Isobaric Stable Isotope N‐Phosphorylation Labeling (iSIPL) for Ultrasensitive Proteome Quantification

细胞培养中氨基酸的稳定同位素标记 定量蛋白质组学 化学 蛋白质组学 等压标记 磷酸肽 质谱法 蛋白质组 磷酸化 串联质谱法 计算生物学 色谱法 生物化学 生物 基因
作者
Xiaoyu Wang,Chun‐Jing Chen,Yaohui He,Lian‐Shuai Ding,Yifan Wu,Cheng‐Ting Huang,Jun Wu,Rong Ding,Yuhua Xue,Zhiwei Lin,Pengxiang Xu,Yile Wu,Wen Liu,Jijun Li,Siming Chen,Yufen Zhao,Jiyang Dong,Qiang Zhou,Xiang Gao
出处
期刊:Angewandte Chemie [Wiley]
卷期号:62 (22) 被引量:3
标识
DOI:10.1002/anie.202303656
摘要

Stable isotope chemical labeling methods have been widely used for high-throughput mass spectrometry (MS)-based quantitative proteomics in biological and clinical applications. However, the existing methods are far from meeting the requirements for high sensitivity detection. In the present study, a novel isobaric stable isotope N-phosphorylation labeling (iSIPL) strategy was developed for quantitative proteome analysis. The tryptic peptides were selectively labeled with iSIPL tag to generate the novel reporter ions containing phosphoramidate P-N bond with high intensities under lower collision energies. iSIPL strategy are suitable for peptide sequencing and quantitative analysis with high sensitivity and accuracy even for samples of limited quantity. Furthermore, iSIPL coupled with affinity purification and mass spectrometry was applied to measure the dynamics of cyclin dependent kinase 9 (CDK9) interactomes during transactivation of the HIV-1 provirus. The interaction of CDK9 with PARP13 was found to significantly decrease during Tat-induced activation of HIV-1 gene transcription, suggesting the effectiveness of iSIPL strategy in dynamic analysis of protein-protein interaction in vivo. More than that, the proposed iSIPL strategy would facilitate large-scale accurate quantitative proteomics by increasing multiplexing capability.
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