Your search keyword '"Hepatitis B Virus, Duck isolation & purification"' showing total 56 results

1. Simple and visible detection of duck hepatitis B virus in ducks and geese using loop-mediated isothermal amplification.

Author

Ji J, Xu X, Wu Q, Wang X, Li W, Yao L, Kan Y, Yuan L, Bi Y, and Xie Q

Subjects

Animals, Hepadnaviridae Infections diagnosis, Hepadnaviridae Infections virology, Hepatitis, Viral, Animal virology, Nucleic Acid Amplification Techniques methods, Poultry Diseases virology, Sensitivity and Specificity, Ducks, Geese, Hepadnaviridae Infections veterinary, Hepatitis B Virus, Duck isolation & purification, Hepatitis, Viral, Animal diagnosis, Nucleic Acid Amplification Techniques veterinary, Poultry Diseases diagnosis

Abstract

In this study, loop-mediated isothermal amplification (LAMP) was used to establish a rapid, specific, and visual detection method for duck hepatitis B virus (DHBV). The design and synthesis of 4 specific LAMP primers were based on the conserved gene region of the DHBV genome, and the optimum temperature and time of the LAMP reaction were 63°C and 50 min, respectively. The LAMP assay was confirmed to be specific for DHBV detection and had the same sensitivity as the quantitative PCR assay. A visual detection method for rapid determination of results was developed using a color indicator containing phenol red and cresol red. A color change was produced based on a pH change in the reaction system, indicating a positive reaction. For the detection of samples from ducks and geese, the LAMP method has the advantages of simplicity, high sensitivity and specificity, good visibility, and low cost. Moreover, it is more practical and convenient than PCR-related assays for the clinical detection of DHBV., (Copyright © 2019 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2020

2. [Establishment of a method to detect duck hepatitis B virus covalently closed circular DNA based on rolling circle amplification].

Author

Su HL, Wang HM, Ran JY, Wang Z, Li HY, Yang Y, Xu DP, and Liu YM

Subjects

Animals, DNA Primers genetics, Ducks, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck genetics, Liver virology, Polymerase Chain Reaction methods, DNA, Circular genetics, DNA, Viral genetics, Hepadnaviridae Infections veterinary, Hepatitis B Virus, Duck isolation & purification, Poultry Diseases virology

Abstract

Rolling circle amplification (RCA) is a newly developed experimental technique that can specific ally amplify circular DNA. Since 2008, RCA has been extensively used in hepatitis B virus (HBV) research, such as the amplification of the full-length sequence of the HBV genome, and the analysis of the drug-resistant mutations of HBV covalently closed circular DNA (cccDNA), amongst others. To create an easy assay for the analysis of duck hepatitis B virus (DHBV) cccDNA, this study established an RCA-based method. DHBV cccDNA was amplified from the DHBV DNA samples of duck liver with four pairs of sulfur-modified primers, which were designed according to the highly conserved sequence of DHBV using sera DHBV DNA as the negative control. DHBV cccDNA was detected in the obtained RCA products by the sequencing of RCA amplicons that were amplified with primer pairs on both sides of the gap of DH BV relaxed circular DNA, rather than by digesting RCA products with a restriction enzyme. The liver and sera DHBV DNA samples of 39 ducks infected with DHBV were examined with the RCA-based DHBV cccDNA detection method, and the results showed that while DHBV cccDNA was detected from all 39 liver DHBV DNA samples, no DHBV cccDNA was found in any of the sera DHBV DNA samples. These results suggest that the method established in the study is highly specific and sensitive for the detection of DHBV cccDNA. The establishment of this RCA-based DHBV method for cccDNA detection lays the groundwork for using a DHBV model to study the role of cccDNA in the pathogenesis of hepatitis B and to evaluate the effect of anti-virus therapies.

Published

2014

3. Antiviral activity of methyl helicterate isolated from Helicteres angustifolia (Sterculiaceae) against hepatitis B virus.

Author

Huang Q, Huang R, Wei L, Chen Y, Lv S, Liang C, Zhang X, Yin F, Li H, Zhuo L, and Lin X

Subjects

Animals, Antiviral Agents isolation & purification, Cell Line, DNA, Viral genetics, DNA, Viral isolation & purification, Ducks, Hepadnaviridae Infections drug therapy, Hepatitis B Virus, Duck genetics, Hepatitis B Virus, Duck isolation & purification, Hepatocytes virology, Histocytochemistry, Humans, Liver pathology, Liver virology, Plant Extracts isolation & purification, Poultry Diseases drug therapy, Serum virology, Triterpenes isolation & purification, Viral Load, Antiviral Agents pharmacology, Hepatitis B virus drug effects, Hepatitis, Viral, Animal drug therapy, Malvaceae chemistry, Plant Extracts pharmacology, Triterpenes pharmacology

Abstract

The anti-HBV effect of methyl helicterate (MH), a triterpenoid isolated from the Chinese herb Helicteres angustifolia, was explored both in vitro and in vivo. In the HBV-transfected cell line HepG2.2.15, the secretion of HBsAg/HBeAg, the levels of HBV DNA and cccDNA, and the amount of viral RNA were significantly decreased after treatment with MH for 144h. In addition, MH had no inhibitory effect on the mitochondrial DNA content. In DHBV-infected ducklings, MH significantly reduced the serum DHBV DNA, liver total viral DNA, and cccDNA levels. Furthermore, analysis of the liver pathological changes confirmed the hepatoprotective effect of MH. These results indicate that MH efficiently inhibits HBV replication both in vitro and in vivo and that MH may be a major bioactive ingredient in H. angustifolia., (Copyright © 2013 Elsevier B.V. All rights reserved.)

Published

2013

4. Development and application of a universal Taqman real-time PCR for quantitation of duck hepatitis B virus DNA.

Author

Wang Y, Li Y, Yang C, Hui L, Han Q, Ma L, Wang Q, Yang G, and Liu Z

Subjects

Animals, Blood virology, China, DNA Primers genetics, DNA, Viral genetics, Ducks, Hepadnaviridae Infections diagnosis, Hepadnaviridae Infections veterinary, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck genetics, Hepatitis, Viral, Animal diagnosis, Hepatitis, Viral, Animal virology, Liver virology, Oligonucleotide Probes genetics, Reproducibility of Results, Sensitivity and Specificity, DNA, Viral isolation & purification, Hepatitis B Virus, Duck isolation & purification, Real-Time Polymerase Chain Reaction methods, Viral Load methods

Abstract

To develop a quantitative assay for universal detection of duck hepatitis B virus (DHBV) DNA, a Taqman real-time fluorescent quantitative polymerase chain reaction (FQ-PCR) assay was developed using primers and probes based on genomic sequences located at nucleotide 241-414 of the DHBV Core region which possesses the highest homology among the 44 DHBV genomes available in Genbank. The DHBV Core gene cloned in pGEM-T was used to generate DHBV DNA standard. The assay had a lowest detection limit of 10(3) copies/ml and a good linear standard curve (Y=-3.989X+49.086, r(2)=0.9993) over a wide range of input DHBV DNA (10(3) to 10(10) copies/ml). The standard deviation of intra- and inter-assay was 0.01-0.06 and 0.05-0.16, respectively, and the coefficient of variation was 1.3-1.8%. The specificity of the assay was validated using duck hepatitis virus type 1, hepatitis B virus, and E. coli DNA. Comparison of ABI 7300 and Bio-Rad iQ5 PCR instruments yielded highly consistent results. The assay showed a positive rate of 63.8% (51/80) DHBV DNA in peripheral blood and liver tissue from ducks from Xi'an, China. The FQ-PCR developed is highly sensitive, specific, reproducible and versatile, and may be used to universally detect DHBV DNA of different DHBV strains., (Copyright © 2013 Elsevier B.V. All rights reserved.)

Published

2013

5. [Cloning and sequence analysis of the DHBV genome of the brown ducks in Guilin region and establishment of the quantitative method for detecting DHBV].

Author

Su HL, Huang RD, He SQ, Xu Q, Zhu H, Mo ZJ, Liu QB, and Liu YM

Subjects

Animals, Base Sequence, China epidemiology, Ducks, Hepadnaviridae Infections diagnosis, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck classification, Hepatitis B Virus, Duck genetics, Molecular Sequence Data, Phylogeny, Poultry Diseases diagnosis, Cloning, Molecular, Genome, Viral, Hepadnaviridae Infections veterinary, Hepatitis B Virus, Duck isolation & purification, Polymerase Chain Reaction methods, Poultry Diseases virology

Abstract

Brown ducks carrying DHBV were widely used as hepatitis B animal model in the research of the activity and toxicity of anti-HBV dugs. Studies showed that the ratio of DHBV carriers in the brown ducks in Guilin region was relatively high. Nevertheless, the characters of the DHBV genome of Guilin brown duck remain unknown. Here we report the cloning of the genome of Guilin brown duck DHBV and the sequence analysis of the genome. The full length of the DHBV genome of Guilin brown duck was 3 027bp. Analysis using ORF finder found that there was an ORF for an unknown peptide other than S-ORF, PORF and C-ORF in the genome of the DHBV. Vector NTI 8. 0 analysis revealed that the unknown peptide contained a motif which binded to HLA * 0201. Aligning with the DHBV sequences from different countries and regions indicated that there were no obvious differences of regional distribution among the sequences. A fluorescence quantitative PCR for detecting DHBV was establishment based on the recombinant plasmid pGEM-DHBV-S constructed. This study laid the groundwork for using Guilin brown duck as a hepatitis B animal model.

Published

2013

6. [Research on the gene structure of duck hepatitis B virus and its encoding proteins].

Author

Liu Q and Jia RY

Subjects

Animals, Ducks, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck chemistry, Hepatitis B Virus, Duck isolation & purification, Open Reading Frames, Protein Structure, Tertiary, Viral Proteins chemistry, Hepadnaviridae Infections veterinary, Hepatitis B Virus, Duck genetics, Hepatitis, Viral, Animal virology, Viral Proteins genetics

Abstract

Duck hepatitis B virus (DHBV) belongs to the Avihepadnavirus genus of the Hepadnaviridae, and it not only has the same replication pattern, but also has the similar genomic and antigenic structures to Hepatitis B virus (HBV). The genome of DHBV is a partially double-stranded closed circular DNA. The genome consists of three distinct open reading frames (ORFs): ORF-PreS/S, ORF-PreC/C and ORF-P, which all locate on the negative DNA strand and encode four separate proteins. The ORF-PreS/S encodes envelope proteins L and S, and the ORF-PreC/C and ORF-P encode capsid proteins C and polymerase proteins P, respectively. The characteristics of genome structure,viral proteins features and functions were described in this review in order to provide useful information for the further study of DHBV and the duck model infected by DHBV.

Published

2012

7. [Dynamic detection of duck hepatitis B virus cccDNA in serum of ducks with liver injury].

