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High-yield production of major T-cell ESAT6-CFP10 fusion antigen of M tuberculosis complex employing codon-optimized synthetic gene

Int J Biol Macromol. 2021-01; 
A Gutiérrez-Ortega, D A Moreno, S A Ferrari, H Espinosa-Andrews, E P Ortíz, F Milián-Suazo, A H Alvarez
Products/Services Used Details Operation
Plasmid DNA Preparation … Plasmid pUC57-rESAT6-CFP10 was manufactured by GenScript (Piscataway NJ). Commercial bovine IFN-γ-microplate enzyme-linked immunosorbent assay from Prionics AG (USA) was used. 2.2. Design and structure prediction of the target ESAT6-CFP10-(His6x) protein … Get A Quote

摘要

Translation engineering and bioinformatics have accelerated the rate at which gene sequences can be improved to generate multi-epitope proteins. Strong antigenic proteins for tuberculosis diagnosis include individual ESAT6 and CFP10 proteins or derived peptides. Obtention of heterologous multi-component antigens in E. coli without forming inclusion bodies remain a biotechnological challenge. The gene sequence for ESAT6-CFP10 fusion antigen was optimized by codon bias adjust for high-level expression as a soluble protein. The obtained fusion protein of 23.7 kDa was observed by SDS-PAGE and Western blot analysis after Ni-affinity chromatography and the yield of expressed soluble protein reached a concentration o... More

关键词

Antigenicity, Codon optimization, Fusion protein, Soluble ESAT6-CFP10, Synthetic gene