A Glycosidic‐Bond‐Based Mass‐Spectrometry‐Cleavable Cross‐linker Enables In Vivo Cross‐linking for Protein Complex Analysis

Author:

Chen Jing12,Zhao Qun1,Gao Hang13,Zhao Lili13,Chu Huiying4,Shan Yichu1,Liang Zhen1,Zhang Yukui1,Zhang Lihua1ORCID

Affiliation:

1. CAS Key Labratory of Separation Science for Analytical Chemistry Dalian Institute of Chemical Physics Chinese Academy of Sciences 457 Zhongshan Road Dalian 116023 China

2. School of Chemistry and Material Science University of Science and Technology of China 96 Jinzhai Road Hefei 230026 China

3. University of Chinese Academy of Sciences Beijing 100039 China

4. Laboratory of Molecular Modeling and Design State Key Laboratory of Molecular Reaction Dynamics Dalian Institute of Chemical Physics Chinese Academy of Sciences 457 Zhongshan Road Dalian 116023 China

Abstract

AbstractChemical cross‐linking mass spectrometry (CXMS) has emerged as a powerful technology to analyze protein complexes. However, the progress of in vivo CXMS studies has been limited by cross‐linking biocompatibility and data analysis. Herein, a glycosidic bond‐based MS‐cleavable cross‐linker of trehalose disuccinimidyl ester (TDS) was designed and synthesized, which was fragmented in MS under CID/HCD to simplify the cross‐linked peptides into conventional single peptides via selective cleavage between glycosidic and peptide bonds under individual MS collision energy. Consequently, the cross‐linking identification accuracy and throughput were significantly enhanced, and the popular MS mode of stepped HCD was allowed. In addition, TDS showed proper cell‐penetrating properties while being highly water‐soluble, making it non‐DMSO dependent during solubilization. Collectively, TDS provides a promising toolkit for CXMS characterization of living systems with high biocompatibility and accuracy.

Funder

National Key Research and Development Program of China

Publisher

Wiley

Subject

General Medicine

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