重组梅利特布鲁氏菌Bp26基因间接ELISA试剂盒诊断人布鲁氏菌病的准确性

S. Hoseini, E. Ghaznavirad, A. Farazi
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引用次数: 0

摘要

背景:考虑到布鲁氏菌病在伊朗的流行,有必要选择一种特定而敏感的实验室方法来快速及时地诊断。本研究的目的是评估间接酶联免疫吸附试验(ELISA)检测人类布鲁氏菌病的准确性,以便为Wright、2ME和商业ELISA试剂盒等常规检测提供合适的替代方案。材料与方法:本研究以(omp28)bp26基因产生的重组蛋白为抗原,包被微孔板。共有124份经STA和2次ME测试批准的正常健康人(n=62)和急性布鲁氏菌病患者(n=62)的血清样本被纳入研究。结果:患者组平均年龄39.8±13.5岁,健康组平均年龄36.1±12.7岁。此外,66.1%的患者是男性,62.9%的患者生活在农村地区,而健康组的这一数字分别为71%和45.2%。本研究中使用的ELISA试剂盒的敏感性为92%,特异性为87%,阳性预测值为88%,阴性预测值为92%,准确率为90%。结论:ELISA诊断试剂盒对大多数阳性人血清均有反应。然而,该试剂盒需要用来自不同地区的更大样本量的临床标本和各种临床形式的人类布鲁氏菌病进行进一步评估。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Accuracy of Indirect ELISA Prepared from Recombinant Bp26 Gene of Brucella melitensis in Diagnosis of Human Brucellosis
Background: Considering the prevalence of brucellosis in Iran, it is necessary to choose a specific and sensitive laboratory method to diagnose it in a rapid and timely manner. The aim of this study was to assess the accuracy of indirect enzyme-linked immunosorbent assay (ELISA) for detecting brucellosis in humans in order to have an appropriate alternative to conventional tests such as Wright, 2ME, and commercial ELISA kits. Materials and Methods: In this study, the recombinant protein produced from the gene (omp28) bp26 Brucella melitensis was used as an antigen for coating microplate wells. A total of 124 serum samples of normal healthy individuals (n=62) and patients with acute brucellosis (n=62) approved by STA and 2 ME tests were entered into the study. The data were analyzed in SPSS (ver.18). Results: The mean age was 39.8±13.5 years in the patient group and 36.1±12.7 years in the healthy group. Furthermore, 66.1% of the patients were male and 62.9% lived in rural regions, while these figures were respectively 71% and 45.2% in the healthy group. The sensitivity of 92% and specificity of 87% and a positive predictive value of 88% and a negative predictive value of 92% and an accuracy of 90% were determined for ELISA kit used in this study. Conclusion: The ELISA diagnostic kit reacted to most of the positive human sera. However, this kit needs to be further evaluated with a larger sample size of clinical specimens from different regions and with various clinical forms of human brucellosis.
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