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Design and Production of a Novel Polypeptide with Immunogenic Potentials for Immunoassay of Brucella Melitensis

机译:一种新型的具有免疫原性潜力的多肽用于布鲁氏菌免疫分​​析的设计和生产

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Brucellosis is one of the most common diseases in humans and it has a worldwide spread. The design and production of newly synthesized proteins can be served as a goal for the rapid and accurate detection of brucellosis. To this aim, finding the antigenic epitopes is the first step to design a diagnostic method. In this study, the epitope mapping procedure was carried out by IEDB analysis resource using Flagellin and Porin amino acid sequences. The selected sequences were linked by GS linkers and cloned into pET26b vector. After confirmation of the expressed recombinant polypeptide by western blotting, it was immunologically analyzed by gel diffusion assay. The SDS PAGE and western blot analysis confirmed the 27 KDa polypeptide production and observing an arc in gel diffusion test demonstrated the precipitation of serum antibodies and the presence of specific antigen complexes. The results showed that the recombinant polypeptide produced in E. coli BL21, could interact with antibodies present in Brucella immunized sheep serum. HIGHLIGHTS ?Prediction of antigenic epitopes for Brucella membrane proteins. ?Production of designed polypeptide in E. coli BL21 (DE3). ?Interaction of produced polypeptide with Brucella specific antibodies.
机译:布鲁氏菌病是人类最常见的疾病之一,已在世界范围内传播。新合成蛋白质的设计和生产可以作为快速准确检测布鲁氏菌病的目标。为了这个目的,发现抗原表位是设计诊断方法的第一步。在这项研究中,表位作图程序是由IEDB分析资源使用鞭毛蛋白和孔蛋白氨基酸序列进行的。选定的序列通过GS接头连接,并克隆到pET26b载体中。通过蛋白质印迹确认表达的重组多肽后,通过凝胶扩散测定法对其进行免疫学分析。 SDS PAGE和蛋白质印迹分析证实了27 KDa多肽的产生,并且在凝胶扩散测试中观察到电弧证明血清抗体沉淀并且存在特定抗原复合物。结果表明,在大肠杆菌BL21中产生的重组多肽可以与布鲁氏菌免疫的绵羊血清中存在的抗体相互作用。要点?布鲁氏菌膜蛋白的抗原表位预测。在大肠杆菌BL21(DE3)中生产设计的多肽。产生的多肽与布鲁氏菌特异性抗体的相互作用。

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