2019
DOI: 10.1021/acs.jproteome.8b00898
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Comparison of Protein Quantification in a Complex Background by DIA and TMT Workflows with Fixed Instrument Time

Abstract: Label-free quantification (LFQ) and isobaric labeling quantification (ILQ) are among the most popular protein quantification workflows in discovery proteomics. Here, we compared the TMT SPS/MS3 10-plex workflow to a label free single shot data-independent acquisition (DIA) workflow on a controlled sample set. The sample set consisted of ten samples derived from 10 biological replicates of mouse cerebelli spiked with the UPS2 protein standard in five different concentrations. For a fair comparison, we matched t… Show more

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Cited by 134 publications
(154 citation statements)
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References 48 publications
(81 reference statements)
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“…In this commonly used strategy for DIA experiments, sample-specific proteins could be potentially missed, because of dilution of these proteins in the pooled sample. This effect has been described previously for a protein spike-in experiment in complex background 30 and will likely get more prominent the more samples are pooled to generate the project-specific library. The largest improvement in quantified precursors (+27%), peptides (+12%) and proteins (+10%) using the hybrid library approach was found for the resource library which was based on DDA data from unrelated samples and on a different LC-MS setup.…”
Section: Esi †) the Overlap On Protein Levelmentioning
confidence: 72%
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“…In this commonly used strategy for DIA experiments, sample-specific proteins could be potentially missed, because of dilution of these proteins in the pooled sample. This effect has been described previously for a protein spike-in experiment in complex background 30 and will likely get more prominent the more samples are pooled to generate the project-specific library. The largest improvement in quantified precursors (+27%), peptides (+12%) and proteins (+10%) using the hybrid library approach was found for the resource library which was based on DDA data from unrelated samples and on a different LC-MS setup.…”
Section: Esi †) the Overlap On Protein Levelmentioning
confidence: 72%
“…Compared to library-based analysis of the DIA data, a database search resulted in less identified proteins, but an improved quantitative performance. 30 A marriage of both of these approaches, i.e. combining data from a database search of DIA data with results of a search of DDA, holds the potential to the improve DIA data analysis in terms of quantitative precision and number of quantified proteins.…”
Section: Introductionmentioning
confidence: 99%
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“…Specifically, one set of controlled mixtures had defined spike-in of few proteins in a constant background (Spike-in-HEK293-OT dataset). Additionally, a set of controlled mixtures had defined spike-in of few proteins in a background with realistic biological variation (Spikein-biol-var-OT) (23). The third type consisted of sets of controlled mixtures at defined ratios (MP-LFC-OT, MP-SFC-OT, MP-LFC-TTOF, and MP-LFC-MS1var-OT).…”
Section: Methodsmentioning
confidence: 99%
“…Peptides were loaded onto the column with 100% buffer A (99% H2O, 0.1% formic acid) and eluted with increasing buffer B (80% acetonitrile, 0.1% formic acid) over a nonlinear gradient for 120min. The DIA method (Muntel et al, 2019) contained 40 DIA segments of 30,000 resolution with IT set to 55ms, AGC of 1×106, and a survey scan of 120,000 resolution with 50 ms max IT and AGC of 5×105. The mass range was set to 350-1650 m/z.…”
Section: Methodsmentioning
confidence: 99%