2018
DOI: 10.1021/acs.jproteome.8b00523
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NormalyzerDE: Online Tool for Improved Normalization of Omics Expression Data and High-Sensitivity Differential Expression Analysis

Abstract: Technical biases are introduced in omics data sets during data generation and interfere with the ability to study biological mechanisms. Several normalization approaches have been proposed to minimize the effects of such biases, but fluctuations in the electrospray current during liquid chromatography–mass spectrometry gradients cause local and sample-specific bias not considered by most approaches. Here we introduce a software named NormalyzerDE that includes a generic retention time (RT)-segmented approach c… Show more

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Cited by 174 publications
(141 citation statements)
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“…For quantification both unique and razor peptides were requested. Protein raw data abundance was first filtered for empty rows with in house script and quantile-normalize using R package NormalyzerDE 29 . Principal component analysis (PCA) was applied to explore sample-to-sample relationships.…”
Section: Methodsmentioning
confidence: 99%
“…For quantification both unique and razor peptides were requested. Protein raw data abundance was first filtered for empty rows with in house script and quantile-normalize using R package NormalyzerDE 29 . Principal component analysis (PCA) was applied to explore sample-to-sample relationships.…”
Section: Methodsmentioning
confidence: 99%
“…Regarding computational solutions, the new version of the statTarget package with a user-friendly graphical interface integrating a QC-based random forests signal correction algorithm has been released to remove inter-and intra-batch variations in omics study [82]. NormalyzerDE, an R package, provides 12 different normalization methods for omics data to enable researchers the correct technical variation, and decide the most suitable strategy for particular datasets [83]. NOREVA is another powerful online tool that implements various normalization methods of which five well-established criteria were supported for the comparison of different normalization approaches [84].…”
Section: The Assessment Of Systematic Errors In Clinical Metabolomicsmentioning
confidence: 99%
“…Statistical visualizations require columns with p-value, false discovery rate (FDR) corrected p-values, fold change (difference of means between the two compared groups) and average feature level. These values are provided by up-stream software such as NormalyzerDE [7] or R packages such as Limma [8] for most types of omics or DESeq2 [9], for RNA-seq expression data. After loading the data in the web interface, the visualizations can be accessed immediately.…”
Section: Software Implementationmentioning
confidence: 99%
“…They were subsequently log2-transformed and rolled up to protein level using an R-reimplementation (github.com/ComputationalProteomics/ProteinRollup) of the DanteR RRollup [26], using default settings and excluding proteins supported by a single peptide. Statistical contrasts between the two concentration levels were subsequently calculated using Limma [8] as provided by NormalyzerDE [7], and resulting p-values adjusted for multiple hypothesis testing using the Benjamini-Hochberg procedure [27].…”
Section: Case 1: Technical Spike-in Datasetmentioning
confidence: 99%