Molecular detection of human papillomavirus HPV) in highly fragmented DNA from cervical cancer biopsies using double-nested PCR
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Date
2018Author
Tawe, Leabaneng
Grover, Surbhi
Moyo, Sikhulile
Narasimhamurthy, Mohan
Kasvosve, Ishmael
Gaseitsiwe, Simani
Paganotti, Giacomo M.
Publisher
Elsevier, www.elsevier.comType
Published ArticleMetadata
Show full item recordAbstract
Archived Formalin-Fixed Paraffin-Embedded (FFPE) tissue specimens can be a valuable source of human
papillomavirus (HPV) nucleic acids for molecular biological analyses in retrospective studies. Although successful
amplification with polymerase chain reaction (PCR) is essential for analysis of HPV DNA extracted from cervical
FFPE specimens, extensive DNA damage due to cross-linking and fragmentation results in poor yield. Therefore,
techniques to improve the diagnostic rate and sensitivity from FFPE tissues through PCR is highly desired and of
wider interest. To overcome this, a highly sensitive double-nested PCR methodology was designed and optimized
for limited-resource laboratories coupled with an organic extraction of DNA. This method allows the detection of
a broad range of HPV genotypes and also allowing the sequencing of the final amplicon. Validation of the new
approach developed was done with an automated DNA extraction coupled with Real Time PCR. Results showed
that the proposed method achieves 96.3% of HPV detection as compared to 100% Abbott m2000rt used as ‘gold
standard’. Moreover, the concordance rate between the two methods was equal for detecting HPV -16 or -18
genotypes. Nevertheless, the newly introduced assay has an advantage of:
Simultaneously identifying broad range of HPV genotypes besides HPV-16 and -18 from clinical samples.
It is an easy and cost-effective method that can be beneficial in resource-limited setting and can be employed
for various molecular applications.