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The Fh8 tag : a fusion partner for simple and cost-effective protein purification in Escherichia coli

机译:Fh8标签:融合伴侣,可在大肠杆菌中进行简单且经济高效的蛋白质纯化

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摘要

Downstream processing is still a major bottleneck in recombinant protein production representing most of its costs. Hence, there is a continuing demand of novel and cost-effective purification processes aiming at the recovery of pure and active target protein. In this work, a novel purification methodology is presented, using the Fh8 solubility enhancer tag as fusion handle. The binding properties of Fh8 tag to a hydrophobic matrix were first studied via hydrophobic interaction chromatography (HIC). The Fh8 tag was then evaluated as a purification handle by its fusion to green fluorescent protein and superoxide dismutase. The purification efficiency of the Fh8-HIC strategy was compared to the immobilized metal ion affinity chromatography (IMAC) using the His6 tag. Results showed that the Fh8-HIC binding mechanism is calcium-dependent in a low salt medium, making the purification process highly selective. Both target proteins were biologically active, even when fused to Fh8, and were successfully purified by HIC, achieving efficiencies identical to those of IMAC. Thus, the Fh8 acts as an effective affinity tag that, together with its previously reported solubility enhancer capability, allows for the design of inexpensive and successful recombinant protein production processes in Escherichia coli.
机译:下游加工仍是重组蛋白生产的主要瓶颈,代表了其大部分成本。因此,持续需要新颖且具有成本效益的纯化方法,其目的是回收纯的和活性的靶蛋白。在这项工作中,提出了一种新颖的纯化方法,使用Fh8溶解度增强剂标签作为融合柄。 Fh8标签与疏水基质的结合特性首先通过疏水相互作用色谱法(HIC)研究。然后通过将Fh8标签与绿色荧光蛋白和超氧化物歧化酶融合来评估其纯化工艺。 Fh8-HIC策略的纯化效率与使用His6标签的固定金属离子亲和色谱(IMAC)进行了比较。结果表明,Fh8-HIC的结合机制在低盐培养基中是钙依赖性的,从而使纯化过程具有高度的选择性。两种靶蛋白均具有生物学活性,即使与Fh8融合也是如此,并已通过HIC成功纯化,获得了与IMAC相同的效率。因此,Fh8可作为有效的亲和标签,与其先前报道的溶解度增强剂功能一起,可用于设计大肠杆菌中廉价而成功的重组蛋白生产工艺。

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