HBV‐RNA Co‐amplification May Influence HBV DNA Viral Load Determination

Despite effective hepatitis B virus (HBV)‐DNA suppression, HBV RNA can circulate in patients receiving nucleoside/nucleotide analogues (NAs). Current assays quantify HBV DNA by either real‐time polymerase chain reaction (PCR), which uses DNA polymerase, or transcription‐mediated amplification, which uses reverse‐transcriptase (RT) and RNA polymerase. We assessed the effect of RT capability on HBV‐DNA quantification in samples from three cohorts, including patients with quantified HBV RNA. We compared the HBV‐DNA levels by real‐time PCR (cobas HBV, Roche 6800/8800; Xpert HBV, Cepheid), transcription‐mediated amplification (Aptima HBV, Hologic), and real‐time PCR with added RT capability (cobas HBV+RT). In the first cohort (n = 45) followed over 192 weeks of NA therapy, on‐treatment HBV‐DNA levels were higher with cobas HBV+RT than cobas HBV (mean difference: 0.14 log10 IU/mL). In a second cohort (n = 50) followed over 96 weeks of NA therapy, HBV‐DNA viral load was significantly higher with the cobas HBV+RT and Aptima HBV compared with the cobas HBV test at all time points after initiation of NA therapy (mean difference: 0.65‐1.16 log10 IU/mL). A clinically significant difference was not detected between the assays at baseline. In a third cohort (n = 53), after a median of 2.2 years of NA therapy, we detected HBV RNA (median 5.6 log10 copies/mL) in 23 patients (43.4%). Median HBV‐DNA levels by Aptima HBV were 2.4 versus less than 1 log10 IU/mL in samples with HBV RNA and without HBV RNA, respectively (P = 0.0006). In treated patients with HBV RNA, Aptima HBV measured higher HBV‐DNA levels than Xpert HBV and cobas HBV. Conclusion: Tests including an RT step may overestimate HBV DNA, particularly in samples with low viral loads as a result of NA therapy. This overestimation is likely due to amplification of HBV RNA and may have an impact on clinical decisions.

[1]  J. Izopet,et al.  Performance of the Xpert HBV Viral Load assay versus the Aptima Quant assay for quantifying hepatitis B virus DNA. , 2019, Diagnostic microbiology and infectious disease.

[2]  K. Agarwal,et al.  Pregenomic HBV RNA and Hepatitis B Core‐Related Antigen Predict Outcomes in Hepatitis B e Antigen–Negative Chronic Hepatitis B Patients Suppressed on Nucleos(T)ide Analogue Therapy , 2019, Hepatology.

[3]  B. Pinsky,et al.  Comparison of Transcription-Mediated Amplification and Real-Time PCR Assays for Hepatitis B Virus DNA Quantitation in Serum. , 2019, The journal of applied laboratory medicine.

[4]  Haitao Guo,et al.  Serum Hepatitis B Virus RNA: A New Potential Biomarker for Chronic Hepatitis B Virus Infection , 2019, Hepatology.

[5]  N. Terrault,et al.  New and Old Biomarkers for Diagnosis and Management of Chronic Hepatitis B Virus Infection. , 2019, Gastroenterology.

[6]  B. McMahon,et al.  Update on prevention, diagnosis, and treatment of chronic hepatitis B: AASLD 2018 hepatitis B guidance , 2018, Hepatology.

[7]  A. Speicher,et al.  Evaluation of the Aptima HBV Quant assay vs. the COBAS TaqMan HBV test using the high pure system for the quantitation of HBV DNA in plasma and serum samples , 2017, Clinical chemistry and laboratory medicine.

[8]  V. Calvez,et al.  Multicenter comparison of the new Cobas 6800 system with Cobas Ampliprep/Cobas TaqMan and Abbott RealTime for the quantification of HIV, HBV and HCV viral load. , 2017, Journal of clinical virology : the official publication of the Pan American Society for Clinical Virology.

[9]  A. Lok,et al.  Hepatitis B cure: From discovery to regulatory approval , 2017, Journal of hepatology.

[10]  A. Lombardi,et al.  A European multicientre study on the comparison of HBV viral loads between VERIS HBV assay and Roche COBAS® TAQMAN® HBV test, Abbott RealTime HBV assay, Siemens VERSANT HBV assay, and Qiagen artus HBV RG kit. , 2017, Journal of clinical virology : the official publication of the Pan American Society for Clinical Virology.

[11]  M. Manns,et al.  Commutability and concordance of four hepatitis B virus DNA assays in an international multicenter study , 2017, Therapeutic advances in gastroenterology.

[12]  D. Sinn,et al.  Low‐level viremia and the increased risk of hepatocellular carcinoma in patients receiving entecavir treatment , 2017, Hepatology.

[13]  Thomas Berg,et al.  EASL 2017 Clinical Practice Guidelines on the management of hepatitis B virus infection. , 2017, Journal of hepatology.

[14]  J. Pawlotsky,et al.  The New Aptima HCV Quant Dx Real-time TMA Assay Accurately Quantifies Hepatitis C Virus Genotype 1-6 RNA. , 2017, Journal of clinical virology : the official publication of the Pan American Society for Clinical Virology.

[15]  N. Xia,et al.  Serum hepatitis B virus RNA is encapsidated pregenome RNA that may be associated with persistence of viral infection and rebound. , 2016, Journal of hepatology.

[16]  G. Marx,et al.  International Journal of Molecular Sciences the Ribonuclease a Superfamily in Humans: Canonical Rnases as the Buttress of Innate Immunity , 2022 .

[17]  A. Heim Evaluation of the Procleix Ultrio Elite Assay and the Panther-System for Individual NAT Screening of Blood, Hematopoietic Stem Cell, Tissue and Organ Donors , 2016, Transfusion Medicine and Hemotherapy.

[18]  N. Terrault,et al.  AASLD guidelines for treatment of chronic hepatitis B , 2016, Hepatology.

[19]  M. Kumar,et al.  Asian-Pacific clinical practice guidelines on the management of hepatitis B: a 2015 update , 2015, Hepatology International.

[20]  A. Geretti,et al.  Comparative performance of the new Aptima HIV-1 Quant Dx assay with three commercial PCR-based HIV-1 RNA quantitation assays. , 2015, Journal of clinical virology : the official publication of the Pan American Society for Clinical Virology.

[21]  T. Berg,et al.  Serum hepatitis B virus RNA levels as an early predictor of hepatitis B envelope antigen seroconversion during treatment with polymerase inhibitors , 2015, Hepatology.

[22]  Anders Kallner,et al.  Measurement Procedure Comparison and Bias Estimation Using Patient Samples; Approved Guideline—Third Edition , 2013 .