The uncalibrated prothrombinase-induced clotting time test

W. Korte; R. Jovic; M. Hollenstein; P. Degiacomi; M. Gautschi; A. Ferrández

doi:10.1055/s-0037-1619058

Hämostaseologie, Inhaltsverzeichnis

Hamostaseologie 2010; 30(04): 212-216
DOI: 10.1055/s-0037-1619058

Original article

Schattauer GmbH

The uncalibrated prothrombinase-induced clotting time test

Equally convenient but more precise than the aPTT for monitoring of unfractionated heparinDer PiCT UC-Test ist gleichermaßen einfach aber präziser als die aPTT zur Überwachung von unfraktioniertem Heparin

W. Korte

¹Institute for Clinical Chemistry and Haematology, Kantonsspital St. Gallen, Basel, Switzerland

²University of Bern, Basel, Switzerland

,

R. Jovic

¹Institute for Clinical Chemistry and Haematology, Kantonsspital St. Gallen, Basel, Switzerland

,

M. Hollenstein

¹Institute for Clinical Chemistry and Haematology, Kantonsspital St. Gallen, Basel, Switzerland

,

P. Degiacomi

¹Institute for Clinical Chemistry and Haematology, Kantonsspital St. Gallen, Basel, Switzerland

,

M. Gautschi

³DSM Nutritional Products Ltd. Branch Pentapharm, Basel, Switzerland

,

A. Ferrández

³DSM Nutritional Products Ltd. Branch Pentapharm, Basel, Switzerland

› Institutsangaben

Abstract

Summary

The activated partial thromboplastin time test (aPTT) represents one of the most commonly used diagnostic tools in order to monitor patients undergoing heparin therapy. Expression of aPTT coagulation time in seconds represents common practice in order to evaluate the integrity of the coagulation cascade. The prolongation of the aPTT thus can indicate whether or not the heparin level is likely to be within therapeutic range. Unfortunately aPTT results are highly variable depending on patient properties, manufacturer, different reagents and instruments among others but most importantly aPTT’s dose response curve to heparin often lacks linearity. Furthermore, aPTT assays are insensitive to drugs such as, for example, low molecular weight heparin (LMWH) and direct factor Xa (FXa) inhibitors among others. On the other hand, the protrombinase-induced clotting time assay (PiCT^®) has been show to be a reliable functional assay sensitive to all heparinoids as well as direct thrombin inhibitors (DTIs). So far, the commercially available PiCT assay (Pefakit^®-PiCT^®, DSM Nutritional Products Ltd. Branch Pentapharm, Basel, Switzerland) is designed to express results in terms of units with the help of specific calibrators, while aPTT results are most commonly expressed as coagulation time in seconds. In this report, we describe the results of a pilot study indicating that the Pefakit PiCT UC assay is superior to the aPTT for the efficient monitoring of patients undergoing UFH therapy; it is also suitable to determine and quantitate the effect of LMWH therapy. This indicates a distinct benefit when using this new approach over the use of aPPT for heparin monitoring.

Zusammenfassung

Die aPTT ist eine der meist verwendeten Überwachungsmöglichkeiten bei Patienten mit He-parin-Therapie. Die Beurteilung der Gerin-nungszeit mittels aPTT ist ein viel genutztes Instrument, um die Integrität der Gerinnungskaskade zu untersuchen. Die aPTT-Verlängerung unter Heparin kann daher als Marker dafür verwendet werden, ob der Heparinspiegel im gewünschten therapeutischen Bereich ist. Unglücklicherweise sind die aPTT-Resultate stark abhängig von Patienteneigenschaften, unterschiedlichen Herstellern, verschiedenen Reagenzien und Instrumenten, so dass die Dosisantwort der aPTT auf Heparin oft nicht linear ist. Außerdem ist die aPTT nicht sensitiv genug, um niedermolekulare Heparine bzw. direkte Faktor-Xa-Inhibitoren zu monitieren. An-dererseits ist die PiCT (prothrombinase induced clotting time) ein zuverlässiger funktioneller Assay, um alle Heparin- und Heparinoide sowie direkte Thrombininhibitoren zu monitieren. Bis jetzt wurde der kommerziell erhältliche PiCT-Assay verwendet, um mit Hilfe spezifischer Ka-libratoren die Konzentration der genannten In-hibitoren direkt anzugeben; aPTT-Resultate werden jedoch in Sekunden angegeben. Wir beschreiben die Resultate einer Pilot-Studie, die ergibt, dass die “PiCT-UC” der aPTT zum Monitoring bei Patienten mit unfraktionierter Heparintherapie überlegen ist. PiCT-UC ist auch geeignet den Einfluss von niedrig-molekularem Heparin quantitativ adäquat wi-derzuspiegeln. Diese Resultate zeigen, dass der Gebrauch der PiCT-UC gegenüber dem Gebrauch der aPTT eine deutliche Verbes-serung des Heparin-Monitorings darstellt.

