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使用单一临床样本对两种市售登革病毒(DENV)NS1捕获酶联免疫吸附测定法进行比较,以诊断急性登革病毒感染。

Comparison of two commercially available dengue virus (DENV) NS1 capture enzyme-linked immunosorbent assays using a single clinical sample for diagnosis of acute DENV infection.

作者信息

Bessoff Kovi, Delorey Mark, Sun Wellington, Hunsperger Elizabeth

机构信息

Centers for Disease Control and Prevention, Division of Vector-Borne Infectious Diseases, Dengue Branch, SanJuan, Puerto Rico 00920.

出版信息

Clin Vaccine Immunol. 2008 Oct;15(10):1513-8. doi: 10.1128/CVI.00140-08. Epub 2008 Aug 6.

Abstract

Dengue virus (DENV) nonstructural protein 1 (NS1) has shown promise as a novel diagnostic marker of acute DENV infection. Current techniques used to diagnose acute DENV infection, including virus isolation and reverse transcription-PCR (RT-PCR), are costly and difficult to perform, while traditional serological assays have low sensitivities during the acute stage of infection. Two commercially available NS1 antigen capture enzyme-linked immunosorbent assays (ELISAs), the Platelia dengue NS1Ag test (Bio-Rad Laboratories, Marnes La Coquette, France) and the Pan-E dengue early ELISA test (Panbio Diagnostics, Brisbane, Australia), were evaluated against a well-characterized panel of 208 real-time RT-PCR- and virus isolation-positive sera, as well as 45 real-time RT-PCR- and serologically negative sera from patients with other acute febrile illnesses. The overall sensitivities were 64.9% (95% confidence interval [CI(95)], 58.2 to 71.1%) for the Panbio test and 83.2% (CI(95), 77.5 to 87.7%) for the Bio-Rad test, with interserotype variation, especially for DENV serotype 4. Predictive models were constructed to identify factors that had a significant influence on a test's outcome with respect to this panel of samples in order to identify the conditions in which the test will be most effective as a diagnostic tool. The immunoglobulin G titer was found to be the only covariate that significantly influenced results in the Bio-Rad test, while serotype and the day postonset were found to significantly influence results in the Panbio test. We concluded that the NS1 capture ELISA is a useful tool that can improve testing algorithms to diagnose DENV infection in single samples from acute and early convalescent cases.

摘要

登革病毒(DENV)非结构蛋白1(NS1)已显示出有望成为急性登革病毒感染的新型诊断标志物。目前用于诊断急性登革病毒感染的技术,包括病毒分离和逆转录-聚合酶链反应(RT-PCR),成本高昂且操作困难,而传统血清学检测在感染急性期的敏感性较低。针对一组经过充分鉴定的208份实时RT-PCR和病毒分离阳性血清,以及45份来自其他急性发热性疾病患者的实时RT-PCR和血清学阴性血清,对两种市售的NS1抗原捕获酶联免疫吸附测定(ELISA),即Platelia登革热NS1Ag检测(伯乐生命医学产品公司,法国马恩拉科凯特)和泛E登革热早期ELISA检测(Panbio诊断公司,澳大利亚布里斯班)进行了评估。Panbio检测的总体敏感性为64.9%(95%置信区间[CI(95)],58.2%至71.1%),伯乐检测为83.2%(CI(95),77.5%至87.7%),存在血清型间差异,尤其是对于登革病毒血清型4。构建预测模型以识别对此组样本而言对检测结果有显著影响的因素,以便确定该检测作为诊断工具最有效的条件。发现免疫球蛋白G滴度是唯一显著影响伯乐检测结果的协变量,而血清型和发病后天数被发现显著影响Panbio检测结果。我们得出结论,NS1捕获ELISA是一种有用的工具,可改进检测算法以诊断急性和早期恢复期病例单一样本中的登革病毒感染。

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