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A Clinical Approach for Defining the Threshold between Low and Medium Anti-Cardiolipin Antibody Levels for QUANTA Flash Assays

机译:定义QUANTA快速测定中低抗心磷脂抗体水平阈值的临床方法

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摘要

The threshold between low and medium antibody levels for anticardiolipin (aCL) and anti-β2 glycoprotein I antibodies (aβ2GPI) for the diagnosis of antiphospholipid syndrome (APS) remains a matter of discussion. Our goal was to create a protocol for determining the low/medium antibody cut-off for aCL antibody methods based on a clinical approach, and utilize it to establish the clinically-relevant low/medium threshold for QUANTA Flash aCL chemiluminescent immunoassay (CIA) results. The study included 288 samples from patients with primary APS (n = 70), secondary APS (n = 42), suspected APS (n = 36), systemic lupus erythematosus (SLE) without APS (n = 96) and other connective tissue diseases (n = 44). All samples were tested for IgG and IgM aCL antibodies with QUANTA Flash CIA, along with traditional enzyme-linked immunosorbent assays (ELISAs) (QUANTA Lite). The assay specific low/medium threshold for QUANTA Flash aCL IgG and IgM assays (i.e., the equivalent of 40 GPL and MPL units) was established as 95 and 31 chemiluminescent units (CU), respectively, based on clinical performance and comparison to QUANTA Lite ELISAs. Agreement between CIA and ELISA assay results improved substantially when the platform-specific low/medium antibody threshold was used, as compared to agreement obtained on results generated with the assay cutoff: Cohen’s kappa increased from 0.85 to 0.91 for IgG aCL, and from 0.59 to 0.75 for IgM aCL results. This study describes a clinical approach for establishing the low/medium antibody threshold for aPL antibody assays, and successfully employs it to define 95 and 31 CU, respectively, as the low/medium cut point for QUANTA Flash aCL IgG and IgM results. This study can serve as a model for labs wishing to establish the appropriate low/medium aPL antibody threshold when implementing new aPL antibody assays.
机译:用于诊断抗磷脂综合症(APS)的抗心磷脂(aCL)和抗β2糖蛋白I抗体(aβ2GPI)的中低抗体水平之间的阈值仍然是讨论的问题。我们的目标是创建一种基于临床方法确定aCL抗体方法的低/中抗体临界值的方案,并利用该协议为QUANTA Flash aCL化学发光免疫分析(CIA)结果建立与临床相关的低/中阈值。该研究包括来自原发性APS(n = 70),继发性APS(n = 42),疑似APS(n = 36),无APS的系统性红斑狼疮(SLE)(n = 96)和其他结缔组织疾病患者的288个样本(n = 44)。使用QUANTA Flash CIA和传统的酶联免疫吸附测定(ELISA)(QUANTA Lite)对所有样品的IgG和IgM aCL抗体进行了测试。根据临床表现和与QUANTA Lite的比较,将QUANTA Flash aCL IgG和IgM分析的特定分析低/中阈值(相当于40 GPL和MPL单位)分别设置为95和31个化学发光单位(CU)。 ELISA。与使用平台特定的低/中抗体阈值时相比,CIA和ELISA分析结果之间的一致性有了显着改善,与通过分析截止产生的结果所达成的一致:IgG aCL的Cohen卡帕值从0.85增加到0.91,从0.59到0.59 IgM aCL结果为0.75。这项研究描述了建立aPL抗体测定的低/中抗体阈值的临床方法,并成功地将其用于分别定义95和31 CU,作为QUANTA Flash aCL IgG和IgM结果的低/中切点。这项研究可以为希望在实施新的aPL抗体测定时建立适当的低/中等aPL抗体阈值的实验室提供模型。

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