An integrated workflow for crosslinking mass spectrometry
pmid: 31556486
pmc: PMC6753376
An integrated workflow for crosslinking mass spectrometry
We present a concise workflow to enhance the mass spectrometric detection of crosslinked peptides by introducing sequential digestion and the crosslink identification software Xi. Sequential digestion enhances peptide detection by selective shortening of long tryptic peptides. We demonstrate our simple 12-fraction protocol for crosslinked multi-protein complexes and cell lysates, quantitative analysis, and high-density crosslinking, without requiring specific crosslinker features. This overall approach reveals dynamic protein-protein interaction sites, which are accessible, have fundamental functional relevance and are therefore ideally suited for the development of small molecule inhibitors.
- Max Planck Society Germany
- Wellcome Trust United Kingdom
- Imperial College London United Kingdom
- Technische Universitat Berlin Germany
- MAX PLANCK INSTITUTE OF BIOCHEMISTRY
Models, Molecular, Proteomics, Medicine (General), Bioinformatics, QH301-705.5, Protein Conformation, 0699 Other Biological Sciences, protein-protein interactions, protein–protein interactions, 0601 Biochemistry and Cell Biology, Mass Spectrometry, proteomics, R5-920, Cytosol, Protein Interaction Mapping, Methods, structural biology, Humans, crosslinking mass spectrometry, Biology (General), software, Proteins, 540, Peptide Fragments, 620, K562 Cells, Software
Models, Molecular, Proteomics, Medicine (General), Bioinformatics, QH301-705.5, Protein Conformation, 0699 Other Biological Sciences, protein-protein interactions, protein–protein interactions, 0601 Biochemistry and Cell Biology, Mass Spectrometry, proteomics, R5-920, Cytosol, Protein Interaction Mapping, Methods, structural biology, Humans, crosslinking mass spectrometry, Biology (General), software, Proteins, 540, Peptide Fragments, 620, K562 Cells, Software
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