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采用源内碎裂和 CID MS/MS 相结合的方法阐明聚乙二醇化位点。

Elucidation of PEGylation site with a combined approach of in-source fragmentation and CID MS/MS.

机构信息

Bioproduct Research and Development, Lilly Research Laboratories, Eli Lilly and Company, Lilly Corporate Center, Indianapolis, Indiana 46285, USA.

出版信息

J Am Soc Mass Spectrom. 2010 May;21(5):810-8. doi: 10.1016/j.jasms.2010.01.011. Epub 2010 Jan 25.

Abstract

Poly(ethylene glycol) (PEG)ylation of peptides and proteins creates significant challenges for detailed structural characterization, such as PEG heterogeneity, site of addition and number of attached PEGylated moieties. Recently, we published a novel LC/MS methodology with a post-column addition of amines to obtain accurate masses of PEGylated peptides and proteins. The accurate masses can be used to assign the structures and number of attached PEGs [15], but the PEGylation site remains unclear in situations where multiple potential attachments are involved. Here, we present a methodology combining in-source fragmentation (ISF) with CID-MS/MS to elucidate the PEGylated sites in PEGylated products. All PEGylated samples, either prepared in acidic solution, or collected from a RP-HPLC stream, were first ionized via ISF to produce products containing small PEG fragment attachment, and then those fragment ions obtained were sequenced via CID MS/MS to deduce the PEGylation site. The methodology was successfully applied to PEGylated glucagon and IgG4 antibody light chain, which demonstrated that the small PEG fragments attached were stable during the CID activation.

摘要

聚乙二醇(PEG)化的肽和蛋白质对详细的结构特征分析造成了巨大的挑战,如 PEG 的不均一性、加成位置和连接的 PEG 化部分的数量。最近,我们发表了一种新型的 LC/MS 方法,通过在柱后添加胺来获得 PEG 化肽和蛋白质的精确质量。精确的质量可用于分配结构和连接的 PEG 数量[15],但在涉及多个潜在连接点的情况下,PEG 化位点仍然不清楚。在这里,我们提出了一种结合源内碎裂(ISF)和 CID-MS/MS 的方法,以阐明 PEG 化产物中的 PEG 化位点。所有 PEG 化样品,无论是在酸性溶液中制备的,还是从反相高效液相色谱流中收集的,首先通过 ISF 进行离子化,产生含有小 PEG 片段连接的产物,然后通过 CID MS/MS 对这些片段离子进行测序,以推断 PEG 化位点。该方法成功应用于 PEG 化胰高血糖素和 IgG4 抗体轻链,证明在 CID 激活过程中连接的小 PEG 片段是稳定的。

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