首页> 外文期刊>Journal of clinical laboratory analysis. >Evaluation of a new automated enzyme fluoroimmunoassay using recombinant plasmid dsDNA for the detection of anti-dsDNA antibodies in SLE.
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Evaluation of a new automated enzyme fluoroimmunoassay using recombinant plasmid dsDNA for the detection of anti-dsDNA antibodies in SLE.

机译:使用重组质粒DSDNA评估新的自动酶氟汞法测定,用于检测SLE中的抗DSDNA抗体。

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摘要

ELISA methods to detect anti-double-stranded DNA (anti-dsDNA) antibodies are highly sensitive, but are less specific for the diagnosis of SLE than the immunofluorescence test on Crithidia luciliae (CLIFT) and the Farr assay because they also detect low-avidity antibodies. This study evaluated the specificity, sensitivity, positive predictive value (PPV), and negative predictive value (NPV) of a new automated fluoroimmunoassay (EliA dsDNA; Pharmacia, Freiburg, Germany). We compared the results with those obtained using a commercial CLIFT and an in-house anti-dsDNA IgG ELISA method, and verified its putative ability to detect only high-avidity anti-dsDNA antibodies. Sera from 100 SLE patients and 120 controls were studied. The control group included 20 healthy donors, 70 patients with other rheumatic diseases (32 systemic sclerosis (SSc); 18 primary Sjogren syndrome (pSS), 20 rheumatoid arthritis (RA)), and 30 patients with various infectious diseases (ID). Anti-dsDNA avidity was estimated using an ELISA method based upon the law of mass action, and a simplified Scatchard plot analysis for data elaboration; the apparent affinity constant (Kaa) was calculated and expressed as arbitrary units (L/U). Sensitivity, specificity, PPV, and NPV for SLE were 64%, 95.8%, 93.8% and 72.7%, respectively, for the EliA anti-dsDNA assay; 55%, 99.2%, 98.5%, and 68.8%, respectively, for the CLIFT; and 64%, 93.3%, 90.6%, and 72.3%, respectively, for the in-house ELISA. Although EliA anti-dsDNA was positive mainly in SLE patients with high- (Kaa>80 L/U) and intermediate- (Kaa 30-80 L/U) avidity antibodies (45.3% and 49.9%, respectively), it was also positive in five (7.8%) SLE patients with low-avidity anti-dsDNA antibodies, and five controls (three SSc, one pSS, and one ID) (mean Kaa = 16.4 +/- 9.04 L/U). In conclusion, EliA anti-dsDNA assay showed a higher sensitivity than the CLIFT, and a good specificity and PPV for SLE. Its putative ability to detect only high-avidity anti-dsDNA antibodies remains questionable. J. Clin. Lab. Anal. 16:227-232, 2002.
机译:以检测抗双链DNA(抗DSDNA)抗体的ELISA方法是高度敏感的,但对SLE的诊断而言比临时荧光素(Clift)和Farr测定的诊断较少,因为它们也检测到低耐酸性抗体。该研究评估了新自动化氟莫莫纳斯的特异性,敏感性,阳性预测值(PPV)和负预测值(NPV)(ELIA dsdna; Pharmacia,Freiburg,德国)。我们将结果与使用商业Clift和内部抗DSDNA IgG ELISA方法进行比较,并验证了其仅检测高耐酸性抗DSDNA抗体的推定能力。研究了100名SLE患者和120种对照的血清。对照组包括20名健康供体,70例其他风湿性疾病(32例全身硬化症(SSC); 18次初级Sjogren综合征(PSS),20例类风湿性关节炎(RA))和30名各种传染病(ID)患者。使用基于大规模作用规律的ELISA方法估计抗DSDNA亲经,以及用于数据阐述的简化旋涡曲线图分析;表观亲和力常数(KAA)计算并表示为任意单位(L / U)。对于ELIA抗DSDNA测定,SLE的敏感性,特异性,PPV和NPV分别为64%,95.8%,93.8%和72.7%; 55%,99.2%,98.5%和68.8%,克拉夫特分别为68.8%;对于内部ELISA,分别为64%,93.3%,90.6%和72.3%。虽然ELIA抗DSDNA主要是SLE患者,但在SLE患者中,患者高(KAA> 80L / U)和中间体 - (KAA 30-80L / u / U)亲经抗体(分别为45.3%和49.9%),也是阳性的在五(7.8%)的SLE患者中,具有低耐酸性抗DSDNA抗体,五种对照(三个SSC,一个PSS和一个ID)(平均KAA = 16.4 +/- 9.04 L / U)。总之,ELIA抗DSDNA测定显示比克拉夫更高的敏感性,以及SLE的良好特异性和PPV。其仅检测高耐酸性抗DSDNA抗体的推定能力仍然是可疑的。 J. Clin。实验室。肛门。 16:227-232,2002。

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