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Hepatitis B Virus

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Cover of 'Hepatitis B Virus'

Table of Contents

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    Book Overview
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    Chapter 1 NTCP-Reconstituted In Vitro HBV Infection System
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    Chapter 2 Hepatitis B Virus Infection of HepaRG Cells, HepaRG-hNTCP Cells, and Primary Human Hepatocytes
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    Chapter 3 Live Cell Imaging Confocal Microscopy Analysis of HBV Myr-PreS1 Peptide Binding and Uptake in NTCP-GFP Expressing HepG2 Cells
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    Chapter 4 Intracytoplasmic Transport of Hepatitis B Virus Capsids
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    Chapter 5 A Homokaryon Assay for Nucleocytoplasmic Shuttling Activity of HBV Core Protein
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    Chapter 6 Analyses of HBV cccDNA Quantification and Modification
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    Chapter 7 Detection of HBV cccDNA Methylation from Clinical Samples by Bisulfite Sequencing and Methylation-Specific PCR
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    Chapter 8 A T7 Endonuclease I Assay to Detect Talen-Mediated Targeted Mutation of HBV cccDNA
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    Chapter 9 Detection of Hepatocyte Clones Containing Integrated Hepatitis B Virus DNA Using Inverse Nested PCR
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    Chapter 10 Highly Sensitive Detection of HBV RNA in Liver Tissue by In Situ Hybridization
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    Chapter 11 Immunofluorescent Staining for the Detection of the Hepatitis B Core Antigen in Frozen Liver Sections of Human Liver Chimeric Mice
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    Chapter 12 Measuring Changes in Cytosolic Calcium Levels in HBV- and HBx-Expressing Cultured Primary Hepatocytes
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    Chapter 13 In Vitro Assays for RNA Binding and Protein Priming of Hepatitis B Virus Polymerase
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    Chapter 14 In Vitro Enzymatic and Cell Culture-Based Assays for Measuring Activity of HBV RNaseH Inhibitors
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    Chapter 15 Detection of Hepatitis B Virus Particles Released from Cultured Cells by Particle Gel Assay
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    Chapter 16 Microtiter-Format Assays for HBV Antigen Quantitation in Nonclinical Applications
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    Chapter 17 Deep Sequencing of the Hepatitis B Virus Genome: Analysis of Multiple Samples by Implementation of the Illumina Platform
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    Chapter 18 Generation of Replication-Competent Hepatitis B Virus Genome from Blood Samples for Functional Characterization
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    Chapter 19 Hydrodynamic HBV Transfection Mouse Model
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    Chapter 20 An ELISPOT-Based Assay to Measure HBV-Specific CD8 + T Cell Responses in Immunocompetent Mice
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    Chapter 21 Advanced Method for Isolation of Mouse Hepatocytes, Liver Sinusoidal Endothelial Cells, and Kupffer Cells
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    Chapter 22 Partial Hepatectomy and Castration of HBV Transgenic Mice
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    Chapter 23 Studying HBV Infection and Therapy in Immune-Deficient NOD-Rag1−/−IL2RgammaC-null (NRG) Fumarylacetoacetate Hydrolase (Fah) Knockout Mice Transplanted with Human Hepatocytes
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    Chapter 24 Measurement of Antiviral Effect and Innate Immune Response During Treatment of Primary Woodchuck Hepatocytes
Attention for Chapter 13: In Vitro Assays for RNA Binding and Protein Priming of Hepatitis B Virus Polymerase
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Chapter title
In Vitro Assays for RNA Binding and Protein Priming of Hepatitis B Virus Polymerase
Chapter number 13
Book title
Hepatitis B Virus
Published in
Methods in molecular biology, January 2017
DOI 10.1007/978-1-4939-6700-1_13
Pubmed ID
Book ISBNs
978-1-4939-6698-1, 978-1-4939-6700-1
Authors

Daniel N. Clark, Scott A. Jones, Jianming Hu

Abstract

The hepatitis B virus (HBV) polymerase synthesizes the viral DNA genome from the pre-genomic RNA (pgRNA) template through reverse transcription. Initiation of viral DNA synthesis is accomplished via a novel protein priming mechanism, so named because the polymerase itself acts as a primer, whereby the initiating nucleotide becomes covalently linked to a tyrosine residue on the viral polymerase. Protein priming, in turn, depends on specific recognition of the packaging signal on pgRNA called epsilon. These early events in viral DNA synthesis can now be dissected in vitro as described here.The polymerase is expressed in mammalian cells and purified by immunoprecipitation. The purified protein is associated with host cell factors, is enzymatically active, and its priming activity is epsilon dependent. A minimal epsilon RNA construct from pgRNA is co-expressed with the polymerase in cells. This RNA binds to and co-immunoprecipitates with the polymerase. Modifications can be made to either the epsilon RNA or the polymerase protein by manipulating the expression plasmids. Also, the priming reaction itself can be modified to assay for the initiation or subsequent DNA synthesis during protein priming, the susceptibility of the polymerase to chemical inhibitors, and the precise identification of the DNA products upon their release from the polymerase. The identity of associated host factors can also be evaluated. This protocol closely mirrors our current understanding of the RNA binding and protein priming steps of the HBV replication cycle, and it is amenable to modification. It should therefore facilitate both basic research and drug discovery.

Mendeley readers

Mendeley readers

The data shown below were compiled from readership statistics for 4 Mendeley readers of this research output. Click here to see the associated Mendeley record.

Geographical breakdown

Country Count As %
Unknown 4 100%

Demographic breakdown

Readers by professional status Count As %
Unspecified 1 25%
Professor 1 25%
Student > Ph. D. Student 1 25%
Unknown 1 25%
Readers by discipline Count As %
Unspecified 1 25%
Biochemistry, Genetics and Molecular Biology 1 25%
Immunology and Microbiology 1 25%
Unknown 1 25%