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Title: Quantitative analysis of cell surface membrane proteins using membrane-impermeable chemical probe coupled with 18O labeling

Journal Article · · Journal of Proteome Research, 9(5):2160-2169
DOI:https://doi.org/10.1021/pr9009113· OSTI ID:982569

We report a mass spectrometry-based strategy for quantitative analysis of cell surface membrane proteome changes. The strategy includes enrichment of surface membrane proteins using a membrane-impermeable chemical probe followed by stable isotope 18O labeling and LC-MS analysis. We applied this strategy for enriching membrane proteins expressed by Shewanella oneidensis MR-1, a gram-negative bacterium with known metal-reduction capability via extracellular electron transfer between outer membrane proteins and environmental electron receptors. LC/MS/MS analysis resulted in the identification of about 79% membrane proteins among all proteins identified from the enriched sample. To illustrate the quantification of membrane proteome changes, enriched membrane protein samples from wild-type and mutant cells (generated from deletion of a type II secretion protein, GspD) were further labeled with 16O and 18O at the peptide level prior to LC-MS analysis. A chemical-probe-labeled pure protein has also been used as an internal standard for normalization purpose. The quantitative data revealed reduced abundances of many outer membrane proteins such as OmcA and MtrC in ΔgspD mutant cells, which agreed well with previously published studies.

Research Organization:
Pacific Northwest National Lab. (PNNL), Richland, WA (United States). Environmental Molecular Sciences Lab. (EMSL)
Sponsoring Organization:
USDOE
DOE Contract Number:
AC05-76RL01830
OSTI ID:
982569
Report Number(s):
PNNL-SA-67314; ISSN 1535-3907; 34708; 18427; KP1601010; TRN: US201014%%389
Journal Information:
Journal of Proteome Research, 9(5):2160-2169, Vol. 9, Issue 5; ISSN 1535-3893
Country of Publication:
United States
Language:
English