Author

Zhao KK, Wang Q, Miao XH, and Xu WS

Subjects

Animals, Ducks, Hepatitis B Virus, Duck genetics, Hepatitis, Viral, Animal pathology, Serum, Chemical and Drug Induced Liver Injury virology, DNA, Viral blood, Hepatitis B Virus, Duck isolation & purification, Hepatitis, Viral, Animal virology, Liver virology

Abstract

Objective: To confirm whether DHBV cccDNA could be detected in serum of DHBV-infected ducks after liver injury., Methods: Twenty four ducks with persistent DHBV infection were divided into 4 groups with the following treatments: A, D-galactosamine (D-GalN, 2.2 g/kg) and lipopolysaccharide (LPS, 100 µg/kg); B, 10 mg/kg of carbon tetrachloride (CCl4) every 12 h twice following D-GalN and LPS; C, 15 mg/kg of CCl4 every 12 h twice following D-GalN and LPS; D, normal saline as normal control (NC). At 0 h, 24 h, 36 h and 48 h post-treatment, sera were collected from each duck for determination of serum DHBV load, DHBV cccDNA and alanine aminotransferase (ALT). And ducks were eventually sacrificed to obtain liver specimens for pathological assessment of liver lesions and determination of intrahepatic total DHBV DNA and DHBV cccDNA., Results: (1) No obvious pathological change was observed in the liver of ducks from NC group while the indices of liver injury were significantly different between Groups A, B and C; (2) DHBV cccDNA was undetectable in the sera of ducks from NC and A group at all time points. In contrast, DHBV cccDNA, varying from 3.17 × 10(3) copies/ml to 1.72 × 10(4) copies/ml, was detected in the sera of 2 ducks from Group B and 3 ducks from Group C at 36 h post-treatment. The occurrence of DHBV cccDNA in serum was significantly correlated with the degree of liver injury while no significant association with serum ALT level and DHBV load as well as with the level of intrahepatic total DHBV DNA and DHBV cccDNA was observed., Conclusion: DHBV cccDNA may be detected in the serum when the liver of duck is seriously damaged. The incidence of DHBV cccDNA occurrence in the serum is significantly associated with the severity of liver injury.

Published

2010

8. Identification of natural recombination in duck hepatitis B virus.

Author

Liu W, Zhai J, Liu J, and Xie Y

Subjects

Animals, China, Cluster Analysis, DNA, Viral genetics, Genome, Viral, Hepatitis B Virus, Duck isolation & purification, Phylogeny, Sequence Analysis, DNA, Ducks virology, Hepatitis B Virus, Duck genetics, Recombination, Genetic

Abstract

Due to its high similarity to human hepatitis B virus (HBV), duck HBV (DHBV) is often used as an important model for HBV research. While inter-genotypic recombination of HBV is common, it has not been reported with DHBV. In this study, 32 non-redundant DHBV complete genomes were analyzed using phylogenetic methods and classified into two clusters, corresponding to the 'Chinese' and 'Western country' branches previously reported based on geographical distribution. One 'Chinese' branch strain was isolated in Australia and three 'Western country' branch strains were isolated in China, suggesting cross-geographical distribution of both branches. Recombination analyses of the 32 DHBV genomes identified two possible inter-genotypic recombination events with high confidence value. These recombination events occurred between the lineages represented, respectively, by the Chinese isolate GD3 (AY536371, 'Chinese' branch) and the American isolate DHBV16 (K01834, 'Western country' branch), giving rise to two Chinese recombinant isolates CH4 (EU429324) and CH6 (EU429326). The identification of inter-genotypic recombination among circulating DHBV isolates suggests the usefulness of DHBV as a model for studying the mechanism of HBV recombination., ((c) 2010 Elsevier B.V. All rights reserved.)

Published

2010

9. The early host innate immune response to duck hepatitis B virus infection.

Author

Tohidi-Esfahani R, Vickery K, and Cossart Y

Subjects

Age Factors, Animals, Apoptosis, Cells, Cultured, Female, Hepadnaviridae Infections immunology, Hepadnaviridae Infections physiopathology, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck isolation & purification, Hepatitis, Viral, Animal physiopathology, Hepatitis, Viral, Animal virology, Hepatocytes cytology, Hepatocytes immunology, Immunity, Cellular, Immunity, Innate, Lymphocytes immunology, Male, Poultry Diseases physiopathology, Poultry Diseases virology, Ducks, Hepadnaviridae Infections veterinary, Hepatitis B Virus, Duck immunology, Hepatitis, Viral, Animal immunology, Poultry Diseases immunology

Abstract

The early phase after hepatitis B virus infection could play a crucial role in clearance and/or persistence of the virus, particularly in neonates. This work compared the early phase of duck hepatitis B virus infection in 1-day-old (D1) and 28-day-old (D28) ducks to determine whether differences in viral or host innate immune response can be related to the difference in outcome. In the first phase, almost immediately after inoculation, virus was taken up by components of the reticulo-endothelial systems, particularly liver-specific macrophages, Kupffer cells. Very early after infection, the induction of alpha interferon by infected hepatocytes occurred and was rapidly reinforced by recruitment of effector lymphocytes, which directly or indirectly caused apoptosis, eliminating infected hepatocytes, as was seen in mature birds. In addition, a lack of lymphocytic infiltration of the liver was found in D1 ducks, which supports the suggestion that the innate immune network is less effective in D1 ducks. Taken together, these results suggest that failure of the co-ordinated innate immune response rather than a defect in induced antiviral cell-mediated immunity may be the key factor which makes baby ducks vulnerable to persistence of hepadnavirus infection.

Published

2010

10. Viral load in 1-day-old ducklings acutely infected with duck hepatitis B virus by different doses and routes of inoculation.

Author

Chen ZY, Cheng AC, Wang MS, Xu DW, Jia R, Guo YF, and Zeng W

Subjects

Animals, DNA Primers, DNA, Viral blood, DNA, Viral isolation & purification, Ducks, Gene Amplification, Genome, Viral, Hepatitis B pathology, Hepatitis B virology, Hepatitis B Virus, Duck genetics, Hepatitis, Viral, Animal genetics, Hepatitis, Viral, Animal virology, Hepatocytes virology, Liver pathology, Liver virology, Viremia blood, Viremia veterinary, Hepatitis B veterinary, Hepatitis B Virus, Duck isolation & purification, Hepatitis, Viral, Animal pathology, Poultry Diseases virology, Viral Load

Abstract

In order to define clearly the conditions leading to the outcome of acute duck hepatitis B virus (DHBV) infection, 1-day-old Pekin ducklings were infected with DHBV by different routes and given different doses of inoculum. Groups of 24 ducklings were inoculated either intravenously via the vena cruralis, or intraperitoneally with pooled serum containing either 1.6 x 10(7) or 1.6 x 10(4) DHBV genomes. One control duck from each group was inoculated with an equal volume of normal duck serum. A sensitive and reproducible real-time polymerase chain reaction assay based on TaqMan technology was developed for the detection and quantitation of DHBV DNA in the serum and liver. DHBAg was observed in the hepatocytes by immunohistochemistry. Histological changes in the liver tissue were also observed. The results demonstrate that ducklings at each time point and in all groups developed detectable viraemia. In each group, DHBV DNA in the liver was at a lower level than in serum and the peak DNA titre was found in serum earlier than in the liver. In the low-dose groups it was always at a lower level than in the high-dose groups. The DHBV replication levels appeared to be directly related to the number of DHBAg-positive hepatocytes. The variation trends of DHBAg-positive hepatocytes were similar in the high-dose groups. Histological changes were associated with liver viral DNA levels. We suggest that this dose and route of inoculation can be used as a model to study acute DHBV infections.

Published

2009

11. Assembly and budding of a hepatitis B virus is mediated by a novel type of intracellular vesicles.

Author

Mhamdi M, Funk A, Hohenberg H, Will H, and Sirma H

Subjects

Animals, Cell Fractionation, Cell Membrane virology, Ducks, Endoplasmic Reticulum virology, Hepatitis B Virus, Duck growth & development, Hepatitis B Virus, Duck isolation & purification, Hepatitis B virus growth & development, Hepatitis B virus isolation & purification, Hepatocytes ultrastructure, Organelles virology, Plasmids, Virus Replication, Hepatitis B Virus, Duck genetics, Hepatitis B virus physiology, Hepatocytes virology

Abstract

Unlabelled: Formation of enveloped viruses involves assembly and budding at cellular membranes. In this study, we elucidated the morphogenesis of hepadnaviruses on the ultrastructural and biochemical level using duck hepatitis B virus (DHBV) as a model system. Formation of virus progeny initiates at the endoplasmic reticulum (ER) and is conserved both in vitro and in vivo. The morphogenesis proceeds via membrane-surrounded vesicles containing both virions and subviral particles, indicating a common morphogenetic pathway. The virus particle-containing vesicles (VCVs) are generated and maintained by reorganization of endomembranes accompanied by a striking disorganization of the rough ER (rER). VCVs are novel organelles with unique identity and properties of ER, intermediate compartment, endosomes, and multivesicular bodies. VCVs are dynamic structures whose size and shape are regulated by both membrane fusion and fission., Conclusion: Our data indicate a strong reorganization of endomembranes during DHBV infection, resulting in the biogenesis of novel organelles serving as multifunctional platforms for assembly and budding of virus progeny.

Published

2007

12. LC-MS characterization of efficacy substances in serum of experimental animals treated with Sophora flavescens extracts.

Author

Ye G, Zhu HY, Li ZX, Ma CH, Fan MS, Sun ZL, and Huang CG

Subjects

Alkaloids blood, Animals, Cell Survival drug effects, Cells, Cultured, Ducks, Flavonoids blood, Formazans chemistry, Formazans metabolism, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck isolation & purification, Hepatitis B Virus, Duck physiology, Molecular Structure, Quinolizines blood, Sophora chemistry, Spectrophotometry, Ultraviolet methods, Tetrazolium Salts chemistry, Tetrazolium Salts metabolism, Matrines, Antiviral Agents administration & dosage, Chromatography, High Pressure Liquid methods, Hepadnaviridae Infections drug therapy, Hepatitis B Virus, Duck drug effects, Plant Extracts administration & dosage, Spectrometry, Mass, Electrospray Ionization methods, Virus Replication drug effects

Abstract

Anti-DHBV (duck hepatitis B virus) activity was found in the aqueous extracts of Sophora flavescens Ait. in vivo. Liquid chromatography/electrospray ionization ion trap mass spectrometry was applied to characterize the components in duck serum after oral administration of S. flavescens extract. Oxymatrine (1), sophoranol (2), sophoridine (3) and matrine (4) were identified in the serum. Further research on the four compounds was evaluated for their antiviral activity against HBV (hepatitis B virus) in cell culture. The results suggested that oxymatrine, sophoranol and matrine were the efficacy substances for anti-HBV activity in aqueous extracts of S. flavescens Ait., (Copyright 2007 John Wiley & Sons, Ltd.)

Published

2007

13. Enzymatic treatment of duck hepatitis B virus: topology of the surface proteins for virions and noninfectious subviral particles.

Author

Franke C, Matschl U, and Bruns M

Subjects

Animals, Blotting, Western, Chymotrypsin metabolism, Ducks, Electrophoresis, Polyacrylamide Gel, Hepatitis B Virus, Duck isolation & purification, Iodine Isotopes, Models, Biological, Phosphoric Monoester Hydrolases metabolism, Phosphorylation, Serum virology, Staining and Labeling, Ultracentrifugation, Viral Envelope Proteins chemistry, Viral Envelope Proteins metabolism, Virion isolation & purification, Hepatitis B Virus, Duck chemistry, Viral Envelope Proteins analysis, Virion chemistry

Abstract

The large surface antigen L of duck hepatitis B virus exhibits a mixed topology with the preS domains of the protein alternatively exposed to the particles' interior or exterior. After separating virions from subviral particles (SVPs), we compared their L topologies and showed that both particle types exhibit the same amount of L with the following differences: 1--preS of intact virions was enzymatically digested with chymotrypsin, whereas in SVPs only half of preS was accessible, 2--phosphorylation of L at S118 was completely removed by phosphatase treatment only in virions, 3--iodine-125 labeling disclosed a higher ratio of exposed preS to S domains in virions compared to SVPs. These data point towards different surface architectures of virions and SVPs. Because the preS domain acts in binding to a cellular receptor of hepatocytes, our findings implicate the exclusion of SVPs as competitors for the receptor binding and entry of virions.

