Lysine-specific chemical cross-linking of protein complexes and identification of cross-linking sites using LC-MS/MS and the xQuest/xProphet software pipeline

被引:0
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作者
Alexander Leitner
Thomas Walzthoeni
Ruedi Aebersold
机构
[1] Institute of Molecular Systems Biology,Department of Biology
[2] Eidgenössische Technische Hochschule (ETH) Zürich,undefined
[3] PhD Program in Molecular Life Sciences,undefined
[4] University of Zurich–ETH Zurich,undefined
[5] Faculty of Science,undefined
[6] University of Zurich,undefined
来源
Nature Protocols | 2014年 / 9卷
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摘要
Chemical cross-linking in combination with LC-MS/MS (XL-MS) is an emerging technology to obtain low-resolution structural (distance) restraints of proteins and protein complexes. These restraints can also be used to characterize protein complexes by integrative modeling of the XL-MS data, either in combination with other types of structural information or by themselves, to establish spatial relationships of subunits in protein complexes. Here we present a protocol that has been successfully used to generate XL-MS data from a multitude of native proteins and protein complexes. It includes the experimental steps for performing the cross-linking reaction using disuccinimidyl suberate (a homobifunctional, lysine-reactive cross-linking reagent), the enrichment of cross-linked peptides by peptide size-exclusion chromatography (SEC; to remove smaller, non-cross-linked peptides), instructions for tandem MS analysis and the analysis of MS data via the open-source computational software pipeline xQuest and xProphet (available from http://proteomics.ethz.ch). Once established, this robust protocol should take ∼4 d to complete, and it is generally applicable to purified proteins and protein complexes.
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页码:120 / 137
页数:17
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