首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Comparison of Two Widely Used Human Papillomavirus Detection and Genotyping Methods GP5+/6+-Based PCR Followed by Reverse Line Blot Hybridization and Multiplex Type-Specific E7-Based PCR
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Comparison of Two Widely Used Human Papillomavirus Detection and Genotyping Methods GP5+/6+-Based PCR Followed by Reverse Line Blot Hybridization and Multiplex Type-Specific E7-Based PCR

机译:两种广泛使用的人类乳头瘤病毒检测和基因分型方法基于GP5 + / 6 +的PCR反向印迹杂交和基于多重类型E7的PCR的比较

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摘要

GP5+/6+-based PCR followed by reverse line blot hybridization (GP5+/6+RLB) and multiplex type-specific PCR (E7-MPG) are two human papillomavirus (HPV) genotyping methodologies widely applied in epidemiological research. We investigated their relative analytical performance in 4,662 samples derived from five studies in Bhutan, Rwanda, and Mongolia coordinated by the International Agency for Research on Cancer (IARC). A total of 630 samples were positive by E7-MPG only (13.5%), 24 were positive by GP5+/6+RLB only (0.5%), and 1,014 were positive (21.8%) by both methods. Ratios of HPV type-specific positivity of the two tests (E7-MPG:GP5+/6+RLB ratio) were calculated among 1,668 samples that were HPV positive by one or both tests. E7-MPG:GP5+/6+RLB ratios were >1 for all types and highly reproducible across populations and sample types. E7-MPG:GP5+/6+RLB ratios were highest for HPV53 (7.5) and HPV68 (7.1). HPV16 (1.6) and HPV18 (1.7) had lower than average E7-MPG:GP5+/6+RLB ratios. Among E7-MPG positive infections, median mean fluorescence intensity (MFI; a semiquantitative measure of viral load) tended to be higher among samples positive for the same virus type by GP5+/6+RLB than for those negative for the same type by GP5+/6+RLB. Exceptions, however, included HPV53, -59, and -82, for which the chances of being undetected by GP5+/6+RLB appeared to be MFI independent. Furthermore, the probability of detecting an additional type by E7-MPG was higher when another type was already detected by GP5+/6+RLB, suggesting the existence of masking effects due to competition for GP5+/6+ PCR primers. In conclusion, this analysis is not an evaluation of clinical performance but may inform choices for HPV genotyping methods in epidemiological studies, when the relative merits and dangers of sensitivity versus specificity for individual types should be considered, as well as the potential to unmask nonvaccine types following HPV vaccination.
机译:基于GP5 + / 6 +的PCR,然后进行反向线杂交(GP5 + / 6 + RLB)和多重特异性PCR(E7-MPG)是两种在流行病学研究中广泛应用的人类乳头瘤病毒(HPV)基因分型方法。在国际癌症研究机构(IARC)的协调下,我们在不丹,卢旺达和蒙古的五项研究中获得了4,662个样品的相对分析性能。两种方法总共仅通过E7-MPG阳性(13.5%)阳性,仅通过GP5 + / 6 + RLB阳性(0.5%)24例,以及1,014阳性(21.8%)阳性。在一项或两项测试均为HPV阳性的1,668份HPV阳性样本中,计算了两项测试的HPV型特异性阳性比率(E7-MPG:GP5 + / 6 + RLB比)。所有类型的E7-MPG:GP5 + / 6 + RLB比率均> 1,并且在所有人群和样本类型之间均具有很高的重现性。 HPV53(7.5)和HPV68(7.1)的E7-MPG:GP5 + / 6 + RLB比率最高。 HPV16(1.6)和HPV18(1.7)低于平均E7-MPG:GP5 + / 6 + RLB比率。在E7-MPG阳性感染中,GP5 + / 6 + RLB对相同病毒类型呈阳性的样本中位数平均荧光强度(MFI;病毒载量的半定量测量)往往高于GP5 + / 6 + RLB。但是,例外情况包括HPV53,-59和-82,GP5 + / 6 + RLB无法检测到的可能性似乎与MFI无关。此外,当GP5 + / 6 + RLB已经检测到另一种类型时,通过E7-MPG检测到另一种类型的可能性更高,这表明存在由于GP5 + / 6 + PCR引物竞争而产生的掩盖效应。总之,这种分析不是对临床表现的评估,而是可以在流行病学研究中为HPV基因分型方法的选择提供信息,应考虑每种类型敏感性和特异性的相对优点和危险,以及揭示非疫苗类型的潜力HPV疫苗接种后。

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