Sequence Variation in Amplification Target Genes and Standards Influences Interlaboratory Comparison of BK Virus DNA Load Measurement

Author:

Solis Morgane12,Meddeb Mariam1,Sueur Charlotte12,Domingo-Calap Pilar2,Soulier Eric2,Chabaud Angeline1,Perrin Peggy3,Moulin Bruno23,Bahram Seiamak2,Stoll-Keller Françoise12,Caillard Sophie23,Barth Heidi12,Fafi-Kremer Samira12

Affiliation:

1. Laboratoire de Virologie, Hôpitaux Universitaires de Strasbourg, Strasbourg, France

2. Inserm UMR S1109, LabEx Transplantex, Fédération de Médecine Translationnelle de Strasbourg (FMTS), Université de Strasbourg, Strasbourg, France

3. Département de Néphrologie-Transplantation, Hôpitaux Universitaires de Strasbourg, Strasbourg, France

Abstract

ABSTRACT International guidelines define a BK virus (BKV) load of ≥4 log 10 copies/ml as presumptive of BKV-associated nephropathy (BKVN) and a cutoff for therapeutic intervention. To investigate whether BKV DNA loads (BKVL) are comparable between laboratories, 2 panels of 15 and 8 clinical specimens (urine, whole blood, and plasma) harboring different BKV genotypes were distributed to 20 and 27 French hospital centers in 2013 and 2014, respectively. Although 68% of the reported results fell within the acceptable range of the expected result ±0.5 log 10 , the interlaboratory variation ranged from 1.32 to 5.55 log 10 . Polymorphisms specific to BKV genotypes II and IV, namely, the number and position of mutations in amplification target genes and/or deletion in standards, arose as major sources of interlaboratory disagreements. The diversity of DNA purification methods also contributed to the interlaboratory variability, in particular for urine samples. Our data strongly suggest that (i) commercial external quality controls for BKVL assessment should include all major BKV genotypes to allow a correct evaluation of BKV assays, and (ii) the BKV sequence of commercial standards should be provided to users to verify the absence of mismatches with the primers and probes of their BKV assays. Finally, the optimization of primer and probe design and standardization of DNA extraction methods may substantially decrease interlaboratory variability and allow interinstitutional studies to define a universal cutoff for presumptive BKVN and, ultimately, ensure adequate patient care.

Publisher

American Society for Microbiology

Subject

Microbiology (medical)

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