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Multicenter comparison of PCR assays for detection of human herpesvirus 6 DNA in serum
Authors:Flamand Louis  Gravel Annie  Boutolleau David  Alvarez-Lafuente Roberto  Jacobson Steve  Malnati Mauro S  Kohn Debra  Tang Yi-Wei  Yoshikawa Tetsushi  Ablashi Dharam
Affiliation:Rheumatology and Immunology Research Center, CHUL Research Center, Room T1-49, 2705 Laurier Blvd., Quebec, Quebec, Canada G1V 4G2. louis.flamand@crchul.ulaval.ca
Abstract:Human herpesvirus 6 (HHV-6) is a ubiquitous virus with which infections have been associated with pathologies ranging from delayed bone marrow engraftment to a variety of neurological diseases. The lack of a standardized assay that can be used to detect and estimate HHV-6 DNA contents in various clinical specimens can lead and has led to discordant results among investigators and on the potential association of HHV-6 to diseases. To identify the most reliable and sensitive assays, an identical set of 11 coded serum samples spiked with various quantities of the HHV-6A variant (range, 4 to 400,000 genome copies/ml) was sent to eight independent laboratories around the world. Each laboratory was asked to estimate the HHV-6 DNA content by use of its own protocols and assays. Among the various assays, three TaqMan-based real-time PCR assays yielded quantities that were closest to the quantity of HHV-6 that had been spiked. To provide better homogeneity between the results from the different laboratories working on HHV-6, we propose that investigators interested in quantifying HHV-6 in clinical samples adopt one of these assays.
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