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8 results on '"Dai, Chang-bai"'

2. PRODUCTION IN PICHIA PASTORIS AND CHARACTERIZATION OF GENETIC ENGINEERED CHIMERIC HBV/HEV VIRUS-LIKE PARTICLES.

Author

Li, Hong-zhao, Gang, Hong-ying, Sun, Qiang-ming, Liu, Xiao, Ma, Yan-bing, Sun, Mao-sheng, and Dai, Chang-bai

Subjects
*PICHIA pastoris, *EPITOPES, *GENETIC engineering, *HEPATITIS B virus, *HEPATITIS E, *ENZYME-linked immunosorbent assay, *MOSAICISM, *IMMUNE system
Abstract

Objective To investigate the presentation of a neutralization epitope-containing peptide antigen of hepatitis E virus (HEV) on chimeric virus-like particles (VLPs) of hepatitis B surface antigen (HBsAg). Method The gene fragment corresponding to amino acids (aa) 551-607 (HEnAg) of HEV capsid protein, which contains the only neutralization epitope identified to date, was fused via a synthetic glycine linker in frame with the gene of HBsAg. The resulted fusion gene was then integrated through transformation into the genome of Pichia pastoris under the control of a methanol-induced alcohol oxidase 1 (A 0X1) promoter and expressed intracellularly. The expression products in the soluble ceil extracts were characterized by Western blot, ELISA, CsCl density gradient analysis, and electron microscopic visualization. Results The novel fusion protein incorporating HBsAg and the neutralization epitope-containing HEnAg was expressed successfully in Pichia pastoris with an expected molecular weight of approximately 32 kD. It was found to possess the ability to assemble into chimeric HBV/HEV VLPs with immunological, physical and morphological characteristics akin to HBsAg particles. Not only did the chimeric VLPs show high activity levels in a HBsAg particle-specific ELISA but they were also strongly immunoreactive with hepatitis E (HE) positive human serum in a HEY specific ELISA, indicating that HEnAg peptide fragments were exposed on VLP surfaces and would be expected to be readily accessible by cells and molecules of the immune system. Similarity between chimeric VLPs to highly immunogenic HBsAg particles may confer good immunogenicity on surface-displayed HEnAg. Conclusion The chimeric HEY/HEY VLPs produced in this study may have potential to be a recombinant HEY/HEY bivalent vaccine candidate. [ABSTRACT FROM AUTHOR]

Published
2004

3. High-level expression and purification of recombinant huGM-CSF (9-127)/IL-6 (29-184) fusion protein in Escherichia coil.

Author

Sun QM, Jiang HC, Xu WM, Liu X, Dai CB, and Sun MS

Subjects
Base Sequence, Escherichia coli, Granulocyte-Macrophage Colony-Stimulating Factor genetics, Granulocyte-Macrophage Colony-Stimulating Factor isolation & purification, Humans, Interleukin-6 genetics, Interleukin-6 isolation & purification, Molecular Sequence Data, Peptide Fragments genetics, Peptide Fragments isolation & purification, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins isolation & purification, Granulocyte-Macrophage Colony-Stimulating Factor biosynthesis, Interleukin-6 biosynthesis, Peptide Fragments biosynthesis, Recombinant Fusion Proteins biosynthesis
Abstract

As HuGM-CSF and huIL-6 seem to have synergistic and complementary actions, researchers have proposed that fusion proteins incorporating these two cytokines could show increased biological activity, especially in terms of hematopoietic function. Here, we sought to obtain a functional GM-CSF/IL-6 fusion protein and to investigate its biological activities in vitro. A novel construct encoding a fusion protein of huGM-CSF (9-127) and IL-6 (29-184) was generated in the pBV220 expression vector by step-by-step cloning. Amino acids 1-8 of huGM-CSF and amino acids 1-28 of huIL-6 were deleted by PCR. The mutant huGM-CSF (9-127) and huIL-6 (29-184) cDNAs were linked via a linker sequence encoding 15 amino acid residues (G-G-S-G-S)3. Direct sequencing was used to confirm the validity of the desired construct, and the fusion protein was expressed in Escherichia coli host strain BL21 (DE3) in the form of inclusion bodies (IBs). The expression level was more than 25% of the total cell lysate, and a novel purification and refolding strategy was used to isolate the fusion protein product. Inclusion bodies were purified by Q Sepharose H.P. ion exchange in 8 mol/L urea, followed by in situ refolding by Sephacryl S-200. The renatured fusion proteins were obtained at a purity of >95%, and the strategy of refolding on the gel filtration column was found to be efficient, with a relative refolding rate of 80%. This entire refolding and purification procedure could be performed within one day and may prove applicable to large-scale purification and refolding of recombinant proteins from IBs in E. coli. This new method was used to obtain huGM-CSF (9-127)/IL-6 (29-184) fusion protein with high purity and biological activity. MTT assays in TF-1 and B9 cell lines showed that the specific biological activity of huGM-CSF was 1.14+/-0.10 x 10(8) U/mg, and that for huIL-6 was 1.89+/-0.11 x 10(7) U/mg. The fusion protein exhibited enhanced huGM-CSF, but similar huIL-6 biological activities compared with those of either GM-CSF or IL-6 alone. This suggests that our novel huGM-CSF (9-127)/IL-6 (29-184) fusion protein may hold future promise as a therapeutic agent.

