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全自动毛细管等电聚焦-质谱联用超高分辨技术用于鉴定完整蛋白质复合物的微异质性和等电点。

Automated Capillary Isoelectric Focusing-Mass Spectrometry with Ultrahigh Resolution for Characterizing Microheterogeneity and Isoelectric Points of Intact Protein Complexes.

机构信息

Department of Chemistry, Michigan State University, 578 S Shaw Lane, East Lansing, Michigan 48824, Unites States.

New Biological Entities (NBE), Analytical R&D, AbbVie Inc., 1 Waukegan Rd, North Chicago, Illinois 60064, United States.

出版信息

Anal Chem. 2022 Jul 12;94(27):9674-9682. doi: 10.1021/acs.analchem.2c00975. Epub 2022 Jun 29.

DOI:10.1021/acs.analchem.2c00975
PMID:35766479
Abstract

Protein complexes are the functional machines in the cell and are heterogeneous due to protein sequence variations and post-translational modifications (PTMs). Here, we present an automated nondenaturing capillary isoelectric focusing-mass spectrometry (ncIEF-MS) methodology for uncovering the microheterogeneity of intact protein complexes. The method exhibited superior separation resolution for protein complexes than conventional native capillary zone electrophoresis (nCZE-MS). In our study, ncIEF-MS achieved liquid-phase separations and MS characterization of seven different forms of a streptavidin homotetramer with variations of N-terminal methionine removal, acetylation, and formylation and four forms of the carbonic anhydrase-zinc complex arising from variations of PTMs (succinimide, deamidation, etc.). In addition, ncIEF-MS resolved different states of an interchain cysteine-linked antibody-drug conjugate (ADC1) as a new class of anticancer therapeutic agents that bears a distribution of varied drug-to-antibody ratio (DAR) species. More importantly, ncIEF-MS enabled precise measurements of isoelectric points (pIs) of protein complexes, which reflect the surface electrostatic properties of protein complexes. We studied how protein sequence variations/PTMs modulate the pIs of protein complexes and how drug loading affects the pIs of antibodies. We discovered that keeping the N-terminal methionine residue of one subunit of the streptavidin homotetramer decreased its pI by 0.1, adding one acetyl group onto the streptavidin homotetramer reduced its pI by nearly 0.4, incorporating one formyl group onto the streptavidin homotetramer reduced its pI by around 0.3, and loading two more drug molecules on one ADC1 molecule increased its pI by 0.1. The data render the ncIEF-MS method a valuable tool for delineating protein complexes.

摘要

蛋白质复合物是细胞中的功能机器,由于蛋白质序列的变异和翻译后修饰(PTMs)而具有异质性。在这里,我们提出了一种自动化的非变性毛细管等电聚焦-质谱(ncIEF-MS)方法,用于揭示完整蛋白质复合物的微观异质性。该方法对蛋白质复合物的分离分辨率优于传统的天然毛细管区带电泳(nCZE-MS)。在我们的研究中,ncIEF-MS 实现了七种不同形式的链霉亲和素四聚体的液相分离和 MS 特征分析,这些四聚体在 N 端甲硫氨酸缺失、乙酰化和甲酰化以及碳酸酐酶-锌复合物的四个形式上存在差异,这些差异源于 PTMs 的变化(琥珀酰亚胺、脱酰胺等)。此外,ncIEF-MS 还解析了一种链间半胱氨酸连接的抗体药物偶联物(ADC1)的不同状态,ADC1 作为一种新型抗癌治疗药物,具有不同药物抗体比(DAR)物种的分布。更重要的是,ncIEF-MS 能够精确测量蛋白质复合物的等电点(pI),这反映了蛋白质复合物的表面静电特性。我们研究了蛋白质序列的变异/PTMs 如何调节蛋白质复合物的 pI,以及药物加载如何影响抗体的 pI。我们发现,保持链霉亲和素四聚体一个亚基的 N 端甲硫氨酸残基可使其 pI 降低 0.1,在链霉亲和素四聚体上添加一个乙酰基可使其 pI 降低近 0.4,在链霉亲和素四聚体上添加一个甲酰基可使其 pI 降低约 0.3,在一个 ADC1 分子上再加载两个药物分子可使其 pI 增加 0.1。这些数据表明,ncIEF-MS 方法是描绘蛋白质复合物的一种有价值的工具。

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