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酶联免疫吸附试验检测人水通道蛋白-4 抗体:敏感性、特异性及与免疫组化的直接比较。

Testing for antibodies to human aquaporin-4 by ELISA: sensitivity, specificity, and direct comparison with immunohistochemistry.

机构信息

Division of Molecular Neuroimmunology, Department of Neurology, University of Heidelberg, Heidelberg, Germany.

出版信息

J Neurol Sci. 2012 Sep 15;320(1-2):32-7. doi: 10.1016/j.jns.2012.06.002. Epub 2012 Jun 16.

DOI:10.1016/j.jns.2012.06.002
PMID:22705047
Abstract

BACKGROUND

Several assays have been developed to detect antibodies to aquaporin-4 (NMO-IgG/AQP4-Ab). However, many of these assays require sophisticated techniques and are thus only available at specialized laboratories. This is problematic since NMO-IgG/AQP4-Ab testing has important prognostic and therapeutic implications.

OBJECTIVE

To evaluate a newly developed, commercial, enzyme-linked immunosorbent assay (ELISA) for detecting NMO-IgG/AQP4-Ab.

METHODS

Serum samples from 261 patients with NMO spectrum disorders (NMOSD; n=108) and controls (n=153) were tested for AQP4-Ab by using ELISA. Of these patients, 207 were tested in parallel using a standard immunohistochemical (IHC) assay.

RESULTS

Fifty of 66 (75.8%) patients with NMO, 17/25 (68%) with LETM, 3/14 (21.4%) with ON, 2/3 (66.7%) with ON and non-extensive transverse myelitis, and 2/153 (1.3%) controls tested positive in the ELISA. Of those NMOSD patients tested by both ELISA and IHC, 10 were positive only in the ELISA and 3 exclusively in the IHC assay, suggesting that the overall sensitivity of the ELISA was higher than that of the standard IHC assay. The ELISA yielded very good intra- and inter-run reproducibility with regard to AQP4-Ab detection and good intrarun, but only moderate inter-run reproducibility with regard to AQP4-Ab quantification. Anti-AQP4 serum concentrations correlated with disease activity (p<0.00001), but did not differ between patients with NMO and patients with isolated LETM or ON.

CONCLUSION

The ELISA evaluated here provides a relatively sensitive and easy-to-use diagnostic tool for detecting antibodies to AQP4 and could make AQP4-Ab testing, which is of high clinical relevance, more widely available.

摘要

背景

已经开发出几种检测水通道蛋白 4(NMO-IgG/AQP4-Ab)抗体的检测方法。然而,其中许多方法需要复杂的技术,因此仅在专门的实验室可用。这是有问题的,因为 NMO-IgG/AQP4-Ab 检测具有重要的预后和治疗意义。

目的

评估一种新开发的商业酶联免疫吸附试验(ELISA)用于检测 NMO-IgG/AQP4-Ab。

方法

使用 ELISA 检测了 261 名 NMO 谱障碍(NMOSD;n=108)和对照组(n=153)患者的血清样本中的 AQP4-Ab。其中 207 名患者使用标准免疫组织化学(IHC)检测方法进行平行检测。

结果

66 名 NMO 患者中有 50 名(75.8%)、25 名 LETM 中有 17 名(68%)、14 名 ON 中有 3 名(21.4%)、3 名 ON 和非广泛性横贯性脊髓炎中有 2 名(66.7%)和 153 名对照组中有 2 名(1.3%)检测为阳性。在通过 ELISA 和 IHC 检测的 NMOSD 患者中,有 10 名仅在 ELISA 中呈阳性,3 名仅在 IHC 检测中呈阳性,这表明 ELISA 的总体敏感性高于标准 IHC 检测。ELISA 在 AQP4-Ab 检测方面具有良好的内和重复性,并且在 AQP4-Ab 定量方面具有良好的内重复性,但仅具有中等的间重复性。抗 AQP4 血清浓度与疾病活动相关(p<0.00001),但 NMO 患者与单独的 LETM 或 ON 患者之间无差异。

结论

这里评估的 ELISA 提供了一种相对敏感且易于使用的诊断工具,用于检测抗 AQP4 抗体,并且可以使具有高临床相关性的 AQP4-Ab 检测更广泛地可用。

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