Abstract
Technical biases reduces the ability to see the desired biological changes when performing omics experiments. There are numerous normalization techniques available to counter the biases, but to find the optimal normalization is often a non-trivial task. Furthermore there are limited tools available to counter biases such as retention-time based biases caused by fluctuating electrospray intensities. NormalyzerDE helps this process by performing a wide range of normalization techniques including a general and openly available approach to countering retention-time based biases. More importantly it calculates and visualizes a number of performance measures to guide the users selection of normalization technique. Furthermore, NormalyzerDE provides means to easily perform differential expression statistics using either the empirical Bayes Limma approach or ANOVA. Evaluation visualizations are available for both normalization performance measures and as P-value histograms for the subsequent differential expression analysis comparisons. NormalyzerDE package version: 1.25.0
Installation is preferably performed using BiocManager (requires R version >= 3.5):
install.packages("BiocManager")
BiocManager::install("NormalyzerDE")
Willforss, J., Chawade, A., Levander, F. Submitted article.
NormalyzerDE expects a raw data file. Columns can contain annotation information or sample data. Each column should start with a header.
pepseq s1 s2 s3 s4
ATAAGG 20.0 21.2 19.4 18.5
AWAG 23.3 24.1 23.5 17.3
ACATGM 22.1 22.3 22.5 23.2
This data should be provided with a design matrix where all data samples should be represented. One column (default header “sample”) should match the columns containing samples in the raw data. Another column (default header “group”) should contain condition levels which could be used for group-based evaluations.
sample group
s1 condA
s2 condA
s3 condB
s4 condB
Alternatively the data can be provided as an instance of a
SummarizedExperiment
S4 class.
The evaluation step can be performed with one command,
normalyzer
. This command expects a path to the data file, a
name for the run-job, a path to a design matrix and finally a path to an
output directory.
Alternatively the designPath
and dataPath
arguments can be replaced with the experimentObj
argument
where the first assay should contain the data matrix of interest, the
colData
attribute the design matrix and the
rowData
attribute the annotation columns.
library(NormalyzerDE)
outDir <- tempdir()
designFp <- system.file(package="NormalyzerDE", "extdata", "tiny_design.tsv")
dataFp <- system.file(package="NormalyzerDE", "extdata", "tiny_data.tsv")
normalyzer(jobName="vignette_run", designPath=designFp, dataPath=dataFp,
outputDir=outDir)
## You are running version 1.25.0 of NormalyzerDE
## [Step 1/5] Load data and verify input
## Input data checked. All fields are valid.
## Sample check: More than one sample group found
## Sample replication check: All samples have replicates
## RT annotation column found (5)
## [Step 1/5] Input verified, job directory prepared at:/tmp/Rtmpwbkmgr/vignette_run
## [Step 2/5] Performing normalizations
## [Step 2/5] Done!
## [Step 3/5] Generating evaluation measures...
## [Step 3/5] Done!
## [Step 4/5] Writing matrices to file
## [Step 4/5] Matrices successfully written
## [Step 5/5] Generating plots...
## [Step 5/5] Plots successfully generated
## All done! Results are stored in: /tmp/Rtmpwbkmgr/vignette_run, processing time was 0.3 minutes
When you after performing the evaluation and having evaluated the report have decided for which normalization approach seems to work best you can continue to the statistical step.
Here, expected parameters are the path to the target normalization matrix, the sample design matrix as in the previous step, a job name, the path to an output directory and a list of the pairwise comparisons for which you want to calculate contrasts. They are provided as a character vector with conditions to compare separated by a dash (“-”).
Similarly as for the normalization step the designPath
and dataPath
arguments can be replaced with an instance of
SummarizedExperiment
sent to the experimentObj
argument.
normMatrixPath <- paste(outDir, "vignette_run/CycLoess-normalized.txt", sep="/")
normalyzerDE("vignette_run",
comparisons=c("4-5"),
designPath=designFp,
dataPath=normMatrixPath,
outputDir=outDir,
condCol="group")
## You are running version 1.25.0 of NormalyzerDE
## [1] "Setting up statistics object"
## [1] "Calculating statistical contrasts..."
## [1] "Contrast calculations done!"
## [1] "Writing 100 annotated rows to /tmp/Rtmpwbkmgr/vignette_run/vignette_run_stats.tsv"
## [1] "Writing statistics report"
## [1] "All done! Results are stored in: /tmp/Rtmpwbkmgr/vignette_run, processing time was 0 minutes"
A benefit of using a SummarizedExperiment object as input is that it allows executing NormalyzerDE using variables as input instead of loading from file.
