Chloride-Mediated Peroxide-Free Photochemical Oxidation of Proteins (PPOP) in Mass Spectrometry-Based Structural Analysis.
Pan LuoZheyi LiuTingting ZhangXiaolei WangJing LiuYiqiang LiuXiaohu ZhouYang ChenWenrui DongChunlei XiaoYan JinXueming YangFang-Jun WangPublished in: Analytical chemistry (2021)
Ultraviolet (UV) laser photolysis of hydrogen peroxide (H 2 O 2 ) for the in situ generation of hydroxyl radicals ( • OH) is a widely utilized strategy in the oxidation footprinting of native proteins and mass spectrometry (MS)-based structural analysis. However, it remains challenging to realize peroxide-free photochemical oxidation footprinting. Herein, we describe the footprinting of native proteins by chloride-mediated peroxide-free photochemical oxidation of proteins (PPOP). The protein samples are prepared within biocompatible phosphate-buffered saline (PBS) containing 10 mM Gln as radical scavengers and oxidized in a capillary flow reactor directly under a single-pulse (10 ns) irradiation of a 193 nm ArF UV laser. The main oxidized protein residues are CMYWFHLI. We demonstrate that the PPOP-MS strategy is highly sensitive to the protein high-order structures and can be applied to monitor the protein-drug interfaces, which provides a promising footprinting alternative for protein structure-function explorations.
Keyphrases
- hydrogen peroxide
- mass spectrometry
- protein protein
- amino acid
- multiple sclerosis
- binding protein
- liquid chromatography
- high resolution
- nitric oxide
- blood pressure
- emergency department
- capillary electrophoresis
- small molecule
- high performance liquid chromatography
- photodynamic therapy
- high speed
- single molecule
- radiation induced
- electron transfer
- molecularly imprinted
- electronic health record
- fluorescent probe
- tandem mass spectrometry
- anaerobic digestion