annotate small_rna_maps.r @ 15:82fedc576024 draft

planemo upload for repository https://github.com/ARTbio/tools-artbio/tree/master/tools/small_rna_maps commit c1d96f7f028512aa4d8fcae3dd5f967cd445708e
author artbio
date Sat, 06 Oct 2018 05:24:15 -0400
parents cd75c72e1d75
children b585cb347a26
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1 ## Setup R error handling to go to stderr
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2 options( show.error.messages=F,
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3 error = function () { cat( geterrmessage(), file=stderr() ); q( "no", 1, F ) } )
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4 options(warn = -1)
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5 library(RColorBrewer)
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6 library(lattice)
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7 library(latticeExtra)
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8 library(grid)
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9 library(gridExtra)
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10 library(optparse)
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13 option_list <- list(
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14 make_option(c("-i", "--ymin"), type="double", help="set min ylimit. e.g. '-100.0'"),
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15 make_option(c("-a", "--ymax"), type="double", help="set max ylimit. e.g. '100.0'"),
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16 make_option(c("-f", "--first_dataframe"), type="character", help="path to first dataframe"),
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17 make_option(c("-e", "--extra_dataframe"), type="character", help="path to additional dataframe"),
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18 make_option(c("-n", "--normalization"), type="character", help="space-separated normalization/size factors"),
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19 make_option("--first_plot_method", type = "character", help="How additional data should be plotted"),
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20 make_option("--extra_plot_method", type = "character", help="How additional data should be plotted"),
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21 make_option("--global", type = "character", help="data should be plotted as global size distribution"),
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22 make_option("--output_pdf", type = "character", help="path to the pdf file with plots")
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23 )
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25 parser <- OptionParser(usage = "%prog [options] file", option_list = option_list)
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26 args = parse_args(parser)
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27
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28 # data frames implementation
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29 ## first table
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30 Table = read.delim(args$first_dataframe, header=T, row.names=NULL)
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31 if (args$first_plot_method == "Counts" | args$first_plot_method == "Size") {
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32 Table <- within(Table, Counts[Polarity=="R"] <- (Counts[Polarity=="R"]*-1))
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33 }
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34 n_samples=length(unique(Table$Dataset))
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35 samples = unique(Table$Dataset)
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36 if (args$normalization != "") {
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37 norm_factors = as.numeric(unlist(strsplit(args$normalization, " ")))
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38 } else {
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39 norm_factors = rep(1, n_samples)
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40 }
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41 if (args$first_plot_method == "Counts" | args$first_plot_method == "Size" | args$first_plot_method == "Coverage") {
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42 i = 1
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43 for (sample in samples) {
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44 Table[, length(Table)][Table$Dataset==sample] <- Table[, length(Table)][Table$Dataset==sample]*norm_factors[i]
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45 i = i + 1
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46 }
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47 }
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48 genes=unique(Table$Chromosome)
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49 per_gene_readmap=lapply(genes, function(x) subset(Table, Chromosome==x))
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50 per_gene_limit=lapply(genes, function(x) c(1, unique(subset(Table, Chromosome==x)$Chrom_length)) )
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51 n_genes=length(per_gene_readmap)
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52 # second table
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53 if (args$extra_plot_method != '') {
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54 ExtraTable=read.delim(args$extra_dataframe, header=T, row.names=NULL)
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55 if (args$extra_plot_method == "Counts" | args$extra_plot_method=='Size') {
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56 ExtraTable <- within(ExtraTable, Counts[Polarity=="R"] <- (Counts[Polarity=="R"]*-1))
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57 }
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58 if (args$extra_plot_method == "Counts" | args$extra_plot_method == "Size" | args$extra_plot_method == "Coverage") {
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59 i = 1
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60 for (sample in samples) {
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61 ExtraTable[, length(ExtraTable)][ExtraTable$Dataset==sample] <- ExtraTable[, length(ExtraTable)][ExtraTable$Dataset==sample]*norm_factors[i]
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62 i = i + 1
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63 }
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64 }
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65 per_gene_size=lapply(genes, function(x) subset(ExtraTable, Chromosome==x))
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66 }
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67
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68 ## functions
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69 globalbc = function(df, global="", ...) {
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70 if (global == "yes") {
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71 bc <- barchart(Counts~as.factor(Size)|factor(Dataset, levels=unique(Dataset)),
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72 data = df, origin = 0,
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73 horizontal=FALSE,
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74 col=c("darkblue"),
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75 scales=list(y=list(tick.number=4, rot=90, relation="free", cex=0.5, alternating=T), x=list(rot=0, cex=0.6, tck=0.5, alternating=c(3,3))),
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76 xlab=list(label=bottom_first_method[[args$first_plot_method]], cex=.85),
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77 ylab=list(label=legend_first_method[[args$first_plot_method]], cex=.85),
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78 main=title_first_method[[args$first_plot_method]],
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79 layout = c(2, 6), newpage=T,
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80 as.table=TRUE,
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81 aspect=0.5,
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82 strip = strip.custom(par.strip.text = list(cex = 1), which.given=1, bg="lightblue"),
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83 ...
