Targeting proline in (phospho)proteomics

Targeting proline in (phospho)proteomics

Mass spectrometry‐based proteomics experiments typically start with the digestion of proteins using trypsin, chosen because of its high specificity, availability, and ease of use. It has become apparent that the sole use of trypsin may impose certain limits on our ability to grasp the full proteome,...

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Veröffentlicht in:The FEBS journal 2020-07, Vol.287 (14), p.2979-2997
Hauptverfasser: Laarse, Saar A. M., Gelder, Charlotte A. G. H., Bern, Marshall, Akeroyd, Michiel, Olsthoorn, Maurien M. A., Heck, Albert J. R.
Format: Artikel
Sprache:eng
Schlagworte:
(phospho)proteomics
EndoPro
HeLa Cells
Humans
Mass spectrometry
Mass spectroscopy
Neoplasm Proteins - metabolism
Original
Peptide Hydrolases - metabolism
Peptides
pH effects
Phosphoproteins - metabolism
Phosphoproteomes
Phosphorylation
Proline
Proline - metabolism
proline effect
protease
Proteins
Proteolysis
Proteome - analysis
Proteome - metabolism
Proteomes
Proteomics
Proteomics - methods
Search algorithms
Trypsin
Trypsin - metabolism
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Zusammenfassung:Mass spectrometry‐based proteomics experiments typically start with the digestion of proteins using trypsin, chosen because of its high specificity, availability, and ease of use. It has become apparent that the sole use of trypsin may impose certain limits on our ability to grasp the full proteome, missing out particular sites of post‐translational modifications, protein segments, or even subsets of proteins. To tackle this problem, alternative proteases have been introduced and shown to lead to an increase in the detectable (phospho)proteome. Here, we argue that there may be further room for improvement and explore the protease EndoPro. For optimal peptide identification rates, we explored multiple peptide fragmentation techniques (HCD, ETD, and EThcD) and employed Byonic as search algorithm. We obtain peptide IDs for about 40% of the MS2 spectra (66% for trypsin). EndoPro cleaves with high specificity at the C‐terminal site of Pro and Ala residues and displays activity in a broad pH range, where we focused on its performance at pH = 2 and 5.5. The proteome coverage of EndoPro at these two pH values is rather distinct, and also complementary to the coverage obtained with trypsin. As about 40% of mammalian protein phosphorylations are proline‐directed, we also explored the performance of EndoPro in phosphoproteomics. EndoPro extends the coverable phosphoproteome substantially, whereby both the, at pH = 2 and 5.5, acquired phosphoproteomes are complementary to each other and to the phosphoproteome obtained using trypsin. Hence, EndoPro is a powerful tool to exploit in (phospho)proteomics applications. To improve (phospho)proteome coverage, we characterized EndoPro, a proline‐specific protease. The protease exhibits high specificity for cleavage C‐terminal to proline and alanine and is interestingly not hindered by phosphorylations near the cleavage site. EndoPro is complementary to trypsin and enabled us to detect over 2200 unique proteins not observed by trypsin and contributed 49% of the uniquely identified phosphosites.
ISSN:1742-464X
1742-4658
DOI:10.1111/febs.15190