Internal Fragment Ions Disambiguate and Increase Identifications in Top-Down Proteomics

2021 ◽  
Author(s):  
Zach Rolfs ◽  
Lloyd M. Smith
Keyword(s):  
Top Down ◽  
Fragment Ions ◽  
Internal Fragment

scholarly journals Using 10,000 Fragment Ions to Inform Scoring in Native Top-down Proteomics

2020 ◽  
Vol 31 (7) ◽  
pp. 1398-1409 ◽  
Author(s):  
Ashley N. Ives ◽  
Taojunfeng Su ◽  
Kenneth R. Durbin ◽  
Bryan P. Early ◽  
Henrique dos Santos Seckler ◽  
...  
Keyword(s):  
Top Down ◽  
Fragment Ions

scholarly journals TDFragMapper: a visualization tool for evaluating experimental parameters in top-down proteomics

2021 ◽  
Author(s):  
Jonathan Steven Dhenin ◽  
Diogo Borges Lima ◽  
Mathieu Dupre ◽  
Julia Chamot-Rooke
Keyword(s):  
Software Tool ◽  
Rapid Evaluation ◽  
Visualization Tool ◽  
Sequence Coverage ◽  
Top Down ◽  
Intact Proteins ◽  
Fragment Ions ◽  
Experimental Parameters ◽  
Demonstration Video

We present a new software-tool allowing an easy visualization of fragment ions and thus a rapid evaluation of key experimental parameters on the sequence coverage obtained for the MS/MS analysis of intact proteins. Our tool can deal with multiple fragmentation methods. We demonstrate that TDFragMapper can rapidly highlight the experimental fragmentation parameters that are critical to the characterization of intact proteins of various size using top-down proteomics. TDFragMapper, a demonstration video and user tutorial are freely available at https://msbio.pasteur.fr/tdfragmapper, for academic use; all data are thus available from the ProteomeXchange consorti-um (identifier PXD024643).

Isotope Depletion Mass Spectrometry (ID-MS) for Enhanced Top-Down Protein Fragmentation

2018 ◽  
Author(s):  
Kelly J. Gallagher ◽  
Michael Palasser ◽  
Sam Hughes ◽  
C. Logan Mackay ◽  
David P. A. Kilgour ◽  
...  
Keyword(s):  
Mass Spectrometry ◽  
Molecular Mass ◽  
Posttranslational Modifications ◽  
Recombinant Expression ◽  
Expression System ◽  
Single Amino Acid ◽  
Sequence Coverage ◽  
Top Down ◽  
Fragment Ions ◽  
Signal Overlap

<div>Top-down mass spectrometry has become an important technique for the identification of proteins and characterisation of chemical and posttranslational modifications. However, as the molecular mass of proteins increases intact mass determination and top-down fragmentation efficiency become more challenging due to the partitioning of the mass spectral signal into many isotopic peaks. In large proteins, this results in reduced sensitivity and increased spectral complexity and signal overlap. This phenomenon is a consequence of the natural isotopic heterogeneity of the elements which comprise proteins (notably 13C). Here we present a bacterial recombinant expression system for the production of proteins depleted in 13C and 15N and use this strategy to prepare a range of isotopically depleted proteins. High resolution MS of isotope depleted proteins reveal dramatically reduced isotope distributions, which results in increases in sensitivity and deceased spectral complexity. We demonstrate that the monoisotopic signal is observed in mass spectra of proteins up to ~50 kDa. This allows confident assignment of accurate molecular mass, and facile detection of low mass modifications (such as deamidation). We outline the benefits of this isotope depletion strategy for top-down fragmentation. The reduced spectral complexity alleviates problems of signal overlap; the presence of monoisotopic signals allow more accurate assignment of fragment ions; and the dramatic increase in single-to-noise ratio (up to 7-fold increases) permits vastly reduced data acquisition times. Together, these compounding benefits allow the assignment of ca. 3-fold more fragment ions than analysis of proteins with natural isotopic abundances. Thus, more comprehensive sequence coverage can be achieved; we demonstrate near single amino-acid resolution of the 29 kDa protein carbonic anhydrase from a single top-down MS experiment. Finally, we demonstrate that the ID-MS strategy allows far greater sequence coverage to be obtained in time limited top-down data acquisitions – highlighting potential advantages for top-down LC-MS/MS workflows and top-down proteomics. </div><div><br></div>

scholarly journals The Ups and Downs of Repeated Cleavage and Internal Fragment Production in Top-Down Proteomics

