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线性判别分析在提取核抗原免疫分析系统性能评估中的应用及其在系统性自身免疫性风湿病筛查和诊断中的价值。

Application of linear discriminant analysis in performance evaluation of extractable nuclear antigen immunoassay systems in the screening and diagnosis of systemic autoimmune rheumatic diseases.

机构信息

Department of Pathology, Vancouver General Hospital, 855 West 12th Ave, Vancouver, BC, Canada V5Z 1M9.

出版信息

Am J Clin Pathol. 2012 Oct;138(4):596-603. doi: 10.1309/AJCPX1SQXKI3MWNN.

DOI:10.1309/AJCPX1SQXKI3MWNN
PMID:23010715
Abstract

This study applied a linear discriminant analysis model to evaluate the performance of 2 types of commercially available extractable nuclear antigen (ENA) immunoassays for the screening and diagnosis of systemic autoimmune rheumatic diseases (SARDs) in a large tertiary hospital reference laboratory: (1) an enzyme-linked immunosorbent assay (ELISA) and (2) a multiplex bead-based immunoassay (MPBI). The results of the study showed both ENA immunoassays had comparable sensitivity for the detection of SARDs compared with the antinuclear antigen immunofluorescence (ANA-IF) method (ANA-IF: 85.6%, ENA-ELISA: 91.5%, ENA-MPBI: 83.1%, pairwise comparisons with ANA-IF: P > .05). However, both ENA immunoassays offered improved specificity compared with the ANA-IF (ANA-IF: 24.2%; ENA-ELISA: 39.8%; ENA-MPBI: 53.1%; pairwise comparison with ANA-IF: P < .001). The use of a more specific screening immunoassay with comparable sensitivity to ANA-IF is important in a tertiary hospital with high prevalence of non-SARD immune diseases. Diagnostic performance of the ENA/dsDNA components by the MPBI and ELISA methods did not differ significantly (area under the curve [AUC], 81.0% vs 83.0%, respectively, P > .05), but the key ENA/dsDNA variables contributing to the discriminating power of the assays for the diagnosis of specific SARDs were reagent/method dependent.

摘要

本研究应用线性判别分析模型评估了两种市售可提取核抗原(ENA)免疫分析在大型三级医院参考实验室中筛查和诊断系统性自身免疫性风湿病(SARD)的性能:(1)酶联免疫吸附测定(ELISA)和(2)多指标 bead 基免疫分析(MPBI)。研究结果表明,与抗核抗体免疫荧光(ANA-IF)方法相比,两种 ENA 免疫分析在检测 SARD 方面具有相当的敏感性(ANA-IF:85.6%,ENA-ELISA:91.5%,ENA-MPBI:83.1%,两两比较与 ANA-IF:P>0.05)。然而,与 ANA-IF 相比,两种 ENA 免疫分析均提供了更好的特异性(ANA-IF:24.2%;ENA-ELISA:39.8%;ENA-MPBI:53.1%;两两比较与 ANA-IF:P<0.001)。在自身免疫性疾病高发的三级医院中,使用具有与 ANA-IF 相当敏感性的更特异性筛查免疫分析很重要。MPBI 和 ELISA 方法的 ENA/dsDNA 成分的诊断性能没有显著差异(曲线下面积[AUC],分别为 81.0%和 83.0%,P>0.05),但有助于区分特定 SARD 诊断的检测能力的关键 ENA/dsDNA 变量取决于试剂/方法。

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