Abstract
The development of high-performance technology platforms for generating detailed protein expression profiles, or protein atlases, is essential. Recently, we presented a novel platform that we termed global proteome survey, where we combined the best features of affinity proteomics and mass spectrometry, to probe any proteome in a species independent manner while still using a limited set of antibodies. We used so called context-independent-motif-specific antibodies, directed against short amino acid motifs. This enabled enrichment of motif-containing peptides from a digested proteome, which then were detected and identified by mass spectrometry. In this study, we have demonstrated the quantitative capability, reproducibility, sensitivity, and coverage of the global proteome survey technology by targeting stable isotope labeling with amino acids in cell culture-labeled yeast cultures cultivated in glucose or ethanol. The data showed that a wide range of motif-containing peptides (proteins) could be detected, identified, and quantified in a highly reproducible manner. On average, each of six different motif-specific antibodies was found to target about 75 different motif-containing proteins. Furthermore, peptides originating from proteins spanning in abundance from over a million down to less than 50 copies per cell, could be targeted. It is worth noting that a significant set of peptides previously not reported in the PeptideAtlas database was among the profiled targets. The quantitative data corroborated well with the corresponding data generated after conventional strong cation exchange fractionation of the same samples. Finally, several differentially expressed proteins, with both known and unknown functions, many relevant for the central carbon metabolism, could be detected in the glucose- versus ethanol-cultivated yeast. Taken together, the study demonstrated the potential of our immunoaffinity-based mass spectrometry platform for reproducible quantitative proteomics targeting classes of motif-containing peptides.
Highlights
In the quest for disease-associated biomarkers, the deciphering of the human proteome(s) will be central (1)
We have demonstrated the GPS set-up with respect to its quantitative capability, reproducibility, sensitivity, and coverage, by using the stable isotope labeling by amino acids in cell culture (SILAC) approach (26), targeting SILAC-labeled yeast cultivated in either glucose or ethanol
The total number of identified peptides and proteins were lower in biosample 2 than biosample 1, but as this was noticed for both the GPS and strong cation exchange chromatography (SCX) set-up, this was attributed to the sample and not the experimental set-ups
Summary
In the quest for disease-associated biomarkers, the deciphering of the human proteome(s) will be central (1). We have demonstrated the GPS set-up with respect to its quantitative capability, reproducibility, sensitivity, and coverage, by using the stable isotope labeling by amino acids in cell culture (SILAC) approach (26), targeting SILAC-labeled yeast cultivated in either glucose or ethanol.
Sign-in/Register to view highlights & summary Sign-in/Register to access full text options 
Free) 
Talk to us
Join us for a 30 min session where you can share your feedback and ask us any queries you have
Schedule a call
