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Rapid detection of glycoprotein G gene for the diagnosis and typing of herpes simplex virus infection in genital herpes

机译:糖蛋白G基因的快速检测用于生殖器疱疹单纯疱疹病毒感染的诊断和分型

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摘要

OBJECTIVE: To develop a new, rapid, and convenient technique for the diagnosis and typing of herpes simplex virus (HSV) in genital herpes (GH). METHODS: Using samples from skin vesicle fluid and urogenital mucosal swabs of subjects with GH, conventional polymerase chain reaction (PCR) (directed to polymerase gene: PCRpG) were compared with a newly developed PCR (directed to HSV glycoprotein gene: PCRgG). Both PCR methods were compared with virus isolation culture (VI) with indirect immunofluorescent staining (IIF). RESULTS: 80 samples from 40 GH patients (25 males) were tested. Positive results were seen in 52.5% (42/80) using PCRgG compared with 40% (32/80) by VI. Most of PCRgG positive samples (95.1%) were caused by HSV-2 infection. In samples from healing lesions, HSV was detected more often by PCRgG, than by VI. The results of typing by PCRgG and IIF were highly consistent. CONCLUSION: PCRgG is more sensitive than VI and PCRgG in detecting HSV in urogenital samples from subjects with GH. PCRgG is a convenient technique for the rapid detection and typing of GH.




机译:目的:开发一种新的,快速,便捷的技术,用于生殖器疱疹(GH)的单纯疱疹病毒(HSV)的诊断和分型。方法:使用GH患者皮肤囊泡液和泌尿生殖道粘膜拭子样本,将常规聚合酶链反应(PCR)(针对聚合酶基因:PCRpG)与新开发的PCR(针对HSV糖蛋白基因:PCRgG)进行比较。两种PCR方法都与带有间接免疫荧光染色(IIF)的病毒分离培养物(VI)进行了比较。结果:从40名GH患者(25名男性)中检测了80个样本。使用PCRgG的阳性结果为52.5%(42/80),相比之下VI的阳性结果为40%(32/80)。大多数PCRgG阳性样品(95.1%)是由HSV-2感染引起的。在来自治愈性病变的样本中,PCRgG检出HSV的频率高于VI检出HSV的频率。 PCRgG和IIF进行分型的结果高度一致。结论:PCRgG在检测GH患者泌尿生殖道样本中的HSV方面比VI和PCRgG更为灵敏。 PCRgG是用于GH快速检测和分型的便捷技术。




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