Multicentric evaluation of a new commercial cytomegalovirus real-time PCR quantitation assay

S Gouarin; A Vabret; C Scieux; F Agbalika; J Cherot; C Mengelle; C Deback; J Petitjean; J Dina; F Freymuth

doi:10.1016/j.jviromet.2007.06.013

Multicentric evaluation of a new commercial cytomegalovirus real-time PCR quantitation assay

J Virol Methods. 2007 Dec;146(1-2):147-54. doi: 10.1016/j.jviromet.2007.06.013. Epub 2007 Jul 27.

Authors

S Gouarin¹, A Vabret, C Scieux, F Agbalika, J Cherot, C Mengelle, C Deback, J Petitjean, J Dina, F Freymuth

Affiliation

¹ Laboratory of Virology, University Hospital, Avenue Georges Clemenceau, 14033 Caen Cedex, France. gouarin-s@chu-caen.fr

PMID: 17673304
DOI: 10.1016/j.jviromet.2007.06.013

Abstract

Automated real-time PCR systems have become the most common method in the quantitation of viral load during cytomegalovirus (CMV) infection in immuno-compromised patients. In order to evaluate a new commercially available CMV real-time PCR assay (CMV R-gene, Argene, France), a pp65 antigenemia assay and four different "in-house" real-time PCR assays were compared to the CMV R-gene for the detection and the quantitation of CMV load in 506 specimens of whole blood from transplant patients in four French hospital laboratories. The CMV R-gene was more sensitive than the pp65 antigenemia: there were 18% antigenemia-negative versus CMV R-gene-positive samples. A significant correlation was found between DNA quantitation by CMV R-gene and the number of positive cells detected by the pp65 antigenemia test (Spearman's rank test, r=0.63, p<0.0001). A CMV DNA load equivalent to 50 pp65-positive cells/200000 polymorphonuclear leukocytes was 5.26log(10)copies/mL of whole blood. When the CMV R-gene kit was compared to the four other "in-house" real-time PCR assays, there were few discordant results (6.7% total for the four laboratories), all detected with a weak positive CMV DNA viral load. Spearman's coefficients showed a good (r=0.82 for laboratory 1, r=0.66 for laboratory 3) to excellent (r=0.99 for laboratory 2, r=0.94 for laboratory 4) correlation between CMV R-gene and the four real-time "in-house" PCR assays. However, the results of CMV DNA viral load generated by CMV R-gene test were constantly higher than those generated by three out of four "in-house" PCR assays. This mean variation in CMV DNA viral load measured by CMV R-gene and "in-house" PCRs was of 0.77log(10), 0.04log(10), 0.77log(10) and 0.97log(10), for laboratories 1, 2, 3 and 4, respectively. We concluded that there was variability between results of different real-time PCR assays for CMV DNA quantitation. This observation emphasized the need of a standardised commercial assay to allow an "inter-laboratory" comparison of results. Our study showed that CMV R-gene is an accurate, efficient, reliable and versatile tool for rapid diagnosis and monitoring of CMV disease in transplantation recipients.

Publication types

Comparative Study
Evaluation Study
Multicenter Study

MeSH terms

Cytomegalovirus / isolation & purification*
Cytomegalovirus Infections / virology*
France
Humans
Polymerase Chain Reaction / methods*
Sensitivity and Specificity
Viral Load / methods*