Differences in sequences between HBV-relaxed circular DNA and covalently closed circular DNA

Rybicka, Magda; Woziwodzka, Anna; Romanowski, Tomasz; Stalke, Piotr; Dręczewski, Marcin; Bielawski, Krzysztof Piotr

doi:10.1038/emi.2017.41

Cited by 6 publications

(6 citation statements)

References 19 publications

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“…For comparison, the HBeAg-positive capuchin monkey HBV (CMHBV) showed significantly more SNPs in serum (1.8 SNPs per 100 nucleotides; χ 2 , P < 0.0001) (24). This difference is noteworthy because liver contains the covalently closed circular DNA reservoir showing relatively higher virus diversity than the relaxed circular DNA found in circulating virions (31). Of note, significant differences in SNP occurrence rates were observed neither between coding nor noncoding shrew HBV genomic regions, nor between single or overlapping ORFs, nor between the different shrew genera (SI Appendix, Table S5).…”

Section: Shrews Carry Hbvs Across a Broad Geographic And Host Rangementioning

confidence: 99%

Highly diversified shrew hepatitis B viruses corroborate ancient origins and divergent infection patterns of mammalian hepadnaviruses

Rasche

Lehmann

König

et al. 2019

Proc. Natl. Acad. Sci. U.S.A.

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Shrews, insectivorous small mammals, pertain to an ancient mammalian order. We screened 693 European and African shrews for hepatitis B virus (HBV) homologs to elucidate the enigmatic genealogy of HBV. Shrews host HBVs at low prevalence (2.5%) across a broad geographic and host range. The phylogenetically divergent shrew HBVs comprise separate species termed crowned shrew HBV (CSHBV) and musk shrew HBV (MSHBV), each containing distinct genotypes. Recombination events across host orders, evolutionary reconstructions, and antigenic divergence of shrew HBVs corroborated ancient origins of mammalian HBVs dating back about 80 million years. Resurrected CSHBV replicated in human hepatoma cells, but human-and tupaiaderived primary hepatocytes were resistant to hepatitis D viruses pseudotyped with CSHBV surface proteins. Functional characterization of the shrew sodium taurocholate cotransporting polypeptide (Ntcp), CSHBV/MSHBV surface peptide binding patterns, and infection experiments revealed lack of Ntcp-mediated entry of shrew HBV. Contrastingly, HBV entry was enabled by the shrew Ntcp. Shrew HBVs universally showed mutations in their genomic preCore domains impeding hepatitis B e antigen (HBeAg) production and resembling those observed in HBeAg-negative human HBV. Deep sequencing and in situ hybridization suggest that HBeAg-negative shrew HBVs cause intense hepatotropic monoinfections and low within-host genomic heterogeneity. Geographical clustering and low MSHBV/CSHBVspecific seroprevalence suggest focal transmission and high virulence of shrew HBVs. HBeAg negativity is thus an ancient HBV infection pattern, whereas Ntcp usage for entry is not evolutionarily conserved. Shrew infection models relying on CSHBV/MSHBV revertants and human HBV will allow comparative assessments of HBeAg-mediated HBV pathogenesis, entry, and species barriers.hepatitis B virus | viral evolution | zoonosis | shrew | E antigen T he hepatitis B virus (HBV, genus Orthohepadnavirus) is a ubiquitous pathogen that causes 887,000 deaths annually, predominantly due to cirrhosis and hepatocellular carcinoma after chronic hepatitis B (CHB) (1). Distantly related hepadnaviruses were identified recently in animals other than humans and apes (1). The newly discovered animal viruses revealed that prototypic properties of HBV such as envelopment (2) and presence of an X gene (3) emerged de novo during orthohepadnavirus evolution.Hepadnaviruses are ancient pathogens, likely infecting vertebrates for over 200 million years (3). Placental mammals evolved ∼99 million years ago (mya) and form 2 major clades termed Laurasiatheria and Euarchontoglires (4). The known laurasiatherian HBV hosts belong to several species within the orders Chiroptera (bats) and to one species each within the orders Carnivora (cat) and Artiodactyla (duiker). HBV hosts within the Euarchontoglires include Significance Hepatitis B viruses (HBVs) have existed for millions of years. We describe divergent HBV species in shrews, which are ancient insectivorous mammals. The shrew viruses co...

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Section: Shrews Carry Hbvs Across a Broad Geographic And Host Rangementioning

confidence: 99%

Highly diversified shrew hepatitis B viruses corroborate ancient origins and divergent infection patterns of mammalian hepadnaviruses

Rasche

Lehmann

König

et al. 2019

Proc. Natl. Acad. Sci. U.S.A.

