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用于定量16重蛋白质组学的新型等压标记试剂

New Set of Isobaric Labeling Reagents for Quantitative 16Plex Proteomics.

作者信息

Ning Xiaolian, Li Qidan, Zi Jin, Mei Zhanlong, Liu Jie, Zhang Yuxing, Bi Mao, Ren Yan, Liu Xingang, Lv Chao, Yao Hequan, Sun Jianguo, Rao Feng, Li Shuwei, Liu Siqi

机构信息

College of Life Sciences, University of Chinese Academy of Sciences, Beijing 100049, China.

BGI-Shenzhen, Shenzhen, Guangdong 518083, China.

出版信息

Anal Chem. 2023 Apr 4;95(13):5788-5795. doi: 10.1021/acs.analchem.3c00235. Epub 2023 Mar 23.

DOI:10.1021/acs.analchem.3c00235
PMID:36958307
Abstract

Peptide labeling by isobaric tags is a powerful approach for the relative quantitative analysis of proteomes in multiple groups. There has been a revolution in the innovation of new isobaric reagents; however, great effort is being made to expand simultaneous labeling groups to identify more labeled peptides and reduce reporter ion signal suppression. We redesigned the original chemical structure of the deuterium isobaric amine-reactive tag developed in our laboratory. We optimized the synthetic pathway to create a new set of 16-plex isobaric tags (IBT-16plex). The novel reagent enabled almost complete labeling of peptides within 90 min, with all labeling reporter ions exhibiting comparable MS/MS signals. Compared to a typical 16plex reagent, TMTpro-16plex, the peptides and proteins identified by IBT-16plex in trypsinized HeLa cells were significantly increased by 14.8 and 8.6%, respectively. Moreover, differences in peptide abundance within 10-fold among multiple groups were barely suppressed in IBT-16plex, whereas the dynamic range in TMTpro-16plex-labeled groups was smaller. After quantitative examination of MCF7 cell proteins, IBT-16plex was confirmed as feasible and useful for evaluating protein responses of glucose-starved MCF7 cells to a glucose-rich medium.

摘要

使用等压标签进行肽段标记是一种用于多组蛋白质组相对定量分析的强大方法。新型等压试剂的创新取得了革命性进展;然而,人们正在付出巨大努力来扩大同时标记的组数,以识别更多标记的肽段并减少报告离子信号抑制。我们重新设计了我们实验室开发的氘代等压胺反应性标签的原始化学结构。我们优化了合成途径,创建了一组新的16重等压标签(IBT-16plex)。这种新型试剂能够在90分钟内几乎完全标记肽段,所有标记的报告离子都表现出可比的串联质谱信号。与典型的16重试剂TMTpro-16plex相比,IBT-16plex在胰蛋白酶消化的HeLa细胞中鉴定出的肽段和蛋白质分别显著增加了14.8%和8.6%。此外,IBT-16plex几乎没有抑制多组中10倍以内肽段丰度的差异,而TMTpro-16plex标记组的动态范围较小。在对MCF7细胞蛋白质进行定量检测后,IBT-16plex被证实对于评估葡萄糖饥饿的MCF7细胞对富含葡萄糖培养基的蛋白质反应是可行且有用的。

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