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无鞘毛细管电泳-质谱法分离和分析完整单克隆抗体

Intact monoclonal antibodies separation and analysis by sheathless capillary electrophoresis-mass spectrometry.

作者信息

Giorgetti Jérémie, Lechner Antony, Del Nero Elise, Beck Alain, François Yannis-Nicolas, Leize-Wagner Emmanuelle

机构信息

1 Laboratoire de Spectrométrie de Masse des Interactions et des Systèmes (LSMIS) UMR 7140 (Unistra-CNRS), Université de Strasbourg, Strasbourg, France.

2 Centre d'immunologie Pierre Fabre, Saint-Julien-en-Genevois, France.

出版信息

Eur J Mass Spectrom (Chichester). 2019 Jun;25(3):324-332. doi: 10.1177/1469066718807798. Epub 2018 Oct 23.

DOI:10.1177/1469066718807798
PMID:30351978
Abstract

Capillary electrophoresis-mass spectrometry coupling is a growing technique in biopharmaceutics characterization. Assessment of monoclonal antibodies is well known at middle-up and bottom-up levels to obtain information about the sequence, post-translational modifications and degradation products. Intact protein analysis is an actual challenge to be closer to the real protein structure. At this level, actual techniques are time consuming or cumbersome processes. In this work, a 20 minutes separation method has been developed to optimize characterization of intact monoclonal antibodies. Thus, separation has been done on a positively charged coated capillary with optimized volatile background electrolyte and sample buffer. Three world-wide health authorities approved monoclonal antibodies have been used to set up a rapid and ease of use method. Intact trastuzumab, rituximab and palivizumab isoforms have been partially separated with this method in less than 20 minutes under denaturing conditions. For each monoclonal antibody, 2X-glycosylated and 1X-glycosylated structures have been identified and separated. Concerning basic and acidic variants, potential aspartic acid isomerization modification and asparagine deamidation have been observed. Accurate mass determination for high-mass molecular species remains a challenge, but the progress in intact monoclonal antibodies separation appears very promising for biopharmaceutics characterization.

摘要

毛细管电泳-质谱联用是生物制药表征中一种不断发展的技术。在中上游和下游水平对单克隆抗体进行评估以获取有关序列、翻译后修饰和降解产物的信息是众所周知的。完整蛋白质分析是一项实际挑战,目的是更接近真实的蛋白质结构。在此层面,现有的技术要么耗时,要么操作繁琐。在这项工作中,已开发出一种20分钟的分离方法,以优化完整单克隆抗体的表征。因此,在带有优化的挥发性背景电解质和样品缓冲液的带正电荷涂层毛细管上进行了分离。三种获得全球卫生当局批准的单克隆抗体被用于建立一种快速且易于使用的方法。在变性条件下,使用该方法在不到20分钟的时间内已部分分离出完整的曲妥珠单抗、利妥昔单抗和帕利珠单抗异构体。对于每种单克隆抗体,已鉴定并分离出2X-糖基化和1X-糖基化结构。关于碱性和酸性变体,已观察到潜在的天冬氨酸异构化修饰和天冬酰胺脱酰胺作用。对高质量分子物种进行精确质量测定仍然是一项挑战,但完整单克隆抗体分离方面的进展在生物制药表征中似乎非常有前景。

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