Literature DB >> 1951850

Sensitivity and specificity of a universal primer set for the rapid diagnosis of dengue virus infections by polymerase chain reaction and nucleic acid hybridization.

E A Henchal1, S L Polo, V Vorndam, C Yaemsiri, B L Innis, C H Hoke.   

Abstract

A set of sense and anti-sense oligomeric DNA primers, degenerate in the third "wobble" base position of codons so as to match all known dengue virus sequences, was evaluated as universal primers in a polymerase chain reaction (PCR) assay for the rapid diagnosis of dengue virus infections. Virus-specific complementary DNA (cDNA) was prepared by reverse transcription (RT) of total RNA extracted from serum. Amplified cDNA was identified by nucleic acid hybridization with four serotype-specific, oligomeric DNA probes. Using sera from patients admitted with dengue fever, RT/PCR followed by nucleic acid hybridization using radiolabeled probes was 68% sensitive (50/74; 95% confidence interval [CI] = 57-78%) and 100% specific. Chemiluminescent detection of hybridized products was 62% sensitive (26/42; 95% CI = 46-75%). Using specimens from which a virus isolate had been obtained, RT/PCR followed by nucleic acid hybridization with radiolabeled probes was 80% sensitive (40/50; 95% CI = 69-91%) and 100% specific. The results suggest that RT/PCR using degenerate primers is a sensitive and specific method for the detection of dengue viruses in clinical specimens.

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Year:  1991        PMID: 1951850     DOI: 10.4269/ajtmh.1991.45.418

Source DB:  PubMed          Journal:  Am J Trop Med Hyg        ISSN: 0002-9637            Impact factor:   2.345


  18 in total

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Review 2.  Advances in dengue diagnosis.

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Journal:  Clin Diagn Lab Immunol       Date:  1996-11

3.  Use of NS3 consensus primers for the polymerase chain reaction amplification and sequencing of dengue viruses and other flaviviruses.

Authors:  V T Chow; C L Seah; Y C Chan
Journal:  Arch Virol       Date:  1993       Impact factor: 2.574

4.  Dengue virus RNA purification from human plasma: a comparison of two techniques.

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5.  Detection of dengue virus RNA in patients after primary or secondary dengue infection by using the TaqMan automated amplification system.

Authors:  T Laue; P Emmerich; H Schmitz
Journal:  J Clin Microbiol       Date:  1999-08       Impact factor: 5.948

6.  Factors influencing dengue virus isolation by C6/36 cell culture and mosquito inoculation of nested PCR-positive clinical samples.

Authors:  Richard G Jarman; Ananda Nisalak; Kathryn B Anderson; Chonticha Klungthong; Butsaya Thaisomboonsuk; Winai Kaneechit; Siripen Kalayanarooj; Robert V Gibbons
Journal:  Am J Trop Med Hyg       Date:  2011-02       Impact factor: 2.345

7.  Typing of dengue viruses in clinical specimens and mosquitoes by single-tube multiplex reverse transcriptase PCR.

Authors:  E Harris; T G Roberts; L Smith; J Selle; L D Kramer; S Valle; E Sandoval; A Balmaseda
Journal:  J Clin Microbiol       Date:  1998-09       Impact factor: 5.948

8.  A rapid method for detection and identification of flaviviruses by polymerase chain reaction and nucleic acid hybridization.

Authors:  B Puri; E A Henchal; J Burans; K R Porter; W Nelson; D M Watts; C G Hayes
Journal:  Arch Virol       Date:  1994       Impact factor: 2.574

9.  Enhancement by tumor necrosis factor alpha of dengue virus-induced endothelial cell production of reactive nitrogen and oxygen species is key to hemorrhage development.

Authors:  Yu-Ting Yen; Hsuen-Chin Chen; Hseun-Chin Chen; Yang-Ding Lin; Chi-Chang Shieh; Betty A Wu-Hsieh
Journal:  J Virol       Date:  2008-10-08       Impact factor: 5.103

10.  Simultaneous detection and serotyping of dengue infection using single tube multiplex CDC Dengue Real-Time RT-PCR from India.

Authors:  Shashi Sharma; Kundan Tandel; Surabhi Danwe; Puneet Bhatt; P K Dash; Praveer Ranjan; K R Rathi; Rajiv Mohan Gupta; M M Parida
Journal:  Virusdisease       Date:  2018-02-03
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