annotate template_script_edgeR_CL.r @ 2:d86ccac2a660 draft

New release of SARTools (1.3.2)
author lgueguen
date Wed, 17 May 2017 05:09:10 -0400
parents 581d217c7337
children de6d0b7c17af
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1 #!/local/gensoft2/exe/R/3.1.2/bin/Rscript
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2
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3 # to run this script, use one of these commands:
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4 # Rscript --no-save --no-restore --verbose template_script_edgeR_CL.r -r raw -v group -c T0 > log.txt 2>&1
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5 # Rscript template_script_edgeR_CL.r -r raw -v group -c T0
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6
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7 # to get help:
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8 # Rscript template_script_edgeR_CL.r --help
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9
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10 ################################################################################
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11 ### R script to compare several conditions with the SARTools and edgeR packages
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12 ### Hugo Varet
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13 ### April 20th, 2015
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14 ### designed to be executed with SARTools 1.1.0
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15 ################################################################################
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16
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17 rm(list=ls()) # remove all the objects from the R session
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18 library(optparse) # to run the script in command lines
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19
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20 # options list with associated default value.
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21 option_list <- list(
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22 make_option(c("-P", "--projectName"),
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23 default=basename(getwd()),
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24 dest="projectName",
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25 help="name of the project used for the report [default: name of the current directory]."),
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26
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27 make_option(c("-A", "--author"),
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28 default=Sys.info()[7],
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29 dest="author",
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30 help="name of the report author [default: %default]."),
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31
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32 make_option(c("-t", "--targetFile"),
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33 default="target.txt",
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34 dest="targetFile",
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35 help="path to the design/target file [default: %default]."),
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36
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37 make_option(c("-r", "--rawDir"),
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38 default="raw",
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39 dest="rawDir",
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40 help="path to the directory containing the HTSeq files [default: %default]."),
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41
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42 make_option(c("-F", "--featuresToRemove"),
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43 default="alignment_not_unique,ambiguous,no_feature,not_aligned,too_low_aQual",
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44 dest="FTR",
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45 help="names of the features to be removed, more than once can be specified [default: %default]"),
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46
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47 make_option(c("-v", "--varInt"),
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48 default="group",
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49 dest="varInt",
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50 help="factor of interest [default: %default]"),
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51
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52 make_option(c("-c", "--condRef"),
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53 default="WT",
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54 dest="condRef",
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55 help="reference biological condition [default: %default]"),
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56
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57 make_option(c("-b", "--batch"),
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58 default=NULL,
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59 dest="batch",
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60 help="blocking factor [default: %default] or \"batch\" for example"),
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61
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62 make_option(c("-a", "--alpha"),
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63 default=0.05,
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64 dest="alpha",
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65 help="threshold of statistical significance [default: %default]"),
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66
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67 make_option(c("-p", "--pAdjustMethod"),
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68 default="BH",
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69 dest="pAdjustMethod",
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70 help="p-value adjustment method: \"BH\" or \"BY\" [default: %default]"),
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71
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72 make_option(c("-m", "--cpmCutoff"),
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73 default=1,
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74 dest="cpmCutoff",
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75 help="counts-per-million cut-off to filter low counts"),
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76
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77 make_option(c("-g", "--gene.selection"),
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78 default="pairwise",
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79 dest="gene.selection",
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80 help="selection of the features in MDSPlot [default: %default]"),
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81
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82 make_option(c("-n", "--normalizationMethod"),
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83 default="TMM",
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84 dest="normalizationMethod",
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85 help="normalization method in calcNormFactors: \"TMM\", \"RLE\" or \"upperquartile\" [default: %default]"),
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86
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87 make_option(c("-C", "--colors"),
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88 default="dodgerblue,firebrick1,MediumVioletRed,SpringGreen,chartreuse,cyan,darkorchid,darkorange",
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89 dest="cols",
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90 help="colors of each biological condition on the plots\n\t\t\"col1,col2,col3,col4\"\n\t\t[default: %default]")
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91 )
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92
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93 # now parse the command line to check which option is given and get associated values
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94 parser <- OptionParser(usage="usage: %prog [options]",
