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首页> 外文期刊>Journal of Clinical Microbiology >Performance of HerpeSelect and Kalon Assays in Detection of Antibodies to Herpes Simplex Virus Type 2
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Performance of HerpeSelect and Kalon Assays in Detection of Antibodies to Herpes Simplex Virus Type 2

机译:HerpeSelect和Kalon分析在检测2型单纯疱疹病毒抗体中的性能

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摘要

The performances of commercial enzyme-linked immunosorbent assays (ELISAs) in detecting herpes simplex virus type 2 (HSV-2) antibodies have been inconsistent for African and human immunodeficiency virus (HIV)-positive populations. We compared the performances of the HerpeSelect and Kalon glycoprotein G2 ELISAs for patients with genital ulcer disease in Ghana and the Central African Republic. Sera from 434 women were tested with the HerpeSelect assay, and a subsample (n = 199) was tested by the Kalon assay. Ulcer swabs and cervicovaginal lavage samples were tested for HSV-2 DNA by PCR. HSV-2-seronegative women with detectable genital HSV-2 DNA were retested for HSV-2 antibodies 14 and 28 days later by the two ELISAs. A total of 346 (80%) women were positive by HerpeSelect at baseline, and 225 (54%) had detectable genital (lesional or cervicovaginal) HSV-2 DNA. Sixty-six (19%) HerpeSelect-positive samples had low-positive index values (1.1 to 3.5), and 58% of these samples had detectable genital HSV-2 DNA. Global agreement between the two serological assays was 86%. Concordance was high (99%) for sera that were negative by HerpeSelect or had high index values (>3.5). Defining infection detected by HSV-2 DNA PCR and/or Kalon assay as true infection, 71% of sera with low-positive index values were associated with true HSV-2 infection. Twenty-five women were identified as having nonprimary first-episode genital HSV-2 infection. Rates of HSV-2 seroconversion at day 14 were 77% (10/13 patients) by HerpeSelect assay and 23% (3/13 patients) by Kalon assay, with four additional seroconversions detected by Kalon assay at day 28. HIV serostatus did not influence assay performance. Low index values obtained with the HerpeSelect assay may correspond to true HSV-2 infection, in particular to nonprimary first episodes of genital HSV-2 infection, and need to be interpreted in the context of clinical history.
机译:对于非洲和人类免疫缺陷病毒(HIV)阳性人群,商业酶联免疫吸附测定(ELISA)在检测2型单纯疱疹病毒(HSV-2)抗体方面的性能一直不一致。我们比较了在加纳和中非共和国患有生殖器溃疡疾病的患者使用HerpeSelect和Kalon糖蛋白G2 ELISA的性能。用HerpeSelect分析法检测了434名女性的血清,通过Kalon分析法检测了一个子样本( n = 199)。通过PCR测试溃疡拭子和宫颈阴道灌洗样品的HSV-2 DNA。在14天和28天后,通过两次ELISA对具有可检测到的生殖器HSV-2 DNA的HSV-2阴性女性进行了HSV-2抗体的重新测试。共有346名(80%)妇女在基线时通过HerpeSelect呈阳性,而225名(54%)妇女具有可检测到的生殖器(病变或宫颈阴道)HSV-2 DNA。六十六(19%)个HerpeSelect阳性样本的阳性指数值较低(1.1至3.5),其中58%的样本具有可检测的生殖器HSV-2 DNA。两种血清学检测之间的总体一致性为86%。对于HerpeSelect阴性或具有高指数值(> 3.5)的血清,一致性较高(99%)。将通过HSV-2 DNA PCR和/或Kalon分析检测到的感染定义为真实感染,低阳性指数值的血清中有71%与真实HSV-2感染相关。确认有25名妇女患有非原发性首发生殖器HSV-2感染。通过HerpeSelect分析,在第14天的HSV-2血清转化率为77%(10/13例),通过Kalon分析,为23%(3/13例),在第28天通过Kalon分析又检测到4种血清转化。影响测定性能。通过HerpeSelect分析获得的低指数值可能对应于真正的HSV-2感染,特别是生殖器HSV-2感染的非原发性第一发作,需要在临床病史中加以解释。

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