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一种新的用于抗心磷脂抗体IgM的铕(Eu³⁺)标记方法。

A new Eu(3+)-labeled method for anticardiolipin antibody IgM.

作者信息

Ye Yan, Hu Zhigang, Liu Jie, Chen Guoqian, Zhou Yaohong

机构信息

Department of Clinical Laboratory, Affiliated Wuxi People's Hospital of Nanjing Medical University, Wuxi, China.

出版信息

J Clin Lab Anal. 2014 Jul;28(4):335-40. doi: 10.1002/jcla.21690. Epub 2014 Mar 22.

Abstract

BACKGROUND

The anticardiolipin antibodies (aCL) test has become a laboratory standard for the clinical diagnosis of antiphospholipid syndrome (APS). To better the quantitative detection of aCL-IgM so as to classify patients correctly and timely as APS positive, we established herein a new immunoassay based on a time-resolved fluoroimmunoassay (TRFIA).

METHODS

The complex of cardiolipin plus bovine anti-β2 glycoprotein-I was used as antigen fixed on microtiter plates to detect serum aCL-IgM, and Eu(3+) -labeled rabbit antihuman IgM was used as conjugate. The precision, sensitivity, specificity, coefficient of recovery, and stability of the assay were evaluated, and comparison with the traditional, classical enzyme-linked immunosorbent assay (ELISA) was also made.

RESULTS

The detection limit of the aCL-IgM TRFIA kit we established was 0.1 MPL U/ml, with a wider detectable range than commercial ELISA ones when a strong-positive specimen was diluted from 2,630.9 to 0.08 MPL U/ml. There was a good liner range within 0.16 to 2,630.9 MPL U/ml, whereas it was within 5.14 to 328.86 MPL U/ml when using three commercial ELISA ones. The average intra- and interassay variability was 3.19 and 3.70%, respectively. The mean recovery rate was 101.95%. The clinical diagnostic specificity was 98%. Additionally, the established assay kit presented good characteristics of stability and correlated well with the ELISA, and the correlation coefficient was 0.955.

CONCLUSION

The aCL-IgM TRFIA provides an approach to a more sensitive and reliable diagnosis of APS. Further validation of its use is required.

摘要

背景

抗心磷脂抗体(aCL)检测已成为抗磷脂综合征(APS)临床诊断的实验室标准。为了更好地定量检测aCL-IgM,以便正确、及时地将患者分类为APS阳性,我们在此建立了一种基于时间分辨荧光免疫分析(TRFIA)的新免疫分析方法。

方法

将心磷脂与牛抗β2糖蛋白-I的复合物用作固定在微量滴定板上的抗原,以检测血清aCL-IgM,并用铕(Eu3+)标记的兔抗人IgM作为结合物。评估了该分析方法的精密度、灵敏度、特异性、回收率和稳定性,并与传统的经典酶联免疫吸附测定(ELISA)进行了比较。

结果

我们建立的aCL-IgM TRFIA试剂盒的检测限为0.1 MPL U/ml,当强阳性标本从2630.9稀释至0.08 MPL U/ml时,其可检测范围比市售ELISA试剂盒更宽。在0.16至2630.9 MPL U/ml范围内有良好的线性范围,而使用三种市售ELISA试剂盒时,线性范围在5.14至328.86 MPL U/ml之间。平均批内和批间变异分别为3.19%和3.70%。平均回收率为101.95%。临床诊断特异性为98%。此外,所建立的检测试剂盒具有良好的稳定性,与ELISA相关性良好,相关系数为0.955。

结论

aCL-IgM TRFIA为APS的更敏感、可靠诊断提供了一种方法。需要对其使用进行进一步验证。

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