These results demonstrate that while the qualitative performance of HBV detection has considerably improved compared to that of a previously published HBV proficiency study, the detection levels of many commercial quantitative assays are still too high to allow adequate quantitation of all relevant clinical samples.Direct detection and quantitation of hepatitis B virus (HBV) DNA in plasma or serum are now used routinely to evaluate viremia in HBV-infected persons, to identify infectious chronic carriers, and to predict and monitor the efficacy of antiviral therapy (2,8,11). Since the early 1980s, a variety of molecular detection and quantitation methods have been developed, including dot and slot blot hybridization with radioactive and nonradioactive DNA probes (19-21), chemiluminescent detection of HBV DNA-RNA hybrids (14), PCR amplification of HBV DNA followed by hybridization to probes bound to a microwell plate (10, 12, 22) or magnetic beads (13), branched DNA (bDNA) signal amplification of an HBV DNA-DNA hybrid (7), transcription-mediated amplification (9), and fluorescent real-time detection of amplified HBV DNA (1). Each method, calibrated uniquely, exhibits its own sensitivity, specificity, and dynamic range. Standardization is ongoing (5, 6).To assess the relative value of these methods in detecting and quantitating HBV DNA, international proficiency studies with well-characterized, simulated clinical samples would be required. In the first and only such study published to date (17), 39 laboratories analyzed 22 samples, including 12 undiluted samples with and without HBV DNA. (The lowest positive sample contained 3.5 pg/ml, or approximately 980,000 copies/ml.) Only 27.9% of the data sets had all 12 samples correct, and 34.9% showed false-positive results. Clearly, a majority of the participating laboratories had problems with both sensitivity and specificity.The present report describes two recent HBV proficiency panels (lowest viral load of 1,000 copies/ml) designed by the European Union Concerted Action on Quality Control (EU QCCA) of Nucleic Acid Amplification in Diagnostic Virology and prepared by Boston Biomedica, Inc. (BBI; West Bridgewater, Mass.). The results obtained with these panels demonstrate that while the qualitative detection of HBV DNA has significantly improved, the detection levels of many commercial quantitative assays are still too high to allow adequate quantitation of the clinical samples seen in routine diagnostic laboratories.
MATERIALS AND METHODSPanels. (i) Preparation. Panels were prepared by BBI from human plasma containing HBV DNA of subtype ad or ay by appropriate dilution in sterile filtered defibrinated plasma (Basematrix) with 0.09% sodium azide as preservative in accordance with the ISO 9001 Quality System Standards and the 21CFR 820 "Good Manufacturing Practice for Medical Devices: General." Plasma units were obtained from Food and Drug Administration-licensed facilities that comply with the applicable federal regulations (21CFR, part 600).The pilot dilutions made for...