Published
2005
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4. Expression and immunoreactivity of an epitope of HCV in a foreign epitope presenting system.

Author

Peng M, Dai CB, and Chen YD

Subjects
Animals, Capsid Proteins genetics, Capsid Proteins immunology, Escherichia coli, Humans, Insecta, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins immunology, Viral Envelope Proteins genetics, Viral Envelope Proteins immunology, Antigen Presentation genetics, Antigen Presentation immunology, Epitopes genetics, Epitopes immunology, Hepacivirus genetics, Hepacivirus immunology
Abstract

Aim: To construct and highly express an epitope of hepatitis C virus (HCV) in a foreign epitope presenting vector based on an insect virus, and to study the antigenicity of the epitope., Methods: The HCV epitope sequence (amino acid residues 315 to 328: EGHRMAWDMMMNWS) of the E1 region was constructed at different positions of a foreign epitope presenting vector based on an insect virus, flock house virus (FHV) capsid protein encoding gene as a vector, and expressed in E. coli cells. Western blotting and ELISA were used to detect the immunoreactivity of these recombinant proteins., Results: The gene encoding of the concerned B-cell epitope of HCV E1 envelope protein was expressed on FHV capsid carrier protein at positions I1 (aa 106), I2 (aa 153) and I3 (aa 305), respectively, on the surface of FHV capsid protein. The recombinant proteins in this system could be highly expressed in more than 40% of total cell protein of E. coli BL21. All the expressed recombinant proteins were in inclusion body form, and showed obvious immunoreactivity by Western blotting. Further purified recombinant proteins were detected by indirect ELISA as coating antigen respectively. All recombinant proteins could still show immunoreactivity., Conclusion: The epitope of HCV E1 envelope protein can be highly expressed in FHV carrier system as a chimeric protein with high immunoreactivity. This system has multiple entry sites conferring many possible conformations closer to the native one for a given sequence.

Published
2005
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5. [Construction, expression and biologic activities of two rhIL-6/GM-CSF fusion proteins].

Author

Sun QM, Sun MS, Yi S, Cao Z, Bie J, Dai CB, and Xu WM

Subjects
Blotting, Western, Cell Line, Escherichia coli genetics, Granulocyte-Macrophage Colony-Stimulating Factor pharmacology, Humans, Interleukin-6 pharmacology, Polymerase Chain Reaction, Recombinant Fusion Proteins isolation & purification, Recombinant Fusion Proteins pharmacology, Granulocyte-Macrophage Colony-Stimulating Factor genetics, Interleukin-6 genetics, Recombinant Fusion Proteins biosynthesis
Abstract

Aim: To construct and express the gene encoding hIL-6/GM-CSF fusion protein., Methods: The genes encoding the two hIL-6/GM-CSF fusion proteins were constructed in pBV220 expression vector. Fusion proteins were expressed in E.coli BL-21 and purified through Q Sepharose HP ion exchange chromatography and Sephacryl S-200 gel filtration columns. The biologic activities of the fusion proteins were detected by proliferation of hIL-6 dependent cell line B9 and hGM-CSF dependent cell line TF1 with MTT assay., Results: Both fusion proteins were expressed in E.coli BL-21 in the form of inclusion body. The expression levels were more than 25% of the total cell lysates. Both fusion proteins were obtained with high purity which had both hIL-6 and hGM-CSF biologic activities., Conclusion: Two hIL-6/GM-CSF fusion proteins with high purity and bilolgic activities have been acquired successfully.

Published
2004

6. [Construction of a recombinant human adenovirus expressing the ORF2 antigen of HEV and immunization of mice by mucosal system].

