Rachel Gehlen , Roxanne G. Moesbergen , CuiCui Bai , Philip G. de Groot , A.J.Gerard Jansen , Joost C.M. Meijers , Bas de Laat , Jasper A. Remijn
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Concerns have been raised about the validity of international normalized ratio (INR) measurements in lupus anticoagulant (LA)-positive APS patients because LA may interfere with phospholipid-dependent coagulation tests and could elevate INR measurements.</p></div><div><h3>Objectives</h3><p>Here, we aimed to determine the interference of antigen-specific monoclonal and isolated patient antibodies with LA activity on INR measurements.</p></div><div><h3>Methods</h3><p>Pooled normal plasma and control plasma from patients on VKA (without LA) were incubated with monoclonal and isolated patient immunoglobulin G antiprothrombin and anti–beta-2-glycoprotein I antibodies that express LA activity. INR was determined before and after addition using 3 laboratory assays (Owren STA-Hepato Prest, Quick STA-NeoPTimal, and Quick STA-Neoplastine R) and 1 point-of-care test device (CoaguChek Pro II).</p></div><div><h3>Results</h3><p>Antiprothrombin and anti–beta-2-glycoprotein I antibodies with LA activity interfered with recombinant human thromboplastin reagents (Quick STA-Neoplastine R and CoaguChek Pro II), particularly when added to plasma of VKA-treated controls. This effect was most evident on point-of-care test INR measurements, while the recombinant Quick reagent exhibited a lesser degree of interference. In contrast, tissue-derived thromboplastin reagents (Owren STA-Hepato Prest and Quick STA-NeoPTimal) remained largely unaffected by these antibodies, both in pooled normal plasma and VKA anticoagulated control plasma. Among these reagents, the Owren INR reagent exhibited the lowest sensitivity to the influence of LA antibodies. This observed difference in sensitivity is independent of the plasma dilution factor or the presence of factor V or fibrinogen in Owren reagent.</p></div><div><h3>Conclusion</h3><p>INR reagents that utilize recombinant human thromboplastin are more sensitive to the presence of monoclonal and patient-derived antibodies with LA activity. Consequently, APS patients positive for LA should be monitored using tissue-derived thromboplastin reagents, given its reduced susceptibility to interference by LA-causing antibodies.</p></div>","PeriodicalId":20893,"journal":{"name":"Research and Practice in Thrombosis and Haemostasis","volume":null,"pages":null},"PeriodicalIF":3.4000,"publicationDate":"2024-07-01","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://www.sciencedirect.com/science/article/pii/S2475037924001596/pdfft?md5=907440664fb64fd45bb59c757e8a972f&pid=1-s2.0-S2475037924001596-main.pdf","citationCount":"0","resultStr":"{\"title\":\"Interference of lupus anticoagulant causing antiprothrombin and anti–beta-2-glycoprotein I antibodies on international normalized ratio measurements: comparative analysis of international normalized ratio methods\",\"authors\":\"Rachel Gehlen , Roxanne G. Moesbergen , CuiCui Bai , Philip G. de Groot , A.J.Gerard Jansen , Joost C.M. 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INR was determined before and after addition using 3 laboratory assays (Owren STA-Hepato Prest, Quick STA-NeoPTimal, and Quick STA-Neoplastine R) and 1 point-of-care test device (CoaguChek Pro II).