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“…Simultaneous, competing evolutionary pressures can create different subpopulations of HBV within patients (quasispecies) and at the population level. These can produce a more diverse RC-DNA population and a less diverse and stable cccDNA population, with different sequence polymorphisms potentially archived in the cccDNA pool 128 (Figure 2 Bv ).…”

Section: Virus Evolution and Diversitymentioning

confidence: 99%

Insights From Deep Sequencing of the HBV Genome—Unique, Tiny, and Misunderstood

et al. 2019

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Hepatitis B virus (HBV) is a unique, tiny, partially double-stranded, reverse-transcribing DNA virus with proteins encoded by multiple overlapping reading frames. The substitution rate is surprisingly high for a DNA virus, but lower than that of other reverse transcribing organisms. More than 260 million people worldwide have chronic HBV infection, which causes 0.8 million deaths a year. Because of the high burden of disease, international health agencies have set the goal of eliminating HBV infection by 2030. Nonetheless, the intriguing HBV genome has not been well characterized. We summarize data on the HBV genome structure and replication cycle, explain and quantify diversity within and among infected individuals, and discuss advances that can be offered by application of next-generation sequencing technology. In-depth HBV genome analyses could increase our understanding of disease pathogenesis and allow us to better predict patient outcomes, optimize treatment, and develop new therapeutics.

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“…15 Rolling circle amplification is a potential alternative to increase the sensitivity of cccDNA detection, 16,17 but this has not been widely accepted. 6,18 To increase the specificity, a cccDNA PCR, using specific primers and probes to selectively amplify cccDNA and exclude rcDNA, was developed. This is achieved as a result of using primers spanning the nick of rcDNA and hybridizing the probe to its gap region.…”

mentioning

confidence: 99%

“…19 Reducing rcDNA copy number is another way to increase the accuracy of cccDNA detection. Pretreatment of HBV-DNA with Plasmid-Safe ATP-Dependent DNase (PSAD) (Epicentre, Madison, WI) 15 or T5 exonuclease (NEB, Beverly, MA) 18 to degrade DNA with free ends can improve discriminatory power up to 1000-fold. 15 Although cccDNA-selective PCR provides a relative discrimination between cccDNA and rcDNA, additional means are still required to reduce the false-positive amplification of rcDNA.…”

mentioning

confidence: 99%

A Highly Sensitive and Robust Method for Hepatitis B Virus Covalently Closed Circular DNA Detection in Single Cells and Serum

Huang

Yang

et al. 2018

The Journal of Molecular Diagnostics

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Despite implications of persistence of hepatitis B virus (HBV) covalently closed circular DNA (cccDNA) in the development of hepatocellular carcinoma (HCC), little is known about serum cccDNA in HBV-infected diseases. We developed a cccDNA-selective droplet digital PCR (ddPCR) to assess cccDNA content and dynamics across different stages of HCC development. One hundred forty-seven serum samples and 35 formalin-fixed, paraffin-embedded tumor tissues were derived from patients with HCC or HBV hepatitis/cirrhosis. After specific amplification and selective digestion, probe-based ddPCR was used to quantify cccDNA copy numbers in single cells and clinical samples. The cccDNA in single HepG2.2.15 cells ranged from 0 to 10.8 copies/cell. Compared with non-HCC patients, HCC patients showed a higher cccDNA-positive rate (89.9% versus 53.2%; P = 4.22 × 10) and increased serum cccDNA contents (P = 0.002 and P = 0.041 for hepatitis and cirrhosis patients, respectively). Serum cccDNA ranged from 84 to 1.07 × 10 copies/mL. Quantification of serum cccDNA and HBV-DNA was an effective way to discriminate HCC patients from non-HCC patients, with areas under the curve of receiver operating characteristic of 0.847 (95% CI, 0.759-0.935; sensitivity, 74.5%; specificity, 93.7%). cccDNA-selective ddPCR is sensitive to detect cccDNA in single cells and different clinical samples. Combined analysis of serum cccDNA and HBV-DNA may be a promising strategy for HBV-induced HCC surveillance and antiviral therapy evaluation.

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Differences in sequences between HBV-relaxed circular DNA and covalently closed circular DNA

Cited by 6 publications

References 19 publications

Highly diversified shrew hepatitis B viruses corroborate ancient origins and divergent infection patterns of mammalian hepadnaviruses

Highly diversified shrew hepatitis B viruses corroborate ancient origins and divergent infection patterns of mammalian hepadnaviruses

Insights From Deep Sequencing of the HBV Genome—Unique, Tiny, and Misunderstood

A Highly Sensitive and Robust Method for Hepatitis B Virus Covalently Closed Circular DNA Detection in Single Cells and Serum

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