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Identification of utilized phosphorylation sites in tagged proteins

External protocol Created on 30 Apr 2014

Authors

Nicholas Sherman and Jay Fox

Summary

Examination of utilized phosphorylation sites in an expressed, tagged protein requires a robust method that allows for maximum sequence coverage and identification of even low stoichiometry sites. The following protocol uses two to four enzymes to achieve high sequence coverage. Each of these digestions is analyzed un-enriched (C18) and enriched by TiO chromatography. By using this strategy and the high dynamic range and mass accuracy of the LTQFT hybrid linear ion trap – FTICR, sites modified at least down to the 0.1% level can be determined.

Further details

The protocol was published on Protocol Exchange in 2008. To see the entire protocol, click on the source link.

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