Publication | Closed Access
Rapid and sensitive profiling and quantification of the human cell line proteome by LC‐MS/MS without prefractionation
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Citations
34
References
2014
Year
Lc‐ms/ms ConditionsBiological Mass SpectrometryCell CycleProteomic TechnologyPlasma ProteomicsProteomicsProtein DegradationProtein Quality ControlLc‐ms/ms WorkflowTranslational ProteomicsBioinformaticsCell BiologySensitive ProfilingHuman Cell LinePrognostic BiomarkersNatural SciencesProtein Mass SpectrometrySystems BiologyMedicine
In this paper, we demonstrate a rapid and reproducible 1D LC‐MS/MS workflow for fast quantitative proteomic research. We have optimized the LC‐MS/MS conditions, including digestion and gradient conditions, sample loading amount, and MS parameter settings. As a result, we were able to obtain twice as many protein identifications compared with the LC‐MS/MS conditions before optimization. More than 4500 protein groups and 50 000 peptides were identified in less than 8 h without any fractionation. This 1D workflow was then applied to the analysis of the MLN4924 treated/untreated human umbilical vein endothelial cell (HUVEC) samples with label‐free quantification. In these experiments, a total of 179 proteins showed a statistically significant expression change after the MLN4924 treatment. Functional analysis showed that these proteins are associated with cell death and survival; gene expression; cell cycle; and DNA replication, recombination, and repair.
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