Nilvebrant Johan, Alm Tove, Hober Sophia
School of Biotechnology, Department of Proteomics, Royal Institute of Technology.
J Vis Exp. 2012 Jan 16(59):3370. doi: 10.3791/3370.
Due to the high costs associated with purification of recombinant proteins the protocols need to be rationalized. For high-throughput efforts there is a demand for general methods that do not require target protein specific optimization . To achieve this, purification tags that genetically can be fused to the gene of interest are commonly used. The most widely used affinity handle is the hexa-histidine tag, which is suitable for purification under both native and denaturing conditions. The metabolic burden for producing the tag is low, but it does not provide as high specificity as competing affinity chromatography based strategies. Here, a bispecific purification tag with two different binding sites on a 46 amino acid, small protein domain has been developed. The albumin-binding domain is derived from Streptococcal protein G and has a strong inherent affinity to human serum albumin (HSA). Eleven surface-exposed amino acids, not involved in albumin-binding, were genetically randomized to produce a combinatorial library. The protein library with the novel randomly arranged binding surface (Figure 1) was expressed on phage particles to facilitate selection of binders by phage display technology. Through several rounds of biopanning against a dimeric Z-domain derived from Staphylococcal protein A, a small, bispecific molecule with affinity for both HSA and the novel target was identified. The novel protein domain, referred to as ABDz1, was evaluated as a purification tag for a selection of target proteins with different molecular weight, solubility and isoelectric point. Three target proteins were expressed in Escherishia coli with the novel tag fused to their N-termini and thereafter affinity purified. Initial purification on either a column with immobilized HSA or Z-domain resulted in relatively pure products. Two-step affinity purification with the bispecific tag resulted in substantial improvement of protein purity. Chromatographic media with the Z-domain immobilized, for example MabSelect SuRe, are readily available for purification of antibodies and HSA can easily be chemically coupled to media to provide the second matrix. This method is especially advantageous when there is a high demand on purity of the recovered target protein. The bifunctionality of the tag allows two different chromatographic steps to be used while the metabolic burden on the expression host is limited due to the small size of the tag. It provides a competitive alternative to so called combinatorial tagging where multiple tags are used in combination.
由于重组蛋白纯化成本高昂,因此需要对实验方案进行优化。对于高通量研究,需要通用方法,而无需针对目标蛋白进行特定优化。为实现这一目标,通常使用可通过基因融合到目标基因上的纯化标签。使用最广泛的亲和配基是六组氨酸标签,它适用于天然和变性条件下的纯化。产生该标签的代谢负担较低,但与基于亲和色谱的竞争策略相比,其特异性不高。在此,已开发出一种双特异性纯化标签,该标签在一个由46个氨基酸组成的小蛋白结构域上具有两个不同的结合位点。白蛋白结合结构域源自链球菌蛋白G,对人血清白蛋白(HSA)具有很强的固有亲和力。将11个不参与白蛋白结合的表面暴露氨基酸进行基因随机化处理,以产生一个组合文库。具有新型随机排列结合表面的蛋白文库(图1)在噬菌体颗粒上表达,以便通过噬菌体展示技术筛选结合剂。通过针对源自葡萄球菌蛋白A的二聚体Z结构域进行几轮生物淘选,鉴定出一种对HSA和新型靶标均具有亲和力的小双特异性分子。将这种新型蛋白结构域称为ABDz1,并将其作为纯化标签用于一系列具有不同分子量、溶解度和等电点的目标蛋白。三种目标蛋白在大肠杆菌中表达,新型标签融合在其N端,然后进行亲和纯化。在固定化HSA或Z结构域的柱上进行初步纯化可得到相对纯的产物。使用双特异性标签进行两步亲和纯化可显著提高蛋白纯度。例如,固定化Z结构域的色谱介质(如MabSelect SuRe)可随时用于抗体纯化,并且HSA可轻松化学偶联到介质上以提供第二种基质。当对回收的目标蛋白纯度要求很高时,该方法特别有利。标签的双功能性允许使用两个不同的色谱步骤,同时由于标签尺寸小,对表达宿主的代谢负担有限。它为所谓的组合标签(其中多个标签组合使用)提供了一种有竞争力的替代方案。