Keywords

Anticoagulation monitoring - aPTT - PiCT - universal functional assay

Schlüsselwörter

Heparin - aPTT - Monitoring - PiCT

Volltext

Referenzen

References
1 Kher A, Samama MM. Primary and secondary prophylaxis of venous thromboembolism with low-molecular-weight heparins: prolonged thrombo-prophylaxis, an alternative to vitamin K antagonists. J Thromb Haemost 2005; 03: 473-481.
2 Iorio A. Prevention of venous thromboembolism after major orthopedic surgery: summing up evidence about old and new antithrombotic agents. J Thromb Haemost 2004; 02: 1055-1057.
3 Hirsh J, O’Donnell M, Weitz JI. New anticoagulants. Blood 2005; 105: 453-463.
4 Brill-Edwards P, Ginsberg JS, Johnston M. et al. Establishing a therapeutic range for heparin therapy. Annals of internal medicine 1993; 119: 104-109.
5 Harenberg J. Is laboratory monitoring of low-molecular-weight heparin therapy necessary? Yes. J Thromb Haemost 2004; 02: 547-550.
6 Bounameaux H, de Moerloose P. Is laboratory monitoring of low-molecular-weight heparin therapy necessary? No. J Thromb Haemost 2004; 02: 551-554.
7 Shojania AM. More on: is laboratory monitoring of low-molecular-weight heparin necessary?. J Thromb Haemost 2004; 02: 2276-2277.
8 Bachmann F. Laboratory monitoring of low-molecular-weight heparin therapy. J Thromb Haemost 2004; 02: 1005-1006.
9 Kearon C. Laboratory monitoring of low-molecular-weight heparin therapy. J Thromb Haemost 2004; 02: 1006-1007.
10 Nurmohamed MT, Berckmans RJ, Morrien-Salo-mons WM. et al. Monitoring anticoagulant therapy by activated partial thromboplastin time: hirudin assessment. An evaluation of native blood and plasma assays. Thrombosis and haemostasis 1994; 72: 685-692.
11 Rosborough TK. Comparing different lots of activated partial thromboplastin time reagent: analysis of two methods. American journal of clinical pathology 1998; 110: 173-177.
12 Walenga JM, Hoppensteadt DA. Monitoring the new antithrombotic drugs. Seminars in thrombosis and hemostasis 2004; 30: 683-695.
13 Mischke R. Effect of reagent batch on activated partial thromboplastin time in canine plasma and use of the ratio system for standardization. Berliner und Münchener tierärztliche Wochenschrift 2002; 115: 225-229.
14 Girolami A, Vettore S. Discrepancies between clotting and chromogenic assays in congenital coagulation disorders: the hemostatic coin has only one face, chromogenic substrates many. Blood Coagul Fibrinolysis 2009; 20: 484-485.
15 Calatzis A, Peetz D, Haas S. et al. Prothrombinaseinduced clotting time assay for determination of the anticoagulant effects of unfractionated and low-molecular-weight heparins, fondaparinux, and thrombin inhibitors. Am J Clin Pathol 2008; 130: 446-454.