One-Step Rapid Reverse Transcription-PCR Assay for Detecting and Typing Dengue Viruses with GC Tail and Induced Fluorescence Resonance Energy Transfer Techniques for Melting Temperature and Color Multiplexing

doi:10.1373/clinchem.2006.077446

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Clinical Chemistry 0: clinchem.2006.077446v1, 2007; 10.1373/clinchem.2006.077446

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Received on July 29, 2006
Accepted on January 25, 2007

Molecular Diagnostics and Genetics

One-Step Rapid Reverse Transcription-PCR Assay for Detecting and Typing Dengue Viruses with GC Tail and Induced Fluorescence Resonance Energy Transfer Techniques for Melting Temperature and Color Multiplexing

Constance L.H. Lo ¹, Shea Ping Yip ¹, Peter K.C. Cheng ², Tony S.S. To ¹, Wilina W.L. Lim ², Polly H.M. Leung ¹^*

¹ Department of Health Technology and Informatics, The Hong Kong Polytechnic University, Hong Kong SAR, China
² Public Health Laboratory Centre, Centre for Health Protection, Department of Health, Hong Kong SAR, China

^* To whom correspondence should be addressed. E-mail: htpolly{at}inet.polyu.edu.hk.

Background: Dengue fever is an arthropod-borne infection causedby dengue viruses (DVs; DEN-1 to DEN-4). Early diagnosis iscritical to prevent severe disease progression and the spreadingof DV because no vaccine or specific treatment is available;therefore, a rapid and specific diagnostic assay capable ofdetecting and typing all serotypes would be ideal.

Methods:We amplified RNA samples from all 4 DV serotypes and Japaneseencephalitis virus with 4 serotype-specific forward primersand a universal species-specific reverse primer. DEN-1 and DEN-3forward primers were labeled at their 5' ends with BODIPY 630/650and Cy5.5, respectively. DEN-1 and DEN-3 amplicons were detectedby their characteristic emission generated from induced fluorescenceresonance energy transfer. The presence of DEN-2 and DEN-4 ampliconswas indicated by SYBR Green I (SGI) signals at specific ampliconmelting temperatures (T_ms).

Results: Fluorescence signals withspecific emission wavelengths were obtained from DEN-1 and DEN-3.SGI melting profiles showed a T_m difference between DEN-2 andDEN-4 of 4.7 °C, which was sufficient for differentiatingthese 2 serotypes. The primers did not amplify the Japaneseencephalitis virus. The detection limits of DEN-1 to DEN-4 were1.64 x 10^-4, 1.05 x 10^-3, 8.15 x 10^-4, and 5.80 x 10^-3 plaque-formingunits per reaction, respectively. The assay had a dynamic rangeof 10³-10⁸ plaque-forming units/L and could be performed in2 h.

Conclusions: A single-tube, 1-step reverse transcription-PCRassay based on T_m and color multiplexing was developed for detectingand typing all 4 DV serotypes.