A Recombinant Multiepitope Protein for Hepatitis B Diagnosis

被引:20
作者
de Souza, Marilen Queiroz [1 ]
Galdino, Alexsandro Sobreira [2 ]
dos Santos, Jose Carlos [1 ]
Soares, Marcus Vinicius [1 ]
de Nobrega, Yanna C. [3 ]
Morales Alvares, Alice da Cunha [4 ]
de Freitas, Sonia Maria [4 ]
Goncalves Torres, Fernando Araripe [1 ]
Soares Felipe, Maria Sueli [1 ,5 ]
机构
[1] Univ Brasilia, Med Biol Lab, BR-70910900 Brasilia, DF, Brazil
[2] Univ Fed Sao Joao Del Rei, Lab Biotecnol Microrganismos, BR-35501296 Divinopolis, MG, Brazil
[3] Univ Brasilia, Dept Patol Mol, Lab Imunopatol, BR-70910900 Brasilia, DF, Brazil
[4] Univ Brasilia, Inst Ciencias Biol, Lab Biofis, BR-70910900 Brasilia, DF, Brazil
[5] Univ Catolica Brasilia, Posgrad Ciencias Genom & Biotecnol, BR-70910900 Brasilia, DF, Brazil
关键词
CIRCULAR-DICHROISM; GENETIC DIVERSITY; ANTIGENIC REGIONS; FUSION PROTEIN; CORE ANTIGEN; VIRUS; IDENTIFICATION; SERODIAGNOSIS; GENOTYPES; PEPTIDE;
D O I
10.1155/2013/148317
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
Hepatitis B is a liver inflammation caused by hepatitis B virus (HBV) and can be diagnosed in clinical stage by hepatitis B core antibody from IgM class (anti-HBcIgM). Hepatitis B core antibody from IgG class (Anti-HBcIgG) appears quickly after IgM, reaching high titers in chronic hepatitis, and remains even after cure. Since hepatitis B core antibody (anti-HBc) is the first antibody identified and sometimes the only marker detected during the course of infection, it can be used both to indicate HBV acute infection (anti-HBc-IgM) and to identify individuals who have come into contact with the virus (anti-HBc-IgG). In this work we propose a recombinant hepatitis B core multiepitope antigen (rMEHB) to be used for diagnosis of hepatitis B. For this purpose, a synthetic gene coding for rMEHB was designed and cloned into vector pET21a with a 6xHis tag at the C-terminal. Time course induction in E. coli showed an induced protein with an apparent molecular mass of similar to 21 kDa. Protein purification was performed by a single step with affinity chromatography Ni-NTA. Circular dichroism spectroscopy indicated rMEHB as a thermal stable protein at pH 7.0 and 8.0. In these conditions rMEHB was successfully used to perform an enzyme linked immuno sorbent assay (ELISA) with positive and negative sera.
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页数:7
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