The comparative results of three different real-time PCR assays: MY09/11 primers failed to detect multiple infections
HPV-DNA testing is widely used worldwide today and it has become an important part of cervical cancer screening programs. The aim of this study is re-evaluating the effectiveness of MY09/11 consensus primer system, which is one of the most widely used HPVDNA tests, by using a different approach. In...
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| Veröffentlicht in: | Gülhane tıp dergisi 2014-06, Vol.56 (2), p.65 |
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| creator | Sahiner, Fatih Sener, Kenan Gumral, Ramazan Yapar, Mehmet Dede, Murat Yigit, Nuri Kubar, Ayhan |
| description | HPV-DNA testing is widely used worldwide today and it has become an important part of cervical cancer screening programs. The aim of this study is re-evaluating the effectiveness of MY09/11 consensus primer system, which is one of the most widely used HPVDNA tests, by using a different approach. In this study, MY09/11 consensus PCR and two different TaqMan-based type-specific PCR assays were used for investigation of the presence of 17 different HPV types in cervical smear samples. Of the 470 samples, 33.2% (156/470) were HPV-DNA positive by at least one of the three methods and remains were negative by all methods. A total of 220 different HPV isolates were identified in 149 samples by the type specific PCR, while the nine samples were positive by consensus PCR only. A single HPV type was detected in 64.4% (96/149) of the genotyped samples, and multiple HPV types were detected in the remaining 35.6% (53/149). MY09/11 PCR failed to detect 21.2% (33/156) of all HPV-DNA positive samples and the rates of false negative results were 18.75% (18/96) and 28.3% (15/53) in single and multiple infections, respectively. We conclude that highly sensitive type-specific PCR tests may be a useful tool for screening of cervical cancer. |
| doi_str_mv | 10.5455/gulhane.41476 |
| format | Article |
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The aim of this study is re-evaluating the effectiveness of MY09/11 consensus primer system, which is one of the most widely used HPVDNA tests, by using a different approach. In this study, MY09/11 consensus PCR and two different TaqMan-based type-specific PCR assays were used for investigation of the presence of 17 different HPV types in cervical smear samples. Of the 470 samples, 33.2% (156/470) were HPV-DNA positive by at least one of the three methods and remains were negative by all methods. A total of 220 different HPV isolates were identified in 149 samples by the type specific PCR, while the nine samples were positive by consensus PCR only. A single HPV type was detected in 64.4% (96/149) of the genotyped samples, and multiple HPV types were detected in the remaining 35.6% (53/149). MY09/11 PCR failed to detect 21.2% (33/156) of all HPV-DNA positive samples and the rates of false negative results were 18.75% (18/96) and 28.3% (15/53) in single and multiple infections, respectively. We conclude that highly sensitive type-specific PCR tests may be a useful tool for screening of cervical cancer.</description><identifier>ISSN: 1302-0471</identifier><identifier>EISSN: 2146-8052</identifier><identifier>DOI: 10.5455/gulhane.41476</identifier><language>eng ; tur</language><publisher>Ankara: Gulhane Medical Journal</publisher><subject>Cervical cancer ; Deoxyribonucleic acid ; DNA ; Human papillomavirus ; Medical screening</subject><ispartof>Gülhane tıp dergisi, 2014-06, Vol.56 (2), p.65</ispartof><rights>2014. This work is published under https://creativecommons.org/licenses/by-nc-nd/4.0/ (the “License”). 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MY09/11 PCR failed to detect 21.2% (33/156) of all HPV-DNA positive samples and the rates of false negative results were 18.75% (18/96) and 28.3% (15/53) in single and multiple infections, respectively. 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| language | eng ; tur |
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| source | EZB-FREE-00999 freely available EZB journals; Alma/SFX Local Collection |
| subjects | Cervical cancer Deoxyribonucleic acid DNA Human papillomavirus Medical screening |
| title | The comparative results of three different real-time PCR assays: MY09/11 primers failed to detect multiple infections |
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