Published

2007

14. The effect of surgical immunomodulation on liver inflammation and clearance of DHBV infection.

Author

Vickery K, Tohidi-Esfahani R, Pouliopoulos J, Welschinger R, Dixon R, Deva A, and Cossart Y

Subjects

Animals, B-Lymphocytes immunology, Bursa of Fabricius immunology, Female, Hepadnaviridae Infections virology, Hepatitis, Viral, Animal virology, Leukocyte Count, Liver immunology, Liver pathology, Male, Spleen pathology, T-Lymphocytes immunology, Bursa of Fabricius surgery, Hepadnaviridae Infections immunology, Hepatitis B Virus, Duck isolation & purification, Hepatitis, Viral, Animal immunology, Inflammation immunology, Liver physiopathology, Thymectomy

Abstract

The key to developing a therapeutic vaccine for chronic hepadnavirus infection lies in the characteristics of the host-immune response which leads to clearance of acute infection. Groups of 28-day-old ducks which had been surgically bursectomized (n = 10) or thymectomized (n = 13) on the day of hatch or were untreated (n = 21) were inoculated with 10(9) viral genome equivalents (vge) DHBV, then bled twice a week, and euthanased 40 days later. Serum and liver were tested for DHBV DNA and total leukocytes and peripheral blood mononuclear cells (PBMCs) counted. Liver and spleen sections were either stained with hematoxylin and eosin, and graded for inflammation or stained with peroxidase-labeled anti-human CD3 antibody and examined for T lymphocyte distribution. PBMC counts were similar in all groups. DHBV infection combined with bursectomy increased significantly, while thymectomy decreased significantly the total leukocyte count. The spleen and liver bursectomy increased T lymphocyte number while B cells were decreased. Converse changes were observed in thymectomized ducks. Histological evidence of hepatitis was present in infected control and bursectomized ducks but not in the uninfected control or infected thymectomized ducks. In control animals, DHBV challenge caused viremia in 17 and persistent infection in 11 (56%). Fewer thymectomized ducks (3/13, 23%) and significantly more (100%) bursectomized ducks remained persistently infected (P < 0.001). Unexpectedly, bursectomy led to persistence of infection while clearance of infection occurred normally in thymectomized ducks despite decreased T lymphocyte numbers. This suggests that clearance requires T and B lymphocyte collaboration., ((c) 2006 Wiley-Liss, Inc.)

Published

2006

15. Rise in gamma interferon expression during resolution of duck hepatitis B virus infection.

Author

Narayan R, Buronfosse T, Schultz U, Chevallier-Gueyron P, Guerret S, Chevallier M, Saade F, Ndeboko B, Trepo C, Zoulim F, and Cova L

Subjects

Animals, DNA, Viral analysis, DNA, Viral genetics, Ducks, Hepadnaviridae Infections blood, Hepadnaviridae Infections metabolism, Hepadnaviridae Infections virology, Hepatitis B Antibodies blood, Hepatitis B Surface Antigens immunology, Hepatitis B Surface Antigens metabolism, Hepatitis, Viral, Animal blood, Hepatitis, Viral, Animal virology, Interferon-gamma genetics, Liver virology, Polymerase Chain Reaction, RNA, Viral analysis, RNA, Viral genetics, Time Factors, Viremia, Hepadnaviridae Infections veterinary, Hepatitis B Virus, Duck isolation & purification, Hepatitis, Viral, Animal metabolism, Interferon-gamma metabolism, Leukocytes, Mononuclear metabolism, Liver metabolism

Abstract

Gamma interferon (IFN-gamma) expression plays a crucial role in the control of mammalian hepatitis B virus (HBV) infection. However, the role of duck INF-gamma (DuIFN-gamma) in the outcome of duck HBV (DHBV) infection, a reference model for hepadnavirus replication studies, has not yet been investigated. This work explored the dynamics of DuIFN-gamma expression in liver and peripheral blood mononuclear cells (PBMCs) during resolution of DHBV infection in adolescent ducks in relation to serum and liver markers of virus replication, histological changes and humoral response induction. DHBV infection of 3-week-old ducks resulted in transient expression of intrahepatic preS protein (days 3-14) and mild histological changes. Low-level viraemia was detected only during the first 10 days of infection and was accompanied by early anti-preS antibody response induction. Importantly, a strong increase in intrahepatic DuIFN-gamma RNA was detected by real-time RT-PCR at days 6-14, which coincided with a sharp decrease in both viral DNA and preS protein in the liver. Interestingly, liver DuIFN-gamma expression remained augmented to the end of the follow-up period (day 66) and correlated with portal lymphocyte infiltration and persistence of trace quantities of intrahepatic DHBV DNA in animals that had apparently completely resolved the infection. Moreover, in infected ducks, a moderate increase was detected in the levels of DuIFN-gamma in PBMCs (days 12-14), which coincided with the peak in liver DuIFN-gamma RNA levels. These data reveal that increased DuIFN-gamma expression in liver and PBMCs is concomitant with viral clearance, characterizing the resolution of infection, and provide new insights into the host-virus interactions that control DHBV infection.

Published

2006

16. Molecular characterization of duck hepatitis B virus isolated from Hubei brown ducks.

Author

Hu Q, Zhang X, Lei Y, Zhang Z, Mengji L, and Yang D

Subjects

Animals, China, Cloning, Molecular, Genome, Viral, Hepatitis B Virus, Duck isolation & purification, Molecular Sequence Data, Phylogeny, Poultry Diseases virology, Sequence Analysis, Carrier State virology, Ducks virology, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck genetics, Hepatitis, Viral, Animal virology

Abstract

The objective of this study was to characterize the genome structure of duck hepatitis B virus (DHBV) isolated from Hubei brown ducks. The natural carrier rate of DHBV in adult ducks from Hubei area was investigated and the DHBV DNA-positive serum screened out. The complete genome of a DHBV strain was amplified by polymerase chain reaction (PCR) and cloned into T vector and sequenced. The results showed that the carrier rate of DHBV in Hubei brown ducks was 10 %. This strain (GenBank accession number DQ276978) had a genome of 3024 nucleotides with three overlapping open reading frames encoding the surface, core and polymerase proteins respectively. Comparison of the strain with 17 DHBV strains registered in GenBank revealed a homology from 89.3 % to 93.5 % at the nucleotide level. The sequences of the structural and functional domains of these proteins were highly conserved. The strain was found to share more signature amino acids in the polymerase genes with the "Chinese" DHBV strains than those of the "Western" country strains. This finding was also corroborated by a phylogenetic tree analysis. Therefore, the DQ276978 might belong to a subtype of the Chinese DHBV strains.

Published

2006

17. Alternative methods for validation of cell culture infection with duck hepatitis B virus.

Author

Sauerbrei A, Schacke M, Schultz U, Egerer R, Merkle I, Glebe D, Gerlich W, and Wutzler P

Subjects

Animals, Antigens, Viral analysis, DNA, Viral genetics, Ducks, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck immunology, Hepatitis B Virus, Duck isolation & purification, Hepatocytes virology, Microscopy, Fluorescence, Time Factors, Transfection, Hepadnaviridae Infections veterinary, Hepatitis B Virus, Duck growth & development, Hepatitis, Viral, Animal virology, Virus Cultivation methods

Abstract

Hepatitis B virus (HBV) is an important virus used in disinfection procedures for blood spillage. However, validation of HBV inactivation is difficult, since there are no feasible infectivity assays. In some countries, the duck HBV (DHBV) is recognized as a suitable model for testing antiviral activity of chemical biocides against HBV. Currently, DHBV-infected ducks are required for preparation of the test virus as well as eggs from DHBV-free flocks for testing DHBV infectivity. To improve the practicality of the system, we suggested to use commercially available embryonated duck eggs for preparation of DHBV-susceptible hepatocyte cultures and to exclude infected hepatocytes by pre-screening with qualitative detection of DHBV DNA using polymerase chain reaction (PCR). A standardized DHBV test virus was prepared from the DHBV DNA-transfected hepatoma cell line D2, which contained 10(11)DHBV DNA molecules per mL detected by light cycler real-time PCR. Infection of cell cultures was most efficient 4 days after plating. The best identification of infected cultures was possible 6 days after infection with immunofluorescence using an antiserum against DHBV surface antigen.

Published

2005

18. [The possibility of hepatitis B virus transmission through dental handpieces].

Author

Deng XH, Sun Z, Qiao H, Deng HY, Xiao X, and Su J

Subjects

Animals, DNA, Viral blood, Ducks virology, Hepatitis B Virus, Duck genetics, Hepatitis B Virus, Duck isolation & purification, Sterilization standards, Dental Instruments virology, Equipment Contamination, Hepatitis B transmission, Sterilization methods

Abstract

Objective: To discuss the possibility of hepatitis B virus (HBV) transmission through dental handpieces., Methods: Investigation was carried on methods for disinfecting and sterilizing dental handpieces and the condition of HBsAg contamination on dental handpieces before and after disinfection and sterilization by randomly sampling all special stomatological hospitals and dental clinics in a same city and 10 dental departments from the third, second and first class hospitals. The possibility of HBV transmission through dental handpieces was probed by investigating whether ducks can be infected by bath liquid of dental handpieces contaminated by DHBV, while in such bath liquid, DHBV can not be detected by serum dot hybridization., Results: From 2001 to 2004, in methods to disposing dental handpieces, the use of autoclave was remarkably increased while of the disinfectant wipe, immersion and other methods was remarkably decreased. The positive rate of HBsAg from dental handpieces in practice was 1.65%. It was evident that the bath liquid of dental handpieces contaminated by DHBV can conduct infection in vivo test of duck, while DHBV can not be detected in such bath liquid by serum dot hybridization, it is proved that the negative result of HBsAg in non-sterilized dental handpieces can not eliminate the possibility of HBV transmission through dental handpieces., Conclusion: There might exist the possibility of HBV transmission through dental handpieces however, the autoclaves might kill the virus contaminating on dental handpieces.

Published

2005

19. Establishment and assessment of two methods for quantitative detection of serum duck hepatitis B virus DNA.

Author

Chen YX, Huang AL, Qi ZY, and Guo SH

Subjects

Alkaline Phosphatase, Animals, DNA Probes, DNA, Viral analysis, Digoxigenin, Ducks, Hepadnaviridae Infections blood, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck genetics, Hepatitis, Viral, Animal blood, Hepatitis, Viral, Animal virology, Polymerase Chain Reaction, Sensitivity and Specificity, DNA, Viral blood, Hepadnaviridae Infections diagnosis, Hepatitis B Virus, Duck isolation & purification, Hepatitis, Viral, Animal diagnosis

Abstract

Aim: To establish and assess the methods for quantitative detection of serum duck hepatitis B virus (DHBV) DNA by quantitative membrane hybridization using DHBV DNA probe labeled directly with alkaline phosphatase and fluorescence quantitative PCR (qPCR)., Methods: Probes of DHBV DNA labeled directly with alkaline phosphatase and chemiluminescent substrate CDP-star were used in this assay. DHBV DNA was detected by autoradiography, and then scanned by DNA dot-blot. In addition, three primers derived from DHBV DNA S gene were designed. Semi-nested primer was labeled by AmpliSensor. Standard curve of the positive standards of DHBV DNA was established after asymmetric preamplification, semi-nested amplification and on-line detection. Results from 100 samples detected separately by alkaline phosphatase direct-labeled DHBV DNA probe with dot-blot hybridization and digoxigenin-labeled DHBV DNA probe hybridization. Seventy samples of duck serum were tested by fluorescent qPCR and digoxigenin-labeled DHBV DNA probe in dot-blot hybridization assay and the correlation of results was analysed., Results: Sensitivity of alkaline phosphatase direct-labeled DHBV DNA probe was 10 pg. The coincidence was 100% compared with digoxigenin-labeled DHBV DNA probe assay. After 30 cycles, amplification products showed two bands of about 180 bp and 70 bp by 20 g/L agarose gel electrophoresis. Concentration of amplification products was in direct proportion to the initial concentration of positive standards. The detection index was in direct proportion to the quantity of amplification products accumulated in the current cycle. The initial concentration of positive standards was in inverse proportion to the number of cycles needed for enough quantities of amplification products. Correlation coefficient of the results was (0.97, P<0.01) between fluorescent qPCR and dot-blot hybridization., Conclusion: Alkaline phosphatase direct-labeled DHBV DNA probe in dot-blot hybridization and fluorescent qPCR can be used as valuable means to quantify DHBV DNA in serum.

