首页> 外文期刊>Virchows Archiv: an international journal of pathology >Detection of human papillomavirus in cervical intra-epithelial neoplasia, using in situ hybridization and various polymerase chain reaction techniques.
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Detection of human papillomavirus in cervical intra-epithelial neoplasia, using in situ hybridization and various polymerase chain reaction techniques.

机译:使用原位杂交和各种聚合酶链反应技术检测宫颈上皮内瘤变中的人乳头瘤病毒。

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One hundred and forty-eight randomly chosen neutral-buffered formaldehyde-fixed cervical biopsies in which cervical intra-epithelial neoplasia (CIN) I-III had been diagnosed were tested for HPV (human papilloma virus) DNA by in situ hybridization (ISH) and polymerase chain reaction (PCR). For ISH, we utilized a biotinylated panprobe and type-specific, genomic probe sets. For PCR, we used the general primers GP5/GP6 and their recently described, elongated version GP5+/GP6+, and included the modification of hot-start PCR. Amplified DNA was detected by gel electrophoresis and slot blot hybridization. The positivity rate of ISH was 59% for all biopsies and 69%, 62% and 46% for CIN I, II and III, respectively. The sensitivity of GP5/GP6 was 74% with cold-start PCR and 78% with hot-start PCR. When GP5+/GP6+ was used, the sensitivity increased to 89% with cold-start PCR and to 95% with hot-start PCR. Based on the most sensitive PCR technique, HPV detection was 93%, 95% and 96% in CIN I, II and III, respectively. The number of HPV types decreased with the severity of the lesion, and HPV 16 was the predominant type. Multiple HPVs were rare and almost all HPV-positive cases could be typed. ISH and slot blot hybridization correlated well regarding HPV typing specificity. Our results confirm that distinct HPV types are present in a high proportion of cases of CIN. The sensitivity of ISH is lower than that of PCR. Furthermore, the modified general primers GP5+/GP6+ give a higher yield than GP5/GP6, while hot-start PCR increases sensitivity even further.
机译:通过原位杂交(ISH)对148例随机选择的中性缓冲液固定甲醛的宫颈活检组织进行了HPV(人乳头瘤病毒)DNA检测,其中已诊断出宫颈上皮内瘤变(CIN)I-III。聚合酶链反应(PCR)。对于ISH,我们利用了生物素化的泛探针和特定类型的基因组探针组。对于PCR,我们使用了通用引物GP5 / GP6及其最近描述的加长版GP5 + / GP6 +,并包括了热启动PCR的修饰。通过凝胶电泳和缝隙印迹杂交检测扩增的DNA。所有活检的ISH阳性率分别为CIN I,II和III的69%,62%和46%。 GP5 / GP6的灵敏度在冷启动PCR下为74%,在热启动PCR下为78%。当使用GP5 + / GP6 +时,冷启动PCR的灵敏度提高到89%,热启动PCR的灵敏度提高到95%。基于最灵敏的PCR技术,在CIN I,II和III中HPV检出率分别为93%,95%和96%。 HPV类型的数量随病变的严重程度而减少,而HPV 16是主要类型。多种HPV很少见,几乎所有HPV阳性病例均可分型。 ISH和狭缝印迹杂交与HPV分型特异性相关性很好。我们的结果证实,在高比例的CIN病例中存在截然不同的HPV类型。 ISH的敏感性低于PCR。此外,修饰的通用引物GP5 + / GP6 +比GP5 / GP6的产率更高,而热启动PCR进一步提高了灵敏度。

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