XTract: Software for characterizing conformational changes of protein complexes by quantitative cross-linking mass spectrometry

Thomas Walzthoeni; Lukasz A. Joachimiak; George Rosenberger; Hannes L. Röst; Lars Malmström; Alexander Leitner; Judith Frydman; Ruedi Aebersold

doi:10.1038/nmeth.3631

XTract: Software for characterizing conformational changes of protein complexes by quantitative cross-linking mass spectrometry

Thomas Walzthoeni, Lukasz A. Joachimiak, George Rosenberger, Hannes L. Röst, Lars Malmström, Alexander Leitner, Judith Frydman, Ruedi Aebersold

Research output: Contribution to journal › Article › peer-review

67 Scopus citations

Abstract

Chemical cross-linking in combination with mass spectrometry generates distance restraints of amino acid pairs in close proximity on the surface of native proteins and protein complexes. In this study we used quantitative mass spectrometry and chemical cross-linking to quantify differences in cross-linked peptides obtained from complexes in spatially discrete states. We describe a generic computational pipeline for quantitative cross-linking mass spectrometry consisting of modules for quantitative data extraction and statistical assessment of the obtained results. We used the method to detect conformational changes in two model systems: firefly luciferase and the bovine TRiC complex. Our method discovers and explains the structural heterogeneity of protein complexes using only sparse structural information.

Original language	English (US)
Pages (from-to)	1185-1190
Number of pages	6
Journal	Nature methods
Volume	12
Issue number	12
DOIs	https://doi.org/10.1038/nmeth.3631
State	Published - Dec 1 2015
Externally published	Yes

ASJC Scopus subject areas

Biotechnology
Biochemistry
Molecular Biology
Cell Biology

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10.1038/nmeth.3631

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title = "XTract: Software for characterizing conformational changes of protein complexes by quantitative cross-linking mass spectrometry",

abstract = "Chemical cross-linking in combination with mass spectrometry generates distance restraints of amino acid pairs in close proximity on the surface of native proteins and protein complexes. In this study we used quantitative mass spectrometry and chemical cross-linking to quantify differences in cross-linked peptides obtained from complexes in spatially discrete states. We describe a generic computational pipeline for quantitative cross-linking mass spectrometry consisting of modules for quantitative data extraction and statistical assessment of the obtained results. We used the method to detect conformational changes in two model systems: firefly luciferase and the bovine TRiC complex. Our method discovers and explains the structural heterogeneity of protein complexes using only sparse structural information.",

author = "Thomas Walzthoeni and Joachimiak, {Lukasz A.} and George Rosenberger and R{\"o}st, {Hannes L.} and Lars Malmstr{\"o}m and Alexander Leitner and Judith Frydman and Ruedi Aebersold",

note = "Funding Information: This work was supported by the European Union 7th Framework project PROSPECTS (Proteomics Specification in Time and Space; grant HEALTH-F4-2008-201648). R.A. is supported by European Research Council (ERC) advanced grant “Proteomics v.3.0” (grant 233226), ERC advanced grant “Proteomics 4D—the proteome in context” (grant 670821) and ETH Zurich. We thank M. Beck (EMBL Heidelberg) for helpful discussions. Publisher Copyright: {\textcopyright} 2015 Nature America, Inc.",

year = "2015",

month = dec,

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doi = "10.1038/nmeth.3631",

language = "English (US)",

volume = "12",

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T2 - Software for characterizing conformational changes of protein complexes by quantitative cross-linking mass spectrometry

AU - Walzthoeni, Thomas

AU - Joachimiak, Lukasz A.

AU - Rosenberger, George

AU - Röst, Hannes L.

AU - Malmström, Lars

AU - Leitner, Alexander

AU - Frydman, Judith

AU - Aebersold, Ruedi

N1 - Funding Information: This work was supported by the European Union 7th Framework project PROSPECTS (Proteomics Specification in Time and Space; grant HEALTH-F4-2008-201648). R.A. is supported by European Research Council (ERC) advanced grant “Proteomics v.3.0” (grant 233226), ERC advanced grant “Proteomics 4D—the proteome in context” (grant 670821) and ETH Zurich. We thank M. Beck (EMBL Heidelberg) for helpful discussions. Publisher Copyright: © 2015 Nature America, Inc.

PY - 2015/12/1

Y1 - 2015/12/1

N2 - Chemical cross-linking in combination with mass spectrometry generates distance restraints of amino acid pairs in close proximity on the surface of native proteins and protein complexes. In this study we used quantitative mass spectrometry and chemical cross-linking to quantify differences in cross-linked peptides obtained from complexes in spatially discrete states. We describe a generic computational pipeline for quantitative cross-linking mass spectrometry consisting of modules for quantitative data extraction and statistical assessment of the obtained results. We used the method to detect conformational changes in two model systems: firefly luciferase and the bovine TRiC complex. Our method discovers and explains the structural heterogeneity of protein complexes using only sparse structural information.

AB - Chemical cross-linking in combination with mass spectrometry generates distance restraints of amino acid pairs in close proximity on the surface of native proteins and protein complexes. In this study we used quantitative mass spectrometry and chemical cross-linking to quantify differences in cross-linked peptides obtained from complexes in spatially discrete states. We describe a generic computational pipeline for quantitative cross-linking mass spectrometry consisting of modules for quantitative data extraction and statistical assessment of the obtained results. We used the method to detect conformational changes in two model systems: firefly luciferase and the bovine TRiC complex. Our method discovers and explains the structural heterogeneity of protein complexes using only sparse structural information.

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XTract: Software for characterizing conformational changes of protein complexes by quantitative cross-linking mass spectrometry

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