Published

2004

20. [Study on the detection of duck hepatitis B virus with SYBR based quantitative real-time PCR].

Author

Zou W, Yang X, Yang LP, Lai LY, Lei JH, Luo HY, and Zhang YH

Subjects

Animals, Benzothiazoles, DNA, Viral genetics, Diamines, Ducks, Hepatitis B Virus, Duck genetics, Hepatitis, Viral, Animal virology, Organic Chemicals, Quinolines, Sensitivity and Specificity, DNA, Viral isolation & purification, Hepatitis B Virus, Duck isolation & purification, Polymerase Chain Reaction methods

Published

2004

21. Molecular characterization of duck hepatitis B virus isolates from South African ducks.

Author

Mangisa NP, Smuts HE, Kramvis A, Linley CW, Skelton M, Tucker TJ, De La M Hall P, Kahn D, Jilbert AR, and Kew MC

Subjects

Animals, Base Sequence, Cloning, Molecular, DNA, Viral blood, DNA, Viral genetics, Hepadnaviridae Infections veterinary, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck classification, Hepatitis, Viral, Animal virology, Nucleic Acid Conformation, Phylogeny, Poultry Diseases virology, RNA, Viral chemistry, RNA, Viral genetics, South Africa, Ducks virology, Hepatitis B Virus, Duck genetics, Hepatitis B Virus, Duck isolation & purification

Abstract

The objective of the study was to characterize the genome of duck hepatitis B virus (DHBV) isolates from South African Pekin ducks. Duck serum and liver samples were collected from two commercial duck farms from geographically distinct regions of South Africa. In total, 498 duck serum samples were tested for the presence of DHBV DNA using either sub-genomic or full-length polymerase chain reaction (PCR) assays. The overall prevalence of DHBV infection in South African ducks was 47%. In addition, 30% of 59 liver tissues tested were DHBV DNA-positive. Six randomly selected serum or liver samples were used to clone and sequence the genomes of the South African DHBV strains. All six isolates had DHBV genomes of 3,021 nucleotides with three characteristic overlapping reading frames encoding the polymerase, surface and core gene products. No X-like gene with a traditional start codon was found. Following phylogenetic analysis, the South African DHBV isolates clustered with DHBV isolates from other "Western" countries, including United States of America, Canada, Germany and India. On translation of the open reading frames, the South African isolates were found to share signature amino acids in the polymerase and surface genes with the "Western" country isolates as opposed to those of Chinese DHBV isolates.

Published

2004

22. High prevalence of hepatitis B virus pre-s mutant in countries where it is endemic and its relationship with genotype and chronicity.

Author

Huy TT, Ushijima H, Win KM, Luengrojanakul P, Shrestha PK, Zhong ZH, Smirnov AV, Taltavull TC, Sata T, and Abe K

Subjects

Amino Acid Sequence, Animals, Asia epidemiology, Genetic Variation, Genotype, Geography, Hepatitis B virology, Hepatitis B Surface Antigens blood, Hepatitis B Virus, Duck genetics, Hepatitis B Virus, Duck isolation & purification, Hepatitis B virus isolation & purification, Humans, Molecular Sequence Data, Prevalence, Sequence Alignment, Sequence Homology, Amino Acid, Viral Envelope Proteins isolation & purification, Hepatitis B epidemiology, Hepatitis B virus genetics

Abstract

It has been reported that hepatitis B virus (HBV) mutants carrying mutations in the pre-S region can be found in infected patients. In this study, we investigated the prevalence of the HBV variant with the pre-S mutant in different geographic regions, including countries with low and high levels of endemic HBV infection, and analyzed the correlation with clinical findings. We examined 387 HBV DNA-positive serum samples from individuals among 12 countries, consisting of Vietnam, Myanmar, Thailand, China, Korea, Nepal, Japan, Russia, Spain, United States, Bolivia, and Ghana. HBV pre-S mutants were detected in 71 (18.3%) of 387 serum samples tested. This mutant was the most prevalent in Vietnam (36%), followed by Nepal (27.3%), Myanmar (23.3%), China (22.4%), Korea (14.3%), Thailand (10.5%), Japan (7.7%), and Ghana (4.3%). In contrast, no case with this mutation was found in Russia, Spain, United States, and Bolivia. Among the HBV deletion mutations, 15.5% (11 of 71) occurred in the pre-S1 and 46.5% (33 of 71) in the pre-S2 regions. Eight (11.3%) cases had a mutation in both the pre-S1 and pre-S2 regions. In addition, a point mutation at the pre-S2 starting codon was observed in 19 (26.7%) cases. The detection rate of the HBV mutant in patients with hepatocellular carcinoma was significantly higher than in other patients (P < 0.05). Furthermore, these mutants were found more frequently in genotype B (25%) and genotype C (24.5%) than in the other genotypes (P < 0.05). Our results indicated that there was a high prevalence of HBV pre-S mutation in regions of endemic HBV infection in Asia. Furthermore, the pre-S mutation appeared to be correlated with hepatocellular carcinoma and HBV genotypes.

Published

2003

23. Single-cell analysis of covalently closed circular DNA copy numbers in a hepadnavirus-infected liver.

Author

Zhang YY, Zhang BH, Theele D, Litwin S, Toll E, and Summers J

Subjects

Animals, Base Sequence, Cell Nucleus virology, DNA, Circular genetics, DNA, Viral genetics, Ducks, Female, Gene Dosage, Hepatitis B Virus, Duck genetics, Interferon-alpha genetics, Liver virology, Polymerase Chain Reaction, DNA, Circular analysis, DNA, Viral analysis, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck isolation & purification, Hepatitis, Viral, Animal virology

Abstract

Hepatitis B virus (hepadnavirus) infections are maintained by the presence of a small and regulated number of episomal viral genomes [covalently closed circular DNA (cccDNA)] in the nuclei of infected cells. Although a number of studies have measured the mean copy number of cccDNA molecules in hepadnaviral-infected cells, the distribution of individual copy numbers have not been reported. Using a PCR-based assay, we examined the number of cccDNA molecules of the duck hepatitis B virus in single nuclei isolated from the liver of a chronically infected duck over the course of 131 days of infection. Nuclei were isolated from frozen serial biopsies and individually deposited into PCR microplates by flow sorting. Each nucleus was assayed by nested PCR for cccDNA and for cellular IFN-alpha genes as an internal control. We found that 90% of the nuclei assayed contained between 1 and 17 cccDNA molecules, with the remaining 10% containing more (90% confidence), and that differences in the mean number of copies and distribution of copy numbers occurred within the same animal at different times postinfection. Overall, the data suggest (i) that the number of cccDNA molecules per cell may fluctuate over time, and (ii) that, according to these fluctuations, a substantial fraction of cells may contain only one or a few copies. We infer from the results that infected hepatocytes express virus at different levels and that during cell division it is possible to segregate cells containing no cccDNA.

Published

2003

24. Detection of duck hepatitis B virus DNA on filter paper by PCR and SYBR green dye-based quantitative PCR.

Author

Wang CY, Giambrone JJ, and Smith BF

Subjects

Animals, Base Sequence, DNA Primers genetics, Fluorescent Dyes, Hepadnaviridae Infections virology, Hepatitis B virus genetics, Hepatitis, Viral, Animal virology, Humans, Models, Biological, DNA, Viral genetics, DNA, Viral isolation & purification, Ducks virology, Hepatitis B Virus, Duck genetics, Hepatitis B Virus, Duck isolation & purification, Polymerase Chain Reaction methods

Abstract

Duck hepatitis B virus (DHBV) belongs to the Hepadnaviridae family, which includes human Hepatitis B virus (HBV) and Woodchuck hepatitis virus. It is widely distributed in wild and domestic ducks due to congenital transmission. HBV is a worldwide health problem, with carriers at risk of developing cirrhosis and liver cancer. Medical staff and scientists working with HBV must be vaccinated because of its contagious nature. DHBV is a safe surrogate for HBV because of their similarities. Collection of serum and blood samples on filter paper has been used to screen for metabolic disorders, genetic diseases, and viral infection and for evolutionary studies of the genome. In this study, DHBV from serum and blood dried on filters was detected by PCR. A 0.1-microl sample was sufficient for detection. The immobilization potential of filter papers for DHBV was examined, and the highest yield of PCR products was observed with Whatman paper. Dried serum was stable under different storage temperatures for 4 weeks, but the yields of PCR products decreased when the temperature was >or=4 degrees C. The optimal condition for storage was -70 degrees C. A newly developed quantitative PCR based on monitoring the amplification by measuring the increase in fluorescence caused by the binding of SYBR green dye to double-stranded products was applied herein. DHBV genomic DNA cloned in a plasmid was used for the generation of standard DHBV DNA for quantitative PCR. It validated results from PCR in terms of the copy number of DHBV particles. The specificity of PCR was demonstrated by melting curve analysis, and the differentiation of two DHBV isolates amplified from dried serum was demonstrated based on their melting temperatures determined by GC contents and sequence. It was easier and simpler than other PCR-based DNA techniques. The use of serum dried on filters allows samples from distant field for which cold storage and transportation are a problem to be mailed to the diagnostic laboratory. Samples can be archived for comparison and used as a source of DNA for cloning and sequencing.

Published

2002

25. A quantitative competitive PCR assay for the covalently closed circular form of the duck hepatitis B virus.

Author

Addison WR, Wong WW, Fischer KP, and Tyrrell DL

Subjects

Animals, Biopsy, Blotting, Southern, Ducks, Hepatitis B Virus, Duck genetics, Liver virology, Reproducibility of Results, Sensitivity and Specificity, DNA, Circular analysis, DNA, Viral analysis, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck isolation & purification, Polymerase Chain Reaction methods

Abstract

A crucial step in the establishment and maintenance of a hepadnavirus infection is the formation of a pool of covalently closed circular viral genomes in the nucleus. Changes in the size of this pool occur when an infection is established, when acute infections are resolved, and when chronic infections are treated with antiviral drugs. However, the lack of a quantitative assay for the cccDNA form of the virus has hampered study of the biology of this replication intermediate. In response to this need we have devised a sensitive and accurate competitive PCR assay that is highly selective for the cccDNA form of the duck hepatitis B virus. Since only small amounts of DNA are needed for the assay, cccDNA pool sizes can be monitored in live animals using DNA derived from needle biopsies of infected liver.

Published

2000

26. The majority of duck hepatitis B virus reverse transcriptase in cells is nonencapsidated and is bound to a cytoplasmic structure.

