Design and Application of Nucleic Acid Standards for Quantitative Detection of Enteric Viruses by Real-Time PCR

Artigo Acesso aberto Revisado por pares

Design and Application of Nucleic Acid Standards for Quantitative Detection of Enteric Viruses by Real-Time PCR

2011; Springer Science+Business Media; Volume: 3; Issue: 2 Linguagem: Inglês

10.1007/s12560-011-9062-9

ISSN

1867-0342

Autores

Mónica Martínez‐Martínez, Marta Diez‐Valcarce, Marta Hernández, David Rodrı́guez-Lázaro,

Tópico(s)

Animal Virus Infections Studies

Resumo

Synthetic multiple-target RNA and DNA oligonucleotides were constructed for use as quantification standards for nucleic acid amplification assays for human norovirus genogroup I and II, hepatitis E virus, murine norovirus, human adenovirus, porcine adenovirus and bovine polyomavirus. This approach overcomes the problems related to the difficulty of obtaining practical quantities of viral RNA and DNA from these viruses. The quantification capacity of assays using the standards was excellent in each case (R(2) > 0.998 and PCR efficiency > 0.89). The copy numbers of the standards were equivalent to the genome equivalents of representative viruses (murine norovirus and human adenovirus), ensuring an accurate determination of virus presence. The availability of these standards should facilitate the implementation of nucleic acid amplification-based methods for quantitative virus detection.

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Design and Application of Nucleic Acid Standards for Quantitative Detection of Enteric Viruses by Real-Time PCR