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通过多维 LC/MS 对重组单克隆抗体进行靶向从头分析。

Targeted Bottom-up Characterization of Recombinant Monoclonal Antibodies by Multidimensional LC/MS.

机构信息

Protein Analytical Chemistry, Genentech, 1 DNA Way, South San Francisco, California 94080, United States.

School of Pharmaceutical Sciences, University of Geneva, CMU, Rue Michel-Servet, 1, 1206 Geneva, Switzerland.

出版信息

Anal Chem. 2020 Oct 6;92(19):13420-13426. doi: 10.1021/acs.analchem.0c02780. Epub 2020 Sep 18.

DOI:10.1021/acs.analchem.0c02780
PMID:32901474
Abstract

On-line bottom-up approaches have recently emerged as promising alternatives to standard off-line processes for characterizing post-translational modifications (PTMs) of therapeutic monoclonal antibodies (mAbs). The benefits of on-line processing include reductions in required sample amount and sample handling, as well as reducing the overall turnaround time. However, shortening digestion time for the on-line approach of an intact mAb can cause incomplete peptide cleavages, leading to low sequence coverage and poor repeatability of analyses. For the first time, we describe a novel, automated targeted bottom-up strategy consisting of reducing the complexity of intact mAb by digesting the product into small ∼25 kDa fragments, followed by an on-line peptide mapping analysis of each fragment. For this purpose, a four-dimensional-liquid chromatography/mass spectrometry (4D-LC/MS) method was developed using an immobilized -high-performance liquid chromatography (HPLC) column as a first dimension (D) for on-line digestion, followed by a (D) on-column reversed-phase liquid chromatography (RPLC) for reduction and fragments separation. Then, only one fragment was selected for digestion using a (D) immobilized trypsin cartridge and, finally, the obtained peptides were analyzed by (D) RPLC-MS. This strategy considerably improved the on-line digestion efficiency with higher sequence coverages (LC and HC >97%), thus allowing various PTMs including oxidation, deamidation, and isomerization located in the complementarity-determining regions (CDRs), as well as -glycans present on the Fc/2 fragment, to be monitored with similar sensitivity to those obtained with standard off-line approaches. Additional investigations at a middle-up level were also performed via a three-dimensional-LC/MS (3D-LC/MS) approach within the same system, demonstrating the feasibility to achieve a multilevel comprehensive characterization of mAbs.

摘要

在线自下而上的方法最近作为一种很有前途的替代方法出现,用于对治疗性单克隆抗体 (mAb) 的翻译后修饰 (PTM) 进行离线标准过程进行特征描述。在线处理的好处包括减少所需的样品量和样品处理量,以及减少整体周转时间。然而,缩短完整 mAb 的在线方法的消化时间可能会导致肽裂解不完全,从而导致序列覆盖率低和分析重复性差。我们首次描述了一种新颖的、自动化的靶向自下而上策略,该策略通过将产物消化成小的约 25 kDa 片段来降低完整 mAb 的复杂性,然后对每个片段进行在线肽图谱分析。为此,开发了一种四维度液相色谱/质谱 (4D-LC/MS) 方法,该方法使用固定化高效液相色谱 (HPLC) 柱作为在线消化的第一维 (D),然后进行 (D) 柱上反相液相色谱 (RPLC) 用于还原和片段分离。然后,仅使用一个片段使用固定化胰蛋白酶筒进行消化,最后通过 (D) RPLC-MS 分析获得的肽。该策略极大地提高了在线消化效率,具有更高的序列覆盖率 (LC 和 HC>97%),从而允许包括氧化、脱酰胺和异构化在内的各种 PTM 位于互补决定区 (CDR) 中,以及 Fc/2 片段上的 -聚糖,与使用标准离线方法获得的灵敏度相似。还通过同一系统内的三维液相色谱/质谱 (3D-LC/MS) 方法在中量级水平上进行了额外的研究,证明了实现 mAb 多级综合特征描述的可行性。

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