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Cloning, expression, and purification of recombinant protein from a single synthetic multivalent construct of Mycobacterium tuberculosis

机译:从结核分枝杆菌的单一合成多价构建体克隆,表达和纯化重组蛋白

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Tuberculosis remains a major infectious disease with over 8 million new cases and 2 million deaths annually. Therefore, a vaccine more potent than BCG is desperately needed. In this regard, an approximately 800 bp DNA encoding a mycobacterial synthetic gene designated as VacIII (containing ubiquitin gene UbGR and four immunogenic mycobacterial epitopes or genes of ESAT-6, Phos1, Hsp 16.3, and Mtb8.4) was sub-cloned into a bacterial expression vector of pRSET-B resulting in a 6x His-VaeIII fusion gene construction. This recombinant clone was over expressed in Escherichia coli BL-21 (DE-3). The expressed fusion protein was found almost entirely in the insoluble form (inclusion bodies) in cell lysate. The inclusion bodies were solubilized with 8 M urea and the recombinant protein was purified by Ni-NTA column and dialyzed by urea gradient dialysis. This method produced a relatively high yield of recombinant VacIII protein and the cloned VacIII gene offers the potential development of other vaccine formats such as DNA vaccine and recombinant vaccine. (c) 2006 Elsevier Inc. All rights reserved.
机译:结核病仍然是一种主要的传染病,每年新增病例超过800万,死亡200万。因此,迫切需要比BCG更有效的疫苗。在这方面,将编码称为VacIII的分枝杆菌合成基因(包含泛素基因UbGR和四个免疫原性分枝杆菌抗原决定簇或ESAT-6,Phos1,Hsp 16.3和Mtb8.4的基因)的大约800 bp DNA亚克隆到一个pRSET-B的细菌表达载体导致6x His-VaeIII融合基因的构建。该重组克隆在大肠杆菌BL-21(DE-3)中过表达。发现表达的融合蛋白几乎完全以不溶形式(包涵体)存在于细胞裂解物中。用8M尿素溶解包涵体,并通过Ni-NTA柱纯化​​重组蛋白,并通过尿素梯度透析进行透析。该方法产生了相对较高产率的重组VacIII蛋白,并且克隆的VacIII基因提供了其他疫苗形式的潜在发展,例如DNA疫苗和重组疫苗。 (c)2006 Elsevier Inc.保留所有权利。

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