Fast Fluoroalkylation of Proteins Uncovers the Structure and Dynamics of Biological Macromolecules.
Lukáš FojtíkJan FialaPetr PompachJosef ChmelíkVáclav MatoušekPetr BeierZdeněk KukačkaPetr NovákPublished in: Journal of the American Chemical Society (2021)
Covalent labeling of proteins in combination with mass spectrometry has been established as a complementary technique to classical structural methods, such as X-ray, NMR, or cryogenic electron microscopy (Cryo-EM), used for protein structure determination. Although the current covalent labeling techniques enable the protein solvent accessible areas with sufficient spatial resolution to be monitored, there is still high demand for alternative, less complicated, and inexpensive approaches. Here, we introduce a new covalent labeling method based on fast fluoroalkylation of proteins (FFAP). FFAP uses fluoroalkyl radicals formed by reductive decomposition of Togni reagents with ascorbic acid to label proteins on a time scale of seconds. The feasibility of FFAP to effectively label proteins was demonstrated by monitoring the differential amino acids modification of native horse heart apomyoglobin/holomyoglobin and the human haptoglobin-hemoglobin complex. The obtained data confirmed the Togni reagent-mediated FFAP is an advantageous alternative method for covalent labeling in applications such as protein footprinting and epitope mapping of proteins (and their complexes) in general. Data are accessible via the ProteomeXchange server with the data set identifier PXD027310.
Keyphrases
- high resolution
- amino acid
- mass spectrometry
- electron microscopy
- electronic health record
- protein protein
- magnetic resonance imaging
- heart failure
- magnetic resonance
- big data
- endothelial cells
- liquid chromatography
- machine learning
- binding protein
- small molecule
- computed tomography
- artificial intelligence
- data analysis
- atrial fibrillation
- simultaneous determination
- gas chromatography
- pluripotent stem cells