2017 ◽  
Vol 29 (1) ◽  
pp. 150-157 ◽  
Author(s):  
Yana A. Lyon ◽  
Dylan Riggs ◽  
Luca Fornelli ◽  
Philip D. Compton ◽  
Ryan R. Julian
Keyword(s):  
Top Down ◽  
Fragment Production ◽  
Internal Fragment

scholarly journals ClipsMS: An Algorithm for Analyzing Internal Fragments Resulting from Top-Down Mass Spectrometry

2021 ◽  
Author(s):  
Carter Lantz ◽  
Muhammad A. Zenaidee ◽  
Benqian Wei ◽  
Zachary Hemminger ◽  
Rachel R. Ogorzalek Loo ◽  
...  
Keyword(s):  
Mass Spectrum ◽  
Protein Sequence ◽  
Sequence Coverage ◽  
Top Down ◽  
Mass Spectrum Analysis ◽  
Single Top ◽  
Product Ions ◽  
Methionine Residues ◽  
Protein Fragmentation ◽  
Internal Fragment

<p>Here we describe ClipsMS, an algorithm that can assign both terminal and internal fragments generated by top-down MS fragmentation. Further, ClipsMS can be used to locate various modifications on the protein sequence. Using ClipsMS to assign TD-MS generated product ions, we demonstrate that for apo-myoglobin, the inclusion of internal fragments increases the sequence coverage up to 78%. Interestingly, many internal fragments cover complimentary regions to the terminal fragments that enhance the information that is extracted from a single top-down mass spectrum. Analysis of oxidized apo-myoglobin using terminal and internal fragment matching by ClipsMS confirmed the locations of oxidation sites on the two methionine residues. Internal fragments can be beneficial for top-down protein fragmentation analysis, and ClipsMS can be a valuable tool for assigning both terminal and internal fragments present in a top-down mass spectrum.</p>

scholarly journals ClipsMS: An Algorithm for Analyzing Internal Fragments Resulting from Top-Down Mass Spectrometry

2021 ◽  
Author(s):  
Carter Lantz ◽  
Muhammad A. Zenaidee ◽  
Benqian Wei ◽  
Zachary Hemminger ◽  
Rachel R. Ogorzalek Loo ◽  
...  
Keyword(s):  
Mass Spectrum ◽  
Protein Sequence ◽  
Sequence Coverage ◽  
Top Down ◽  
Mass Spectrum Analysis ◽  
Single Top ◽  
Product Ions ◽  
Methionine Residues ◽  
Protein Fragmentation ◽  
Internal Fragment

<p>Here we describe ClipsMS, an algorithm that can assign both terminal and internal fragments generated by top-down MS fragmentation. Further, ClipsMS can be used to locate various modifications on the protein sequence. Using ClipsMS to assign TD-MS generated product ions, we demonstrate that for apo-myoglobin, the inclusion of internal fragments increases the sequence coverage up to 78%. Interestingly, many internal fragments cover complimentary regions to the terminal fragments that enhance the information that is extracted from a single top-down mass spectrum. Analysis of oxidized apo-myoglobin using terminal and internal fragment matching by ClipsMS confirmed the locations of oxidation sites on the two methionine residues. Internal fragments can be beneficial for top-down protein fragmentation analysis, and ClipsMS can be a valuable tool for assigning both terminal and internal fragments present in a top-down mass spectrum.</p>

Isotope Depletion Mass Spectrometry (ID-MS) for Enhanced Top-Down Protein Fragmentation