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84 )
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85 } else {
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86 bc <- barchart(Counts~as.factor(Size)|factor(Dataset, levels=unique(Dataset)),
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87 data = df, origin = 0,
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88 horizontal=FALSE,
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89 group=Polarity,
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90 stack=TRUE,
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91 col=c('red', 'blue'),
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92 scales=list(y=list(tick.number=4, rot=90, relation="free", cex=0.5, alternating=T), x=list(rot=0, cex=0.6, tck=0.5, alternating=c(3,3))),
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93 xlab=list(label=bottom_first_method[[args$first_plot_method]], cex=.85),
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94 ylab=list(label=legend_first_method[[args$first_plot_method]], cex=.85),
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95 main=title_first_method[[args$first_plot_method]],
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96 layout = c(2, 6), newpage=T,
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97 as.table=TRUE,
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98 aspect=0.5,
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99 strip = strip.custom(par.strip.text = list(cex = 1), which.given=1, bg="lightblue"),
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100 ...
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101 )
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102 }
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103 return(bc)
7
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104 }
5
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105 plot_unit = function(df, method=args$first_plot_method, ...) {
12
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106 if (exists('ymin', where=args)){
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107 min=args$ymin
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108 }else{
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109 min=''
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110 }
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111 if ((exists('ymax', where=args))){
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112 max=args$ymax
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113 }else{
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114 max=''
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115 }
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116 ylimits=c(min,max)
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117 if (method == 'Counts') {
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118 p = xyplot(Counts~Coordinate|factor(Dataset, levels=unique(Dataset))+factor(Chromosome, levels=unique(Chromosome)),
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119 data=df,
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120 type='h',
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121 lwd=1.5,
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122 scales= list(relation="free", x=list(rot=0, cex=0.7, axs="i", tck=0.5), y=list(tick.number=4, rot=90, cex=0.7)),
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123 xlab=NULL, main=NULL, ylab=NULL, ylim=ylimits,
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124 as.table=T,
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125 origin = 0,
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126 horizontal=FALSE,
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127 group=Polarity,
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128 col=c("red","blue"),
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129 par.strip.text = list(cex=0.7),
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130 ...)
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131 p=combineLimits(p)
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132 } else if (method != "Size") {
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133 p = xyplot(eval(as.name(method))~Coordinate|factor(Dataset, levels=unique(Dataset))+factor(Chromosome, levels=unique(Chromosome)),
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134 data=df,
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135 type='p',
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136 pch=19,
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137 cex=0.35,
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138 scales= list(relation="free", x=list(rot=0, cex=0.7, tck=0.5), y=list(tick.number=4, rot=90, cex=0.7)),
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139 xlab=NULL, main=NULL, ylab=NULL, ylim=ylimits,
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140 as.table=T,
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141 origin = 0,
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142 horizontal=FALSE,
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143 group=Polarity,
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144 col=c("red","blue"),
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145 par.strip.text = list(cex=0.7),
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146 ...)
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147 } else {
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148 p = barchart(Counts~as.factor(Size)|factor(Dataset, levels=unique(Dataset))+Chromosome, data = df, origin = 0,
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149 horizontal=FALSE,
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150 group=Polarity,
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151 stack=TRUE,
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152 col=c('red', 'blue'),
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153 scales=list(y=list(rot=90, relation="free", cex=0.7), x=list(rot=0, cex=0.7, axs="i", tck=c(1,0))),
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154 xlab = NULL,
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155 ylab = NULL,
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156 main = NULL,
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157 as.table=TRUE,
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158 par.strip.text = list(cex=0.6),
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159 ...)
