Literature DB >> 11469514

One-step RT-PCR for the detection of infectious bursal disease virus in clinical samples.

R S Kataria1, A K Tiwari, T Nanthakumar, P P Goswami.   

Abstract

A single-tube, non-interrupted, one-step RT-PCR has been standardized to amplify the hypervariable region of the VP2 gene sequence of infectious bursal disease virus (IBDV). The technique standardized on purified viral RNA was successfully applied to the detection of the virus directly in clinical samples. The amplified products were confirmed to be IBDV specific by their size in ethidium bromide-stained agarose gel, nested PCR and restriction enzyme digestion. Digestion of the amplicons with StyI restriction enzyme also differentiated classical virus from six very virulent field isolates. The sensitivity of the one-step RT-PCR was found to be 0.2 pg of viral RNA.

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Year:  2001        PMID: 11469514     DOI: 10.1023/a:1010607229688

Source DB:  PubMed          Journal:  Vet Res Commun        ISSN: 0165-7380            Impact factor:   2.459


  17 in total

1.  Continuous RT-PCR using AMV-RT and Taq DNA polymerase: characterization and comparison to uncoupled procedures.

Authors:  F Mallet; G Oriol; C Mary; B Verrier; B Mandrand
Journal:  Biotechniques       Date:  1995-04       Impact factor: 1.993

2.  Outbreak of virulent infectious bursal disease in East Anglia.

Authors:  N Chettle; J C Stuart; P J Wyeth
Journal:  Vet Rec       Date:  1989-09-02       Impact factor: 2.695

3.  Differentiation of infectious bursal disease virus strains by restriction analysis of RT-PCR-amplified VP2 gene sequences.

Authors:  R S Kataria; A K Tiwari; G Butchaiah; J M Kataria
Journal:  Acta Virol       Date:  1999-08       Impact factor: 1.162

4.  VP2 sequences of recent European 'very virulent' isolates of infectious bursal disease virus are closely related to each other but are distinct from those of 'classical' strains.

Authors:  M D Brown; P Green; M A Skinner
Journal:  J Gen Virol       Date:  1994-03       Impact factor: 3.891

5.  Observations on polymerase chain reaction amplification of infectious bursal disease virus dsRNA.

Authors:  B Qian; F S Kibenge
Journal:  J Virol Methods       Date:  1994-04       Impact factor: 2.014

6.  Development of probes for differentiation of infectious bursal disease virus strains of various virulence by dot-blot hybridization.

Authors:  R S Katari; A K Tiwari; G Butchaiah; J M Kataria
Journal:  Acta Virol       Date:  2000-10       Impact factor: 1.162

7.  Diagnosis of the African horse sickness virus serotype 4 by a one-tube, one manipulation RT-PCR reaction from infected organs.

Authors:  S Zientara; C Sailleau; S Moulay; C Cruciere
Journal:  J Virol Methods       Date:  1994-02       Impact factor: 2.014

8.  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

9.  Characteristics and serologic studies of two serotypes of infectious bursal disease virus in turkeys.

Authors:  D J Jackwood; Y M Saif; J H Hughes
Journal:  Avian Dis       Date:  1982 Oct-Dec       Impact factor: 1.577

10.  Sequence comparisons of a highly virulent infectious bursal disease virus prevalent in Japan.

Authors:  Z Lin; A Kato; Y Otaki; T Nakamura; E Sasmaz; S Ueda
Journal:  Avian Dis       Date:  1993 Apr-Jun       Impact factor: 1.577
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