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Isobaric tag for relative and absolute quantitation

From Wikipedia, the free encyclopedia

8plex iTRAQ kit

Isobaric tags for relative and absolute quantitation (iTRAQ) is an isobaric labeling method used in quantitative proteomics by tandem mass spectrometry to determine the amount of proteins from different sources in a single experiment.[1][2][3] It uses stable isotope labeled molecules that can be covalent bonded to the N-terminus and side chain amines of proteins.

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  • Mod-25 Lec-25 Quantitative Proteomics: iTRAQ and TMT
  • Mod-24 Lec-24 Quantitative Proteomics: Stable Isotope Labeling by Amino Acids in Cell Culture(SILAC)
  • Mod-01 Lec-01 Introduction to Proteomics Course

Transcription

Procedure

The ITRAQ method is based on the covalent labeling of the N-terminus and side chain amines of peptides from protein digestions with tags of varying mass. There are currently two mainly used reagents: 4-plex and 8-plex, which can be used to label all peptides from different samples/treatments.[citation needed] These samples are then pooled and usually fractionated by liquid chromatography and analyzed by tandem mass spectrometry (MS/MS). A database search is then performed using the fragmentation data to identify the labeled peptides and hence the corresponding proteins. The fragmentation of the attached tag generates a low molecular mass reporter ion that can be used to relatively quantify the peptides and the proteins from which they originated.

Data evaluation

At the peptide level, the signals of the reporter ions of each MS/MS spectrum allow for calculating the relative abundance (ratio) of the peptide(s) identified by this spectrum.[citation needed] The abundance of the reporter ions may consist of more than one single signal in the MS/MS data and the signals have to be integrated in some way from the histogram spectrum.

At the protein level, the combined ratios a proteins' peptides represent the relative quantification of that protein.

The MS/MS spectra can be analyzed using software that is freely available: i-Tracker[4] and jTraqX [5][6]

References

  1. ^ Ross PL, Huang YN, Marchese JN, Williamson B, Parker K, Hattan S, Khainovski N, Pillai S, Dey S, Daniels S, Purkayastha S, Juhasz P, Martin S, Bartlet-Jones M, He F, Jacobson A, Pappin DJ (2004). "Multiplexed protein quantitation in Saccharomyces cerevisiae using amine-reactive isobaric tagging reagents". Mol. Cell. Proteomics. 3 (12): 1154–69. doi:10.1074/mcp.M400129-MCP200. PMID 15385600.
  2. ^ Zieske LR (2006). "A perspective on the use of iTRAQ reagent technology for protein complex and profiling studies". J. Exp. Bot. 57 (7): 1501–8. doi:10.1093/jxb/erj168. PMID 16574745.
  3. ^ Gafken PR, Lampe PD (2006). "Methodologies for characterizing phosphoproteins by mass spectrometry". Cell Commun. Adhes. 13 (5–6): 249–62. doi:10.1080/15419060601077917. PMC 2185548. PMID 17162667.
  4. ^ Shadforth IP, Dunnley PJ, Lilley KS, Bessant C (2005). "i-Tracker: For quantitative proteomics using iTRAQ". BMC Genomics. 6: 145. doi:10.1186/1471-2164-6-145. PMC 1276793. PMID 16242023.
  5. ^ Muth, T., et al., jTraqX: a Free, Platform Independent Tool for Isobaric Tag Quantitation at the Protein Level, Proteomics, 2010, 10(6): 1223-1225, doi:10.1002/pmic.200900374
  6. ^ protein-ms - Browse /jTraqX at SourceForge.net

Further reading

  • Ow, Saw Yen; Salim, Malinda; Noirel, Josselin; Evans, Caroline; Rehman, Ishtiaq; Wright, Phillip C. (2009). "iTRAQ Underestimation in Simple and Complex Mixtures: "The Good, the Bad and the Ugly"". Journal of Proteome Research. 8 (11): 5347–5355. doi:10.1021/pr900634c. ISSN 1535-3893. PMID 19754192.


This page was last edited on 28 March 2024, at 02:02
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