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Production of recombinant protein G through high-density fermentation of engineered bacteria as well as purification

机译:通过工程菌的高密度发酵以及纯化生产重组蛋白G

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摘要

Recombinant Streptococcus Protein G (PG) is a cell wall protein, which, when combined with mammal immunoglobulin, is used in separating antibody technology. High-density fermentation technologies using an engineered recombinant PG-producing bacteria as well as PG separation and purification technologies have a direct impact on the availability and application of PG. Through primary and secondary seed cultivation, a recombinant E. coli strain was subjected to high-density fermentation with controlled feed supplement concentration under stimulation with isopropyl beta-D-1-thiogalactopyranoside. The present study investigated the effect of factors including inoculum size, oxygen levels, pH and the cultivating method on the fermentation process, as well as the effect of the separation and purification technologies, including ultrasonication, nickel column affinity chromatography, Sephadex G-25 gel filtration chromatography and diethylaminoethanol-sepharose fast flow ion exchange chromatography on the yield and purity of PG. The efficiency of extraction was detected using SDS-PAGE. High-density fermentation yielded 80-150 g/l of bacteria and 1 g PG was obtained from one liter broth. The present study delivered a highly efficient novel method via which PG can be obtained at a high concentration and a purity >95%.
机译:重组链球菌蛋白G(PG)是一种细胞壁蛋白,当与哺乳动物免疫球蛋白结合使用时,可用于分离抗体技术。使用工程重组PG生产菌的高密度发酵技术以及PG分离和纯化技术直接影响PG的可用性和应用。通过一次和二次种子培养,将重组大肠杆菌菌株在异丙基β-D-1-硫代半乳糖吡喃糖苷的刺激下,以受控的饲料添加物浓度进行高密度发酵。本研究调查了接种量,氧气水平,pH和培养方法等因素对发酵过程的影响,以及超声分离,镍柱亲和层析,Sephadex G-25凝胶等分离纯化技术的影响。过滤色谱法和二乙氨基乙醇-琼脂糖快速流动离子交换色谱法测定PG的收率和纯度。使用SDS-PAGE检测提取效率。高密度发酵产生80-150 g / l的细菌,从1升肉汤中获得1 g PG。本研究提供了一种高效的新方法,通过该方法可以以高浓度和纯度> 95%获得PG。

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