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Quantitative Comparison of IMAC and TiO 2 Surfaces Used in the Study of Regulated, Dynamic Protein Phosphorylation ARTICLE IN PRESS

Title: Quantitative Comparison of IMAC and TiO 2 Surfaces Used in the Study of Regulated, Dynamic Protein Phosphorylation ARTICLE IN PRESS
Authors: Xiquan Liang; Geir Fonnum; Mahbod Hajivandi; Torkel Stene; Nini H Kjus; Erlend Ragnhildstveit; Joseph W Amshey; Paul Predki; R Marshall Pope
Contributors: The Pennsylvania State University CiteSeerX Archives
Source: http://www.glsciencesinc.com/ProductInfo/Proteomics/Documents/TiO2/IMAC_vs_TiO2_Surface_Comparison_Invitrogen.pdf.
Collection: CiteSeerX
Description: Protein phosphorylation regulates many aspects of cellular function, including cell proliferation, migration, and signal transduction. An efficient strategy to isolate phosphopeptides from a pool of unphosphorylated peptides is essential to global characterization using mass spectrometry. We describe an approach employing isotope tagging reagents for relative and absolute quantification (iTRAQ) labeling to compare quantitatively commercial and prototypal immobilized metal affinity chelate (IMAC) and metal oxide resins. Results indicate a prototype iron chelate resin coupled to magnetic beads outperforms either the Ga 3ϩ -coupled analog, Fe 3ϩ , or Ga 3ϩ -loaded, iminodiacetic acid (IDA)-coated magnetic particles, Ga 3ϩ -loaded Captivate beads, Fe 3ϩ -loaded Poros 20MC, or zirconium-coated ProteoExtract magnetic beads. For example, compared with Poros 20MC, the magnetic metal chelate (MMC) studied here improved phosphopeptide recovery by 20% and exhibited 60% less contamination from unphosphorylated peptides. With respect to efficiency and contamination, MMC performed as well as prototypal magnetic metal oxide-coated (TiO 2 ) beads (MMO) or TiO 2 chromatographic spheres, even if the latter were used with 2,5-dihydroxybenzoic acid (DHB) procedures. Thus far, the sensitivity of the new prototypes reaches 50 fmol, which is comparable to TiO 2 spheres. In an exploration of natural proteomes, tryptic (phospho)peptides captured from stable isotopic labeling with amino acids in cell culture (SILAC)-labeled immunocomplexes following EGF-treatment of 5 ϫ 10 7 HeLa cells were sufficient to quantify stimulated response of over 60 proteins and identify 20 specific phosphorylation sites. (J Am Soc Mass Spectrom 2007, xx, xxx) © 2007 American Society for Mass Spectrometry C haracterization of protein phosphorylation status, especially following stimulated transduction events, can provide mechanistic insights into the biological basis of signaling, cell cycle progression, adhesion, migration, and numerous other functions. ...
Document Type: text
File Description: application/pdf
Language: English
Relation: http://citeseerx.ist.psu.edu/viewdoc/summary?doi=10.1.1.1049.3008; http://www.glsciencesinc.com/ProductInfo/Proteomics/Documents/TiO2/IMAC_vs_TiO2_Surface_Comparison_Invitrogen.pdf
Availability: http://citeseerx.ist.psu.edu/viewdoc/summary?doi=10.1.1.1049.3008; http://www.glsciencesinc.com/ProductInfo/Proteomics/Documents/TiO2/IMAC_vs_TiO2_Surface_Comparison_Invitrogen.pdf
Rights: Metadata may be used without restrictions as long as the oai identifier remains attached to it.
Accession Number: edsbas.8344D0C8
Database: BASE