Two distinct types of hepatitis B virus core promoter variants in Yemeni blood donors

• Published in: Journal of medical virology Vol. 68; no. 3; pp. 328 - 334
• Main Authors: Sallam, Talal A., Tong, C.Y. William
• Format: Journal Article
• Language: English
• Published: New York Wiley Subscription Services, Inc., A Wiley Company 01.11.2002; Wiley-Liss
• Subjects: Adolescent; Adult; Amino Acid Substitution; Base Sequence; basic core promoter; Biological and medical sciences; Blood Donors; deletions; DNA, Viral - analysis; DNA, Viral - blood; Fundamental and applied biological sciences. Psychology; Gene Deletion; Genetic Variation; Genetics; Hepatitis B Core Antigens - genetics; Hepatitis B e Antigens; Hepatitis B virus - genetics; Hepatitis B, Chronic - virology; Humans; Male; Microbiology; Middle Aged; Molecular Sequence Data; Phenotype; Polymerase Chain Reaction; precore; Promoter Regions, Genetic - genetics; Protein Precursors - genetics; Sequence Analysis, DNA; substitutions; Viral Load; Virology; Yemen; Asia; Yemen; Human; Genetic variability; Hepatitis B core antigen; Transcription promoter; Orthohepadnavirus; Hepatic disease; Asymptomatic; Virus; Hepatitis; Hepadnaviridae; Digestive diseases; Mutation; Hepatitis B virus; Blood donor
• ISSN: 0146-6615; 1096-9071
• DOI: 10.1002/jmv.10207

Genetic variations in the basic core promoter (BCP) region of hepatitis B virus (HBV) occur during the natural history of chronic HBV infection. This study investigates the presence of basic core promoter variations in 28 asymptomatic Yemeni blood donors, correlating variations with HBeAg phenotype and viral load. The core promoter/precore and surface gene region of HBV DNA were amplified using nested PCRs and the PCR products were sequenced either directly or after cloning. HBeAg and viral load were measured when HBV DNA was detectable. Sequencing of 18 surface PCR products indicated that all were of genotype D. Two distinct types of variants were identified in the basic core promoter: substitution only (N = 14) and major deletion (N = 9). The commonest substitutions were located at nucleotide positions 1753, 1762, and 1764; 10/14 (71.4%) were associated with the precore 1896A substitution resulting in the premature stop of the precore reading frame and 6/14 (42.9%) had viral loads above 400 copies/ml. Two forms of deletion variants were found: 8 bp deletion (1763–1770) (N = 2) and a novel 12 (1746–1757) + 8 bp (1763–1770) deletion (N = 7). The deletion sequences were never associated with the precore 1896A substitution and all had viral load below 400 copies/ml with negative HBeAg phenotype. The polymorphism 1773C was found in 9/14 (64.3%) substitution sequences whereas all deletion sequences had 1773T. Two donors had mixed sequences of basic core promoter substitution and major deletions (both 8 bp and 12 + 8 bp). While the deletion variants in these two donors were similar to others found in isolation, the substitutions were of a different pattern. Further studies are required to understand the selection process behind these variants. J. Med. Virol. 68:328–334, 2002. © 2002 Wiley‐Liss, Inc.