Figure 3

Spectra comparisons between CHCA and DHB. (A, B) CHCA matrix vs DHB matrix. Considerably, in the case of DHB the peptide ions signals are less resolved than other signals in the spectrum, maybe connected to metastable decay of ions in the drift tube or "chemical noises" from matrix ions. On the other hand, CHCA was enabled to identify complement C1r-subcomponent (C1r_MOUSE) and alpha-2-antiplasmin (A2AP_MOUSE). Crosses represent matched peptides to the identification. (C, D) DHB matrix vs CHCA matrix. The spectra from DHB are notably rich of peptides ions fragments (crosses) which belong to the identification, i.e. glutatione peroxidase-secreted form (GPX3_MOUSE) and gelsolin (GELS_MOUSE). The blue circles on CHCA spectra, instead, represent matrix fragments which hide the peaks could be matched to the identifications. The pie chart represents our mouse proteome mapping, where both matrices have the almost same input in the identifications.