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Robust hybridization-based genotyping probes for HPV 6, 11, 16 and 18 obtained via in vitro selection
Author(s) -
Ivan Brukner,
Anne-Marie Larose,
Izabella GorskaFlipot,
Maja Krajinović,
Damian Labuda
Publication year - 2010
Publication title -
journal of nucleic acids investigation
Language(s) - English
Resource type - Journals
eISSN - 2035-6005
pISSN - 2036-7996
DOI - 10.4081/jnai.2010.e3
Subject(s) - genotyping , multiplex , computational biology , oligonucleotide , typing , biology , genome , multiplex polymerase chain reaction , microbiology and biotechnology , dna , polymerase chain reaction , genetics , genotype , gene
This paper describes the technical and analytical performance of a novel set of hybridization probes for the four GARDASIL® vaccine-relevant HPV types (6, 11, 16 and 18). These probes are obtained through in vitro selection from a pool of random oligonucleotides, rather than the traditional “rational design” approach typically used as the initial step in assay development. The type-specific segment of the HPV genome was amplified using a GP5+/6+ PCR protocol and 39 synthetic oligonucleotide templates derived from each of the HPV types, as PCR targets. The robust performance of the 4 selected hybridization probes was demonstrated by monitoring the preservation of the specificity and sensitivity of the typing assay over all 39 HPV types, using a different spectrum of HPV (genome equivalent: 103-109) and human DNA concentrations (10-100 ng) as well as temperature and buffer composition variations. To the Authors’ knowledge, this is a unique hybridization-based multiplex typing assay. It performs at ambient temperatures, does not require the strict temperature control of hybridization conditions, and is functional with a number of different non-denaturing buffers, thereby offering downstream compatibility with a variety of detection methods. Studies aimed at demonstrating clinical performance are needed to validate the applicability of this strategy

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