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Protein interaction landscapes revealed by advanced in vivo cross-linking–mass spectrometry
by
Rychnovsky, Scott D.
, Wang, Xiaorong
, Huang, Lan
, Yu, Clinton
, Chemmama, Ilan E.
, Kaake, Robyn M.
, Yang, Jing
, Wheat, Andrew
, Burke, Anthony M.
, Baker, Peter
in
Biochemistry
/ Biological Sciences
/ Chaperonins - analysis
/ Chaperonins - chemistry
/ Chaperonins - metabolism
/ Chemical synthesis
/ Click Chemistry - methods
/ Cross-Linking Reagents - chemistry
/ Crosslinking
/ HEK293 Cells
/ Histones - metabolism
/ Humans
/ Lysine
/ Lysine - chemistry
/ Mass spectrometry
/ Mass Spectrometry - methods
/ Mass spectroscopy
/ Multiprotein Complexes - chemistry
/ Peptide mapping
/ Peptides
/ Peptides - chemistry
/ Proteasome Endopeptidase Complex - metabolism
/ Protein interaction
/ Protein Interaction Mapping - methods
/ Protein structure
/ Proteins
/ Proteomes
/ Proteomics - methods
/ Reproducibility of Results
/ Sample preparation
/ Scientific imaging
/ Spectroscopy
/ Structure-function relationships
/ Ubiquitin - metabolism
2021
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Protein interaction landscapes revealed by advanced in vivo cross-linking–mass spectrometry
by
Rychnovsky, Scott D.
, Wang, Xiaorong
, Huang, Lan
, Yu, Clinton
, Chemmama, Ilan E.
, Kaake, Robyn M.
, Yang, Jing
, Wheat, Andrew
, Burke, Anthony M.
, Baker, Peter
in
Biochemistry
/ Biological Sciences
/ Chaperonins - analysis
/ Chaperonins - chemistry
/ Chaperonins - metabolism
/ Chemical synthesis
/ Click Chemistry - methods
/ Cross-Linking Reagents - chemistry
/ Crosslinking
/ HEK293 Cells
/ Histones - metabolism
/ Humans
/ Lysine
/ Lysine - chemistry
/ Mass spectrometry
/ Mass Spectrometry - methods
/ Mass spectroscopy
/ Multiprotein Complexes - chemistry
/ Peptide mapping
/ Peptides
/ Peptides - chemistry
/ Proteasome Endopeptidase Complex - metabolism
/ Protein interaction
/ Protein Interaction Mapping - methods
/ Protein structure
/ Proteins
/ Proteomes
/ Proteomics - methods
/ Reproducibility of Results
/ Sample preparation
/ Scientific imaging
/ Spectroscopy
/ Structure-function relationships
/ Ubiquitin - metabolism
2021
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Protein interaction landscapes revealed by advanced in vivo cross-linking–mass spectrometry
by
Rychnovsky, Scott D.
, Wang, Xiaorong
, Huang, Lan
, Yu, Clinton
, Chemmama, Ilan E.
, Kaake, Robyn M.
, Yang, Jing
, Wheat, Andrew
, Burke, Anthony M.
, Baker, Peter
in
Biochemistry
/ Biological Sciences
/ Chaperonins - analysis
/ Chaperonins - chemistry
/ Chaperonins - metabolism
/ Chemical synthesis
/ Click Chemistry - methods
/ Cross-Linking Reagents - chemistry
/ Crosslinking
/ HEK293 Cells
/ Histones - metabolism
/ Humans
/ Lysine
/ Lysine - chemistry
/ Mass spectrometry
/ Mass Spectrometry - methods
/ Mass spectroscopy
/ Multiprotein Complexes - chemistry
/ Peptide mapping
/ Peptides
/ Peptides - chemistry
/ Proteasome Endopeptidase Complex - metabolism
/ Protein interaction
/ Protein Interaction Mapping - methods
/ Protein structure
/ Proteins
/ Proteomes
/ Proteomics - methods
/ Reproducibility of Results
/ Sample preparation
/ Scientific imaging
/ Spectroscopy
/ Structure-function relationships
/ Ubiquitin - metabolism
2021
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Protein interaction landscapes revealed by advanced in vivo cross-linking–mass spectrometry
Journal Article
Protein interaction landscapes revealed by advanced in vivo cross-linking–mass spectrometry
2021
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Overview
Defining protein–protein interactions (PPIs) in their native environment is crucial to understanding protein structure and function. Cross-linking–mass spectrometry (XL-MS) has proven effective in capturing PPIs in living cells; however, the proteome coverage remains limited. Here, we have developed a robust in vivo XL-MS platformto facilitate in-depth PPI mapping by integrating a multifunctional MS-cleavable cross-linker with sample preparation strategies and high-resolution MS. The advancement of click chemistry–based enrichment significantly enhanced the detection of cross-linked peptides for proteome-wide analyses. This platform enabled the identification of 13,904 unique lysine–lysine linkages from in vivo cross-linked HEK 293 cells, permitting construction of the largest in vivo PPI network to date, comprising 6,439 interactions among 2,484 proteins. These results allowed us to generate a highly detailed yet panoramic portrait of human interactomes associated with diverse cellular pathways. The strategy presented here signifies a technological advancement for in vivo PPI mapping at the systems level and can be generalized for charting protein interaction landscapes in any organisms.
Publisher
National Academy of Sciences
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