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在本氏烟中瞬时表达的 IgG 融合蛋白的生产。

Production of IgG Fusion Proteins Transiently Expressed in Nicotiana benthamiana.

机构信息

Center for Immunotherapy, Vaccines and Virotherapy, The Biodesign Institute, Arizona State University; School of Life Sciences, Arizona State University; Molecular Biosciences/Biotechnology Undergraduate Program, Arizona State University.

Center for Immunotherapy, Vaccines and Virotherapy, The Biodesign Institute, Arizona State University; School of Life Sciences, Arizona State University; Department of Microbiology and Immunology, University of Michigan Medical School.

出版信息

J Vis Exp. 2021 Jan 16(167). doi: 10.3791/61774.

DOI:10.3791/61774
PMID:33522504
Abstract

High demand for antibodies as therapeutic interventions for various infectious, metabolic, autoimmune, neoplastic, and other diseases creates a growing need in developing efficient methods for recombinant antibody production. As of 2019, there were more than 70 FDA-approved monoclonal antibodies, and there is exponential growth potential. Despite their promise, limiting factors for widespread use are manufacturing costs and complexity. Potentially, plants offer low-cost, safe, and easily scalable protein manufacturing strategies. Plants like Nicotiana benthamiana not only can correctly fold and assemble complex mammalian proteins but also can add critical post-translational modifications similar to those offered by mammalian cell cultures. In this work, by using native GFP and an acid-stable variant of green fluorescent protein (GFP) fused to human monoclonal antibodies, we were able to visualize the entire transient antibody expression and purification process from N. benthamiana plants. Depending on the experiment's purpose, native GFP fusion can ensure easier visualization during the expression phase in the plants, while acid-stable GFP fusion allows for visualization during downstream processing. This scalable and straightforward procedure can be performed by a single researcher to produce milligram quantities of highly pure antibody or antibody fusion proteins in a matter of days using only a few small plants. Such a technique can be extended to the visualization of any type of antibody purification process and potentially many other proteins, both in plant and other expression systems. Moreover, these techniques can benefit virtual instructions and be executed in a teaching laboratory by undergraduate students possessing minimal prior experience with molecular biology techniques, providing a foundation for project-based exploration with real-world applications.

摘要

对作为各种传染性、代谢性、自身免疫性、肿瘤性和其他疾病治疗干预的抗体的高需求,为开发用于重组抗体生产的有效方法创造了日益增长的需求。截至 2019 年,已有超过 70 种 FDA 批准的单克隆抗体,并且具有指数级增长潜力。尽管它们具有前景,但广泛使用的限制因素是制造成本和复杂性。植物可能提供低成本、安全且易于扩展的蛋白质制造策略。像 Nicotiana benthamiana 这样的植物不仅可以正确折叠和组装复杂的哺乳动物蛋白,还可以添加类似于哺乳动物细胞培养物提供的关键翻译后修饰。在这项工作中,通过使用天然 GFP 和与人单克隆抗体融合的绿色荧光蛋白(GFP)的酸稳定变体,我们能够可视化来自 N. benthamiana 植物的整个瞬时抗体表达和纯化过程。根据实验的目的,天然 GFP 融合可以确保在植物中的表达阶段更容易可视化,而酸稳定 GFP 融合则允许在下游处理过程中可视化。这种可扩展且简单的程序可以由单个研究人员执行,仅使用少数几株小植物,在几天内生产毫克量的高度纯抗体或抗体融合蛋白。这种技术可以扩展到任何类型的抗体纯化过程的可视化,并且可能还有许多其他蛋白质,包括植物和其他表达系统中的蛋白质。此外,这些技术可以受益于虚拟指令,并由具有分子生物学技术最低先验经验的本科生在教学实验室中执行,为具有实际应用的基于项目的探索提供基础。

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