High-level production of a functional recombinant hepatitis B virus polymerase in insect cells with a baculovirus expression system

Xiaoyan Wang , Linlin Gao , Fei Deng , Yanfang Zhang , Yan Li , Jusheng Lin

Current Medical Science ›› 2007, Vol. 27 ›› Issue (13) : 269 -273.

PDF
Current Medical Science ›› 2007, Vol. 27 ›› Issue (13) : 269 -273. DOI: 10.1007/s11596-007-0313-9
Article

High-level production of a functional recombinant hepatitis B virus polymerase in insect cells with a baculovirus expression system

Author information +
History +
PDF

Abstract

HBV polymerase has intrinsic RNA-dependent reverse transcriptase, DNA-dependent DNA polymerase as well as RNaseH activity. Analysis of HBV polymerase has been hampered for many years due to the inability to express functional enzyme in a recombinant system. To obtain active polymerase at a high level, we have taken advantage of baculovirus expression system. The gene of HBV polymerase was amplified by PCR and cloned into pFastBac Dual to construct the recombinant plasmid pFastbac Dual-pol. The recombinant donor plasmid, pFastbac Dual-pol, was constructed by inserting HBV polymerase gene into EcoRI and PstI sites controlled by polyhedrin promoter. The recombinant donor plasmid was transformed into DH10Bac competent cells for transposition. Recombinant bacmid was constructed by inserting of the mini-Tn7 element from the donor plasmid into the mini-attTn7 attachment site on the bacmid. The recombinant bacmid DNA was isolated and transfected into the Sf9 cells to produce the recombinant virus, and healthy insect Sf9 cells were infected with the recombinant virus containing HBV polymerse gene to express the target protein. HBV polymerse expressed in insect cells was analyzed by SDS-PAGE. PCR results showed recombinant donor plasmid, pFastbac Dual-pol, was constructed successfully. The recombinant hepatitis B virus polymerase was expressed in insect cells at high level. The recombinant hepatitis B virus polymerase should facilitate the analysis of HBV polymerase biological characteristics, allow the investigation for new anti-HBV drugs specifically blocking HBV polymerase.

Keywords

hepatitis B virus / polymerase / baculovirus / insect cell

Cite this article

Download citation ▾
Xiaoyan Wang, Linlin Gao, Fei Deng, Yanfang Zhang, Yan Li, Jusheng Lin. High-level production of a functional recombinant hepatitis B virus polymerase in insect cells with a baculovirus expression system. Current Medical Science, 2007, 27(13): 269-273 DOI:10.1007/s11596-007-0313-9

登录浏览全文

4963

注册一个新账户 忘记密码

References

Publishing order | Descend order by publishing year | Descend order by cited within
[1]

GanemD.. FieldsB. N., KnipeD. M., HowleyP. M.. Hapadnaviridae and their replication. Fundamental Virology, 19963rd ed.Philadelphia, Lippincott-Raven Publishers: 1199-1233
[2]

SeegerC., MasonW. S.. Hepatitis B virus biology. Microbiol Mol Biol Rev, 2000, 64: 51-68

[3]

SummersJ., MasonW. S.. Replication of the genome of a hepatitis B-like virus by reverse transcription of an RNA intermediate. Cell, 1982, 29: 403-415

[4]

GanemD., VarmusH. E.. The molecular biology of the hepatitis B viruses. Annu Rev Biochem, 1987, 56: 651-693

[5]

BartenschlagerR., KuhnC., SchallerH.. Expression of the P-protein of the human hepatitis B virus in a vaccine virus system and detection of the nucleocapsid-associated P-gene product by radiolabelling at newly introduced phosphorylation sites. Nucleic Acids Res, 1992, 20: 195-202

[6]

RadziwillG., ZentgrafH., SchallerH., et al.. The duck hepatitis B virus DNA polymerase is tightly associated with the viral core structure and unable to switch to an exogenous template. Virology, 1988, 163: 123-132

[7]

LanfordR. E., NotvallL., BeamesB.. Nucleotide priming and reverse transcriptase activity of hepatitis B virus polymerase expressed in insect cells. J Virol, 1995, 69: 4431-4439
[8]

SeiferM., StandringD. N.. Recombinant human hepatitis B virus reverse transcriptase is active in the absence of the viral nucleocapsid or the replication origin, DR1. J Virol, 1993, 67: 4513-4520
[9]

TavisJ. E., GanemD.. Expression of functional hepatitis B virus polymerase in yeast reveals it to be the sole viral protein required for correct initiation of reverse transcription. Proc Natl Acad Sci USA, 1993, 90: 4107-4111

[10]

WangG. H., SeegerC.. The reverse transcriptase of hepatitis B virus acts as a protein primer for viral DNA synthesis. Cell, 1992, 71: 663-670

[11]

LanfordR. E., NotvallL., LeeH., et al.. Transcomplementation of nucleotide priming and reverse transcription between independently expressed TP and RT domains of the hepatitis B virus reverse transcriptase. J Virol, 1997, 71: 2996-3004
[12]

SeiferM., StandringD. N.. Ribonucleoprotein complex formation by the human hepatitis B virus polymerase. Intervirology, 1995, 38: 295-303
[13]

TavisJ. E., GanemD.. RNA sequences controlling the initiation and transfer of duck hepatitis B virus minus-strand DNA. J Virol, 1995, 69: 4283-4291
[14]

GalibertF., MandartE., FitoussiF., et al.. Nucleotide sequence of the hepatitis B virus genome (subtype ayw) cloned in E. coli. Nature (London), 1979, 281: 646-650

[15]

TaniH., LimnC. K., YapC. C., et al.. In vitro and in vivo gene delivery by recombinant baculoviruses. J Virol, 2003, 77: 9799-9808

[16]

KostT. A., CondreayJ. P., JarvisD. L.. Baculovirus as versatile vectors for protein expression in insect and mammalian cells. Nat Biotechnol, 2005, 23: 567-575

[17]

HuserA., HafmannC.. Baculovirus vectors: novel mammalian cell gene-delivery vehicles and their applications. Am J Pharmacogenomics, 2003, 3: 53-63

[18]

BartenschlagerR., Junker-NiepmannM., SchallerH.. The P gene product of hepatitis B virus is required as a structural component for genomic RNA encapsidation. J Virol, 1990, 64: 5324-5332
[19]

HirschR. C., LavineJ. E., ChangL. J., et al.. Polymerase gene products of hepatitis B viruses are required for genomic RNA packaging as well as for reverse transcription. Nature (London), 1990, 344: 552-555

[20]

BartenschlagerR., SchallerH.. The amino-terminal domain of the hepadnaviral P-gene encodes the terminal protein (genome-linked protein) believed to prime reverse transcription. EMBO J, 1988, 7: 4185-4192
[21]

RadziwillG., TuckerW., SchallerH.. Mutational analysis of the hepatitis B virus P gene product: domain structure and RNase H activity. J Virol, 1990, 64: 613-620
[22]

WangG. H., SeegerC.. Novel mechanism for reverse transcription in hepatitis B viruses. J Virol, 1993, 67: 6507-6512
[23]

TavisJ. E., PerriS., GanemD. E.. Hepadnaviral reverse transcription initiates within a stem-loop of the RNA packaging signal and employs a novel strand transfer. J Virol, 1994, 68: 3536-3543
AI Summary AI Mindmap
PDF

93

Accesses

0

Citation

Detail
Sections
Recommended

AI思维导图

/