par Weyn, Christine 
;Boulenouar, Selma ;Mathys, Vanessa ;Vanhoolandt, Julie;Bernis, Aurore;Fontaine, Véronique ;RIIP and INCTR Workshop Study Group,
Référence Journal of virological methods, 146, 1-2, page (405-408)
Publication Publié, 2007-12
;Boulenouar, Selma ;Mathys, Vanessa ;Vanhoolandt, Julie;Bernis, Aurore;Fontaine, Véronique ;RIIP and INCTR Workshop Study Group, Référence Journal of virological methods, 146, 1-2, page (405-408)
Publication Publié, 2007-12
Article révisé par les pairs
| Résumé : | Human papillomavirus (HPV) types 45 and 51 are both considered as high risk types for the development of human cervical cancer. To optimize the detection of these two types in clinical samples, HPV-45 and HPV-51 specific primers were designed to amplify respectively a 141bp and a 266bp fragment from the L1 gene by polymerase chain reaction (PCR). The sensitivity and the specificity of these two PCR reactions were determined using varying amounts of HPV DNA containing plasmids and negative and positive controls. Overall, the sensitivity for the HPV-45 plasmid DNA is 10fg, while for HPV-51 the sensitivity is 1fg. This is equivalent to approximately 100 and 10 HPV genome copies per PCR reaction, respectively. |
