, Department of Medicine, University of Rochester, School of Medicine and Dentistry, Rochester, New York, USA

› Institutsangaben

Abstract

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Summary

The relationship between lytic state variables and ex vivo clot lysability was investigated in blood drawn from patients during streptokinase administration for acute myocardial infarction. A lytic state was already evident after 5 min of treatment and after 20 min the plasminogen concentration had decreased to 24%, antiplasmin to 7% and fibrinogen 0.2 g/1. Lysis of radiolabeled retracted clots in the patient plasmas decreased from 37 ± 8% after 5 min to 21 ± 8% at 10 min and was significantly lower (8 ± 9%, p <0.005) in samples drawn at 20, 40 and 80 min. Clot lysability correlated positively with the plasminogen concentration (r = 0.78, p = 0.003), but not with plasmin activity. Suspension of radiolabeled clots in normal plasma pre-exposed to 250 U/ml two-chain urokinase for varying time to induce an in vitro lytic state was also associated with decreasing clot lysability in direct proportion with the duration of prior plasma exposure to urokinase. The decreased lysability correlated with the time-dependent reduction in plasminogen concentration (r = 0.88, p <0.0005). Thus, clot lysability decreases in conjunction with the development of the lytic state and the associated plasminogen depletion. The lytic state may therefore limit reperfusion during thrombolytic treatment.

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Referenzen

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