A multi-laboratory assessment of congenital thrombophilia assays performed on the ACL TOP 50 family for harmonisation of thrombophilia testing in a large laboratory network

Author:

Favaloro Emmanuel J.123ORCID,Mohammed Soma1,Vong Ronny1,Chapman Kent4,Swanepoel Priscilla4,Kershaw Geoff5,Cai Nancy5,Just Sarah6,Connelly Lynne6,Brighton Timothy7,Pasalic Leonardo12

Affiliation:

1. Haematology , Institute of Clinical Pathology and Medical Research (ICPMR), NSW Health Pathology, Westmead Hospital , Westmead , NSW , Australia

2. Sydney Centres for Thrombosis and Haemostasis , Westmead , NSW , Australia

3. School of Biomedical Sciences , Charles Sturt University , Wagga Wagga , NSW , Australia

4. Haematology , NSW Health Pathology, John Hunter Hospital , Newcastle , NSW , Australia

5. Haematology , NSW Health Pathology, Prince Alfred Hospital , Camperdown , NSW , Australia

6. Haematology , NSW Health Pathology, Royal North Shore Hospital , St Leonards , NSW , Australia

7. Haematology , NSW Health Pathology, Prince of Wales Hospital , Randwick , NSW , Australia

Abstract

Abstract Objectives Thrombophilia testing is commonly performed within hemostasis laboratories, and the ACL TOP 50 family of instruments represent a new ‘single platform’ of hemostasis instrumentation. The study objective was to evaluate these instruments and manufacturer reagents for utility of congenital thrombophilia assays. Methods Comparative evaluations of various congenital thrombophilia assays (protein C [PC], protein S [PS], antithrombin [AT], activated protein C resistance [APCR]) using newly installed ACL TOPs 550 and 750 as well as comparative assessments with existing, predominantly STAGO, instrumentation and reagents. Verification of manufacturer assay normal reference ranges (NRRs). Results HemosIL PC and free PS assays showed good comparability with existing Stago methods (R>0.9) and could be considered as verified as fit for purpose. HemosIL AT showed high relative bias with samples from patients on direct anti-Xa agents, compromising utility. Manufacturer NRRs for PC, PS and AT were verified with minor variance. Given the interference with direct anti-Xa agents, an alternate assay (Hyphen) was evaluated for AT, and the NRR also verified. The HemosIL Factor V Leiden (APC Resistance V) evidenced relatively poor performance compared to existing assays, and could not be adopted for use in our network. Conclusions This evaluation of HemosIL reagents on ACL TOP 50 family instruments identified overall acceptable performance of only two (PC, free PS) of four thrombophilia assays, requiring use of third-party reagents on ACL instruments for the other two assays (AT, APCR).

Publisher

Walter de Gruyter GmbH

Subject

Biochemistry (medical),Clinical Biochemistry,General Medicine

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