Clinical Validation of a Type-Specific Real-Time Quantitative Human Papillomavirus PCR against the Performance of Hybrid Capture 2 for the Purpose of Cervical Cancer Screening

Depuydt, Christophe; Benoy, Ina; Beert, Johan; Criel, A.; Bogers, Johannes; Arbyn, Marc

doi:10.1128/jcm.01231-12

Cited by 46 publications

(65 citation statements)

References 28 publications

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“…both showing a percentage of agreement with a lower confidence bound not less than 87% (kappa value of at least 0.5)) [4]. Recently a number of different molecular HPV test methods have been subjected to this test criterion and it has become the de facto standard by which new tests are assessed [5][6][7].…”

Section: Introductionmentioning

confidence: 99%

Clinical Validation of the BD Onclarity? HPV Assay Using a Non-Inferiority Test

Ejegod¹

2015

J Med Microb Diagn

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The clinical performance of The BD Onclarity™ HPV Assay, a novel type-specific real-time E6/E7-based PCR assay, was evaluated for clinical and analytical performance using the Meijer et al. international guidelines for validation of high-risk HPV tests. Assay performance was found to be similar to the reference method, Hybrid Capture 2 (HC2, QIAGEN) using PreservCyt ® Specimens (Hologic ® , Inc.). In addition, the fully automated assay was found to have excellent intra-and inter-laboratory reproducibility (98.6% (kappa=0.967) and 98.4% (kappa=0.962), respectively). These data show that the BD Onclarity™ HPV Assay fulfills the clinical validation requirements for a HPV based cervical cancer screening assay (Meijer et al. International journal of cancer 2009; 124: 516-520.).

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Section: Introductionmentioning

confidence: 99%

Clinical Validation of the BD Onclarity? HPV Assay Using a Non-Inferiority Test

Ejegod¹

2015

J Med Microb Diagn

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“…The Hybrid Capture 2 (HC2; Qiagen, Hilden, Germany) assay (2-4) and GP5ϩ/6ϩ PCR-based enzyme immunoassay (EIA) kit HPV GP HR (EIA; Diassay, Rijswijk, the Netherlands) (5-9) were the first HPV tests to be clinically validated for primary screening on the basis of longitudinal results from large screening studies (10). Testing for high-risk HPV (hrHPV) nucleic acids is also useful for triage of women with equivocal or mildly abnormal cytology for colposcopy and as a test of cure of treatment (10).Several novel HPV tests have been fully or partially validated by showing noninferiority to HC2 or EIA and high reproducibility (11), as has been extensively reviewed by Arbyn et al (10) and reported in additional studies (12)(13)(14). These tests usually detect around 14 hrHPVs in aggregate, but some provide concurrent (partial) genotype-specific information.…”

mentioning

confidence: 99%

“…Several novel HPV tests have been fully or partially validated by showing noninferiority to HC2 or EIA and high reproducibility (11), as has been extensively reviewed by Arbyn et al (10) and reported in additional studies (12)(13)(14). These tests usually detect around 14 hrHPVs in aggregate, but some provide concurrent (partial) genotype-specific information.…”

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confidence: 99%

Clinical Evaluation of a GP5+/6+-Based Luminex Assay Having Full High-Risk Human Papillomavirus Genotyping Capability and an Internal Control

