Virology Journal (Apr 2006)

Application of real-time PCR to quantify hepatitis B virus DNA in chronic carriers in The Gambia

  • Waight Pauline A,
  • Rayco-Solon Pura,
  • van der Sande Marianne,
  • Kaye Steve,
  • Mendy Maimuna E,
  • Shipton Deborah,
  • Awi Dorka,
  • Snell Paul,
  • Whittle Hilton,
  • McConkey Samuel J

DOI
https://doi.org/10.1186/1743-422X-3-23
Journal volume & issue
Vol. 3, no. 1
p. 23

Abstract

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Abstract Background/Aim The study aimed at developing a real-time quantitative PCR assay to monitor HBV serum virus load of chronic carriers enrolled in therapeutic trials. Method Quantitative real-time PCR assay was carried out using SYBR-Green signal detection and primers specific to the S gene. Thermal cycling was performed in an ABi 5700 sequence detection system. The assay was calibrated against an international HBV DNA standard and inter- and intra-assay reproducibility determined. Levels of viral load were monitored for 1-year in lamivudine treated carriers. Correlation between HBV DNA levels and HBeAg sero-status was determined in untreated carriers. Results The qPCR assay showed good intra- and inter-assay reproducibility over a wide dynamic range (1.5 × 103 to 1.5 × 108 copies/mL) and correlated well with those from a commercial assay (r = 0.91, (p Conclusion This method is reliable, accurate, and reproducible. HBV DNA Quantification by qPCR can be used to monitor the efficacy of HBV therapy and useful in understanding the natural history of HBV in an endemic area.