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采用化学分析联合质谱技术鉴定大肠杆菌表达的 rhGM-CSF 中新型+70 Da 修饰。

Characterization of a novel + 70 Da modification in rhGM-CSF expressed in E. coli using chemical assays in combination with mass spectrometry.

机构信息

Universitätsklinikum Hamburg-Eppendorf (UKE), Hamburg, Germany.

Alphalyse A/S, Odense, Denmark.

出版信息

Amino Acids. 2022 Apr;54(4):601-613. doi: 10.1007/s00726-021-03004-9. Epub 2021 Aug 28.

Abstract

Granulocyte-macrophage colony-stimulating factor (GM-CSF) is a cytokine and a white blood cell growth factor that has found usage as a therapeutic protein. During analysis of different fermentation batches of GM-CSF recombinantly expressed in E. coli, a covalent modification was identified on the protein by intact mass spectrometry. The modification gave a mass shift of + 70 Da and peptide mapping analysis demonstrated that it located to the protein N-terminus and lysine side chains. The chemical composition of CHO was found to be the best candidate by peptide fragmentation using tandem mass spectrometry. The modification likely contains a carbonyl group, since the mass of the modification increased by 2 Da by reduction with borane pyridine complex and it reacted with 2,4-dinitrophenylhydrazine. On the basis of chemical and tandem mass spectrometry fragmentation behavior, the modification could be attributed to crotonaldehyde, a reactive compound formed during lipid peroxidation. A low recorded oxygen pressure in the reactor during protein expression could be linked to the formation of this compound. This study shows the importance of maintaining full control over all reaction parameters during recombinant protein production.

摘要

粒细胞-巨噬细胞集落刺激因子(GM-CSF)是一种细胞因子和白细胞生长因子,已被用作治疗蛋白。在分析大肠杆菌中重组表达的 GM-CSF 的不同发酵批次时,通过完整质谱法鉴定到蛋白质上存在一种共价修饰。该修饰导致分子量增加了 70 Da,肽图分析表明它位于蛋白质的 N 端和赖氨酸侧链上。通过串联质谱法的肽片段分析,发现 CHO 的化学组成是最佳候选物。由于用硼烷吡啶复合物还原后修饰增加了 2 Da,并且与 2,4-二硝基苯肼反应,因此修饰可能包含羰基。根据化学和串联质谱法的片段化行为,该修饰可以归因于丙烯醛,这是脂质过氧化过程中形成的一种反应性化合物。在蛋白质表达过程中记录到的反应器中氧压低可能与该化合物的形成有关。这项研究表明在重组蛋白生产过程中保持对所有反应参数的完全控制的重要性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/83ca/9117350/3d478267d177/726_2021_3004_Fig1_HTML.jpg

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