2018 ◽  
Author(s):  
Kelly J. Gallagher ◽  
Michael Palasser ◽  
Sam Hughes ◽  
C. Logan Mackay ◽  
David P. A. Kilgour ◽  
...  
Keyword(s):  
Mass Spectrometry ◽  
Molecular Mass ◽  
Posttranslational Modifications ◽  
Recombinant Expression ◽  
Expression System ◽  
Single Amino Acid ◽  
Sequence Coverage ◽  
Top Down ◽  
Fragment Ions ◽  
Signal Overlap

<div>Top-down mass spectrometry has become an important technique for the identification of proteins and characterisation of chemical and posttranslational modifications. However, as the molecular mass of proteins increases intact mass determination and top-down fragmentation efficiency become more challenging due to the partitioning of the mass spectral signal into many isotopic peaks. In large proteins, this results in reduced sensitivity and increased spectral complexity and signal overlap. This phenomenon is a consequence of the natural isotopic heterogeneity of the elements which comprise proteins (notably 13C). Here we present a bacterial recombinant expression system for the production of proteins depleted in 13C and 15N and use this strategy to prepare a range of isotopically depleted proteins. High resolution MS of isotope depleted proteins reveal dramatically reduced isotope distributions, which results in increases in sensitivity and deceased spectral complexity. We demonstrate that the monoisotopic signal is observed in mass spectra of proteins up to ~50 kDa. This allows confident assignment of accurate molecular mass, and facile detection of low mass modifications (such as deamidation). We outline the benefits of this isotope depletion strategy for top-down fragmentation. The reduced spectral complexity alleviates problems of signal overlap; the presence of monoisotopic signals allow more accurate assignment of fragment ions; and the dramatic increase in single-to-noise ratio (up to 7-fold increases) permits vastly reduced data acquisition times. Together, these compounding benefits allow the assignment of ca. 3-fold more fragment ions than analysis of proteins with natural isotopic abundances. Thus, more comprehensive sequence coverage can be achieved; we demonstrate near single amino-acid resolution of the 29 kDa protein carbonic anhydrase from a single top-down MS experiment. Finally, we demonstrate that the ID-MS strategy allows far greater sequence coverage to be obtained in time limited top-down data acquisitions – highlighting potential advantages for top-down LC-MS/MS workflows and top-down proteomics. </div><div><br></div>

scholarly journals Top-down proteomic identification of plasmid and host proteins produced by pathogenic Escherichia coli using MALDI-TOF-TOF tandem mass spectrometry

PLoS ONE ◽  
2021 ◽  
Vol 16 (11) ◽  
pp. e0260650
Author(s):  
Clifton K. Fagerquist ◽  
Claire E. Dodd
Keyword(s):  
Mass Spectrometry ◽  
Escherichia Coli ◽  
Tandem Mass Spectrometry ◽  
Aspartic Acid ◽  
Protein Sequences ◽  
Tandem Mass ◽  
Host Proteins ◽  
Top Down ◽  
Maldi Tof ◽  
Fragment Ions

Fourteen proteins produced by three pathogenic Escherichia coli strains were identified using antibiotic induction, MALDI-TOF-TOF tandem mass spectrometry (MS/MS) and top-down proteomic analysis using software developed in-house. Host proteins as well as plasmid proteins were identified. Mature, intact protein ions were fragmented by post-source decay (PSD), and prominent fragment ions resulted from the aspartic acid effect fragmentation mechanism wherein polypeptide backbone cleavage (PBC) occurs on the C-terminal side of aspartic acid (D), glutamic acid (E) and asparagine (N) residues. These highly specific MS/MS-PSD fragment ions were compared to b- and y-type fragment ions on the C-terminal side of D-, E- and N-residues of in silico protein sequences derived from whole genome sequencing. Nine proteins were found to be post-translationally modified with either removal of an N-terminal methionine or a signal peptide. The protein sequence truncation algorithm of our software correctly identified all full and truncated protein sequences. Truncated sequences were compared to those predicted by SignalP. Nearly complete concurrence was obtained except for one protein where SignalP mis-identified the cleavage site by one residue. Two proteins had intramolecular disulfide bonds that were inferred by the absence of PBC on the C-terminal side of a D-residue located within the disulfide loop. These results demonstrate the utility of MALDI-TOF-TOF for identification of full and truncated bacterial proteins.

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