et al. 2014

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The LMNX genotyping kit HPV GP (LMNX) is based on the clinically validated GP5؉/6؉ PCR, with a genotyping readout as an alternative for the more established enzyme immunoassay (EIA) detection of 14 targeted high-risk human papillomavirus (HPV) types. LMNX is additionally provided with an internal control probe. Here, we present an analysis of the clinical performance of the LMNX using a sample panel and infrastructure provided by the international VALGENT (Validation of Genotyping Tests) project. This panel consisted of cervical specimens from approximately 1,000 women attending routine screening, "enriched" with 300 women with abnormal cytology. Cases were defined as women classified with cervical intraepithelial neoplasia (CIN) grade 2؉ (CIN2؉) (n ‫؍‬ 102) or CIN3؉ (n ‫؍‬ 55) within the previous 18 months. Controls were women who had normal cytology results over two subsequent screening rounds at a 3-year interval (n ‫؍‬ 746). The GP5؉/6؉-PCR EIA (EIA) was used as a comparator assay and showed sensitivities of 94.1% and 98.2% for CIN2؉ and CIN3؉, respectively, with a clinical specificity of 92.4% among women aged >30 years. The LMNX demonstrated clinical sensitivities of 96.1% for CIN2؉ and of 98.2% for CIN3؉ and a clinical specificity of 92.6% for women aged >30 years. The LMNX and EIA were in high agreement (Cohen's kappa ‫؍‬ 0.969) for the detection of 14 hrHPVs in aggregate, and no significant difference was observed (McNemar's P ‫؍‬ 0.629). The LMNX internal control detected 0.6% inadequate specimens. Based on our study results, we consider the LMNX, similarly to the EIA, useful for HPV-based cervical cancer screening.H uman papillomavirus (HPV) tests that have been validated for use in a clinical setting usually target 13 or 14 genotypes. These HPVs have been classified by the International Agency for Research on Cancer (IARC) as carcinogenic, i.e., HPV16, HPV18, HPV31, HPV33, HPV35, HPV39, HPV45, HPV51, HPV52, HPV56, HPV58, and HPV59 (class 1), probably carcinogenic, i.e., HPV68 (class 2A), or possibly carcinogenic, i.e., HPV66 (class 2B) (1). The Hybrid Capture 2 (HC2; Qiagen, Hilden, Germany) assay (2-4) and GP5ϩ/6ϩ PCR-based enzyme immunoassay (EIA) kit HPV GP HR (EIA; Diassay, Rijswijk, the Netherlands) (5-9) were the first HPV tests to be clinically validated for primary screening on the basis of longitudinal results from large screening studies (10). Testing for high-risk HPV (hrHPV) nucleic acids is also useful for triage of women with equivocal or mildly abnormal cytology for colposcopy and as a test of cure of treatment (10).Several novel HPV tests have been fully or partially validated by showing noninferiority to HC2 or EIA and high reproducibility (11), as has been extensively reviewed by Arbyn et al. (10) and reported in additional studies (12)(13)(14). These tests usually detect around 14 hrHPVs in aggregate, but some provide concurrent (partial) genotype-specific information. Concurrent genotyping for HPV16 and HPV18 could be beneficial for the triage of hrHPV-positive women (15), as the...

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“…Intralaboratory testing took place at the AML laboratory (Antwerp, Belgium) and interlaboratory testing took place between AML and the laboratory of the University Hospital of Ghent (Ghent, Belgium). A total of 510 samples collated at the AML laboratory, which had previously been tested with an in-house multiplex real-time PCR (15,16), were assessed. For the validation criteria to be satisfied, the 95% lower confidence bound of both agreements should be Ͼ87%, with a kappa value Ն0.5 (5).…”

Section: Assessment Of Clinical Performance and Comparison With A CLImentioning

confidence: 99%

Performance of a Cartridge-Based Assay for Detection of Clinically Significant Human Papillomavirus (HPV) Infection: Lessons from VALGENT (Validation of HPV Genotyping Tests)

et al. 2016

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Clinical Validation of a Type-Specific Real-Time Quantitative Human Papillomavirus PCR against the Performance of Hybrid Capture 2 for the Purpose of Cervical Cancer Screening

Cited by 46 publications

References 28 publications

Clinical Validation of the BD Onclarity? HPV Assay Using a Non-Inferiority Test

Clinical Validation of the BD Onclarity? HPV Assay Using a Non-Inferiority Test

Clinical Evaluation of a GP5+/6+-Based Luminex Assay Having Full High-Risk Human Papillomavirus Genotyping Capability and an Internal Control

Performance of a Cartridge-Based Assay for Detection of Clinically Significant Human Papillomavirus (HPV) Infection: Lessons from VALGENT (Validation of HPV Genotyping Tests)

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