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95 option_list=option_list,
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96 description="Compare two or more biological conditions in a RNA-Seq framework with edgeR.",
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97 epilogue="For comments, bug reports etc... please contact Hugo Varet <hugo.varet@pasteur.fr>")
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98 opt <- parse_args(parser, args=commandArgs(trailingOnly=TRUE), positional_arguments=0)$options
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99
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100 # get options and arguments
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101 workDir <- getwd()
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102 projectName <- opt$projectName # name of the project
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103 author <- opt$author # author of the statistical analysis/report
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104 targetFile <- opt$targetFile # path to the design/target file
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105 rawDir <- opt$rawDir # path to the directory containing raw counts files
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106 featuresToRemove <- unlist(strsplit(opt$FTR, ",")) # names of the features to be removed (specific HTSeq-count information and rRNA for example)
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107 varInt <- opt$varInt # factor of interest
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108 condRef <- opt$condRef # reference biological condition
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109 batch <- opt$batch # blocking factor: NULL (default) or "batch" for example
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110 alpha <- as.numeric(opt$alpha) # threshold of statistical significance
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111 pAdjustMethod <- opt$pAdjustMethod # p-value adjustment method: "BH" (default) or "BY"
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112 gene.selection <- opt$gene.selection # selection of the features in MDSPlot
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113 normalizationMethod <- opt$normalizationMethod # normalization method in calcNormFactors
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114 cpmCutoff <- opt$cpmCutoff # counts-per-million cut-off to filter low counts
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115 colors <- unlist(strsplit(opt$cols, ",")) # vector of colors of each biologicial condition on the plots
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116
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117 # print(paste("workDir", workDir))
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118 # print(paste("projectName", projectName))
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119 # print(paste("author", author))
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120 # print(paste("targetFile", targetFile))
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121 # print(paste("rawDir", rawDir))
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122 # print(paste("varInt", varInt))
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123 # print(paste("condRef", condRef))
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124 # print(paste("batch", batch))
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125 # print(paste("alpha", alpha))
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126 # print(paste("pAdjustMethod", pAdjustMethod))
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127 # print(paste("featuresToRemove", featuresToRemove))
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128 # print(paste("colors", colors))
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129 # print(paste("gene.selection", gene.selection))
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130 # print(paste("normalizationMethod", normalizationMethod))
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131 # print(paste("cpmCutoff", cpmCutoff))
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132
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133 ################################################################################
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134 ### running script ###
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135 ################################################################################
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136 # setwd(workDir)
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137 library(SARTools)
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138
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139 # checking parameters
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140 problem <- checkParameters.edgeR(projectName=projectName,author=author,targetFile=targetFile,
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141 rawDir=rawDir,featuresToRemove=featuresToRemove,varInt=varInt,
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142 condRef=condRef,batch=batch,alpha=alpha,pAdjustMethod=pAdjustMethod,
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143 cpmCutoff=cpmCutoff,gene.selection=gene.selection,
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144 normalizationMethod=normalizationMethod,colors=colors)
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145 if (problem) quit(save="yes")
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146
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147 # loading target file
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148 target <- loadTargetFile(targetFile=targetFile, varInt=varInt, condRef=condRef, batch=batch)
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149
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150 # loading counts
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151 counts <- loadCountData(target=target, rawDir=rawDir, featuresToRemove=featuresToRemove)
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152
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153 # description plots
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154 majSequences <- descriptionPlots(counts=counts, group=target[,varInt], col=colors)
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155
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156 # edgeR analysis
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157 out.edgeR <- run.edgeR(counts=counts, target=target, varInt=varInt, condRef=condRef,
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158 batch=batch, cpmCutoff=cpmCutoff, normalizationMethod=normalizationMethod,
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159 pAdjustMethod=pAdjustMethod)
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160
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161 # MDS + clustering
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162 exploreCounts(object=out.edgeR$dge, group=target[,varInt], gene.selection=gene.selection, col=colors)
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163
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164 # summary of the analysis (boxplots, dispersions, export table, nDiffTotal, histograms, MA plot)
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165 summaryResults <- summarizeResults.edgeR(out.edgeR, group=target[,varInt], counts=counts, alpha=alpha, col=colors)
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166
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167 # save image of the R session
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168 save.image(file=paste0(projectName, ".RData"))
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169
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170 # generating HTML report
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171 writeReport.edgeR(target=target, counts=counts, out.edgeR=out.edgeR, summaryResults=summaryResults,
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172 majSequences=majSequences, workDir=workDir, projectName=projectName, author=author,
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173 targetFile=targetFile, rawDir=rawDir, featuresToRemove=featuresToRemove, varInt=varInt,
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174 condRef=condRef, batch=batch, alpha=alpha, pAdjustMethod=pAdjustMethod, colors=colors,
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175 gene.selection=gene.selection, normalizationMethod=normalizationMethod)