Author

Yao E, Gong Y, Chen N, and Tavis JE

Subjects

Animals, Blotting, Western, Cell Fractionation, Chickens, Detergents pharmacology, Ducks, Fluorescent Antibody Technique, Hepadnaviridae Infections enzymology, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck isolation & purification, Liver enzymology, Liver virology, Microscopy, Confocal, Poultry Diseases enzymology, Precipitin Tests, RNA-Directed DNA Polymerase isolation & purification, Sodium Dodecyl Sulfate pharmacology, Tumor Cells, Cultured, Capsid metabolism, Cytoplasm virology, Hepadnaviridae Infections veterinary, Hepatitis B Virus, Duck metabolism, Poultry Diseases virology, RNA-Directed DNA Polymerase metabolism

Abstract

The hepadnavirus reverse transcriptase binds cotranslationally to the viral pregenomic RNA. This ribonucleoprotein complex is then encapsidated into nascent viral core particles, where the reverse transcriptase copies the viral RNA into DNA. Here we report that 75% of the duck hepatitis B virus reverse transcriptase present in transfected LMH cells does not follow this well-known pathway but rather exists in the cell separate from the core protein or nucleocapsids. The nonencapsidated reverse transcriptase is also abundant in infected duck liver. The nonencapsidated reverse transcriptase exists as a complex set of isoforms that are most likely produced by posttranslational modification. Interestingly, only the smallest of these isoforms is encapsidated into viral core particles. The nonencapsidated reverse transcriptase is bound to a large cellular cytoplasmic structure(s) in a detergent-sensitive complex. The cellular distribution of the reverse transcriptase only partially overlaps that of the core protein, and this distribution is unaffected by blocking encapsidation. These observations raise the possibilities that the metabolic fate of the reverse transcriptase may be posttranscriptionally regulated and that the reverse transcriptase may have roles in the viral replication cycle beyond its well-known function in copying the viral genome.

Published

2000

27. Low dynamic state of viral competition in a chronic avian hepadnavirus infection.

Author

Zhang YY and Summers J

Subjects

Animals, Chronic Disease, Ducks, Hepatitis B Virus, Duck genetics, Hepatitis B Virus, Duck isolation & purification, Hepatitis B Virus, Duck physiology, Mathematical Computing, Mutagenesis, Virus Replication, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck growth & development

Abstract

The dynamic state of infection of 11 ducks with the duck hepatitis B virus was investigated. Chronic infections were established in newly hatched ducklings by inoculation with a mixture of wild-type virus and a mutant virus with a partial replication defect. As expected, the wild-type virus was rapidly enriched in the virus population during the spread of infection. Enrichment thereafter was correlated with normal growth of the liver, with the average mutant-to-wild-type ratio stabilizing for at least 2 months beyond the time at which the liver mass stabilized. Using experimentally determined growth rates for the mutant and wild-type viruses, we estimated that after the spread of infection, competition between the two virus strains was limited by the amount of replication required to infect new hepatocytes in the growing livers. The results suggest that, in a chronically infected liver, the selection of variants with a replication rate advantage is inefficient and that the emergence of such variants would depend on induced liver cell turnover, such as that occurring during chronic hepatitis.

Published

2000

28. An in vitro system for the enzymological analysis of avian hepatitis B virus replication and inhibition in core particles.

Author

Urban S and Tyrrell DL

Subjects

Animals, Chromatography, Agarose, Chromatography, Gel, Detergents, Ducks, Hepatitis B Virus, Duck enzymology, Hepatitis B Virus, Duck isolation & purification, RNA-Directed DNA Polymerase metabolism, Time Factors, Viral Core Proteins isolation & purification, Virus Replication, Hepatitis B Virus, Duck chemistry, RNA-Directed DNA Polymerase chemistry, Viral Core Proteins chemistry

Abstract

A detailed analysis of the hepatitis B virus (HBV) replication reaction is important both in understanding viral biology and in developing effective antiviral drugs. This can best be achieved by studying the viral reverse transcriptase (RT) in its natural context, encapsidated within viral core particles in a multiprotein complex, rather than as an isolated enzyme. In order to facilitate a precise enzymological analysis of the avian HBV-RT reaction and its inhibition within replicating cores, a scheme for the purification and analysis of intracellular core particles derived from infected liver tissue has been devised, optimized and evaluated. The purification scheme itself is simple and rapid, and results in preparations with a 25-fold increase in endogenous polymerase activity that persists for over 5 h under assay conditions. In order to assess the suitability of these preparations for mechanistic studies, a thorough evaluation of purity was undertaken, revealing predominantly pure viral protein and nucleic acid, free of contaminating cellular polymerases and phosphatase activities that potently degrade nucleotides and antiviral drugs. Parameters governing optimal polymerase activity have been determined, and an assay for DHBV-RT activity has been developed which offers the highest purity and specific polymerase activity currently available to study hepadnaviral replication and inhibition.

Published

2000

29. Evaluation of disinfection and sterilization of reusable angioscopes with the duck hepatitis B model.

Author

Chaufour X, Deva AK, Vickery K, Zou J, Kumaradeva P, White GH, and Cossart YE

Subjects

Animals, Cross Infection prevention & control, DNA, Viral analysis, Disease Models, Animal, Ducks, Jugular Veins virology, Sterilization, Angioscopes, Angioscopy adverse effects, Disinfection, Hepatitis B Virus, Duck isolation & purification, Liver virology

Abstract

Purpose: Nosocomial transmission of viral hepatitis and retrovirus infection has been reported. The expected risk is greatest for the hepatitis B virus (HBV). The duck HBV (DHBV) has similar biologic and structural characteristics to HBV and has been adopted as a suitable model for disinfectant testing., Methods: Angioscopic examination of the external jugular vein was performed on DHBV-infected ducks. After use, the instrument was air dried for 3 minutes. Samples were obtained by flushing the channel with 5 mL of phosphate buffered saline solution. The samples were collected immediately after drying (control), after flushing with 5 mL of water, after glutaraldehyde disinfection for 5, 10, and 20 minutes, and after ethylene oxide gas sterilization. Angioscopes were either precleaned or uncleaned before disinfection/sterilization. Residual infectivity was assessed with inoculation of samples into the peritoneal cavity of day-old ducks (n = 231)., Results: DNA analysis results of liver samples showed that all 38 control ducks became infected. The frequency of DHBV infection was reduced to 93% (14 of 15) by flushing the angioscope with 5 mL of sterile water. No transmission occurred after the use of any of the properly precleaned and disinfected/sterilized angioscopes. However, after the use of the uncleaned angioscopes, the transmission rate was 90% (9 of 10) and 70% (7 of 10) after 5 and 10 minutes of contact time, respectively, in 2% glutaraldehyde. Even after the recommended 20 minutes of contact time, there was still 6% (2 of 35) transmission. After ethylene oxide sterilization, two of the recipient ducklings (2 of 35) were infected with DHBV., Conclusion: There was no disease transmission after reuse of disposable angioscopes adequately cleaned before disinfection or sterilization. However, if the angioscopes are inadequately cleaned, DHBV can survive despite glutaraldehyde disinfection or ethylene oxide sterilization. This contrasts with previous in vitro and in vivo data with solid surgical instruments. It is postulated that the presence of a narrow lumen or residual protein shielding within the lumen may compromise effective inactivation of hepadnaviruses on angioscopes, with the potential risk for patient-to-patient transmission.

Published

1999

30. Inactivation of duck hepatitis B virus by a hydrogen peroxide gas plasma sterilization system: laboratory and 'in use' testing.

Author

Vickery K, Deva AK, Zou J, Kumaradeva P, Bissett L, and Cossart YE

Subjects

Animals, Ducks, Equipment Contamination, Hepadnaviridae Infections transmission, Hepatitis B Virus, Duck isolation & purification, Cross Infection prevention & control, Disinfectants, Hepadnaviridae Infections prevention & control, Hepatitis B Virus, Duck physiology, Hydrogen Peroxide, Sterilization methods

Abstract

Human hepatitis B virus (HBV) is an important cause of nosocomial infections and can be transmitted by contaminated instruments. However, tests of the efficacy of sterilization of materials and equipment contaminated by HBV are difficult to perform because the virus cannot be cultured in the laboratory. In this study, we aimed to evaluate the capability of a low temperature, hydrogen peroxide gas plasma sterilizer (Sterrad, Advanced Sterilization Products, Irvine California,) to inactivate duck hepatitis B virus (DHBV). In laboratory efficacy studies using DHBV dried on to glass filter carriers and exposed to one-half of the hydrogen peroxide gas plasma sterilization process, there was a 10(7) or greater decrease in the viral titer, with no infectivity detected on the carriers after treatment. In-use studies were performed using a laparoscope that was experimentally contaminated with DHBV to mimic the possible transmission of infection between successive patients. Following exposure to the hydrogen peroxide gas plasma sterilization process no transmission of DHBV infection from the laparoscope occurred despite obvious visual soiling with blood (N = 8) while the transmission rate for the unprocessed laparoscope (positive control) was 100% (26/26), and that for instruments after a water wash was 63% (7/11). In conclusion the hydrogen gas plasma sterilization process completely inactivates DHBV a representative of the hepadna group of viruses.

Published

1999

31. Treatment of duck hepatitis B virus by antisense poly-2'-O-(2,4-dinitrophenyl)-oligoribonucleotides.

Author

Xin W and Wang JH

Subjects

Animals, Antiviral Agents chemical synthesis, Base Sequence, DNA Primers, Ducks, Hepatitis B Virus, Duck genetics, Hepatitis B Virus, Duck isolation & purification, Liver pathology, Nitrobenzenes chemical synthesis, Oligoribonucleotides chemical synthesis, Polymerase Chain Reaction, Reverse Transcriptase Inhibitors chemical synthesis, Reverse Transcriptase Inhibitors therapeutic use, Viremia drug therapy, Antiviral Agents therapeutic use, Hepadnaviridae Infections drug therapy, Nitrobenzenes therapeutic use, Oligoribonucleotides therapeutic use

Abstract

The poly-2'-O-(2,4-dinitrophenyl)-oligoribonucleotide (poly-DNP-RNA) with antisense sequence 5'ggguguauggaaaagccguc-3' was designed to target the sequence 2468-2487 in the polymerase gene of duck hepatitis B virus (DHBV). The stereochemically pure RNA was synthesized by using T7 RNA polymerase with synthetic DNA template and subsequently derivatized with 2,4-dinitrofluorobenzene in mild basic conditions to make the poly-DNP-RNA with an average DNP/base ratio of 0.7. In vitro studies showed that this antisense poly-DNP-RNA can hybridize with sense DNA and has high resistance to RNase A digestion. These poly-DNP-RNA were also found to be potent sequence-independent inhibitors of the reverse transcriptase activity of DHBV DNA-polymerase. For in vivo studies, DHBV-infected ducks were treated with antisense, sense, and random noncomplementary sequence poly-DNP-RNA, respectively. The data showed that the antisense poly-DNP-RNA completely inhibited the duck viremia in all nine ducks that had been treated with a dose of 1 mg/kg (i.v.) per day for 25 days. The viremia did not come back after 10 months recession. In the sense group, three of the four ducks showed no inhibition, and in the random group, both ducks maintained their viremia. After 45 days of treatment with the antisense poly-DNP-RNA, followed by 2 weeks of recession, PCR as well as QC-PCR assay and microscopic examination showed that viral DNA had disappeared in liver and that the histology of the damaged liver (filled with fat granules) had returned to normal.