</p></div><div><h3>Results</h3><p>Antiprothrombin and anti–beta-2-glycoprotein I antibodies with LA activity interfered with recombinant human thromboplastin reagents (Quick STA-Neoplastine R and CoaguChek Pro II), particularly when added to plasma of VKA-treated controls. This effect was most evident on point-of-care test INR measurements, while the recombinant Quick reagent exhibited a lesser degree of interference. In contrast, tissue-derived thromboplastin reagents (Owren STA-Hepato Prest and Quick STA-NeoPTimal) remained largely unaffected by these antibodies, both in pooled normal plasma and VKA anticoagulated control plasma. Among these reagents, the Owren INR reagent exhibited the lowest sensitivity to the influence of LA antibodies. This observed difference in sensitivity is independent of the plasma dilution factor or the presence of factor V or fibrinogen in Owren reagent.</p></div><div><h3>Conclusion</h3><p>INR reagents that utilize recombinant human thromboplastin are more sensitive to the presence of monoclonal and patient-derived antibodies with LA activity. 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引用次数: 0
摘要
背景推荐将终身维生素K拮抗剂(VKA)治疗作为抗磷脂综合征(APS)血栓患者的标准治疗方法。由于狼疮抗凝剂(LA)阳性的APS患者的国际标准化比值(INR)测量值可能会干扰磷脂依赖性凝血试验,并使INR测量值升高,因此国际标准化比值(INR)测量值的有效性受到了关注。方法将使用 VKA(不含 LA)患者的池化正常血浆和对照血浆与表达 LA 活性的单克隆和分离患者免疫球蛋白 G 抗凝血酶和抗-beta-2-糖蛋白 I 抗体孵育。结果具有 LA 活性的抗凝血酶和抗-beta-2-糖蛋白 I 抗体会干扰重组人凝血酶试剂(Quick STA-Neoplastine R 和 CoaguChek Pro II),尤其是在加入经 VKA 处理的对照组血浆时。这种影响在床旁检测 INR 测量中最为明显,而重组 Quick 试剂的干扰程度较小。相比之下,组织源性凝血活酶试剂(Owren STA-Hepato Prest 和 Quick STA-NeoPTimal)在汇集的正常血浆和 VKA 抗凝对照血浆中基本不受这些抗体的影响。在这些试剂中,Owren INR 试剂对 LA 抗体影响的敏感性最低。结论 使用重组人凝血活酶的 INR 试剂对具有 LA 活性的单克隆抗体和患者衍生抗体更敏感。因此,应使用组织来源的凝血活酶试剂对 LA 阳性的 APS 患者进行监测,因为这种试剂不易受 LA 致癌性抗体的干扰。
Interference of lupus anticoagulant causing antiprothrombin and anti–beta-2-glycoprotein I antibodies on international normalized ratio measurements: comparative analysis of international normalized ratio methods
Background
Life-long vitamin K antagonist (VKA) therapy is recommended as a standard of care in antiphospholipid syndrome (APS) patients with thrombosis. Concerns have been raised about the validity of international normalized ratio (INR) measurements in lupus anticoagulant (LA)-positive APS patients because LA may interfere with phospholipid-dependent coagulation tests and could elevate INR measurements.
Objectives
Here, we aimed to determine the interference of antigen-specific monoclonal and isolated patient antibodies with LA activity on INR measurements.
Methods
Pooled normal plasma and control plasma from patients on VKA (without LA) were incubated with monoclonal and isolated patient immunoglobulin G antiprothrombin and anti–beta-2-glycoprotein I antibodies that express LA activity. INR was determined before and after addition using 3 laboratory assays (Owren STA-Hepato Prest, Quick STA-NeoPTimal, and Quick STA-Neoplastine R) and 1 point-of-care test device (CoaguChek Pro II).
Results
Antiprothrombin and anti–beta-2-glycoprotein I antibodies with LA activity interfered with recombinant human thromboplastin reagents (Quick STA-Neoplastine R and CoaguChek Pro II), particularly when added to plasma of VKA-treated controls. This effect was most evident on point-of-care test INR measurements, while the recombinant Quick reagent exhibited a lesser degree of interference. In contrast, tissue-derived thromboplastin reagents (Owren STA-Hepato Prest and Quick STA-NeoPTimal) remained largely unaffected by these antibodies, both in pooled normal plasma and VKA anticoagulated control plasma. Among these reagents, the Owren INR reagent exhibited the lowest sensitivity to the influence of LA antibodies. This observed difference in sensitivity is independent of the plasma dilution factor or the presence of factor V or fibrinogen in Owren reagent.
Conclusion
INR reagents that utilize recombinant human thromboplastin are more sensitive to the presence of monoclonal and patient-derived antibodies with LA activity. Consequently, APS patients positive for LA should be monitored using tissue-derived thromboplastin reagents, given its reduced susceptibility to interference by LA-causing antibodies.
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