Automated Phosphopeptide
Identification Using Multiple MS/MS Fragmentation Modes
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Abstract
Phosphopeptide identification is still a challenging
task because fragmentation spectra obtained by mass spectrometry do
not necessarily contain sufficient fragment ions to establish with
certainty the underlying amino acid sequence and the precise phosphosite.
To improve upon this, it has been suggested to acquire pairs of spectra
from every phosphorylated precursor ion using different fragmentation
modes, for example CID, ETD, and/or HCD. The development of automated
tools for the interpretation of these paired spectra has however,
until now, lagged behind. Using phosphopeptide samples analyzed by
an LTQ-Orbitrap instrument, we here assess an approach in which, on
each selected precursor, a pair of CID spectra, with or without multistage
activation (MSA or MS2, respectively), are acquired in the linear
ion trap. We applied this approach on phosphopeptide samples of variable
proteomic complexity obtained from <i>Arabidopsis
thaliana</i>. We present a straightforward computational
approach to reconcile sequence and phosphosite identifications provided
by the database search engine Mascot on the spectrum pairs, using
two simple filtering rules, at the amino acid sequence and phosphosite
localization levels. If multiple sequences and/or phosphosites are
likely, they are reported in the consensus sequence. Using our program
FragMixer, we could assess that on samples of moderate complexity,
it was worth combining the two fragmentation schemes on every precursor
ion to help efficiently identify amino acid sequences and precisely
localize phosphosites. FragMixer can be flexibly configured, independently
of the Mascot search parameters, and can be applied to various spectrum
pairs, such as MSA/ETD and ETD/HCD, to automatically compare and combine
the information provided by these more differing fragmentation modes.
The software is openly accessible and can be downloaded from our Web
site at http://proteomics.fr/FragMixer