• Title of article

    Development and application of a quantitative real-time PCR assay to detect feline leukemia virus RNA

  • Author/Authors

    Torres، نويسنده , , Andrea N. and O’Halloran، نويسنده , , Kevin P. and Larson، نويسنده , , Laurie J. and Schultz، نويسنده , , Ronald D. and Hoover، نويسنده , , Edward A.، نويسنده ,

  • Pages
    9
  • From page
    81
  • To page
    89
  • Abstract
    We previously defined four categories of feline leukemia virus (FeLV) infection, designated as abortive, regressive, latent, and progressive. To determine if detectable viral DNA is transcriptionally active in the absence of antigenemia, we developed and validated a real-time viral RNA qPCR assay. This assay proved to be highly sensitive, specific, reproducible, and allowed reliable quantitation. We then applied this methodology, together with real-time DNA qPCR and p27 capsid antigen capture ELISA, to examine cats challenged with FeLV. We found that circulating viral RNA and DNA levels were highly correlated and the assays were almost in perfect agreement. This indicates that the vast majority of viral DNA is transcriptionally active, even in the absence of antigenemia. The real-time qPCR assays are more sensitive than the most commonly used FeLV diagnostic assay, the p27 capsid antigen capture ELISA. Application of qPCR assays may add greater depth in understanding of FeLV–host relationships.
  • Keywords
    FeLV , Real-Time PCR , immune response , latent
  • Journal title
    Astroparticle Physics
  • Record number

    2057058