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一项基于功能性凝血酶原时间检测法对一组意大利静脉血栓形成患者中因子V莱顿突变携带者进行鉴定的临床评估。

Clinical evaluation of a functional prothrombin time-based assay for identification of factor V Leiden carriers in a group of Italian patients with venous thrombosis.

作者信息

Gessoni Gianluca, Valverde Sara

机构信息

Clinical Pathology Laboratory, Ospedale Civile, Chioggia, Venice, Italy.

出版信息

Blood Coagul Fibrinolysis. 2007 Oct;18(7):603-10. doi: 10.1097/MBC.0b013e3282891e2f.

DOI:10.1097/MBC.0b013e3282891e2f
PMID:17890946
Abstract

The efficiency of a new prothrombin-based activated protein C (APC) resistance test to detect factor V Leiden (FVL) was clinically evaluated in 150 Italian patients with deep venous thrombosis. Patient samples are diluted in factor-V-deficient plasma, an APC-containing reagent, and specific factor V activator; after incubation, clotting is initiated by addition of activated-factor-FV-dependent prothrombin activator. Two prothrombin time determinations were performed under identical assay conditions except that no APC was added to one. A ratio over 4.2 for normal individuals and under 2.0 for FVL patients is expected: between 1.3 and 1.9 for FVL heterozygotes, and between 1.0 and 1.1 for FVL homozygotes. Using a predefined cut-off ratio of 2.0, a specificity and a sensitivity of 1.00 for detection of FVL mutation were found. With a cut-off ratio of 1.1, a specificity of 0.98 and a sensitivity of 1.00 were found for discrimination between FVL heterozygous (n = 60) and homozygous (n = 6). No interferences by heparins, oral contraceptives, oral anticoagulant therapy, protein C, protein S, D-dimer, homocysteine, MTHFR mutations and antiphospholipid autoantibodies were detected. In our experience, this new prothrombin time-based APC resistance assay provides improved discrimination between normal individuals and FVL carriers compared with the classical methods. Moreover, this new assay allows good discrimination between homozygous and heterozygous FVL carriers. In the authors' experience this prothrombin time-based method was not influenced by many factors compared with the classical activated partial thromboplastin time-based method.

摘要

在150例意大利深静脉血栓患者中对一种基于凝血酶原的新型活化蛋白C(APC)抵抗试验检测因子V莱顿(FVL)的效率进行了临床评估。将患者样本在缺乏因子V的血浆、含APC的试剂和特定因子V激活剂中进行稀释;孵育后,通过加入依赖活化因子FV的凝血酶原激活剂启动凝血。在相同的检测条件下进行两次凝血酶原时间测定,只是其中一次不添加APC。正常个体的比值预期超过4.2,FVL患者的比值预期低于2.0:FVL杂合子的比值在1.3至1.9之间,FVL纯合子的比值在1.0至1.1之间。使用预先定义的截断比值2.0,发现检测FVL突变的特异性和敏感性均为1.00。截断比值为1.1时,区分FVL杂合子(n = 60)和纯合子(n = 6)的特异性为0.98,敏感性为1.00。未检测到肝素、口服避孕药、口服抗凝治疗、蛋白C、蛋白S、D - 二聚体、同型半胱氨酸、MTHFR突变和抗磷脂自身抗体的干扰。根据我们的经验,与经典方法相比,这种基于凝血酶原时间的新型APC抵抗试验在区分正常个体和FVL携带者方面有更好的表现。此外,这种新试验能够很好地区分FVL纯合子和杂合子携带者。根据作者的经验,与经典的基于活化部分凝血活酶时间的方法相比,这种基于凝血酶原时间的方法不受许多因素的影响。

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