Trifunctional cross-linker for mapping protein-protein interaction networks and comparing protein conformational states

To improve chemical cross-linking of proteins coupled with mass spectrometry (CXMS), we developed a lysine-targeted enrichable cross-linker containing a biotin tag for affinity purification, a chemical cleavage site to separate cross-linked peptides away from biotin after enrichment, and a spacer ar...

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Veröffentlicht in:eLife 2016-03, Vol.5
Hauptverfasser: Tan, Dan, Li, Qiang, Zhang, Mei-Jun, Liu, Chao, Ma, Chengying, Zhang, Pan, Ding, Yue-He, Fan, Sheng-Bo, Tao, Li, Yang, Bing, Li, Xiangke, Ma, Shoucai, Liu, Junjie, Feng, Boya, Liu, Xiaohui, Wang, Hong-Wei, He, Si-Min, Gao, Ning, Ye, Keqiong, Dong, Meng-Qiu, Lei, Xiaoguang
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Sprache:eng
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Zusammenfassung:To improve chemical cross-linking of proteins coupled with mass spectrometry (CXMS), we developed a lysine-targeted enrichable cross-linker containing a biotin tag for affinity purification, a chemical cleavage site to separate cross-linked peptides away from biotin after enrichment, and a spacer arm that can be labeled with stable isotopes for quantitation. By locating the flexible proteins on the surface of 70S ribosome, we show that this trifunctional cross-linker is effective at attaining structural information not easily attainable by crystallography and electron microscopy. From a crude Rrp46 immunoprecipitate, it helped identify two direct binding partners of Rrp46 and 15 protein-protein interactions (PPIs) among the co-immunoprecipitated exosome subunits. Applying it to E. coli and C. elegans lysates, we identified 3130 and 893 inter-linked lysine pairs, representing 677 and 121 PPIs. Using a quantitative CXMS workflow we demonstrate that it can reveal changes in the reactivity of lysine residues due to protein-nucleic acid interaction.
ISSN:2050-084X
2050-084X
DOI:10.7554/eLife.12509