Isobaric Labeling-Based Relative Quantification in Shotgun Proteomics

Rauniyar, Navin; Yates, John R.

doi:10.1021/pr500880b

Cited by 537 publications

(534 citation statements)

References 110 publications

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“…TMT, an isobaric chemical labeling method, is a powerful and convenient tool to estimate the relative abundance of proteins. In particular, isobaric tagging strategy with MSbased proteins is suitable for low-abundance proteins, such as the ones secreted in CM, due to high signal from native peptides (29). We implemented quality check for the proteins, both from CM and from MS-based proteomics with TMT labeling, via western blot and scatter plot, respectively.…”

Section: Discussionmentioning

confidence: 99%

Comparative Secretome Profiling and Mutant Protein Identification in Metastatic Prostate Cancer Cells by Quantitative Mass Spectrometry-based Proteomics

Kwon

Jeon

Sung

et al. 2018

Cancer Genomics Proteomics

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Section: Discussionmentioning

confidence: 99%

Comparative Secretome Profiling and Mutant Protein Identification in Metastatic Prostate Cancer Cells by Quantitative Mass Spectrometry-based Proteomics

Kwon

Jeon

Sung

et al. 2018

Cancer Genomics Proteomics

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“…Several methods are available to normalize data, such as cyclic LOESS, quantile, and median normalization, etc (43,50). However, when comparing isobaric labeled data from multiple experimental designs, these methods have their shortcomings or require reference samples in each experimental setup to allow for cross-set comparison (51 Therefore, we propose a new and easy to use normalization method, called CONSTANd, which allows accurate normalization of multiplexed, isobaric labeled samples in a datadriven and global manner. Latter terms indicate that all the observed data is used for the normalization procedure.…”

Section: Discussionmentioning

confidence: 99%

CONSTANd : A Normalization Method for Isobaric Labeled Spectra by Constrained Optimization

Maes

Hadiwikarta²,

Mertens

et al. 2016

Molecular & Cellular Proteomics

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In quantitative proteomics applications, the use of isobaric labels is a very popular concept as they allow for multiplexing, such that peptides from multiple biological samples are quantified simultaneously in one mass spectrometry experiment. Although this multiplexing allows that peptide intensities are affected by the same amount of instrument variability, systematic effects during sample preparation can also introduce a bias in the quantitation measurements. Therefore, normalization methods are required to remove this systematic error. At present, a few dedicated normalization methods for isobaric labeled data are at hand. Most of these normalization methods include a framework for statistical data analysis and rely on ANOVA or linear mixed models. However, for swift quality control of the samples or data visualization a simple normalization technique is sufficient. To this aim, we present a new and easy-to-use data-driven normalization method, named CONSTANd. The CONSTANd method employs constrained optimization and prior information about the labeling strategy to normalize the peptide intensities. Further, it allows maintaining the connection to any biological effect while reducing the systematic and technical errors. As a result, peptides can not only be compared directly within a multiplexed experiment, but are also comparable between other isobaric labeled datasets from multiple experimental designs that are normalized by the CONSTANd method, without the need to include a reference sample in every experimental setup. The latter property is especially useful when more than six, eight or ten (TMT/iTRAQ) biological samples are required to detect differential peptides with sufficient statistical power and to optimally make use of the multiplexing capacity of isobaric labels. Molecular & Cellular Proteomics 15:

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“…This technique analyzes relative amounts of cysteine-containing peptides in tryptic digests of paired protein extracts. Isobaric tags for relative and absolute quantitation (iTRAQ) method utilizes a multiplexed isobaric chemical tagging reagent to label primary amines of peptides and proteins (44). iTRAQ reagents usually consist of an Nmethyl piperazine reporter group, a balance group, and an Nhydroxysuccinimide ester group.…”

Section: Chemical Proteomic Techniquesmentioning

confidence: 99%

Chemical Proteomic Approaches Targeting Cancer Stem Cells: A Review of Current Literature

Jung

2017

CGP

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Isobaric Labeling-Based Relative Quantification in Shotgun Proteomics

Cited by 537 publications

References 110 publications

Comparative Secretome Profiling and Mutant Protein Identification in Metastatic Prostate Cancer Cells by Quantitative Mass Spectrometry-based Proteomics

Comparative Secretome Profiling and Mutant Protein Identification in Metastatic Prostate Cancer Cells by Quantitative Mass Spectrometry-based Proteomics

CONSTANd : A Normalization Method for Isobaric Labeled Spectra by Constrained Optimization

Chemical Proteomic Approaches Targeting Cancer Stem Cells: A Review of Current Literature

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