Affinity peptide ligands: new tools for chasing non-canonical N-phosphoproteome

IF 7.6 1区化学 Q1 CHEMISTRY, MULTIDISCIPLINARY

Chemical Science Pub Date : 2025-04-25 DOI:10.1039/d5sc01557j

He Wang, Xiaoyu Zhang, Dongdong Wang, Qianqian Jiang, Yue Sun, Baofeng Zhao, Zhen Liang, Guangyan Qing, Bo Jiang, Lihua Zhang, Yukui Zhang

{"title":"Affinity peptide ligands: new tools for chasing non-canonical N-phosphoproteome","authors":"He Wang, Xiaoyu Zhang, Dongdong Wang, Qianqian Jiang, Yue Sun, Baofeng Zhao, Zhen Liang, Guangyan Qing, Bo Jiang, Lihua Zhang, Yukui Zhang","doi":"10.1039/d5sc01557j","DOIUrl":null,"url":null,"abstract":"The enrichment of protein N-phosphorylation encounters substantial challenges due to the inherent instability of the N–P bond, severely impeding the manifestation of its biological functions. Traditional enrichment methods often rely on antibodies, organic solvents and metal ion interactions, which are limited by lack of universality, potential degradation of sample integrity, or reduced selectivity for N-phosphorylation. To overcome these challenges, we innovatively capitalized phage display technology to identify affinity peptides that specifically bind to the N–PO3 group. By functionalizing magnetic nanoparticles with the affinity peptide, we developed a novel, organic solvent- and metal-free enrichment strategy that enhanced both the selectivity and efficiency for all three types of N-phosphopeptide capture under neutral conditions, ensuring superior preservation of sample integrity and allowing more accurate proteomic analysis. This strategy has demonstrated robust enrichment capabilities for both prokaryotic and eukaryotic samples. In HeLa cells, 1995 novel N-phosphorylation sites were identified, representing a substantial increase of 2- to 5-fold in detection depth over previous approaches and significantly expanding the scale of the N-phosphoproteome database. Additionally, it was discovered that N-phosphorylation modification was highly concentrated in the nucleus. By integrating the nuclear isolation technique, 1296 N-phosphorylation sites were identified for the first time, offering new leads for uncovering the functions of N-phosphorylation in nuclear proteins. Finally, in conjunction with the quantitative proteomics method, the dynamic changes in N-phosphorylation modification during the progression of Alzheimer's disease were investigated, providing fresh perspectives on the research of AD pathogenesis. Overall, this work not only presents a new approach for efficient enrichment of N-phosphopeptides but also advances the functional study of N-phosphorylated proteins in physiological and pathological processes.","PeriodicalId":9909,"journal":{"name":"Chemical Science","volume":"1 1","pages":""},"PeriodicalIF":7.6000,"publicationDate":"2025-04-25","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"0","resultStr":null,"platform":"Semanticscholar","paperid":null,"PeriodicalName":"Chemical Science","FirstCategoryId":"92","ListUrlMain":"https://doi.org/10.1039/d5sc01557j","RegionNum":1,"RegionCategory":"化学","ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"Q1","JCRName":"CHEMISTRY, MULTIDISCIPLINARY","Score":null,"Total":0}

引用次数: 0

Abstract

The enrichment of protein N-phosphorylation encounters substantial challenges due to the inherent instability of the N–P bond, severely impeding the manifestation of its biological functions. Traditional enrichment methods often rely on antibodies, organic solvents and metal ion interactions, which are limited by lack of universality, potential degradation of sample integrity, or reduced selectivity for N-phosphorylation. To overcome these challenges, we innovatively capitalized phage display technology to identify affinity peptides that specifically bind to the N–PO₃ group. By functionalizing magnetic nanoparticles with the affinity peptide, we developed a novel, organic solvent- and metal-free enrichment strategy that enhanced both the selectivity and efficiency for all three types of N-phosphopeptide capture under neutral conditions, ensuring superior preservation of sample integrity and allowing more accurate proteomic analysis. This strategy has demonstrated robust enrichment capabilities for both prokaryotic and eukaryotic samples. In HeLa cells, 1995 novel N-phosphorylation sites were identified, representing a substantial increase of 2- to 5-fold in detection depth over previous approaches and significantly expanding the scale of the N-phosphoproteome database. Additionally, it was discovered that N-phosphorylation modification was highly concentrated in the nucleus. By integrating the nuclear isolation technique, 1296 N-phosphorylation sites were identified for the first time, offering new leads for uncovering the functions of N-phosphorylation in nuclear proteins. Finally, in conjunction with the quantitative proteomics method, the dynamic changes in N-phosphorylation modification during the progression of Alzheimer's disease were investigated, providing fresh perspectives on the research of AD pathogenesis. Overall, this work not only presents a new approach for efficient enrichment of N-phosphopeptides but also advances the functional study of N-phosphorylated proteins in physiological and pathological processes.

Abstract Image

查看原文本刊更多论文

亲和肽配体：追踪非典型n-磷蛋白质组的新工具

由于N-P键固有的不稳定性，蛋白质n -磷酸化的富集遇到了很大的挑战，严重阻碍了其生物学功能的发挥。传统的富集方法通常依赖于抗体、有机溶剂和金属离子相互作用，这些方法由于缺乏通用性、可能降低样品完整性或降低n -磷酸化的选择性而受到限制。为了克服这些挑战，我们创新地利用噬菌体展示技术来鉴定特异性结合N-PO3基团的亲和肽。通过将磁性纳米颗粒与亲和肽功能化，我们开发了一种新型的有机溶剂和无金属富集策略，提高了在中性条件下捕获所有三种n -磷酸肽的选择性和效率，确保了样品完整性的良好保存，并允许更准确的蛋白质组学分析。该策略已被证明对原核和真核生物样品具有强大的富集能力。在HeLa细胞中，鉴定出了1995个新的n -磷酸化位点，比以前的方法检测深度增加了2- 5倍，并显著扩大了n -磷酸化蛋白质组数据库的规模。此外，还发现n -磷酸化修饰高度集中在细胞核中。通过整合核分离技术，首次鉴定出1296个n -磷酸化位点，为揭示n -磷酸化在核蛋白中的功能提供了新的线索。最后，结合定量蛋白质组学方法，研究了阿尔茨海默病进展过程中n -磷酸化修饰的动态变化，为AD发病机制的研究提供了新的视角。总之，这项工作不仅为n -磷酸化肽的高效富集提供了新的途径，而且推动了n -磷酸化蛋白在生理和病理过程中的功能研究。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

求助全文

约1分钟内获得全文求助全文

来源期刊

Chemical Science CHEMISTRY, MULTIDISCIPLINARY-

CiteScore

14.40

自引率

4.80%

发文量

1352

审稿时长

2.1 months

期刊介绍： Chemical Science is a journal that encompasses various disciplines within the chemical sciences. Its scope includes publishing ground-breaking research with significant implications for its respective field, as well as appealing to a wider audience in related areas. To be considered for publication, articles must showcase innovative and original advances in their field of study and be presented in a manner that is understandable to scientists from diverse backgrounds. However, the journal generally does not publish highly specialized research.