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Comparison of Real-Time PCR Signal-Amplified In Situ Hybridization and Conventional PCR for Detection and Quantification of Human Papillomavirus in Archival Cervical Cancer Tissue

机译:实时PCR信号扩增原位杂交与常规PCR在宫颈癌组织中检测和定量人乳头瘤病毒的比较

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摘要

Archival paraffin-embedded tumor specimens offer a wealth of information for both cancer research and for routine clinical applications. However, the use of formalin-fixed, paraffin-embedded specimens for quantitative real-time PCR is not yet a standard diagnostic method in many laboratories, in particular for the quantification of human papillomavirus (HPV). Particularly high-risk HPV types are involved in almost 100% of the carcinogenesis of cervical cancer. We compared the diagnostic applicability and sensitivity of real-time PCR to that of chromogenic tyramide-signal-amplified in situ hybridization and conventional PCR for the detection of HPV from archival tissue in 164 cases of carcinoma in situ and cervical cancer. Furthermore, we examined whether the viral load of HPV is of prognostic relevance. Our findings indicate that patients in tumor stage I with a lower viral load of HPV type 16 (HPV16; up to 1,000 copies/ng of DNA) had a significantly better survival than HPV 16-negative patients (P = 0.037). We observed a greater sensitivity of both real-time PCR and conventional PCR for the detection of HPV16 and -18 compared to signal amplified in situ hybridization. We found a considerable concordance between HPV16 (κ = 0.661) and HPV18 (κ = 0.781) status as measured by real-time PCR and conventional PCR, indicating similar sensitivities. We recognized an inhibitory effect of formalin fixation and paraffin embedding on the evaluation of real-time PCR quantification.
机译:档案石蜡包埋的肿瘤标本为癌症研究和常规临床应用提供了大量信息。但是,在许多实验室中,尤其是在定量人类乳头瘤病毒(HPV)方面,使用福尔马林固定,石蜡包埋的标本进行定量实时PCR尚不是标准的诊断方法。特别高危的HPV类型几乎参与了宫颈癌的100%癌变。我们比较了实时PCR的诊断适用性和敏感性与发色酪氨酰胺信号原位杂交和常规PCR在164例原位癌和宫颈癌中从档案组织中检测HPV的诊断适用性和敏感性。此外,我们检查了HPV的病毒载量是否与预后相关。我们的发现表明,处于I期肿瘤的HPV 16型病毒载量较低(HPV16; DNA高达1,000拷贝/ ng)的患者比HPV 16阴性患者的生存率显着提高(P = 0.037)。我们观察到与扩增的原位杂交信号相比,实时PCR和常规PCR对HPV16和-18的检测灵敏度更高。通过实时PCR和常规PCR测量,我们发现HPV16(κ= 0.661)和HPV18(κ= 0.781)状态之间存在相当大的一致性,表明相似的敏感性。我们认识到福尔马林固定和石蜡包埋对实时PCR定量评估的抑制作用。

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