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Thromb Haemost 1992; 68(04): 413-417
DOI: 10.1055/s-0038-1646288
Original Article
Schattauer GmbH Stuttgart

Multicentric Evaluation of a New Assay for Prothrombin Fragment F1+2 Determination

H D Bruhn
1   The 1. Medizinische Klinik, Kiel, FRG
,
J Conard
2   The Hôtel-Dieu de Paris, Paris, France
,
M Mannucci
3   The Universitá di Milano, Ospedale Policlinico, Italy
,
J Monteagudo
4   The Hosp. Clinico Provincial, Barcelona, Spain
,
H Pelzer
5   The Behringwerke AG, Marburg, FRG
,
J C Reverter
4   The Hosp. Clinico Provincial, Barcelona, Spain
,
M Samama
2   The Hôtel-Dieu de Paris, Paris, France
,
A Tripodi
3   The Universitá di Milano, Ospedale Policlinico, Italy
,
C Wagner
5   The Behringwerke AG, Marburg, FRG
› Author Affiliations
Further Information

Publication History

Received 16 December 1991

Accepted after revision 04 May 1992

Publication Date:
04 July 2018 (online)

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Summary

A multicenter study of a recently developed ELISA for the determination of prothrombin fragment Fl+2 was performed in order to evaluate analytical and clinical aspects.

Mean intra-assay and inter-assay reproducibility were found to be 11.0 and 12.6%, respectively. The measuring range covered by the calibration curve reaches from 0.04 to 10.0 nM/1 Fl+2. Testing 133 healthy subjects a reference range of 0.37 to 1.11 nM/1 Fl+2 (2.5–97.5 percentile) with a median of 0.66 nM/1 F1+2 was calculated. Minor difficulties with blood sampling (venous occlusion for 2 min) did not affect Fl+2 plasma concentrations.

Significantly increased F1+2 levels were measured in patients with leukemia (p <0.0001), severe liver disease (p <0.005) and after myocardial infarction (p <0.01). Elevated F1+2 concentration before the beginning of heparin therapy (1.25 nM/1) decreased to 0.77 nM/1 (p <0.0001) after 1 day of therapy. For patients in the stable phase of oral anticoagulant therapy decreasing Fl+2 concentrations were measured with increasing INR. Fl+2 levels were already significantly reduced in patients with INR <2.0 (0.56 nM/1; p = 0.0005). Thus Fl+2 determination may be helpful in identifying activation processes as well as in monitoring anticoagulant therapy.

 

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