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一种带有用于亲和纯化IgG的肽配体的大孔材料。

A megaporous material harbouring a peptide ligand for affinity IgG purification.

作者信息

Tehrani Najafian Foad, Bibi Noor Shad, Islam Tuhidul, Fernández-Lahore Marcelo

机构信息

Jacobs University Bremen, Bremen D-28759, Germany.

出版信息

Electrophoresis. 2017 Nov;38(22-23):2914-2921. doi: 10.1002/elps.201700198. Epub 2017 Sep 15.

DOI:10.1002/elps.201700198
PMID:28833255
Abstract

Common limitations of Protein A affinity chromatography include high adsorbent costs, ligand instability and possible ligand leakage. In this study, a short peptide with affinity for IgG was synthesized chemically and subsequently immobilized on a megaporous support. The support was prepared utilising the cryogel technique while the peptide-ligand was covalently immobilised via thiol-epoxy click chemistry. The cryogel support was chemically grafted to increase the number of reaction sites. This adsorbent was designated as "MP-Pep". Adsorption isotherms were employed to evaluate protein binding capacity. A maximum static binding capacity within the range of 30-60 mg/mL was observed for hIgG. This parameter compares well with other commercial and non-commercial adsorbents, as reported in the literature. As a control material, a Protein A grafted megaporous cryogel was synthesized. Dynamic binding capacity values were obtained by breakthrough analysis. The peptide cryogel showed a dynamic capacity value 9.0 mg/mL in comparison to 9.7 mg/mL in the case of the Protein A based adsorbent. The ratio of dynamic binding capacity to static binding capacity was 20%, indicating suboptimal product capture. However, the advantage of MP-Pep lies in its cost-effective preparations while maintaining a reasonable binding capacity for the targeted product. The presence of cooperative effects during protein binding could also represent an advantage during the processing of a feedstock containing a product in high concentration.

摘要

蛋白A亲和色谱的常见局限性包括吸附剂成本高、配体不稳定以及可能的配体泄漏。在本研究中,化学合成了一种对IgG具有亲和力的短肽,随后将其固定在大孔载体上。载体采用冷冻凝胶技术制备,而肽配体通过硫醇-环氧点击化学共价固定。对冷冻凝胶载体进行化学接枝以增加反应位点的数量。这种吸附剂被命名为“MP-Pep”。采用吸附等温线来评估蛋白质结合能力。对于人IgG,观察到最大静态结合能力在30-60mg/mL范围内。如文献报道,该参数与其他商业和非商业吸附剂相比具有优势。作为对照材料,合成了一种接枝有蛋白A的大孔冷冻凝胶。通过穿透分析获得动态结合能力值。肽冷冻凝胶的动态结合能力值为9.0mg/mL,而基于蛋白A的吸附剂为9.7mg/mL。动态结合能力与静态结合能力的比率为20%,表明产物捕获效果欠佳。然而,MP-Pep的优势在于其制备成本效益高,同时对目标产物保持合理的结合能力。在蛋白质结合过程中协同效应的存在,在处理含有高浓度产物的原料时也可能是一个优势。

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