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160 p=combineLimits(p)
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161 }
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diff changeset
162 return(p)
5
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163 }
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164
12
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165
5
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166 ## function parameters
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167
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168 #par.settings.firstplot = list(layout.heights=list(top.padding=11, bottom.padding = -14))
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169 #par.settings.secondplot=list(layout.heights=list(top.padding=11, bottom.padding = -15), strip.background=list(col=c("lavender","deepskyblue")))
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170 par.settings.firstplot = list(layout.heights=list(top.padding=-2, bottom.padding=-2),strip.background=list(col=c("lightblue","lightgreen")))
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171 par.settings.secondplot=list(layout.heights=list(top.padding=-1, bottom.padding=-1),strip.background=list(col=c("lightblue","lightgreen")))
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172 title_first_method = list(Counts="Read Counts", Coverage="Coverage depths", Median="Median sizes", Mean="Mean sizes", Size="Size Distributions")
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173 title_extra_method = list(Counts="Read Counts", Coverage="Coverage depths", Median="Median sizes", Mean="Mean sizes", Size="Size Distributions")
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174 legend_first_method =list(Counts="Read count", Coverage="Coverage depth", Median="Median size", Mean="Mean size", Size="Read count")
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175 legend_extra_method =list(Counts="Read count", Coverage="Coverage depth", Median="Median size", Mean="Mean size", Size="Read count")
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176 bottom_first_method =list(Counts="Coordinates (nucleotides)",Coverage="Coordinates (nucleotides)", Median="Coordinates (nucleotides)", Mean="Coordinates (nucleotides)", Size="Sizes of reads")
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177 bottom_extra_method =list(Counts="Coordinates (nucleotides)",Coverage="Coordinates (nucleotides)", Median="Coordinates (nucleotides)", Mean="Coordinates (nucleotides)", Size="Sizes of reads")
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178
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179 ## Plotting Functions
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180
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181 double_plot <- function(...) {
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182 page_height = 15
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183 rows_per_page = 10
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184 graph_heights=c(40,30,40,30,40,30,40,30,40,30,10)
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185 page_width=8.2677 * n_samples / 2
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186 pdf(file=args$output_pdf, paper="special", height=page_height, width=page_width)
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187 for (i in seq(1,n_genes,rows_per_page/2)) {
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188 start=i
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189 end=i+rows_per_page/2-1
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190 if (end>n_genes) {end=n_genes}
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191 if (end-start+1 < 5) {graph_heights=c(rep(c(40,30),end-start+1),10,rep(c(40,30),5-(end-start+1)))}
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192 first_plot.list = lapply(per_gene_readmap[start:end], function(x) update(useOuterStrips(plot_unit(x, par.settings=par.settings.secondplot), strip.left=strip.custom(par.strip.text = list(cex=0.5)))))
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193 second_plot.list = lapply(per_gene_size[start:end], function(x) update(useOuterStrips(plot_unit(x, method=args$extra_plot_method, par.settings=par.settings.firstplot), strip.left=strip.custom(par.strip.text = list(cex=0.5)), strip=FALSE)))
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194 plot.list=rbind(first_plot.list, second_plot.list)
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195 args_list=c(plot.list, list( nrow=rows_per_page+1, ncol=1, heights=unit(graph_heights, rep("mm", 11)),
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196 top=textGrob(paste(title_first_method[[args$first_plot_method]], "and", title_extra_method[[args$extra_plot_method]]), gp=gpar(cex=1), vjust=0, just="top"),
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197 left=textGrob(paste(legend_first_method[[args$first_plot_method]], "/", legend_extra_method[[args$extra_plot_method]]), gp=gpar(cex=1), vjust=0, hjust=0, x=1, y=(-0.38/4)*(end-start-(3.28/0.38)), rot=90),
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198 sub=textGrob(paste(bottom_first_method[[args$first_plot_method]], "/", bottom_extra_method[[args$extra_plot_method]]), gp=gpar(cex=1), just="bottom", vjust=2)
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199 )
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200 )
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201 do.call(grid.arrange, args_list)
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202 }
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203 devname=dev.off()
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204 }
0
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205
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206
