7种高灵敏度人乳头瘤病毒核酸检测技术与SPF10 LiPA-25系统的对比研究

Jian Yin , Shuqian Cheng , Daokuan Liu , Yabin Tian , Fangfang Hu , Zhigao Zhang , Tiancen Zhu , Zheng Su , Yujing Liu , Sumeng Wang , Yiwei Liu , Siying Peng , Linlin Li , Sihong Xu , Chuntao Zhang , Youlin Qiao , Wen Chen
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引用次数: 1

摘要

SPF10 LiPA-25人乳头瘤病毒(HPV)检测系统具有较高的分析性能,广泛应用于HPV疫苗临床试验。为了开发和评估更有价值的HPV疫苗,需要其他操作更简单的可比方法。方法选取1726份宫颈拭子和56份活检样本,比较LiPA-25与其他7种检测方法的性能,包括4种基于反向杂交的检测方法(bohui24、yaneng23、Tellgen-27和Hybribio-16)和3种实时聚合酶链反应(PCR)检测方法(Hybribio-23、Bioperfectus-21和san确定-26)。共有15种HPV基因型(HPV 6、11、16、18、31、33、35、39、45、51、52、56、58、59和66)被考虑用于每种HPV型的比较。结果与LiPA-25相比,Hybribio-23的基因型相容性为94.1%,yaneng23为92.8%,Bioperfectus-21为92.6%,Hybribio-16为92.4%,san确定-26为91.3%,渤慧-24为89.7%,Tellgen-27为88.0%。15种HPV基因型组合的总体一致性最高的是Hybribio-23 (κ = 0.879, McNemar's检验:P = 0.136),其次是Hybribio-16 (κ = 0.877, P<0.001), Yaneng-23 (κ = 0.871, P <0.001), Bioperfectus-21 (κ = 0.848, P <0.001), Bohui-24 (κ = 0.847, P <0.001), Tellgen-27 (κ = 0.831, P <0.001), Sansure-26 (κ = 0.826, P <0.001)。此外,这些系统也与活检标本的LiPA-25高度一致(所有,κ >0.897)。结论其他7种检测方法对15种HPV的检测结果与LiPA-25的一致性均较好,其中Hybribio-23与LiPA-25最具可比性。HPV基因分型的检测操作也应考虑到疫苗和流行病学研究。
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Head-to-head comparison of 7 high-sensitive human papillomavirus nucleic acid detection technologies with the SPF10 LiPA-25 system

Background

The SPF10 LiPA-25 system for human papillomavirus (HPV) detection with high analytical performance is widely used in HPV vaccine clinical trials. To develop and evaluate more valent HPV vaccines, other comparable methods with simpler operations are needed.

Methods

The performance of the LiPA-25 against that of other 7 assays, including 4 systems based on reverse hybridization (Bohui-24, Yaneng-23, Tellgen-27, and Hybribio-16) and 3 real-time polymerase chain reaction (PCR) assays (Hybribio-23, Bioperfectus-21, and Sansure-26), was evaluated in selected 1726 cervical swab and 56 biopsy samples. A total of 15 HPV genotypes (HPV 6, 11, 16, 18, 31, 33, 35, 39, 45, 51, 52, 56, 58, 59, and 66) were considered for comparison for each HPV type.

Results

Among the swab samples, compared to LiPA-25, compatible genotypes were observed in 94.1% of samples for Hybribio-23, 92.8% for Yaneng-23, 92.6% for Bioperfectus-21, 92.4% for Hybribio-16, 91.3% for Sansure-26, 89.7% for Bohui-24, and 88.0% for Tellgen-27. The highest overall agreement of the 15 HPV genotypes combined was noted for Hybribio-23 (κ = 0.879, McNemar's test: P = 0.136), followed closely by Hybribio-16 (κ = 0.877, P< 0.001), Yaneng-23 (κ = 0.871, P < 0.001), Bioperfectus-21 (κ = 0.848, P < 0.001), Bohui-24 (κ = 0.847, P < 0.001), Tellgen-27 (κ = 0.831, P < 0.001), and Sansure-26 (κ = 0.826, P < 0.001). Additionally, these systems were also highly consistent with LiPA-25 for biopsy specimens (all, κ > 0.897).

Conclusions

The levels of agreement for the detection of 15 HPV types between other 7 assays and LiPA-25 were all good, and Hybribio-23 was most comparable to LiPA-25. The testing operation of HPV genotyping should also be considered for vaccine and epidemiological studies.

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