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在使用口服生物利用度糖蛋白IIb/IIIa拮抗剂罗昔非班给药的患者安全性监测临床试验中,药物依赖性抗体检测的验证与实施。

Validation and implementation of drug-dependent antibody assays in clinical trials for safety monitoring of patients dosed with roxifiban, an orally bioavailable glycoprotein IIb/IIIa antagonist.

作者信息

Barrett Yu Chen, Ebling William, Pieniaszek Henry, Billheimer Jeffrey, Seiffert Dietmar

机构信息

Bristol-Myers Squibb Company, Princeton, NJ, USA.

出版信息

J Pharm Biomed Anal. 2007 Aug 15;44(4):938-46. doi: 10.1016/j.jpba.2007.03.030. Epub 2007 Mar 31.

DOI:10.1016/j.jpba.2007.03.030
PMID:17485191
Abstract

Thrombocytopenia exposes patients to increased bleeding risk. This serious adverse event was observed with a frequency of approximately 2% in early clinical trials with the potent, orally bioavailable glycoprotein (GP) IIb/IIIa receptor antagonist roxifiban. We previously reported that drug-dependent antibodies (DDAbs) to GP IIb/IIIa are the main cause of thrombocytopenia with roxifiban. Two ELISA assays for detection of free DDAbs (in citrate plasma) and total DDAbs (in EDTA plasma to elute platelet bound DDAbs) were developed and analytically validated. These tests served two purposes during the clinical development program, to pre-screen patients for pre-existing antibodies and monitor patients for increasing antibody titers as a surrogate for eminent thrombocytopenia. The free DDAb assay showed inter and intra-assay precision of 5-12 and 12-14% CV, respectively. The total DDAb assay showed a precision of 5-10 and 4-12% CV, respectively. Three cycles of freeze-thaw did not significantly alter DDAb values in citrate plasma, EDTA plasma or extraction solution. The clinical qualifications of the two assays were conducted in two phase II clinical trials in coronary arterial disease (CAD) patients dosed with roxifiban. Both assays have demonstrated clinical sensitivity of nearly 99-100% and clinical specificity of nearly 95%.

摘要

血小板减少症会使患者面临更高的出血风险。在早期临床试验中,强效口服生物可利用糖蛋白(GP)IIb/IIIa受体拮抗剂罗昔非班出现这种严重不良事件的频率约为2%。我们之前报道过,针对GP IIb/IIIa的药物依赖性抗体(DDAb)是罗昔非班导致血小板减少症的主要原因。我们开发并通过分析验证了两种用于检测游离DDAb(在枸橼酸盐血浆中)和总DDAb(在EDTA血浆中以洗脱与血小板结合的DDAb)的ELISA检测方法。在临床开发项目中,这些检测有两个目的,一是对患者进行预先筛查以检测其是否预先存在抗体,二是监测患者抗体滴度的升高情况,以此作为即将发生血小板减少症的替代指标。游离DDAb检测的批间和批内精密度分别为5 - 12%和12 - 14%变异系数(CV)。总DDAb检测的精密度分别为5 - 10%和4 - 12% CV。三个冻融循环并未显著改变枸橼酸盐血浆、EDTA血浆或提取溶液中的DDAb值。这两种检测方法的临床验证是在两项针对接受罗昔非班治疗的冠状动脉疾病(CAD)患者的II期临床试验中进行的。两种检测方法均显示出近99 - 100%的临床敏感性和近95%的临床特异性。

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