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207 single_plot <- function(...) {
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208 width = 8.2677 * n_samples / 2
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209 rows_per_page=8
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210 graph_heights=c(rep(40,8),10)
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211 pdf(file=args$output_pdf, paper="special", height=15, width=width)
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212 for (i in seq(1,n_genes,rows_per_page)) {
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213 start=i
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214 end=i+rows_per_page-1
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215 if (end>n_genes) {end=n_genes}
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216 if (end-start+1 < 8) {graph_heights=c(rep(c(40),end-start+1),10,rep(c(40),8-(end-start+1)))}
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217 first_plot.list = lapply(per_gene_readmap[start:end], function(x) update(useOuterStrips(plot_unit(x, par.settings=par.settings.firstplot),strip.left=strip.custom(par.strip.text = list(cex=0.5)))))
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218 plot.list=rbind(first_plot.list)
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219 args_list=c(plot.list, list( nrow=rows_per_page+1, ncol=1, heights=unit(graph_heights, rep("mm", 9)),
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220 top=textGrob(title_first_method[[args$first_plot_method]], gp=gpar(cex=1), vjust=0, just="top"),
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221 left=textGrob(legend_first_method[[args$first_plot_method]], gp=gpar(cex=1), vjust=0, hjust=0, x=1, y=(-0.41/7)*(end-start-(6.23/0.41)), rot=90),
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222 sub=textGrob(bottom_first_method[[args$first_plot_method]], gp=gpar(cex=1), just="bottom", vjust=2)
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223 )
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224 )
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225 do.call(grid.arrange, args_list)
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226 }
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227 devname=dev.off()
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228 }
0
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229
5
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230 # main
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231
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232 if (args$extra_plot_method != '') { double_plot() }
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233 if (args$extra_plot_method == '' & !exists('global', where=args)) {
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234 single_plot()
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235 }
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236 if (exists('global', where=args)) {
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237 pdf(file=args$output, paper="special", height=11.69)
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238 Table <- within(Table, Counts[Polarity=="R"] <- abs(Counts[Polarity=="R"])) # retropedalage
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239 library(reshape2)
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240 ml = melt(Table, id.vars = c("Dataset", "Chromosome", "Polarity", "Size"))
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241 if (args$global == "nomerge") {
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242 castml = dcast(ml, Dataset+Polarity+Size ~ variable, function(x) sum(x))
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243 castml <- within(castml, Counts[Polarity=="R"] <- (Counts[Polarity=="R"]*-1))
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244 bc = globalbc(castml, global="no")
d33263e6e812 planemo upload for repository https://github.com/ARTbio/tools-artbio/tree/master/tools/small_rna_maps commit b0676fd329c2ca50002f9f2fede531d8e550569f
artbio
parents: 11
diff changeset
245 } else {
d33263e6e812 planemo upload for repository https://github.com/ARTbio/tools-artbio/tree/master/tools/small_rna_maps commit b0676fd329c2ca50002f9f2fede531d8e550569f
artbio
parents: 11
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246 castml = dcast(ml, Dataset+Size ~ variable, function(x) sum(x))
d33263e6e812 planemo upload for repository https://github.com/ARTbio/tools-artbio/tree/master/tools/small_rna_maps commit b0676fd329c2ca50002f9f2fede531d8e550569f
artbio
parents: 11
diff changeset
247 bc = globalbc(castml, global="yes")
d33263e6e812 planemo upload for repository https://github.com/ARTbio/tools-artbio/tree/master/tools/small_rna_maps commit b0676fd329c2ca50002f9f2fede531d8e550569f
artbio
parents: 11
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248 }
d33263e6e812 planemo upload for repository https://github.com/ARTbio/tools-artbio/tree/master/tools/small_rna_maps commit b0676fd329c2ca50002f9f2fede531d8e550569f
artbio
parents: 11
diff changeset
249 plot(bc)
d33263e6e812 planemo upload for repository https://github.com/ARTbio/tools-artbio/tree/master/tools/small_rna_maps commit b0676fd329c2ca50002f9f2fede531d8e550569f
artbio
parents: 11
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250 devname=dev.off()
7
a96e6a7df2b7 planemo upload for repository https://github.com/ARTbio/tools-artbio/tree/master/tools/small_rna_maps commit 06472d1bd1365e4f7b385d578a69f4646481e22f
artbio
parents: 6
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251 }
0
6d48150495e3 planemo upload for repository https://github.com/ARTbio/tools-artbio/tree/master/tools/small_rna_maps commit d4d8106d66b65679a1a685ab94bfcf99cdb7b959
artbio
parents:
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252