Perhaps one of the most influential concepts in protein mass spectrometry has been the notion of enzymatic protein digestion to render a collection of peptides of suitable size for conventional tandem mass spectrometry (collisional-activation, CAD).1 Doubtless this methodology has enabled significant progress for global protein identification;however, many investigators now realize this approach has significant limitations.2 This conclusion is based upon the following observations: First, protein posttranslational modifications (PTMs) on multi-domain proteins, and among components of protein-protein machines, work in concert;to determine their biological relevance, these patterns must be detected within the context of one another (across the whole protein).3 Second, transcriptional editing processes are pervasive in higher eukaryotes and difficult to predict, even with a completely sequenced genome. For example, 3/4 of all human proteins are expected to have at least 1 splice variant4-6 - variants that could contain intronic sequences. Skipped codons, frameshifting, gene fusion, and single nucleotide polymorphisms (SNPs) also occur. Thus, the use of short peptides as proxy markers for genes is inadequate and often misleading. Unlike CAD, electron transfer dissociation (ETD), a new fragmentation technique co-invented by the PI, does not require short peptides for successful sequence analysis (i.e., trypsin digestion). ETD is indifferent to peptide length or the presence of PTMs, is performed on a time-scale that permits coupling with chromatography, and can be coupled to other ion/ion reactions. This proposal aims to develop a suite of core ion/ion reaction tools, and automate their use in a hybrid-
Lera, Robert F; Potts, Gregory K; Suzuki, Aussie et al. (2016) Decoding Polo-like kinase 1 signaling along the kinetochore-centromere axis. Nat Chem Biol 12:411-8 |
Wilkerson, Emily M; Johansson, Mats W; Hebert, Alexander S et al. (2016) The Peripheral Blood Eosinophil Proteome. J Proteome Res 15:1524-33 |
Baughman, Joshua M; Rose, Christopher M; Kolumam, Ganesh et al. (2016) NeuCode Proteomics Reveals Bap1 Regulation of Metabolism. Cell Rep 16:583-595 |
Horton, Julie L; Martin, Ola J; Lai, Ling et al. (2016) Mitochondrial protein hyperacetylation in the failing heart. JCI Insight 2: |
Riley, Nicholas M; Coon, Joshua J (2016) Phosphoproteomics in the Age of Rapid and Deep Proteome Profiling. Anal Chem 88:74-94 |
Riley, Nicholas M; Mullen, Christopher; Weisbrod, Chad R et al. (2016) Enhanced Dissociation of Intact Proteins with High Capacity Electron Transfer Dissociation. J Am Soc Mass Spectrom 27:520-31 |
Potts, Gregory K; Voigt, Emily A; Bailey, Derek J et al. (2016) Neucode Labels for Multiplexed, Absolute Protein Quantification. Anal Chem 88:3295-303 |
Rose, Christopher M; Rush, Matthew J P; Riley, Nicholas M et al. (2015) A calibration routine for efficient ETD in large-scale proteomics. J Am Soc Mass Spectrom 26:1848-57 |
Zhao, Yimeng; Riley, Nicholas M; Sun, Liangliang et al. (2015) Coupling capillary zone electrophoresis with electron transfer dissociation and activated ion electron transfer dissociation for top-down proteomics. Anal Chem 87:5422-9 |
Mondal, Arindam; Potts, Gregory K; Dawson, Anthony R et al. (2015) Phosphorylation at the homotypic interface regulates nucleoprotein oligomerization and assembly of the influenza virus replication machinery. PLoS Pathog 11:e1004826 |
Showing the most recent 10 out of 98 publications