2017
DOI: 10.1021/acs.jproteome.6b01056
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Missing Value Monitoring Enhances the Robustness in Proteomics Quantitation

Abstract: In global proteomic analysis, it is estimated that proteins span from millions to less than 100 copies per cell. The challenge of protein quantitation by classic shotgun proteomic techniques relies on the presence of missing values in peptides belonging to low-abundance proteins that lowers intraruns reproducibility affecting postdata statistical analysis. Here, we present a new analytical workflow MvM (missing value monitoring) able to recover quantitation of missing values generated by shotgun analysis. In p… Show more

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Cited by 15 publications
(10 citation statements)
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“…The mass spectrometer was operated in DDA mode as described previously (Matafora et al, 2017): dynamic exclusion enabled (exclusion duration = 15 s), MS1 resolution = 70,000, MS1 automatic gain control target = 3 × 106, MS1 maximum fill time = 60 ms, MS2 resolution = 17,500, MS2 automatic gain control target = 1 × 105, MS2 maximum fill time = 60 ms, and MS2 normalized collision energy = 25. For each cycle, one full MS1 scan range = 300-1,650 m/z was followed by 12 MS2 scans using an isolation window of 2.0 m/z.…”
Section: Secretome Analysismentioning
confidence: 99%
“…The mass spectrometer was operated in DDA mode as described previously (Matafora et al, 2017): dynamic exclusion enabled (exclusion duration = 15 s), MS1 resolution = 70,000, MS1 automatic gain control target = 3 × 106, MS1 maximum fill time = 60 ms, MS2 resolution = 17,500, MS2 automatic gain control target = 1 × 105, MS2 maximum fill time = 60 ms, and MS2 normalized collision energy = 25. For each cycle, one full MS1 scan range = 300-1,650 m/z was followed by 12 MS2 scans using an isolation window of 2.0 m/z.…”
Section: Secretome Analysismentioning
confidence: 99%
“…As protein quantities are inferred from the quantities of measured peptides or even fragment ions, one needs to decide at which level to correct the data. Second, it is known that missing values can be associated with technical factors (Karpievitch et al , 2012 ; Matafora et al , 2017 ). Finally, when dealing with experiments with large sample numbers, typically in the order of hundreds, one needs to account for MS signal drift.…”
Section: Introductionmentioning
confidence: 99%
“…Differences in lipid IDs among each run, in both micro-and nano-flow, are due to the presence of missing values, which are a common problem in omics approaches. Indeed, missing values occur in datasets for several reasons: lipid amount below the limit of detection; stochastic nature of precursor selection in data dependent acquisition methods; missing peak picking by the software and biological variability across different samples [26]. In line with the total identified lipids, also core lipids across replicates are doubled in nano-flow compared the micro-flow datasets (Figure S7B).…”
Section: Lipidomics Analysis Of Mammalian Cells 221 Semi-targeted Lipidomics Analysismentioning
confidence: 90%