Author

Dong X, Hu JY, Xie TH, Sun MS, Dai CB, and Ma YB

Subjects
Animals, Hepatitis Antigens genetics, Immunoglobulin A immunology, Immunoglobulin G immunology, Male, Mice, Mice, Inbred BALB C, Peritoneum immunology, Recombinant Proteins biosynthesis, Recombinant Proteins genetics, Recombinant Proteins immunology, Viral Hepatitis Vaccines, Viral Proteins biosynthesis, Viral Proteins genetics, Adenoviruses, Human genetics, Hepatitis Antigens immunology, Nasal Mucosa immunology, Viral Proteins immunology
Abstract

Objective: To construct a replication-defective recombinant adenovirus expressing the ORF2 (112-660aa) antigen of hepatitis E virus (HEV) and evaluate its immunization effect in BALB/c mice by mucosal inoculation., Methods: The HEV ORF2 gene encoding for 112-660aa was amplified from plasmid pUC-HEV and inserted into the transfer vector pTrack-CMV. The recombinant plasmid and adenoviral backbone plasmid pAdEasy-1 were co-transformed into E. coli strain BJ5183. Taking the advantage of the high efficient homologous recombination machinery presented in bacteria, the recombinant adenovirus backbone plasmid was generated in BJ5183, and then was transfected into 293 cells. Recombinant Adenoviruses were propagated in 293 cells with high titers. 8-week-old BALB/c mice were inoculated intraperitoneally and intranasally with 10(7) pfu recombinant adenovirus each on weeks 0, 3, 5, 7, 10., Results: Both groups of mice induced humoral IgG immune response with the highest titers 1:1,000 and 1:10,000 each. Only the group inoculated intranasally could induce mucosal IgA immune response., Conclusions: The adenoviral recombinant can stimulate specific humoral and mucosal immune response in mice and is potentially to be used as a candidate vaccine for the treatment of HEV infection.

Published
2003

7. [Vaccination of rhesus monkeys with recombinant antigen fragments and protection from hepatitis E virus infection].

Author

Ma YB, Xie TH, Zhang GM, Li CH, Dai XJ, Dai CB, Sun MS, Lu J, and Bi SL

Subjects
Animals, Immunoglobulin G immunology, Macaca mulatta, RNA, Viral blood, Recombinant Proteins immunology, Vaccination, Antigens, Viral immunology, Hepatitis E prevention & control, Hepatitis E virus immunology, Viral Hepatitis Vaccines immunology
Abstract

Objective: To observe anti-HEV IgG response to vaccination of recombinant antigen fragments and evaluate its protection from Hepatitis E Virus infection in rhesus monkeys (Macaca mulatta)., Methods: Twelve monkeys were divided into three groups and immunized respectively with three different recombinant antigens: namely Ag1 (carboxyl terminal 431 amino acids of ORF2), Ag2 (128aa fragment at the carboxyl terminal of ORF2), and Ag3 (full length ORF3 ligated with two ORF2 fragments encoded by 6743-7126nt and 6287-6404nt). The monkeys were challenged intravenously with fecal suspension from experimentally infected rhesus monkeys, and the other three monkeys served as the placebo group for challenge with HEV. The dynamic changes of the levels of ALT and anti-HEV IgG were examined. Pathological changes of liver tissue were observed by light microscope. Excretion of virus was detected by RT-nPCR., Results: Hepatic histopathology of two monkeys in the placebo group was consistent with acute viral hepatitis, and ALT was elevated 3-4 weeks after inoculated with virus, up to 10-20 times higher than normal level. The liver tissue of monkeys immunized with antigen kept normal, ALT in several monkeys elevated mildly, and anti-HEV IgG conversation occurred at 1-2 weeks after vaccination, with the titer reaching 1:12,800. The virus RNA could be detected by RT-nPCR from days 7 to 50 in monkeys of control group, and from days 7 to 21 in vaccinated monkeys after challenged with virus., Conclusions: The recombinant antigens could induce the production of anti-HEV IgG, which protected rhesus monkeys from acute Hepatitis symptoms related to HEV infection.

Published
2002

8. [Refolding and purification of the huGM-CSF(9-127)-IL-6(29-184) fusion protein].

Author

Sun QM, Liu HY, Dai CB, Ma YB, Sun MS, and Xu WM

Subjects
Granulocyte-Macrophage Colony-Stimulating Factor chemistry, Interleukin-6 chemistry, Peptide Fragments chemistry, Protein Folding, Recombinant Fusion Proteins chemistry, Granulocyte-Macrophage Colony-Stimulating Factor isolation & purification, Interleukin-6 isolation & purification, Peptide Fragments isolation & purification, Recombinant Fusion Proteins isolation & purification
Abstract

The huGM-CSF(9-127)-IL-6(29-184) fusion protein was precipitated on column when being purified by Q Sepharose H.P. ion exchange chromatography after renaturation by dilution. To solve this problem, a novel purification and refolding strategy was adopted. Inclusion bodies was first purified by Q Sepharose H.P. ion exchange in 8 mol/L urea, followed by in situ refolding on column by Sephacryl S-200. Renatured fusion protein was obtained in a purity of more than 95%. It was showed that the method of refolding on gel filtration column is efficient, with relative refolding rate at 80%. By the whole procedure, refolding and purification of recombinant protein can be performed within one day. This strategy is also promising to be applied in large scale purification and refolding of recombinant protein from inclusion bodies in E. coli.

Published
2002

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