Streamlined on-column refolding and purification of nanobodies from inclusion bodies expressed as fusion proteins

IF 2.8 3区 医学 Q2 BIOCHEMICAL RESEARCH METHODS Journal of Chromatography B Pub Date : 2024-08-22 DOI:10.1016/j.jchromb.2024.124279
Yiwen Zhang , Yang Guo , Liang Song , Wenshuai Liu , Rui Nian , Xiying Fan
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Abstract

This study introduces an efficient on-column refolding and purification method for preparing nanobodies (Nbs) expressed as inclusion bodies and fusion proteins. The HisTrapTM FF system was successfully employed for the purification of the fusion protein FN1-ΔI-CM-2D5. The intein ΔI-CM cleavage activity was activated at 42 °C, followed by incubation for 4 h. Leveraging the remarkable thermal stability of Nbs, 2D5 was further purified through heat treatment at 80 °C for 1h. This method yielded up to 107.2 mg of pure 2D5 with a purity of 99.2 % from just 1L of bacterial culture grown in a shaker flask. Furthermore, this approach successfully restored native secondary structure and affinity of 2D5. Additionally, the platform was effectively applied to the refolding and purification of a polystyrene-binding nanobody (B2), which exhibited limited expression in the periplasmic and cytoplasmic spaces of E. coli. This endeavor resulted in the isolation of 53.2 mg of pure B2 Nb with a purity exceeding 99.5 % from the same volume of bacterial culture. Significantly, this approach restored the native secondary structure of the Nbs, highlighting its potential for addressing challenges associated with expressing complex Nbs in E. coli. Overall, this innovative platform provides a scientifically rigorous and reproducible method for the efficient preparation of Nbs, offering a valuable tool for antibody research and development.

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从表达为融合蛋白的包涵体中简化柱上重折叠和纯化纳米抗体。
本研究介绍了一种高效的柱上重折叠和纯化方法,用于制备以包涵体和融合蛋白形式表达的纳米抗体(Nbs)。HisTrapTM FF 系统被成功用于纯化融合蛋白 FN1-ΔI-CM-2D5。利用 Nbs 显著的热稳定性,将 2D5 在 80 °C 下加热处理 1 小时后进一步纯化。这种方法只需在摇瓶中培养 1 升细菌,就能得到 107.2 毫克纯 2D5,纯度高达 99.2%。此外,这种方法还成功恢复了 2D5 的原生二级结构和亲和力。此外,该平台还有效地应用于聚苯乙烯结合纳米抗体(B2)的重折叠和纯化,该纳米抗体在大肠杆菌的周质和细胞质空间中表达有限。通过这一努力,从相同体积的细菌培养物中分离出了 53.2 毫克纯净的 B2 Nb,纯度超过 99.5%。值得注意的是,这种方法恢复了 Nbs 的原生二级结构,凸显了它在解决与在大肠杆菌中表达复杂 Nbs 相关的挑战方面的潜力。总之,这一创新平台为高效制备 Nbs 提供了一种科学严谨、可重复的方法,为抗体研究和开发提供了一种宝贵的工具。
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来源期刊
Journal of Chromatography B
Journal of Chromatography B 医学-分析化学
CiteScore
5.60
自引率
3.30%
发文量
306
审稿时长
44 days
期刊介绍: The Journal of Chromatography B publishes papers on developments in separation science relevant to biology and biomedical research including both fundamental advances and applications. Analytical techniques which may be considered include the various facets of chromatography, electrophoresis and related methods, affinity and immunoaffinity-based methodologies, hyphenated and other multi-dimensional techniques, and microanalytical approaches. The journal also considers articles reporting developments in sample preparation, detection techniques including mass spectrometry, and data handling and analysis. Developments related to preparative separations for the isolation and purification of components of biological systems may be published, including chromatographic and electrophoretic methods, affinity separations, field flow fractionation and other preparative approaches. Applications to the analysis of biological systems and samples will be considered when the analytical science contains a significant element of novelty, e.g. a new approach to the separation of a compound, novel combination of analytical techniques, or significantly improved analytical performance.
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