Hepatitis B and D viruses replication interference: Influence of hepatitis B genotype

Antonio Madejón; Míriam Romero; Ángela Hernández; Araceli García-Sánchez; Marta Sánchez-Carrillo; Antonio Olveira; Javier García-Samaniego

doi:10.3748/wjg.v22.i11.3165

Hepatitis B and D viruses replication interference: Influence of hepatitis B genotype

World J Gastroenterol. 2016 Mar 21;22(11):3165-74. doi: 10.3748/wjg.v22.i11.3165.

Authors

Antonio Madejón¹, Míriam Romero¹, Ángela Hernández¹, Araceli García-Sánchez¹, Marta Sánchez-Carrillo¹, Antonio Olveira¹, Javier García-Samaniego¹

Affiliation

¹ Antonio Madejón, Míriam Romero, Ángela Hernández, Araceli García-Sánchez, Marta Sánchez-Carrillo, Antonio Olveira, Javier García-Samaniego, Hepatology Section, Gastroenterology Department, Hospital Universitario La Paz, 28046 Madrid, Spain.

Abstract

Aim: To study the hepatitis B virus (HBV) and hepatitis D virus (HDV) replication interferences in patients with chronic hepatitis delta infected with different HBV genotypes.

Methods: We conducted a transversal study including 68 chronic hepatitis delta (CHD) (37 HIV-positive) patients and a control group of 49 chronic hepatitis B (CHB) (22 HIV-positive) patients. In addition, a dynamic follow-up was performed in 16 CHD patients. In all the samples, the surface antigen of hepatitis B (HBsAg) serum titers were analyzed with the Monolisa HBsAg Ultra system (Bio-Rad), using as quantification standard a serial dilution curve of an international HBsAg standard. Serum HBV-DNA titers were analyzed using the Roche Cobas TaqMan (Roche, Barcelona, Spain), and the serum HDV-RNA using an in-house real-time qRT-PCR method, with TaqMan probes. HBV genotype was determined with the line immunoassay LiPA HBV genotyping system (Innogenetics, Ghent, Belgium). In those patients negative for LiPA assay, a nested PCR method of complete HBsAg coding region, followed by sequence analysis was applied.

Results: No differences in the HBV-DNA levels were found in CHB patients infected with different HBV genotypes. However, in CHD patients the HBV-DNA levels were lower in those infected with HBV-A than in those with HBV-D, both in HIV negative [median (IQR): 1.25 (1.00-1.35) vs 2.95 (2.07-3.93) log10 (copies/mL), P = 0.013] and HIV positive patients [2.63 (1.24-2.69) vs 7.25 (4.61-7.55) log10 (copies/mL), P < 0.001]. This was confirmed in the dynamic study of the HBV/HDV patients. These differences induce an under-estimation of HBV-A incidence in patients with CHD analyzed with LiPA assay. Finally, the HBsAg titers reflected no significant differences in CHD patients infected with HBV-A or D.

Conclusion: Viral replication interference between HBV and HDV is HBV-genotype dependent, and more evident in patients infected with HBV-genotype A, than with HBV-D or E.

Keywords: Delta hepatitis; Hepatitis B virus; Hepatitis D virus; Replication interference; Viral replication.

Publication types

Comparative Study
Research Support, Non-U.S. Gov't

MeSH terms

Adult
Biomarkers / blood
Coinfection*
Cross-Sectional Studies
DNA, Viral / blood
DNA, Viral / genetics
Female
Genotype
HIV Infections / complications
HIV Infections / virology
Hepatitis B / complications
Hepatitis B / diagnosis
Hepatitis B / virology*
Hepatitis B Surface Antigens / blood
Hepatitis B virus / genetics
Hepatitis B virus / growth & development*
Hepatitis B virus / immunology
Hepatitis D, Chronic / complications
Hepatitis D, Chronic / diagnosis
Hepatitis D, Chronic / virology*
Hepatitis Delta Virus / genetics
Hepatitis Delta Virus / growth & development*
Humans
Longitudinal Studies
Male
Middle Aged
RNA, Viral / blood
RNA, Viral / genetics
Retrospective Studies
Time Factors
Viral Load
Virus Replication*

Substances

Biomarkers
DNA, Viral
Hepatitis B Surface Antigens
RNA, Viral