The conversion of designMatrix$sample
is required if
using read.table
as it otherwise is interpreted as a
factor. For more intuitive behaviour you can use read_tsv
from the readr
package instead of
read.table
.
dataMatrix <- read.table(dataFp, sep="\t", header = TRUE)
designMatrix <- read.table(designFp, sep="\t", header = TRUE)
designMatrix$sample <- as.character(designMatrix$sample)
dataOnly <- dataMatrix[, designMatrix$sample]
annotOnly <- dataMatrix[, !(colnames(dataMatrix) %in% designMatrix$sample)]
sumExpObj <- SummarizedExperiment::SummarizedExperiment(
as.matrix(dataOnly),
colData=designMatrix,
rowData=annotOnly
)
normalyzer(jobName="sumExpRun", experimentObj = sumExpObj, outputDir=outDir)
## You are running version 1.25.0 of NormalyzerDE
## [Step 1/5] Load data and verify input
## Input data checked. All fields are valid.
## Sample check: More than one sample group found
## Sample replication check: All samples have replicates
## RT annotation column found (5)
## [Step 1/5] Input verified, job directory prepared at:/tmp/Rtmpwbkmgr/sumExpRun
## [Step 2/5] Performing normalizations
## [Step 2/5] Done!
## [Step 3/5] Generating evaluation measures...
## [Step 3/5] Done!
## [Step 4/5] Writing matrices to file
## [Step 4/5] Matrices successfully written
## [Step 5/5] Generating plots...
## [Step 5/5] Plots successfully generated
## All done! Results are stored in: /tmp/Rtmpwbkmgr/sumExpRun, processing time was 0.2 minutes
Retention time based normalization can be performed with an arbitrary normalization matrix.
There are two points of access for the higher order normalization.
Either by calling getRTNormalizedMatrix
which applies the
target normalization approach stepwise over the matrix based on
retention times, or by calling
getSmoothedRTNormalizedMatrix
which generates multiple
layered matrices and combines them. To use them you need your raw data
loaded into a matrix, a list containing retention times and a
normalization matrix able to take a raw matrix and return a normalized
in similar format.
## Cluster.ID Peptide.Sequence External.IDs Charge Average.RT Average.m.z
## 1 1493882053114 AAAAEINVKD P38156 2 20.25051 501.268
## s_12500amol_1 s_12500amol_2 s_12500amol_3 s_125amol_1 s_125amol_2 s_125amol_3
## 1 115597000 109302000 100314000 98182352 87241776 98702800
## sample group batch
## 1 s_125amol_1 4 2
At this point we have loaded the full data into dataframes. Next, we use the sample names present in the design matrix to extract sample columns from the raw data. Be careful that the sample names is a character vector. If it is a factor it will extract wrong columns.
Make sure that sample names extracted from design matrix are in right format. We expect it to be in ‘character’ format.
## [1] "character"
Now we are ready to extract the data matrix from the full matrix. We also need to get the retention time column from the full matrix.
## s_125amol_1 s_125amol_2 s_125amol_3 s_12500amol_1 s_12500amol_2
## [1,] 98182352 87241776 98702800 115597000 109302000
## s_12500amol_3
## [1,] 100314000
If everything is fine the data matrix should be double
,
and have the same number of rows as the number of retention time values
we have.
## [1] "double"
## [1] "Rows and columns of data"
## [1] 100 6
## [1] "Number of retention times"
## [1] 100
The normalization function is expected to take a raw intensity matrix and return log transformed values. We borrow the wrapper function for Loess normalization from NormalyzerDE. It can be replaced with any custom function as long as the wrapper has the same input/output format.
performCyclicLoessNormalization <- function(rawMatrix) {
log2Matrix <- log2(rawMatrix)
normMatrix <- limma::normalizeCyclicLoess(log2Matrix, method="fast")
colnames(normMatrix) <- colnames(rawMatrix)
normMatrix
}
We are ready to perform the normalization.
rtNormMat <- getRTNormalizedMatrix(dataMat,
retentionTimes,
performCyclicLoessNormalization,
stepSizeMinutes=1,
windowMinCount=100)
Let’s double check the results. We expect a matrix in the same format and shape as before. Furthermore, we expect similar but not the exact same values as if we’d applied the normalization globally.
## [1] 100 6
## [1] 100 6
## s_125amol_1 s_125amol_2 s_125amol_3 s_12500amol_1 s_12500amol_2 s_12500amol_3
## 26.54027 26.36017 26.57715 26.7771 26.70227 26.59205
## s_125amol_1 s_125amol_2 s_125amol_3 s_12500amol_1 s_12500amol_2
## [1,] 26.54027 26.36017 26.57715 26.7771 26.70227
## s_12500amol_3
## [1,] 26.59205
We have everything set up to perform the layered normalization. The result here is expected to be overall similar to the normal retention time approach.
layeredRtNormMat <- getSmoothedRTNormalizedMatrix(
dataMat,
retentionTimes,
performCyclicLoessNormalization,
stepSizeMinutes=1,
windowMinCount=100,
windowShifts=3,
mergeMethod="mean")
dim(layeredRtNormMat)
## [1] 100 6
## s_125amol_1 s_125amol_2 s_125amol_3 s_12500amol_1 s_12500amol_2
## [1,] 26.54027 26.36017 26.57715 26.7771 26.70227
## s_12500amol_3
## [1,] 26.59205
NormalyzerDE consists of a set of steps. The workflow can be run as a whole, or step by step.