Published

1998

32. Characterization of age- and dose-related outcomes of duck hepatitis B virus infection.

Author

Jilbert AR, Botten JA, Miller DS, Bertram EM, Hall PM, Kotlarski J, and Burrell CJ

Subjects

Age Factors, Animals, Animals, Newborn, DNA, Viral blood, DNA, Viral isolation & purification, Disease Models, Animal, Ducks, Hepadnaviridae Infections pathology, Hepadnaviridae Infections virology, Hepatitis Antibodies blood, Hepatitis Antigens blood, Hepatitis Antigens isolation & purification, Hepatitis B Virus, Duck isolation & purification, Hepatitis, Chronic etiology, Hepatitis, Chronic pathology, Hepatitis, Chronic virology, Liver pathology, Liver virology, Viremia etiology, Viremia virology, Virulence, Hepadnaviridae Infections etiology, Hepatitis B Virus, Duck pathogenicity

Abstract

Experimental inoculation of naive ducks with duck hepatitis B virus (DHBV) can lead to one of three outcomes, namely, persistent viremia, transient infection with or without viremia, or no evidence of infection. The ability of individual ducks to resolve DHBV infection was found to be linked to the age of the duck at the time of inoculation and the dose of inoculated virus. (1) In recently hatched ducks inoculated intravenously (i.v.) with 4 x 10(4) DHBV DNA genomes, a switch from persistent viremia to transient antibody appearance was seen at an age of inoculation between 7 and 14 days. A 25-fold increase in the dose of virus (1 x 10(6) DHBV genomes) delayed this switch by 7 days. (2) When 4-month-old ducks were inoculated i.v. with different doses of virus, only those receiving the highest dose (2 x 10(11) DHBV genomes) showed viremia and extensive viral replication and histological changes in the liver; 2/3 ducks in this group had a transient infection, while the third duck had viral replication and histological changes in the liver that were still present at day 120 postinoculation (p.i.). In all ducks receiving lower doses (1 x 10(3), 1 x 10(6), 1 x 10(9) DHBV genomes) antibodies to viral surface and core antigens developed without detectable viral replication in the liver on days 6, 9, or 12 p.i. (3) When 10- to 16-month-old ducks were inoculated i.v. with 2 x 10(11) DHBV genomes, all showed extensive viral replication in hepatocytes and mild to moderate histological changes in the liver on days 4 or 6 p.i. In 4/5 ducks viremia was not detected, anti-surface antibodies were first detected on day 8 p.i., and viral DNA and antigen were cleared from the liver by days 35-47 p.i. The remaining duck became viremic with persistence of virus in the liver until at least day 46 p.i. The findings of the study are consistent with a model for noncytopathic viruses (R. M. Zinkernagel (1996) Science 271, 173-178).

Published

1998

33. Quantification of infectious duck hepatitis B virus by radioimmunofocus assay.

Author

Anderson DA, Grgacic EV, Luscombe CA, Gu X, and Dixon R

Subjects

Animals, Antibodies, Monoclonal, Cell Count, Cells, Cultured, DNA, Viral isolation & purification, Ducks, Evaluation Studies as Topic, Hepatitis B Virus, Duck immunology, Hepatitis B Virus, Duck pathogenicity, Radioimmunoassay statistics & numerical data, Sensitivity and Specificity, Virology statistics & numerical data, Hepatitis B Virus, Duck isolation & purification, Radioimmunoassay methods, Virology methods

Abstract

A simple method is described for the precise quantification of infectious duck hepatitis B virus (DHBV) in cell culture, using a radioimmunofocus assay (RIFA). Primary duck hepatocyte cell cultures were infected with serial dilutions of viral samples as for a plaque assay, but then maintained with liquid overlay medium. After incubation for up to 14 days, cell monolayers were fixed with acetone, then stained with a monoclonal antibody to DHBV L protein followed by secondary antibody labelled with 125I. Foci of infection (representing individual infectious particles in the inoculum) were detected by autoradiography. The number of foci recovered was increased by addition of dimethyl sulphoxide to culture medium, but was not appreciably altered by the use of semi-solid medium. The titre of virus suspensions determined by RIFA correlated well with titration in ducklings. The RIFA is a useful method for titration of DHBV, as it has a wide dynamic range and is well suited to parallel titration of large numbers of samples. This assay will have wide use for the analysis of DHBV growth kinetics, antiviral efficacy, and virus inactivation procedures.

Published

1997

34. Demonstration of duck hepatitis B virus in bile duct epithelial cells: implications for pathogenesis and persistent infection.

Author

Nicoll AJ, Angus PW, Chou ST, Luscombe CA, Smallwood RA, and Locarnini SA

Subjects

Animals, Animals, Newborn, Biomarkers, DNA, Viral analysis, Ducks, Epithelium virology, In Situ Hybridization, Liver metabolism, Liver pathology, Proliferating Cell Nuclear Antigen metabolism, Bile Ducts, Intrahepatic virology, Hepatitis B Virus, Duck isolation & purification

Abstract

Hepatitis B virus (HBV) has been demonstrated in bile duct epithelial cells (BDEC) during chronic infection. The persistence of virus in BDEC may play an important role in disease pathogenesis, and may be at least partly responsible for the relapse phenomenon observed in antiviral treatments using nucleoside analogues. The aims of this study were to examine the morphological changes within the liver in the duck hepatitis B model following bile duct ligation (BDL), and to assess the effect of biliary hyperplasia upon viral DNA and proteins. Seven-day-old ducklings, congenitally infected with the duck hepatitis B virus (DHBV), were subject to BDL. The pathological and virological changes were then followed at 5, 10, 15, and 20 days after ligation. All results were compared with age-matched unligated control birds congenitally infected with DHBV. To assess the early morphological changes, additional animals were sacrificed at 1, 2, 3, and 4 days post-BDL. The proportion of DHBV-infected BDEC, was examined by immunohistochemistry and in situ hybridization. BDL induced rapid biliary hyperplasia, with a doubling time for BDEC of 1.3 days. The proliferated BDEC displayed immunohistochemical features identical to resting BDEC. More than 50% of BDEC in unligated controls, and more than 46% of proliferated BDEC in ligated animals were positive for DHBV DNA and structural proteins. The intensity of immunohistochemical staining and in situ hybridization signal in the BDEC was consistently greater than that of the hepatocytes, both before and after BDL. BDL induces biliary hyperplasia in the duck model, and BDEC division does not reduce the viral burden in infected cells.

Published

1997

35. Preparations of duck hepatitis B virions contain multiple DNA polymerase activities.

Author

Oberhaus SM and Newbold JE

Subjects

Animals, DNA-Directed DNA Polymerase chemistry, Ducks virology, Hepadnaviridae Infections blood, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck isolation & purification, Viral Proteins chemistry, Virion metabolism, DNA-Directed DNA Polymerase metabolism, Hepatitis B Virus, Duck enzymology, Viral Proteins metabolism

Abstract

The hepadnaviral DNA genome is synthesized by a viral-encoded reverse transcriptase, but the nature of this protein(s) in vivo remains obscure. We have previously described studies in which activity gel assays identified multiple DNA polymerase (DNAp) activities associated with highly purified duck hepatitis B virus (DHBV) core particles. We now report that virions isolated from viremic sera are associated with DNA-dependent DNAp activities which are nearly identical to major DNAp activities detected with highly purified DHBV core particles. These results suggest that the virion-associated polymerases are the same as those which are detected with core particles and are likely to represent DHBV pol gene products involved in replication of the genome.

Published

1996

36. In situ DNA polymerase and RNase H activity gel assays as applied to hepadnavirus particles.

Author

Oberhaus SM and Newbold JE

Subjects

Animals, Bird Diseases, DNA-Directed DNA Polymerase isolation & purification, DNA-Directed DNA Polymerase metabolism, Ducks, Electrophoresis, Polyacrylamide Gel methods, Hepadnaviridae physiology, Hepadnaviridae Infections veterinary, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck isolation & purification, Indicators and Reagents, Liver virology, Molecular Weight, Phosphorus Radioisotopes, RNA-Directed DNA Polymerase isolation & purification, RNA-Directed DNA Polymerase metabolism, Radioisotope Dilution Technique, Ribonuclease H isolation & purification, Ribonuclease H metabolism, Substrate Specificity, Ultracentrifugation methods, Virion enzymology, Virion isolation & purification, Virus Replication, DNA-Directed DNA Polymerase analysis, Hepadnaviridae enzymology, Hepatitis B Virus, Duck enzymology, RNA-Directed DNA Polymerase analysis, Ribonuclease H analysis

Published

1996

37. Detection of an RNase H activity associated with hepadnaviruses.

Author

Oberhaus SM and Newbold JE

Subjects

Animals, Blotting, Southern, DNA, Viral analysis, Ducks, Geese, Hepadnaviridae isolation & purification, Hepadnaviridae Infections blood, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck isolation & purification, Kinetics, Liver virology, Magnesium pharmacology, Manganese pharmacology, Ribonuclease H analysis, Ribonuclease H isolation & purification, Viremia blood, Viremia virology, DNA-Directed DNA Polymerase metabolism, Hepadnaviridae enzymology, Hepatitis B Virus, Duck enzymology, RNA-Directed DNA Polymerase metabolism, Ribonuclease H metabolism

Abstract

Replication of the hepadnavirus DNA genome is accomplished via reverse transcription of an intermediate, pregenomic RNA molecule. This process is likely to be carried out by a virally encoded, multifunctional polymerase which possesses DNA- and RNA-dependent DNA polymerase and RNase H activities. However, the nature of the product(s) of the polymerase gene predicted to mediate these functions is unclear. Biochemical studies of the polymerase protein(s) have been limited by its apparent low abundance in virus particles and, until recently, the inability to express active polymerase protein(s) heterologously. We have used activity gel assays to detect DNA- and RNA-dependent DNA polymerase activities associated with highly purified duck hepatitis B virus (DHBV) core particles (S. M. Oberhaus and J. E. Newbold, J. Virol. 67:6558-6566, 1993). Now we report that the same approach identifies a 35-kDa RNase H activity in association with highly purified DHBV core particles and crude preparations of virions from DHBV-infected ducks and woodchuck hepatitis virus-infected woodchucks. This is the first report of the detection of an hepadnavirus-associated RNase H activity. Its apparent size is smaller than any of the DNA polymerase activities that we detected previously and significantly smaller than the full-length protein predicted from the polymerase open reading frame (p85 for DHBV). These data suggest that the viral polymerase and RNase H activities are separable and that these enzymes may coordinate their activities in vivo by forming a complex.

Published

1995

38. Evidence that hepatocyte turnover is required for rapid clearance of duck hepatitis B virus during antiviral therapy of chronically infected ducks.

