Light-Induced Orthogonal Fragmentation of Crosslinked Peptides

Lars Kolbowski; Adam Belsom; Ana M. Pérez-López; Tony Ly; Juri Rappsilber

doi:10.1021/jacsau.3c00199

Light-Induced Orthogonal Fragmentation of Crosslinked Peptides

Lars Kolbowski, Adam Belsom, Ana M. Pérez-López, Tony Ly, Juri Rappsilber

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

Abstract

Crosslinking mass spectrometry provides pivotal information on the structure and interaction of proteins. MS-cleavable crosslinkers are regarded as a cornerstone for the analysis of complex mixtures. Yet they fragment under similar conditions as peptides, leading to mixed fragmentation spectra of the crosslinker and peptide. This hampers selecting individual peptides for their independent identification. Here, we introduce orthogonal cleavage using ultraviolet photodissociation (UVPD) to increase crosslinker over peptide fragmentation. We designed and synthesized a crosslinker that can be cleaved at 213 nm in a commercial mass spectrometer configuration. In an analysis of crosslinked Escherichia coli lysate, the crosslinker-to-peptide fragment intensity ratio increases from nearly 1 for a conventionally cleavable crosslinker to 5 for the UVPD-cleavable crosslinker. This largely increased the sensitivity of selecting the individual peptides for MS3, even more so with an improved doublet detection algorithm. Data are available via ProteomeXchange with identifier PXD040267.

Original language	English
Pages (from-to)	2123-2130
Number of pages	8
Journal	JACS Au
Volume	3
Issue number	8
DOIs	https://doi.org/10.1021/jacsau.3c00199
Publication status	Published - 28 Aug 2023

Keywords / Materials (for Non-textual outputs)

crosslinking mass spectrometry
ultraviolet photodissociation
peptide fragmentation
MS3-triggering
orthogonal cleavage

Access to Document

10.1021/jacsau.3c00199Licence: Creative Commons: Attribution (CC-BY)

jacsau.3c00199 (1)Final published version, 3.55 MBLicence: Creative Commons: Attribution (CC-BY)

Core funding for the Wellcome Centre for Cell Biology
Marston, A.
UK-based charities
1/12/21 → 30/11/23
Project: Research
Understanding the proliferation-quiescence switch using quantitative cellular biochemistry
Ly, T.
UK-based charities
1/10/17 → 30/11/20
Project: Research

Cite this

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title = "Light-Induced Orthogonal Fragmentation of Crosslinked Peptides",

abstract = "Crosslinking mass spectrometry provides pivotal information on the structure and interaction of proteins. MS-cleavable crosslinkers are regarded as a cornerstone for the analysis of complex mixtures. Yet they fragment under similar conditions as peptides, leading to mixed fragmentation spectra of the crosslinker and peptide. This hampers selecting individual peptides for their independent identification. Here, we introduce orthogonal cleavage using ultraviolet photodissociation (UVPD) to increase crosslinker over peptide fragmentation. We designed and synthesized a crosslinker that can be cleaved at 213 nm in a commercial mass spectrometer configuration. In an analysis of crosslinked Escherichia coli lysate, the crosslinker-to-peptide fragment intensity ratio increases from nearly 1 for a conventionally cleavable crosslinker to 5 for the UVPD-cleavable crosslinker. This largely increased the sensitivity of selecting the individual peptides for MS3, even more so with an improved doublet detection algorithm. Data are available via ProteomeXchange with identifier PXD040267.",

keywords = "crosslinking mass spectrometry, ultraviolet photodissociation, peptide fragmentation, MS3-triggering, orthogonal cleavage",

author = "Lars Kolbowski and Adam Belsom and P{\'e}rez-L{\'o}pez, {Ana M.} and Tony Ly and Juri Rappsilber",

note = "Funding Information: This research was funded by the Deutsche Forschungsgemeinschaft (DFG, German Research Foundation) under Germany′s Excellence Strategy–EXC 2008–390540038–UniSysCat and projects 426290502 and 449713269. The Wellcome Centre for Cell Biology is supported by core funding from the Wellcome Trust [203149] and Royal Society (Sir Henry Dale Fellowship to T.L., 206211/A/17/Z). For the purpose of open access, the author has applied a CC BY public copyright license to any author accepted manuscript version arising from this submission. Publisher Copyright: {\textcopyright} 2023 The Authors. Published by American Chemical Society",

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AU - Rappsilber, Juri

N1 - Funding Information: This research was funded by the Deutsche Forschungsgemeinschaft (DFG, German Research Foundation) under Germany′s Excellence Strategy–EXC 2008–390540038–UniSysCat and projects 426290502 and 449713269. The Wellcome Centre for Cell Biology is supported by core funding from the Wellcome Trust [203149] and Royal Society (Sir Henry Dale Fellowship to T.L., 206211/A/17/Z). For the purpose of open access, the author has applied a CC BY public copyright license to any author accepted manuscript version arising from this submission. Publisher Copyright: © 2023 The Authors. Published by American Chemical Society

PY - 2023/8/28

Y1 - 2023/8/28

N2 - Crosslinking mass spectrometry provides pivotal information on the structure and interaction of proteins. MS-cleavable crosslinkers are regarded as a cornerstone for the analysis of complex mixtures. Yet they fragment under similar conditions as peptides, leading to mixed fragmentation spectra of the crosslinker and peptide. This hampers selecting individual peptides for their independent identification. Here, we introduce orthogonal cleavage using ultraviolet photodissociation (UVPD) to increase crosslinker over peptide fragmentation. We designed and synthesized a crosslinker that can be cleaved at 213 nm in a commercial mass spectrometer configuration. In an analysis of crosslinked Escherichia coli lysate, the crosslinker-to-peptide fragment intensity ratio increases from nearly 1 for a conventionally cleavable crosslinker to 5 for the UVPD-cleavable crosslinker. This largely increased the sensitivity of selecting the individual peptides for MS3, even more so with an improved doublet detection algorithm. Data are available via ProteomeXchange with identifier PXD040267.

AB - Crosslinking mass spectrometry provides pivotal information on the structure and interaction of proteins. MS-cleavable crosslinkers are regarded as a cornerstone for the analysis of complex mixtures. Yet they fragment under similar conditions as peptides, leading to mixed fragmentation spectra of the crosslinker and peptide. This hampers selecting individual peptides for their independent identification. Here, we introduce orthogonal cleavage using ultraviolet photodissociation (UVPD) to increase crosslinker over peptide fragmentation. We designed and synthesized a crosslinker that can be cleaved at 213 nm in a commercial mass spectrometer configuration. In an analysis of crosslinked Escherichia coli lysate, the crosslinker-to-peptide fragment intensity ratio increases from nearly 1 for a conventionally cleavable crosslinker to 5 for the UVPD-cleavable crosslinker. This largely increased the sensitivity of selecting the individual peptides for MS3, even more so with an improved doublet detection algorithm. Data are available via ProteomeXchange with identifier PXD040267.

KW - crosslinking mass spectrometry

KW - ultraviolet photodissociation

KW - peptide fragmentation

KW - MS3-triggering

KW - orthogonal cleavage

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DO - 10.1021/jacsau.3c00199

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Light-Induced Orthogonal Fragmentation of Crosslinked Peptides

Abstract

Keywords / Materials (for Non-textual outputs)

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Projects

Core funding for the Wellcome Centre for Cell Biology

Understanding the proliferation-quiescence switch using quantitative cellular biochemistry

Cite this