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克服单克隆抗体非还原肽图分析中人为二硫键错配的实用解决方案。

Practical solutions for overcoming artificial disulfide scrambling in the non-reduced peptide mapping characterization of monoclonal antibodies.

机构信息

Department of Analytical Chemistry, Regeneron Pharmaceuticals, Inc, Tarrytown, NY, USA.

出版信息

MAbs. 2024 Jan-Dec;16(1):2420805. doi: 10.1080/19420862.2024.2420805. Epub 2024 Oct 26.

Abstract

Non-reduced peptide mapping provides essential data for characterizing therapeutic monoclonal antibodies by isolating disulfide connections between specific cysteines. However, conventional digestive strategies used throughout the biopharmaceutical industry have been shown to cause unintentional rearrangement of disulfide connections (disulfide scrambling), thus generating connectivity profiles that do not accurately represent the protein being analyzed. Common misconceptions (e.g. avoiding basic-pH digestion to prevent disulfide scrambling) have led to the development of alternative reagents and conditions that can alleviate this issue, but yield problematic digestion profiles. Herein, we systematically and comprehensively examine the primary considerations for accurate non-reduced peptide mapping, and provide effective, practical solutions to minimize undesired behavior while still yielding high-quality digests. Additionally, we present a method that exploits intentional disulfide scrambling as a reference tool to demonstrate the robustness of our proposed strategies. We also introduce maleimide as a cysteine-alkylating reagent and demonstrate its benefits over industry-leading analogs such as N-ethylmaleimide in terms of compatibility with regulatory reports.

摘要

非还原肽图分析通过分离特定半胱氨酸之间的二硫键连接,为鉴定治疗性单克隆抗体提供了重要数据。然而,已证实整个生物制药行业中使用的传统消化策略会导致二硫键连接的无意重排(二硫键错配),从而产生与正在分析的蛋白质不相符的连接谱。常见的误解(例如避免碱性 pH 消化以防止二硫键错配)导致了替代试剂和条件的开发,这些试剂和条件可以缓解这个问题,但会产生有问题的消化谱。在此,我们系统而全面地检查了准确的非还原肽图分析的主要考虑因素,并提供了有效的实用解决方案,以最小化不良行为,同时仍能获得高质量的消化物。此外,我们提出了一种利用有意二硫键错配作为参考工具的方法,以证明我们提出的策略的稳健性。我们还介绍了马来酰亚胺作为半胱氨酸烷化试剂,并证明了其在与监管报告的兼容性方面优于行业领先的类似物(如 N-乙基马来酰亚胺)的优势。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2621/11520568/d1cb00da2dc6/KMAB_A_2420805_F0001_OC.jpg

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