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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基因的快速检测可用于生殖器疱疹的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:对来自40名GH患者(25名男性)的80个样本进行了测试。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。在来自愈合病变的样本中,PCRgG检出HSV的频率要高于VI检出的HSV。 PCRgG和IIF的打字结果高度一致。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敏感。 PCRgG是用于GH快速检测和分型的便捷技术。

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