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微量肽段样品TMPP标记中过量标记试剂清除技术研究

李紫琳张振鹏吕志堂徐平

分析化学2026，Vol.54Issue(3)：411-420,10.

分析化学2026，Vol.54Issue(3)：411-420,10.DOI:10.19756/j.issn.0253-3820.251328

微量肽段样品TMPP标记中过量标记试剂清除技术研究

Technical Research on Removal of Excess TMPP in Sample Preparation of TMPP-Labeled Peptides

李紫琳 ¹张振鹏 ²吕志堂 ³徐平¹

作者信息

1. 河北大学生命科学学院,河北省微生物多样性研究与应用重点实验室,微生物育种与保育河北省工程中心,保定 071002||中国医学科学院蛋白组学与新药研发创新单元,国家蛋白质科学中心(北京),医学蛋白质组学全国重点实验室,北京 102206
2. 中国医学科学院蛋白组学与新药研发创新单元,国家蛋白质科学中心(北京),医学蛋白质组学全国重点实验室,北京 102206
3. 河北大学生命科学学院,河北省微生物多样性研究与应用重点实验室,微生物育种与保育河北省工程中心,保定 071002
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摘要

Abstract

The labeling reagent(N-Succinimidyloxycarbonylmethyl)tris(2,4,6-trimethoxyphenyl)phosphonium bromide(TMPP-Ac-Osu,abbreviated as TMPP)effectively enhances peptide ionization efficiency and mass spectrometric(MS)detection sensitivity,enabling deep-coverage immunopeptidomic analysis.However,the efficient removal of excess TMPP remains challenging and severely interferes with liquid chromatography(LC)separation and subsequent MS analysis.In this study,an efficient MS sample preparation strategy was established to address residual TMPP contamination during the purification of TMPP-labeled peptides.Using a labeling system with a TMPP-to-peptide mass ratio of 2:1,peptide retention and TMPP removal efficiencies of three commonly used desalting materials,C18,strong cation exchange(SCX),and strong anion exchange(SAX)columns,were systematically compared.Residual TMPP was quantitatively evaluated by extracting characteristic chromatographic peaks and comparing signal intensities and peak areas.SAX achieved a peptide retention efficiency of 84.1%,second only to C18(88.9%),while exhibiting the most effective TMPP removal,with a 184-fold reduction in residual TMPP signal relative to C18.Moreover,SAX-processed peptides showed lower background noise,higher signal-to-noise ratios,improved spectral quality,and higher peptide confidence scores.Collectively,the results indicated that SAX was an optimal sample preparation method for TMPP-labeled peptides,enabling efficient removal of excess labeling reagent and ensuring high-quality immunopeptide identification.This strategy provided a robust methodological foundation for the scalable application of TMPP labeling in immunopeptidomics and related fields.

关键词

N-琥珀酰亚胺基[三(2,4,6-三甲氧苯基)磷基]溴乙酸酯标记/强阴离子交换/质谱前处理/样品前处理/肽段纯化

Key words

(N-Succinimidyloxycarbonylmethyl)tris(2,4,6-trimethoxyphenyl)phosphonium bromide labeling/Strong anion exchange/Mass spectrometry sample preparation/Sample pretreatment/Sample pre-processing/Peptide purification

引用本文复制引用

李紫琳,张振鹏,吕志堂,徐平..微量肽段样品TMPP标记中过量标记试剂清除技术研究[J].分析化学,2026,54(3):411-420,10.

基金项目

国家自然科学基金项目(No.32371503)资助. Supported by the National Natural Science Foundation of China(No.32371503). （No.32371503）

分析化学

ISSN：0253-3820

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