Rapid detection and typing of dengue viruses from clinical samples by using reverse transcriptase-polymerase chain reaction.

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J Clin Microbiol. 1992 March; 30(3): 545-551

Rapid detection and typing of dengue viruses from clinical samples by using reverse transcriptase-polymerase chain reaction.

R S Lanciotti, C H Calisher, D J Gubler, G J Chang and A V Vorndam

Division of Vector-Borne Infectious Diseases, Centers for Disease Control, Fort Collins, Colorado 80522.

ABSTRACT

We report on the development and application of a rapid assayfor detecting and typing dengue viruses. Oligonucleotide consensusprimers were designed to anneal to any of the four dengue virustypes and amplify a 511-bp product in a reverse transcriptase-polymerasechain reaction (PCR). First, we produced a cDNA copy of a portionof the viral genome in a reverse transcriptase reaction in thepresence of primer D2 and then carried out a standard PCR (35cycles of heat denaturation, annealing, and primer extension)with the addition of primer D1. The resulting double-strandedDNA product of the RT-PCR was typed by two methods: dot blothybridization of the 511-bp amplified product to dengue virustype-specific probes or a second round of PCR amplification(nested PCR) with type-specific primers, yielding DNA productsthe unique sizes of which were diagnostic for each dengue virusserotype. The accumulated data demonstrated that dengue virusescan be accurately detected and typed from viremic human serumsamples.

J Clin Microbiol. 1992 March; 30(3): 545-551

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