Literature DB >> 19413330

Lys-N and trypsin cover complementary parts of the phosphoproteome in a refined SCX-based approach.

Sharon Gauci1, Andreas O Helbig, Monique Slijper, Jeroen Krijgsveld, Albert J R Heck, Shabaz Mohammed.   

Abstract

The analysis of proteome-wide phosphorylation events is still a major analytical challenge because of the enormous complexity of protein phosphorylation networks. In this work, we evaluate the complementarity of Lys-N, Lys-C, and trypsin with regard to their ability to contribute to the global analysis of the phosphoproteome. A refined version of low-pH strong cation exchange was used to efficiently separate N-terminally acetylated, phosphorylated, and nonmodified peptides. A total of 5036 nonredundant phosphopeptides could be identified with a false discovery rate of <1% from 1 mg of protein using a combination of the three enzymes. Our data revealed that the overlap between the phosphopeptide data sets generated with different proteases was marginal, whereas the overlap between two similarly generated tryptic data sets was found to be at least 4 times higher. In this way, the parallel use of Lys-N and trypsin enabled a 72% increase in the number of detected phosphopeptides as compared to trypsin alone, whereas a trypsin replicate experiment only led to a 25% increase. Thus, when focusing solely on the trypsin and Lys-N data, we identified 4671 nonredundant phosphopeptides. Further analysis of the detected sites showed that the Lys-N and trypsin data sets were enriched in significantly different phosphorylation motifs, further evidencing that multiprotease approaches are very valuable in phosphoproteome analyses.

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Year:  2009        PMID: 19413330     DOI: 10.1021/ac9004309

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


  101 in total

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4.  Comparative assessment of site assignments in CID and electron transfer dissociation spectra of phosphopeptides discloses limited relocation of phosphate groups.

Authors:  Nikolai Mischerikow; A F Maarten Altelaar; J Daniel Navarro; Shabaz Mohammed; Albert J R Heck
Journal:  Mol Cell Proteomics       Date:  2010-03-16       Impact factor: 5.911

5.  Probing the active site of the deoxynucleotide N-hydrolase Rcl encoded by the rat gene c6orf108.

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6.  Increasing phosphoproteomic coverage through sequential digestion by complementary proteases.

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Review 7.  A structural model for regulation of NHEJ by DNA-PKcs autophosphorylation.

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8.  Quantitative phosphoproteomics after auxin-stimulated lateral root induction identifies an SNX1 protein phosphorylation site required for growth.

Authors:  Hongtao Zhang; Houjiang Zhou; Lidija Berke; Albert J R Heck; Shabaz Mohammed; Ben Scheres; Frank L H Menke
Journal:  Mol Cell Proteomics       Date:  2013-01-17       Impact factor: 5.911

Review 9.  The role of Plk3 in oncogenesis.

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Review 10.  Advanced proteomic liquid chromatography.

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Journal:  J Chromatogr A       Date:  2012-07-09       Impact factor: 4.759

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