Benchmarking Multiple Fragmentation Methods on an Orbitrap Fusion for Top-down Phospho-Proteoform Characterization

Benchmarking Multiple Fragmentation Methods on an Orbitrap Fusion for Top-down Phospho-Proteoform Characterization

Top-down analysis of intact proteins by mass spectrometry provides an ideal platform for comprehensive proteoform characterization, in particular, for the identification and localization of post-translational modifications (PTM) co-occurring on a protein. One of the main bottlenecks in top-down prot...

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Veröffentlicht in:Analytical chemistry (Washington) 2015-04, Vol.87 (8), p.4152-4158
Hauptverfasser: Brunner, Andrea M, Lössl, Philip, Liu, Fan, Huguet, Romain, Mullen, Christopher, Yamashita, Masami, Zabrouskov, Vlad, Makarov, Alexander, Altelaar, A. F. Maarten, Heck, Albert J. R
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Analytical chemistry
Aurora Kinase B - analysis
Aurora Kinase B - metabolism
Auroras
Benchmarking
Benchmarks
Fragmentation
Kinases
Localization
Mass Spectrometry
Phosphorylation
Position (location)
Proteins
Proteomics
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container_end_page 4158
container_issue 8
container_start_page 4152
container_title Analytical chemistry (Washington)
container_volume 87
creator Brunner, Andrea M
Lössl, Philip
Liu, Fan
Huguet, Romain
Mullen, Christopher
Yamashita, Masami
Zabrouskov, Vlad
Makarov, Alexander
Altelaar, A. F. Maarten
Heck, Albert J. R
description Top-down analysis of intact proteins by mass spectrometry provides an ideal platform for comprehensive proteoform characterization, in particular, for the identification and localization of post-translational modifications (PTM) co-occurring on a protein. One of the main bottlenecks in top-down proteomics is insufficient protein sequence coverage caused by incomplete protein fragmentation. Based on previous work on peptides, increasing sequence coverage and PTM localization by combining sequential ETD and HCD fragmentation in a single fragmentation event, we hypothesized that protein sequence coverage and phospho-proteoform characterization could be equally improved by this new dual fragmentation method termed EThcD, recently been made available on the Orbitrap Fusion. Here, we systematically benchmark the performance of several (hybrid) fragmentation methods for intact protein analysis on an Orbitrap Fusion, using as a model system a 17.5 kDa N-terminal fragment of the mitotic regulator Bora. During cell division Bora becomes multiply phosphorylated by a variety of cell cycle kinases, including Aurora A and Plk1, albeit at distinctive sites. Here, we monitor the phosphorylation of Bora by Aurora A and Plk1, analyzing the generated distinctive phospho-proteoforms by top-down fragmentation. We show that EThcD and ETciD on a Fusion are feasible and capable of providing richer fragmentation spectra compared to HCD or ETD alone, increasing protein sequence coverage, and thereby facilitating phosphosite localization and the determination of kinase specific phosphorylation sites in these phospho-proteoforms. Data are available via ProteomeXchange with identifier PXD001845.
doi_str_mv 10.1021/acs.analchem.5b00162
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subjects Analytical chemistry
Aurora Kinase B - analysis
Aurora Kinase B - metabolism
Auroras
Benchmarking
Benchmarks
Fragmentation
Kinases
Localization
Mass Spectrometry
Phosphorylation
Position (location)
Proteins
Proteomics
title Benchmarking Multiple Fragmentation Methods on an Orbitrap Fusion for Top-down Phospho-Proteoform Characterization
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