2009
DOI: 10.1074/mcp.m800232-mcp200
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Identification of Protein-Protein Interactions and Topologies in Living Cells with Chemical Cross-linking and Mass Spectrometry

Abstract: We present results from a novel strategy that enables concurrent identification of protein-protein interactions and topologies in living cells without specific antibodies or genetic manipulations for immuno-/affinity purifications. The strategy consists of ( 1 or a single (e.g. FLAG tag (2)) or double affinity tag (e.g. TAP tag (3, 4)) followed by protein identification with mass spectrometry, protein microarray technology (5, 6), and computational prediction methods (7,8). Although all these approaches demons… Show more

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Cited by 142 publications
(172 citation statements)
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“…Using the protein interaction reporter concept based on gas phase cleavable, affinity tagged crosslinking reagents, Bruce and coworkers have shown applications to a diverse range of organisms such as Shewanella oneidensis [111], Escherichia coli [112 114], Pseudomonas aeruginosa [115], and even human cell lines [116]; other groups have reported similar concepts [117 119]. Recently, the group of Bruce also demonstrated that a quantitative dimension can be added to proteome wide crosslinking data with the help of metabolic stable isotope labeling [120].…”
Section: Box 1 Crosslinking Of Protein Network and Whole Proteomesmentioning
confidence: 99%
“…Using the protein interaction reporter concept based on gas phase cleavable, affinity tagged crosslinking reagents, Bruce and coworkers have shown applications to a diverse range of organisms such as Shewanella oneidensis [111], Escherichia coli [112 114], Pseudomonas aeruginosa [115], and even human cell lines [116]; other groups have reported similar concepts [117 119]. Recently, the group of Bruce also demonstrated that a quantitative dimension can be added to proteome wide crosslinking data with the help of metabolic stable isotope labeling [120].…”
Section: Box 1 Crosslinking Of Protein Network and Whole Proteomesmentioning
confidence: 99%
“…However, these strategies tend not to simultaneously produce sequence ions that would identify the peptide. This leaves the identity of the peptides to be inferred by precursor mass alone (46,47) or requires non-standard instrumentation that permits multiple stages of dissociation (29). With electron transfer dissociation, DEB cross-linking not only produces sequence ions efficiently but also releases the individual molecular ions at equivalent intensity.…”
Section: Cross-linking By Debmentioning
confidence: 99%
“…This can be achieved by the comparison of systematic interaction changes upon a specific stimuli or perturbation using cross-linking snapshots. Some pioneer studies have been applied in bacterial cells [8,10,24]. Another direction is quantitative crosslinking.…”
Section: Conclusion and Perspectivementioning
confidence: 99%
“…First and foremost, cross-linking can take a snap-shot of real-time dynamic interaction networks on the scale of the entire interactome in vitro and in vivo [8][9][10]. Also, cross-linking can not only identify the direct interacting partners but also determine the interaction sites at the same time.…”
Section: Strengths and Challenges Of Chemical Cross-linking Mass Specmentioning
confidence: 99%