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Hybrid mass spectrometry methods reveal lot-to-lot differences and delineate the effects of glycosylation on the tertiary structure of Herceptin®

机译:混合质谱方法揭示了批次间的差异并描述了糖基化对Herceptin®三级结构的影响

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摘要

To quantify the measurable variations in the structure of a biopharmaceutical product we systematically evaluate three lots of Herceptin®, two mAb standards and an intact Fc-hinge fragment. Each mAb is examined in three states; glycan intact, truncated (following endoS2 treatment) and fully deglycosylated. Despite equivalence at the intact protein level, each lot of Herceptin® gives a distinctive signature in three different mass spectrometry approaches. Ion mobility mass spectrometry (IM-MS) shows that in the API, the attached N-glycans reduce the conformational spread of each mAb by 10.5–25%. Hydrogen/deuterium exchange mass spectrometry (HDX-MS) data support this, with lower global deuterium uptake in solution when comparing intact to the fully deglycosylated protein. HDX-MS and activated IM-MS map the influence of glycans on the mAb and reveal allosteric effects which extend far beyond the Fc domains into the Fab region. Taken together, these findings and the supplied interactive data sets establish acceptance criteria with application for MS based characterisation of biosimilars and novel therapeutic mAbs.
机译:为了量化生物制药产品结构中可测量的变化,我们系统地评估了三批Herceptin®,两种mAb标准品和完整的Fc铰链片段。每个mAb均以三种状态进行检查:完整的聚糖,被截短(在endoS2处理之后)并完全去糖基化。尽管在完整蛋白水平上是等效的,但每批Herceptin®在三种不同的质谱方法中均具有独特的特征。离子迁移质谱(IM-MS)表明,在API中,附着的N-聚糖使每个mAb的构象分布降低了10.5-25%。氢/氘交换质谱(HDX-MS)数据支持这一点,与完整的去糖基化蛋白质进行比较时,溶液中的总氘吸收较低。 HDX-MS和激活的IM-MS绘制了聚糖对mAb的影响,并揭示了变构作用,该变构作用远远超出了Fc结构域进入Fab区。总之,这些发现和提供的交互式数据集建立了基于MS的生物仿制药和新型治疗性mAb表征应用的接受标准。

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