Achieving a 35-Plex Tandem Mass Tag Reagent Set through Deuterium Incorporation

Mass spectrometry-based sample multiplexing with isobaric tags permits the development of high-throughput and precise quantitative biological assays with proteome-wide coverage and minimal missing values. Here, we nearly doubled the multiplexing capability of the TMTpro reagent set to a 35-plex thro...

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Veröffentlicht in:Journal of proteome research 2024-11, Vol.23 (11), p.5153-5165
Hauptverfasser: Zuniga, Nathan R., Frost, Dustin C., Kuhn, Karsten, Shin, Myungsun, Whitehouse, Rebecca L., Wei, Ting-Yu, He, Yuchen, Dawson, Shane L., Pike, Ian, Bomgarden, Ryan D., Gygi, Steven P., Paulo, Joao A.
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Sprache:eng
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Zusammenfassung:Mass spectrometry-based sample multiplexing with isobaric tags permits the development of high-throughput and precise quantitative biological assays with proteome-wide coverage and minimal missing values. Here, we nearly doubled the multiplexing capability of the TMTpro reagent set to a 35-plex through the incorporation of one deuterium isotope into the reporter group. Substituting deuterium frequently results in suboptimal peak coelution, which can compromise the accuracy of reporter ion-based quantification. To counteract the deuterium effect on quantitation, we implemented a strategy that necessitated the segregation of nondeuterium and deuterium-containing channels into distinct subplexes during normalization procedures, with reassembly through a common bridge channel. This multiplexing strategy of “design independent sub-plexes but acquire together” (DISAT) was used to compare protein expression differences between human cell lines and in a cysteine-profiling (i.e., chemoproteomics) experiment to identify compounds binding to cysteine-113 of Pin1.
ISSN:1535-3893
1535-3907
1535-3907
DOI:10.1021/acs.jproteome.4c00668