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Proteomic profiling of intact proteins using WAX-RPLC 2-D separations and FTICR mass spectrometry

Journal Article · · Journal of Proteome Research, 6(2):602-610
DOI:https://doi.org/10.1021/pr060354a· OSTI ID:902954

We investigated the combination of weak anion exchange (WAX) fractionation and on-line reversed phase liquid chromatography (RPLC) separation using a 12 T FTICR mass spectrometer for the detection of intact proteins from a Shewanella oneidensis MR-1 cell lysate. 715 intact proteins were detected and the combined results from the WAX fractions and the unfractionated cell lysate were aligned using LC-MS features to facilitate protein abundance measurements. Protein identifications and post translational modifications were assigned for ~10% of the detected proteins by comparing intact protein mass measurements to proteins identified in peptide MS/MS analysis of an aliquot of the same fraction. Intact proteins were also detected for S. oneidensis lysates obtained from cells grown on 13C, 15N depleted media under aerobic and sub-oxic conditions. This work aimed at optimizing intact protein detection for profiling proteins at a level that incorporates their modification complement. The strategy can be readily applied for measuring differential protein abundances, and provides a platform for high-throughput selection of biologically relevant targets for further characterization.

Research Organization:
Pacific Northwest National Laboratory (PNNL), Richland, WA (US), Environmental Molecular Sciences Laboratory (EMSL)
Sponsoring Organization:
USDOE
DOE Contract Number:
AC05-76RL01830
OSTI ID:
902954
Report Number(s):
PNNL-SA-50906; 20496; 400412000
Journal Information:
Journal of Proteome Research, 6(2):602-610, Journal Name: Journal of Proteome Research, 6(2):602-610 Journal Issue: 2 Vol. 6
Country of Publication:
United States
Language:
English

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