Author

Fourel I, Cullen JM, Saputelli J, Aldrich CE, Schaffer P, Averett DR, Pugh J, and Mason WS

Subjects

Animals, Antigens, Viral blood, Antiviral Agents pharmacology, Biopsy, Bromodeoxyuridine, DNA Replication drug effects, DNA, Viral analysis, DNA, Viral biosynthesis, DNA, Viral blood, Deoxyguanosine pharmacology, Deoxyguanosine therapeutic use, Ducks, Emtricitabine analogs & derivatives, Hepadnaviridae Infections metabolism, Hepadnaviridae Infections pathology, Hepatitis B Virus, Duck drug effects, Hepatitis B Virus, Duck isolation & purification, Kinetics, Liver metabolism, Liver pathology, Time Factors, Zalcitabine pharmacology, Zalcitabine therapeutic use, Antiviral Agents therapeutic use, Deoxyguanosine analogs & derivatives, Hepadnaviridae Infections drug therapy, Hepatitis B Virus, Duck physiology, Liver virology, Virus Replication drug effects, Zalcitabine analogs & derivatives

Abstract

Duck hepatitis B virus (DHBV) DNA synthesis in congenitally infected ducks is inhibited by 2'-deoxycarbocyclic guanosine (2'-CDG). Three months of therapy reduces the number of infected hepatocytes at least 10-fold (W.S. Mason, J. Cullen, J. Saputelli, T.-T. Wu, C. Liu, W.T. London, E. Lustbader, P. Schaffer, A.P. O'Connell, I. Fourel, C.E. Aldrich, and A.R. Jilbert, Hepatology 19:393-411, 1994). The present study was performed to determine the kinetics of disappearance of infected hepatocytes and to evaluate the role of hepatocyte turnover in this process. Essentially all hepatocytes were infected before drug therapy. Oral treatment with 2'-CDG resulted in a prompt reduction in the number of infected hepatocytes. After 2 weeks, only 30 to 50% appeared to still be infected, and less than 10% were detectably infected after 5 weeks of therapy. To assess the possible role of hepatocyte turnover in these changes, 5-bromo-2'-deoxyuridine (BUdR) was administered 8 h before liver biopsy to label host DNA in hepatocytes passing through S phase, and stained nuclei were detected in tissue sections by using an antibody reactive to BUdR. The extent of nuclear labeling after 5 weeks was the same as that before therapy (ca. 1%). However, biopsies taken after 2 weeks of therapy showed a ca. 10-fold elevation in the number of nuclei labeled with BUdR. This result suggested that a rapid clearance of infected hepatocytes by 2'-CDG was caused not just by the inhibition of viral replication but also by an acceleration of the rate of hepatocyte turnover. To test this possibility further, antiviral therapy was carried out with another strong inhibitor of DHBV DNA synthesis, 5-fluoro-2',3'-dideoxy-3'-thiacytidine (524W), which did not accelerate hepatocyte turnover in ducks. 524W administration led to a strong inhibition of virus production but to a slower rate of decline in the number of infected hepatocytes, so that ca. 50% (and perhaps more) were still infected after 3 months of therapy. In addition, histopathologic evaluation of 2'-CDG-treated ducks revealed liver injury, especially at the start of therapy. No liver damage was observed during 524W therapy. These results imply that clearance of infected hepatocytes from the liver is correlated with hepatocyte turnover. Thus, in the absence of immune clearance or other sources for the accelerated elimination of infected hepatocytes, inhibitors of virus replication would have to be administered for a long period to substantially reduce the burden of infected hepatocytes in the liver.

Published

1994

39. Characterisation of the Indian strain of duck hepatitis B virus (DHBV) and development of a carrier duck colony for antiviral drug testing.

Author

Munshi A, Mehrotra R, and Panda SK

Subjects

Animals, Base Sequence, Ducks, Genome, Viral, Molecular Sequence Data, Antiviral Agents pharmacology, Hepadnaviridae Infections drug therapy, Hepatitis B Virus, Duck drug effects, Hepatitis B Virus, Duck genetics, Hepatitis B Virus, Duck isolation & purification

Abstract

Duck hepatitis B virus (DHBV) infected carrier ducks serve as a useful model for testing anti-hepadnavirus drugs. This needs a well characterised duck hepatitis B virus strain. We cloned and sequenced the complete genome of duck hepatitis B virus strain of Indian origin. It was 3021 nucleotides in length and had all the recognisable open reading frames (Polymerase: 20-2530 nucletides, Surface: 693-1787 nucleotides and Core: 2518-412). Using an inoculum of 50 microliters serum containing 1 x 10(11) virus particles/ml, we could infect 80% of one day old ducklings and develop a duck colony.

Published

1994

40. Oral famciclovir against duck hepatitis B virus replication in hepatic and nonhepatic tissues of ducklings infected in ovo.

Author

Tsiquaye KN, Slomka MJ, and Maung M

Subjects

2-Aminopurine administration & dosage, 2-Aminopurine pharmacology, 2-Aminopurine therapeutic use, Acyclovir analogs & derivatives, Acyclovir metabolism, Acyclovir pharmacology, Acyclovir therapeutic use, Administration, Oral, Animals, Animals, Newborn, Antiviral Agents administration & dosage, Antiviral Agents pharmacology, Biotransformation, DNA, Viral analysis, Disease Models, Animal, Ducks embryology, Eggs, Famciclovir, Guanine, Hepadnaviridae Infections drug therapy, Hepadnaviridae Infections embryology, Hepadnaviridae Infections microbiology, Hepadnaviridae Infections transmission, Hepatitis B Virus, Duck isolation & purification, Hepatitis B Virus, Duck physiology, Kidney microbiology, Liver embryology, Liver enzymology, Organ Specificity, Pancreas microbiology, Poultry Diseases embryology, Poultry Diseases microbiology, Poultry Diseases transmission, Prodrugs administration & dosage, Prodrugs pharmacology, Spleen microbiology, Viremia drug therapy, Viremia microbiology, Viremia transmission, Xanthine Oxidase metabolism, 2-Aminopurine analogs & derivatives, Antiviral Agents therapeutic use, DNA, Viral isolation & purification, Ducks microbiology, Hepadnaviridae Infections veterinary, Hepatitis B Virus, Duck drug effects, Liver microbiology, Poultry Diseases drug therapy, Prodrugs therapeutic use, Viremia veterinary, Virus Replication drug effects

Abstract

Detection of hepadnaviral DNA in extrahepatic tissues of human and animal models of hepatitis B virus (HBV) has raised the question of whether virus replication in organs other than the liver could be targeted for the treatment of chronic hepatitis B. Since duck hepatitis B virus (DHBV) replication is dynamic in the liver, kidney, pancreas, and spleen of newly hatched ducklings infected in ovo, we used the duck model and the new antiherpesvirus agent, famciclovir (FCV), to determine whether antiviral effect of nucleoside analogues on DHBV replication is pluripotential. Day-old ducklings hatched from eggs laid by a DHBV-carrier duck were bled and administered FCV (25 mg/kg/bd) orally for periods of 1, 2, 3, 6, 9, and 12 days. Seventeen (17) hours after the last dose of each regimen the duckling(s) was bled and postmortem samples of liver, kidney, pancreas, and spleen were snap-frozen and stored at -70 degrees C. Analysis of plasma samples of ducklings treated for 2 days and longer by dot-blot hybridisation showed that levels of DHBV DNA were reduced significantly compared to levels in samples collected before treatment begun. Southern blot hybridisation of tissue DNA corroborated these results and showed that DHBV DNA replicative intermediates in all the tissues examined were reduced to levels that reflected the amount of virus released into the blood of each treated duckling. It is concluded from these results that if antiviral agents could be transformed to active metabolites in any infected tissues including the liver, replication of hepadnaviruses would be inhibited.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1994

41. Dot blot hybridization assay for the detection of duck hepatitis B virus DNA among healthy Indian country ducks.

Author

Valliammai T, Sridhar G, Thyagarajan SP, Ramakrishnan J, Gopal KV, Harrison TJ, and Jayaraman K

Subjects

Animals, India, Nucleic Acid Hybridization, DNA, Viral blood, Ducks microbiology, Hepatitis B Virus, Duck genetics, Hepatitis B Virus, Duck isolation & purification

Abstract

A DNA molecular hybridization technique employing Duck Hepatitis B Virus (DHBV) DNA of 3.0 kilobase pairs as a probe was used to screen for the presence of DHBV DNA in blood samples, collected from 90 apparently healthy Indian country ducks. Six out of 90 ducks showed positivity for DHBV DNA in serum (5.4%) and only 4 out of 6 DHBV DNA positive ducks answered in Counter Immuno Electrophoresis (CIEP) using specific antibody against DHBV surface antigen raised in Guinea pig. The results indicate the pilot observation that (a) DHBV carrier status exists to a tune of 5.4% among apparently healthy Indian country ducks also and (b) DHBV probe can be employed as a sensitive and reliable assay for DHBV DNA detection in DHBV infected ducks.

Published

1994

42. Duck hepatitis B virus (DHBV) infection in Indian domestic ducks: a pilot study.

Author

Sridhar G, Valliammai T, Varalakshmi CS, Udayasankar K, Panchanadam M, Ramakrishna J, Gopal KV, Jayaraman K, and Thyagarajan SP

Subjects

Animals, Antigens, Surface blood, Antigens, Viral blood, Carcinoma, Hepatocellular etiology, Carcinoma, Hepatocellular veterinary, Counterimmunoelectrophoresis veterinary, DNA, Viral blood, Enzyme-Linked Immunosorbent Assay veterinary, Female, Hepadnaviridae Infections complications, Hepadnaviridae Infections diagnosis, Hepadnaviridae Infections epidemiology, Hepatitis B Surface Antigens immunology, Hepatitis B Virus, Duck genetics, Hepatitis B Virus, Duck immunology, India epidemiology, Liver pathology, Liver Cirrhosis etiology, Liver Neoplasms etiology, Liver Neoplasms veterinary, Nucleic Acid Hybridization, Pilot Projects, Poultry Diseases diagnosis, Ducks, Hepadnaviridae Infections veterinary, Hepatitis B Virus, Duck isolation & purification, Poultry Diseases epidemiology

Abstract

One hundred and two apparently healthy Indian domestic ducks from the Poultry Research Station, Madras were screened for duck hepatitis B virus (DHBV) infection by; 1. screening for the duck hepatitis B virus surface antigen (DHBsAg) in their sera using hepatitis B virus (HBV) reagents, 2. screening for DHBsAg using specific duck hepatitis B virus (DHBV) reagents and 3. demonstration of DHBV DNA using DHBV DNA probe by dot blot hybridisation. While 5 ducks (4.9%) were consistently positive with HBV reagents, use of DHBV reagents showed a total of 4 ducks (including 3 of the above 5) to be positive for DHBsAg. DNA hybridisation showed 6 ducks to be positive for DHBV DNA. On clinical examination, 5 out of these 6 ducks did not reveal abnormalities, the other one showed hepatomegaly and ascites. Post-mortem studies showed the presence of nodules on the surface of the liver in all 5 which were positive with HBV reagents including the one with hepatomegaly. On histopathological evaluation, they were found to be hepatocellular carcinoma with or without bile duct carcinoma. The present study is a pilot report on the occurrence of DHBV infection in Indian domestic ducks and the possibility of antigenic cross reactivity between human HBV and duck hepatitis B virus antigens.

Published

1993

43. [The effects of Ara-A on viral markers in duck hepatitis B virus carrier ducks].

Author

Fukuda R, Tokuda A, Kohge N, Xuan NT, Uchida Y, Akagi S, and Fukumoto S

Subjects

Animals, Carrier State microbiology, Hepadnaviridae Infections microbiology, Hepatitis B Virus, Duck isolation & purification, Poultry Diseases microbiology, Carrier State drug therapy, DNA, Viral analysis, DNA-Directed DNA Polymerase analysis, Ducks microbiology, Hepadnaviridae Infections drug therapy, Hepatitis B Virus, Duck drug effects, Poultry Diseases drug therapy, Vidarabine therapeutic use

Abstract

Duck hepatitis B virus (DHBV) carrier ducks of one week old were injected with Ara-A (adenine arabinoside) of different dose including 2.5 (11 ducks), 5.0 (11), 10.0 (10) and 20.0 (10) mg/kg for 14 days. This antiviral effect showed dose-dependence up to 5.0 mg/kg and this dose seemed effective to obtain significant antiviral effect. Viral DNA and DNA polymerase activity were reduced significantly from the 1st week after starting the administration of Ara-A. This antiviral effect was maintained even at the 1st week after discontinuation of the drug. These findings were quite similar to those observed in HBV carriers. With the increasing necessity of Ara-A treatment in patients who will not respond to interferon therapy, DHBV seemed a suitable model for the investigation of the dose and antiviral effect of Ara-A treatment in humans.