This step performs input validation of the data, and generates an object of the class NormalyzerDataset.
jobName <- "vignette_run"
experimentObj <- setupRawDataObject(dataFp, designFp, "default", TRUE, "sample", "group")
normObj <- getVerifiedNormalyzerObject(jobName, experimentObj)
## Input data checked. All fields are valid.
## Sample check: More than one sample group found
## Sample replication check: All samples have replicates
## RT annotation column found (5)
The function setupRawDataObject
returns a
SummarizedExperiment
object. This object can be prepared
directly and should in that case contain the raw data as the default
assay, the design matrix as colData
and annotation rows as
rowData
.
Here, normalizations are performed. This generates a NormalyzerResults object containing both a reference to its original dataset object, but also generated normalization matrices.
Performance measures are calculated for normalizations. These are stored in an object NormalizationEvaluationResults. A NormalyzerResults object similar to the one sent in is returned, but with this field added.
Generated normalization matrices are written to the provided folder.
Performance measures are used to generate evaluation figures which is written in an evaluation report.
## png
## 2
After this evaluation of normalizations and progression to statistics follows as described previously in this report.
For continued processing you select the matrix containing the normalized data from the best performing normalization. The design matrix is the same as for the normalization step.
bestNormMatPath <- paste(jobDir, "RT-Loess-normalized.txt", sep="/")
experimentObj <- setupRawContrastObject(bestNormMatPath, designFp, "sample")
nst <- NormalyzerStatistics(experimentObj, logTrans=FALSE)
Similarly as to for the normalization evaluation step the
experimentObj
above can be prepared directly as a
SummarizedExperiment
object.
Now we are ready to perform the contrasts. Contrasts are provided as
a vector in the format c("condA-condB", "condB-condC")
,
where condX
is the group levels.
Finally we generate a table containing the statistics results for each feature and write it to file together with an evaluation report containing P-value histograms for each comparison.
annotDf <- generateAnnotatedMatrix(nst)
utils::write.table(annotDf, file=paste(jobDir, "stat_table.tsv", sep="/"))
generateStatsReport(nst, "Vignette stats", jobDir)
## png
## 2
NormalyzerDE consists of a number of scripts and classes. They are focused around two separate workflows. One is for normalizing and evaluating the normalizations. The second is for performing differential expression analysis. Classes are contained in scripts with the same name.
Code organization:
The standard workflow for the normalization is the following:
normalyzer
function in the
NormalyzerDE.R
script is called, starting the process.preparsers.R
.inputVerification.R
. This results in an instance of the
NormalyzerDataset
class.normMethods.R
. This yields an instance of
NormalyzerResults
which links to the original
NormalyzerDataset
instance and also contains all the
resulting normalized datasets.normMethods.R
over retention time using
functions present in higherOrderNormMethods.R
.analyzeResults.R
. This yields an instance of
NormalyzerEvaluationResults
containing the evaluation
results. This instance is attached to the NormalyzerResults
object.outputUtils.R
where the
normalizations are written to an output directory, and to
generatePlots.R
which contains visualizations for the
performance measures. It also uses code in printMeta.R
and
printPlots.R
to output the results in a desired
format.When a normalized matrix is selected the analysis proceeds to the statistical analysis.
normalyzerde
function in the
NormalyzerDE.R
script is called starting the differential
expression analysis pipeline.NormalyzerStatistics
is prepared
containing the input data.calculateStatistics.R
script is used to
calculate the statistical contrasts. The results are attached to the
NormalyzerStatistics
object.## R Under development (unstable) (2024-10-21 r87258)
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## Running under: Ubuntu 24.04.1 LTS
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## attached base packages:
## [1] stats graphics grDevices utils datasets methods base
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## other attached packages:
## [1] NormalyzerDE_1.25.0
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## loaded via a namespace (and not attached):
## [1] SummarizedExperiment_1.37.0 gtable_0.3.6
## [3] xfun_0.48 bslib_0.8.0
## [5] ggplot2_3.5.1 Biobase_2.67.0
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## [9] tools_4.5.0 generics_0.1.3
## [11] parallel_4.5.0 stats4_4.5.0
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## [15] vsn_3.75.0 pkgconfig_2.0.3
## [17] Matrix_1.7-1 S4Vectors_0.45.0
## [19] lifecycle_1.0.4 GenomeInfoDbData_1.2.13
## [21] farver_2.1.2 compiler_4.5.0
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## [55] S4Arrays_1.7.0 utf8_1.2.4
## [57] ape_5.8 withr_3.0.2
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## [67] knitr_1.48 GenomicRanges_1.59.0
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## [71] rlang_1.1.4 Rcpp_1.0.13
## [73] glue_1.8.0 BiocManager_1.30.25
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