Variability of cut‐off values for the detection of lupus anticoagulants: results of an international multicenter multiplatform study

Essentials Between‐lab variations of cut‐off values in lupus anticoagulant detection are unknown. Cut‐off values were calculated in 11 labs each testing plasma from 120 donors with 3 platforms. Major variation was observed even within the same platform. Cut‐off values determined in different labs ar...

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Bibliographic Details
Published in:Journal of thrombosis and haemostasis 2017-06, Vol.15 (6), p.1180-1190
Main Authors: Tripodi, A., Chantarangkul, V., Cini, M., Devreese, K., Dlott, J. S, Giacomello, R., Gray, E., Legnani, C., Martinuzzo, M. E., Pradella, P., Siegemund, A., Subramanian, S., Suchon, P., Testa, S.
Format: Article
Language:English
Subjects:
activated partial thromboplastin time
Adolescent
Adult
Aged
Anticoagulants
antiphospholipid syndrome
Antiphospholipid Syndrome - blood
Biochemistry
Biochemistry, Molecular Biology
Blood Coagulation Tests - methods
Cardiology and cardiovascular system
Clotting
dilute Russell viper venom test
Female
Healthy Volunteers
Human health and pathology
Humans
Laboratories
Life Sciences
Lupus
Lupus Coagulation Inhibitor - blood
Male
Middle Aged
Normal Distribution
Parameter estimation
Partial Thromboplastin Time
Plasma - chemistry
Prothrombin Time - methods
Reference Values
Reproducibility of Results
Santé publique et épidémiologie
screening
standardization
Statistical analysis
Systemic lupus erythematosus
Thromboplastin
Venom
Young Adult
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Summary:Essentials Between‐lab variations of cut‐off values in lupus anticoagulant detection are unknown. Cut‐off values were calculated in 11 labs each testing plasma from 120 donors with 3 platforms. Major variation was observed even within the same platform. Cut‐off values determined in different labs are not interchangeable. Summary Background Cut‐off values for interpretation of lupus anticoagulant (LA) detection are poorly investigated. Aims (i) To assess whether results from healthy donors were normally distributed and (ii) the between‐laboratories differences in cut‐off values for screening, mixing and LA confirmation when calculated as 99th or 95th centiles, and (iii) to assess their impact on the detection rate for LA. Methods Each of 11 laboratories using one of the three widely used commercial platforms for LA detection was asked to collect plasmas from 120 healthy donors and to perform screening, mixing and LA confirmation with two methods (activated partial thromboplastin time [APTT] and dilute Russell viper venom [dRVV]). A common set of LA‐positive or LA‐negative freeze‐dried plasmas was used to assess the LA detection rate. Results were centralized (Milano) for statistical analysis. Results and conclusions (i) Clotting times or ratios for healthy subjects were not normally distributed in the majority of cases. The take‐home message is that cut‐off values should be determined preferably by the non‐parametric method based on centiles. (ii) There were relatively large inter‐laboratory cut‐off variations even within the same platform and the variability was marginally attenuated when results were expressed as ratios (test‐to‐normal pooled plasma). The take‐home message is that cut‐off values should be determined locally. (iii) There were differences between cut‐off values calculated as 99th or 95th centiles that translate into a different LA detection rate (the lower the centile the greater the detection rate). The take‐home message is that cut‐off values determined as the 95th centile allow a better LA detection rate.
ISSN:1538-7933
1538-7836
1538-7836
DOI:10.1111/jth.13678