Literature DB >> 23638792

Neutron encoded labeling for peptide identification.

Christopher M Rose1, Anna E Merrill, Derek J Bailey, Alexander S Hebert, Michael S Westphall, Joshua J Coon.   

Abstract

Metabolic labeling of cells using heavy amino acids is most commonly used for relative quantitation; however, partner mass shifts also detail the number of heavy amino acids contained within the precursor species. Here, we use a recently developed metabolic labeling technique, NeuCode (neutron encoding) stable isotope labeling with amino acids in cell culture (SILAC), which produces precursor partners spaced ~40 mDa apart to enable amino acid counting. We implement large scale counting of amino acids through a program, "Amino Acid Counter", which determines the most likely combination of amino acids within a precursor based on NeuCode SILAC partner spacing and filters candidate peptide sequences during a database search using this information. Counting the number of lysine residues for precursors selected for MS/MS decreases the median number of candidate sequences from 44 to 14 as compared to an accurate mass search alone (20 ppm). Furthermore, the ability to co-isolate and fragment NeuCode SILAC partners enables counting of lysines in product ions, and when the information is used, the median number of candidates is reduced to 7. We then demonstrate counting leucine in addition to lysine results in a 6-fold decrease in search space, 43 to 7, when compared to an accurate mass search. We use this scheme to analyze a nanoLC-MS/MS experiment and demonstrate that accurate mass plus lysine and leucine counting reduces the number of candidate sequences to one for ~20% of all precursors selected, demonstrating an ability to identify precursors without MS/MS analysis.

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Year:  2013        PMID: 23638792      PMCID: PMC3827945          DOI: 10.1021/ac400476w

Source DB:  PubMed          Journal:  Anal Chem        ISSN: 0003-2700            Impact factor:   6.986


  58 in total

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2.  Single peptide-based protein identification in human proteome through MALDI-TOF MS coupled with amino acids coded mass tagging.

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3.  Novel linear quadrupole ion trap/FT mass spectrometer: performance characterization and use in the comparative analysis of histone H3 post-translational modifications.

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4.  Open mass spectrometry search algorithm.

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Review 5.  Large-scale database searching using tandem mass spectra: looking up the answer in the back of the book.

Authors:  Rovshan G Sadygov; Daniel Cociorva; John R Yates
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7.  Quantifying the impact of chimera MS/MS spectra on peptide identification in large-scale proteomics studies.

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9.  Neutron-encoded mass signatures for multiplexed proteome quantification.

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Journal:  Nat Methods       Date:  2013-02-24       Impact factor: 28.547

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  17 in total

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Authors:  Camille Lombard-Banek; Erika P Portero; Rosemary M Onjiko; Peter Nemes
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Review 5.  Sample Multiplexing Strategies in Quantitative Proteomics.

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6.  Development and characterization of novel 8-plex DiLeu isobaric labels for quantitative proteomics and peptidomics.

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7.  Peptide dimethylation: fragmentation control via distancing the dimethylamino group.

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8.  Protected amine labels: a versatile molecular scaffold for multiplexed nominal mass and sub-Da isotopologue quantitative proteomic reagents.

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9.  Neucode Labels for Multiplexed, Absolute Protein Quantification.

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10.  NeuCode Proteomics Reveals Bap1 Regulation of Metabolism.

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