2013
DOI: 10.1128/jvi.03328-12
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Novel Recombinant Hepatitis B Virus Vectors Efficiently Deliver Protein and RNA Encoding Genes into Primary Hepatocytes

Abstract: e Hepatitis B virus (HBV) has extremely restricted host and hepatocyte tropism. HBV-based vectors could form the basis of novel therapies for chronic hepatitis B and other liver diseases and would also be invaluable for the study of HBV infection. Previous attempts at developing HBV-based vectors encountered low yields of recombinant viruses and/or lack of sufficient infectivity/ cargo gene expression in primary hepatocytes, which hampered follow-up applications. In this work, we constructed a novel vector bas… Show more

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Cited by 42 publications
(67 citation statements)
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“…Newly synthesized HBsAg was detected in culture supernatants 8 to 10 days later (Fig. 3A) (18). In line with this finding, immunofluorescent staining on day 10 postinfection revealed the foreign-antigenic rHBc, as well as HBsAg, in the cytoplasm.…”
Section: Resultssupporting
confidence: 69%
See 1 more Smart Citation
“…Newly synthesized HBsAg was detected in culture supernatants 8 to 10 days later (Fig. 3A) (18). In line with this finding, immunofluorescent staining on day 10 postinfection revealed the foreign-antigenic rHBc, as well as HBsAg, in the cytoplasm.…”
Section: Resultssupporting
confidence: 69%
“…Huh-7 cells constitutively expressing the HBV core antigen were generated by lentiviral vector transduction. Primary tupaia hepatocytes (PTHs) were isolated by a twostep perfusion protocol (17,18). For viral infection, 1 ϫ 10 6 freshly isolated PTHs were seeded in collagen-coated 6-well plates (BD Biosciences, USA); 1 day after seeding, the PTHs were inoculated with wtHBV isolated from the infectious sera of HBV-infected patients or rHBV virions concentrated from culture supernatants by polyethylene glycol 8000.…”
Section: Methodsmentioning
confidence: 99%
“…However, due to the lack of specific and robust assays for direct measurement of low copy number cccDNA in HBV replicating cells, a cccDNA reporter system is thus needed for identification of cccDNA inhibitors in high throughput screening (Guo and Guo, 2015). Although recombinant HBV reporter viruses have been reported to support cccDNA-dependent infection, replacement or insertion of reporter gene in HBV genome will affect certain step(s) of virus replication and normally require transcomplementation of one or more viral proteins to make the infectious reporter viruses, resulting in decreases in the efficiency of replication or virion formation (Hong et al, 2013; Protzer et al, 1999; Untergasser and Protzer, 2004). In addition, infectious HBV reporter virus systems reproduce only the initial round of infection, and the current HBV in vitro infection systems require large amount of virus inoculum, but still exhibit relatively low infectivity and high variability (Yan et al, 2015a).…”
Section: Discussionmentioning
confidence: 99%
“…The nonviral vectors show less efficiency compared to viral vector in delivering the gene probe and preventing it from degradation of the cell autoimmunity, but good biocompatibility and large-scale production of nonviral vectors make it promising in gene therapy research [4]. Various nonviral gene vectors such as liposomes, [5] cationic polymers, [6] dendritic polymers, [7] polymeric peptides [8], and nanoparticles [9][10][11] have been continuously explored for gene therapy.…”
mentioning
confidence: 99%