Published

1993

44. Immuno disc assay for screening duck hepatitis B surface antigen in serum, liver tissue and cultured hepatocytes.

Author

de Wilde GA and Heijtink RA

Subjects

Animals, Blotting, Southern, Blotting, Western, Cells, Cultured, DNA, Viral analysis, Ducks blood, Ducks immunology, Hepatitis B Virus, Duck immunology, Hepatitis, Viral, Animal blood, Hepatitis, Viral, Animal microbiology, Poultry Diseases blood, Poultry Diseases microbiology, Rabbits, Sensitivity and Specificity, Viremia blood, Viremia immunology, Viremia microbiology, Antigens, Viral analysis, Ducks microbiology, Hepatitis B Virus, Duck isolation & purification, Hepatitis, Viral, Animal immunology, Immunoassay methods, Liver microbiology, Poultry Diseases immunology, Viremia veterinary

Abstract

An immuno disc assay (IDA) for semi-quantitative analysis of the surface antigen (DHBsAg) of duck hepatitis B virus (DHBV) is described. Unpurified antigen preparations were adsorbed onto punched-out nitrocellulose membrane discs. Rabbit antiserum raised against serum-derived gradient-purified DHBsAg was used for detecting the antigen. Cross-reacting antibodies in the rabbit antiserum were removed using normal duck serum and normal duck hepatocytes. The sensitivity of the IDA was compared with that of the Western blot analysis and was observed to be of the same order, but differed slightly for DHBsAg in liver and sera. In contrast to Western blot analysis, antigen specificity for the IDA included the S-protein. Immunodetection was carried out in microtitre plates, but the procedure was accelerated by attaching the antigen-adsorbed discs to an adhesive plate sealer. The IDA was exemplified for measuring DHBsAg in duck serum, duck liver homogenates and viral protein synthesis in cultures of DHBV-infected hepatocytes.

Published

1993

45. Hepatitis B viral clearance studies using duck virus model.

Author

Long Z, Sun CS, White EM, Horowitz B, and Sito AF

Subjects

Animals, Hepadnaviridae Infections microbiology, Hepatitis B Virus, Duck physiology, Hot Temperature, Humans, Pan troglodytes microbiology, Safety, Sensitivity and Specificity, Species Specificity, Biological Assay, Disease Models, Animal, Ducks microbiology, Hepatitis B Virus, Duck isolation & purification, Hepatitis B virus, Viremia microbiology, Virology methods

Abstract

We have shown data to suggest that the in vivo duck hepatitis B virus system represents an excellent animal model system for the study of hepatitis B virus. Because of the similarity of DHBV to human HBV (including comparable results in virus inactivation studies), the high level of sensitivity of the DHBV assay, and the rapidity, ease, and relative low cost of obtaining results, we propose that the in vivo DHBV titration system be used as a model for human HBV in process validation studies. Data generated in such validation studies have, in fact, been submitted by a number of blood products manufacturers to the U.S. F.D.A. in support of IND applications.

Published

1993

46. [A study of duck hepatitis B virus infection in Chinese ducklings].

Author

Leng J and Xu BD

Subjects

Age Factors, Animals, DNA, Viral analysis, DNA, Viral blood, Ducks microbiology, Liver microbiology, Hepatitis B Virus, Duck isolation & purification, Hepatitis, Viral, Animal microbiology

Abstract

Intraperitoneal inoculation of duck hepatitis B virus in three different dosages (9 x 10(7), 1.8 x 10(8), 9 x 10(8) DHBV particles) into 3 to 21 day-old Chinese ducklings provided from a DHBV free flock produced a persistent infection up to 93.3% in 60 animals. The serum and liver specimens of these ducklings were examined by DNA dot blot hybridization on the 30th day after inoculation. The results showed that: (1) examination of viral DNA in liver was more sensitive and reliable than estimation of the DNA in serum for detecting DHBV infection in inoculated ducklings; (2) the liver DHBV DNA level did not coincide with the degree of liver hepatitis induced; (3) 21-day-old Chinese ducklings were also susceptible to DHBV infection, the infection rate of this group was 100% (10/10).

Published

1992

47. Effects of 2'-fluorinated arabinosyl-pyrimidine nucleosides on duck hepatitis B virus DNA level in serum and liver of chronically infected ducks.

Author

Fourel I, Li J, Hantz O, Jacquet C, Fox JJ, and Trépo C

Subjects

Animals, Antiviral Agents pharmacology, Arabinofuranosyluracil pharmacology, Cytarabine pharmacology, DNA, Viral blood, DNA, Viral metabolism, Drug Evaluation, Preclinical, Ducks, Hepatitis B Virus, Duck isolation & purification, Hepatitis B Virus, Duck physiology, Hepatitis, Viral, Animal microbiology, Liver microbiology, Virus Replication drug effects, Arabinofuranosyluracil analogs & derivatives, Cytarabine analogs & derivatives, Hepatitis B Virus, Duck drug effects, Hepatitis, Viral, Animal drug therapy

Abstract

The 2'-fluorinated arabinosyl-pyrimidine nucleosides, 1-(2'-deoxy-2'-fluoro-beta-D-arabinofuranosyl)-5-iodocytosine (FIAC) and 1-(2'-deoxy-2'-fluoro-beta-D-arabinofuranosyl)-5-methyluracil (FMAU), are new antiviral compounds with in vitro inhibitory activity against the DNA polymerase of hepadnaviruses. Those compounds also induced permanent inhibition of viral replication in woodchucks chronically infected by woodchuck hepatitis virus. The effects of these antiviral compounds were assessed in ducks chronically infected by duck hepatitis B virus (DHBV). Following intraperitoneal administration for 5 days, FMAU (2 mg/kg/day) and FIAC (10 mg/kg/day) induced a transient decrease in DHBV replication, as shown by the decrease in both the serum and liver DHBV DNA level. After stopping therapy, DHBV replication rebounded immediately to the pretreatment level. The supercoiled form of liver viral DNA was found to be less affected by the therapy. By contrast, no obvious antiviral effect was observed with vidarabine monophosphate (ara-AMP) (80 mg/kg/day) therapy. No sign of toxicity was observed during the course of the treatment. These preliminary results confirmed in the DHBV model the higher efficacy of FIAC and FMAU as compared to ara-AMP. Pharmacokinetic studies are needed to explain the differences observed in viral replication in these 2 models of HBV infection.

Published

1992

48. Validation of virus inactivation by heat treatment in the manufacture of diaspirin crosslinked hemoglobin.

Author

Farmer M, Ebeling A, Marshall T, Hauck W, Sun CS, White E, and Long Z

Subjects

Aspirin analogs & derivatives, Cross-Linking Reagents, Cytomegalovirus isolation & purification, Drug Contamination, Evaluation Studies as Topic, HIV isolation & purification, Hepatitis B Virus, Duck isolation & purification, Hot Temperature, Humans, Blood Substitutes isolation & purification, Hemoglobins isolation & purification, Viruses isolation & purification

Abstract

Diaspirin crosslinked hemoglobin (DCLHb), a hemoglobin based oxygen carrying solution prepared from outdated human blood, is subjected to a heat treatment step to inactivate viruses in our manufacturing process. To validate the efficacy of this inactivation, we have simulated the heat treatment procedure at a reduced scale using hemoglobin solution spiked with representative viruses. Human Immuno-deficiency Virus (HIV), Cytomegalovirus (CMV), and Duck Hepatitis B Virus (DHBV) were used in this validation. Inoculation with concentrated virus was performed just prior to the heat treatment to determine the effect of that specific process step. Samples were taken before, during, and after heat treatment and assayed for virus titer in an attempt to assess the rate as well as the extent of virus inactivation. CMV was analyzed in a plaque assay using MRC-5 indicator cells. The titer was reduced from 3.3 x 10(6) plaque forming units (PFU) per mL to less than 5 x 10(1) PFU/mL (detection limit) within 30 minutes. DHBV was analyzed by inoculation of serially diluted samples into Pekin ducklings, followed at intervals by screening sera for DHBV DNA by dot blot hybridization. The titer was reduced from 5.0 x 10(6) duck infectious units (DIU) per mL to less than 5 x 10(0) DIU/mL (detection limit) within 1 hour. HIV titers were determined through an ELISA assay for p24 antigen present in peripheral blood lymphocyte cocultivation supernatants. The titer was reduced from 2.0 x 10(4) infectious units (IU) per mL to less than 2 x 10(0) IU/mL (detection limit) within 1 hour. These data indicate that high titers of these blood borne viruses are rapidly inactivated by this heat treatment process.

Published

1992

49. Electron microscopic studies on duck hepatitis B virus particles in hepatocytes and sequential changes in various patterns of infection.

Author

Okinaga S, Fukuda R, Fukumoto S, and Shimada Y

Subjects

Animals, DNA, Viral blood, Hepatitis B Virus, Duck physiology, Microscopy, Electron, Virion ultrastructure, Virus Replication physiology, Ducks microbiology, Hepatitis B Virus, Duck isolation & purification, Hepatitis, Viral, Animal microbiology, Liver microbiology, Poultry Diseases microbiology

Abstract

To investigate the critical factors involved in the elimination of the duck hepatitis B virus (DHBV) in acute infection, the sequential changes in the number of DHBV particles in hepatocytes were studied electron microscopically in ducks experimentally infected by DHBV. Twenty Japanese white Peking ducks were infected with DHBV on the day of hatching, and on the 7th day and 14th day after hatching. Inoculation of DHBV on the day of hatching, and on the 7th and 14th day after hatching resulted in persistent viremia, transient viremia and no viremia, respectively in ducks as tested by spot hybridization assay. The number of DHBV particles in the liver correlated well with the amount of serum DHBV-DNA, DHBV particles decreased in hepatocytes without any interaction of inflammatory cells over the observation period, and the number of particles was not associated with the degree of hepatic inflammation. From these results, the elimination of the virus was thought to be induced by a reduction of viral replication in the hepatocytes and not by destruction of their host cells. There must be an age-dependent factor which strongly suppresses the viral replication.

Published

1991

50. [Duck hepatitis B virus (DHBV) and viral DNA in duck hepatocellular carcinoma and liver tissue].

Author

Yang GX

Subjects

Animals, Antigens, Surface analysis, Carcinoma, Hepatocellular microbiology, Hepatitis, Viral, Animal, Liver Neoplasms microbiology, Carcinoma, Hepatocellular veterinary, DNA, Viral analysis, Ducks microbiology, Hepatitis B Virus, Duck isolation & purification, Liver Neoplasms veterinary, Poultry Diseases microbiology

Abstract

The hybridization test for duck hepatitis B virus DNA was performed in 34 ducks with hepatoma from Qidong, Jiangsu province. Among the 34 hepatoma ducks, 18 were positive for DHBV DNA in the serum and 27 were positive in the tumor and/or liver tissue. Tissue sections were stained with Victoria blue nuclear fast red for detecting DHBV surface antigen. Victoria blue positive cells were found in 11 tumors and 15 paratumorous regions of 23 ducks with hepatocellular carcinoma. Although paratumorous regions were positively stained in 3 of 8 ducks with cholangiocarcinoma, all were negative within their tumors. All paratumorous regions and 2 tumor regions of 3 ducks with hepatocellular-cholangiocarcinoma were positive for Victoria blue. The results suggest that duck hepatocellular carcinoma be closely related to DHBV infection.

Published

1991