定量蛋白质组学
衍生化
细胞培养中氨基酸的稳定同位素标记
化学
肽
色谱法
蛋白质组学
钋
等压标记
同位素
溴化物
同位素标记
无标记量化
质谱法
生物化学
有机化学
物理
量子力学
基因
作者
Hongyan Shen,Mingrui An,Xiao Zou,Xuyang Zhao,Qingsong Wang,Guo‐wen Xing,Jianguo Ji
出处
期刊:Proteomics
[Wiley]
日期:2015-04-30
卷期号:15 (17): 2903-2909
被引量:5
标识
DOI:10.1002/pmic.201400495
摘要
N ‐succinimidyloxycarbonylmethyl tris (2,4,6‐trimethoxyphenyl) phosphonium bromide (TMPP‐Ac‐OSu) reacts rapidly, mildly, and specifically with the N‐terminals of proteins and peptides. Thus, it can be developed as an ideal isotope‐coded tag to be used in quantitative proteomics. Here, we present a strategy for light and heavy TMPP‐based quantitative proteomic analysis, in which peptides in a mixture can be quantified using an on‐tip TMPP derivatization approach. To demonstrate the accuracy of this strategy, light and heavy TMPP‐labeled peptides were combined at different ratios and subsequently analyzed by LC‐MS/MS. The MS spectra and scatter plots show that peptide and protein ratios were both consistent with the mixed ratios. We observed a linear correlation between protein ratios and the predicted ratios. In comparison with SILAC method, the TMPP labeling method produced similarly accurate quantitative results with low CVs. In conclusion, our results suggest that this isotope‐coded TMPP method achieved accurate quantification and compatibility with IEF‐based separation. With the inherent advantages of TMPP derivatization, we believe that it holds great promise for future applications in quantitative proteomics analysis.
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