Author: Lu, Y.Y.; Yan, J.Y.; Feng, Y.; Xu, C.P.; Shi, W.; Mao, H.Y.
Title: Rapid detection of H5 avian influenza virus by TaqManâ€MGB realâ€time RTâ€PCR Cord-id: 9i4frb6k Document date: 2007_10_17
ID: 9i4frb6k
Snippet: Aims: Realâ€time reverse transcriptionâ€polymerase chain reaction (RTâ€PCR) assay based on a TaqManâ€minor groove binder (MGB) probe was developed for the rapid detection of avian influenza virus subtype H5. Methods and Results: Conserved regions in the haemagglutinin genes of avian influenza viruses subtype H5 served as targets for the primers and TaqManâ€MGB probe design. Concentrations of primers and probe were optimized to improve the sensitivity and specificity of the reactions. A plas
Document: Aims: Realâ€time reverse transcriptionâ€polymerase chain reaction (RTâ€PCR) assay based on a TaqManâ€minor groove binder (MGB) probe was developed for the rapid detection of avian influenza virus subtype H5. Methods and Results: Conserved regions in the haemagglutinin genes of avian influenza viruses subtype H5 served as targets for the primers and TaqManâ€MGB probe design. Concentrations of primers and probe were optimized to improve the sensitivity and specificity of the reactions. A plasmid containing the haemagglutinin gene was constructed and in vitro transcribed for a quantitative assay of copy numbers of the target gene. The results revealed that the optimal concentration of primers and probe was 640 and 480 nmol l(−1), respectively. The threshold of 100 copies of target molecules could be detected. The linear range for detection was determined as 10(2) to 10(8) molecules in reaction. Conclusions: It took less than 3 h to complete the detection from viral RNA extraction, with good sensitivity and repeatability. Significance and Impact of the Study: Realâ€time RTâ€PCR assay with MGB probe was an effective means for quick and quantitative laboratory detection and monitoring of H5 avian influenza viruses.
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