R/allPeptidesPlot.R
In Scavetta/ComPrAn: Complexome Profiling Analysis package
Defines functions
allPeptidesPlot
Documented in
allPeptidesPlot
#' Create scatter plot
#'
#' This function creates a plot of all peptides that belong to a single protein
#'
#' @param .listDF list, list containing data frames of peptides for each
#' protein indexed by `Protein Group Accessions`
#' @param protein character, `Protein Group Accession` to show in the plot
#' @param max_frac numeric, total number of fractions
#' @param meanLine logical, specifies whether to plot a mean line
#' @param repPepLine logical, specifies whether to plot a representative
#' peptide line
#' @param separateLabStates logical, specifies whether label states will be
#' separated into facets
#' @param titleLabel character, what to call the plot
#' @param titleAlign character, one of the 'left', 'center'/'centre', 'right',
#' specifies alignment of the title in plot
#' @param ylabel character
#' @param xlabel character
#' @param legendLabel character
#' @param grid logical, specifies presence/absence of gridline in the plot
#' @param labelled character, label to be used for isLabel == TRUE
#' @param unlabelled character, label to be used for isLabel == FALSE
#' @param controlSample character, either labelled or unlabelled, this setting
#' will adjust coloring based on which sample is a control
#' @param textSize numeric, size of text in the plot
#' @param axisTextSize numeric, size of axis labels in the plot
#'
#' @importFrom tibble rowid_to_column
#'
#' @return plot
#' @export
#'
#' @examples
#' ##Use example peptide data set, read in and clean data
#' inputFile <- system.file("extData", "data.txt", package = "ComPrAn")
#' peptides <- peptideImport(inputFile)
#' peptides <- cleanData(peptides, fCol = "Search ID")
#' ## separate chemical modifications and labelling into separate columns
#' peptides <- splitModLab(peptides)
#' ## remove unneccessary columns, simplify rows
#' peptides <- simplifyProteins(peptides)
#' ## Pick representative peptide for each protein for both scenarios
#' peptide_index <- pickPeptide(peptides)
#'
#' ##create a plot showing all peptides of selected protein
#' protein <- "P52815"
#' max_frac <- 23
#' #default plot
#' allPeptidesPlot(peptide_index,protein, max_frac = max_frac)
#' #other plot version
#' allPeptidesPlot(peptide_index,protein, max_frac = max_frac,
#' repPepLine = TRUE, grid = FALSE, titleAlign = "center")
#' #other plot version
#' allPeptidesPlot(peptide_index,protein, max_frac = max_frac,
#' repPepLine = TRUE, meanLine = TRUE, separateLabStates =TRUE,
#' titleLabel = "GN")
allPeptidesPlot <- function(.listDF, protein, max_frac, meanLine = FALSE,
repPepLine = FALSE,separateLabStates = FALSE,grid = TRUE,titleLabel = 'all',
titleAlign = 'left',ylabel = 'Precursor Area', xlabel = 'Fraction',
legendLabel = 'Condition', labelled = "Labeled", unlabelled = "Unlabeled",
controlSample = "",textSize = 12, axisTextSize = 8){
#if controlSample specified, adjust colouring so control is always same
if (controlSample == "labelled"|controlSample == "labeled"){
col_vector_peptides <- c("TRUE" = "#ffc125", "FALSE" = "#a020f0")
}else if(controlSample == "unlabelled"|controlSample == "unlabeled"){
col_vector_peptides <- c("FALSE" = "#ffc125", "TRUE" = "#a020f0")
}
dataFrame <- .listDF[[protein]]
#Next lines: edit data frame to neccessary format before plotting
description <- dataFrame$`Protein Descriptions`[1]
#add mean and repPepValue columns to DF, keep only necessary rows
data.frame(Value = NA, Fraction = seq_len(max_frac)) %>%
spread(Fraction, "Value") -> padding
dataFrame %>%
select(Fraction, `Precursor Area`, isLabel, repPepA) %>%
rowid_to_column() %>% spread(Fraction, `Precursor Area`) %>%
merge(padding, all.x = TRUE)%>%
gather(Fraction, `Precursor Area`, -c(isLabel,repPepA,rowid))%>%
group_by(Fraction, isLabel) %>%
mutate (meanValue = mean(`Precursor Area`, na.rm = TRUE)) %>%
mutate (repPepValue = ifelse(all(is.na(`Precursor Area`)),
NA, mean(`Precursor Area`[repPepA],
na.rm=TRUE))) %>%
ungroup() -> dataFrame
dataFrame$Fraction <- as.numeric(as.character(dataFrame$Fraction))
if (meanLine | repPepLine){alphaValue <- 0.20
} else {alphaValue <- 1} #transparent dots in case of drawing a line
linetype_vector <- c('twodash', 'solid') #define linetype_vector
names(linetype_vector) <- c('mean','representative peptide')
p <- ggplot(dataFrame,aes(Fraction, `Precursor Area`, colour = isLabel)) +
geom_point(na.rm = TRUE, alpha = alphaValue) +
scale_y_log10() +
scale_x_continuous(breaks = seq_len(max_frac), limits = c(0,max_frac))+
scale_colour_manual(legendLabel, values = col_vector_peptides,
labels = c("TRUE" = labelled,
"FALSE" = unlabelled)) +
ylab (ylabel) + xlab (xlabel) +
scale_linetype_manual('Line type', values = linetype_vector)
if(grid){p<- p +theme_minimal() + #add grid
theme(panel.grid.minor = element_blank())
} else {p<- p +theme_classic()}
if (titleAlign == 'left'){adjust <- 0 #title alignment settings
} else if ((titleAlign == 'centre')|(titleAlign=='center')) {adjust <- 0.5
} else if(titleAlign == 'right'){adjust <- 1}
if (titleLabel == 'all'){
p <- p+labs(title=str_remove(str_extract(description, "^.* OS")," OS"),
subtitle = str_extract(str_remove(description," PE=.*$"), "OS=.*$"),
caption = paste('UniProt ID:', protein, sep ='')) +
theme(plot.title = element_text(hjust = adjust))
} else if (titleLabel == 'GN') {
p <- p + labs(title = str_remove(
str_extract(description, "GN=[:alnum:]*"), "GN="),
caption = paste('UniProt ID:', protein, sep ='')) +
theme(plot.title = element_text(hjust = adjust))
} else {p <- p + labs( title = titleLabel,
caption = paste('UniProt ID:', protein, sep ='')) +
theme(plot.title = element_text(hjust = adjust))}
if(meanLine) { ## add line that is a mean of all peptide values
p <- p + geom_line(aes(y=meanValue, colour = isLabel,linetype ='mean'),
size = 1, na.rm = TRUE)
}
if (repPepLine) { ## add rep pep line fir scenario A
p <- p + geom_line(aes(y = repPepValue, colour = isLabel,
linetype = 'representative peptide'),size=1, na.rm = TRUE)+
geom_point(aes(y=repPepValue,colour=isLabel),na.rm=TRUE,alpha = 1)
}
#edit title in case of a multiprotein group
if(str_detect(description,'\\|')){
p <- p + labs(title = protein,
subtitle = 'Multiple proteins group')+
theme(plot.title = element_text(hjust = adjust))
}
#make facets if one wishes to separate label states
if(separateLabStates){
p <- p + facet_wrap(isLabel ~ ., nrow =2,scales = "free_x")+
theme(strip.text = element_blank())
}
p <- p + theme(text = element_text(size = textSize), #adjust text size
axis.text=element_text(size = axisTextSize))
return (p)
}
Scavetta/ComPrAn documentation built on Oct. 3, 2022, 1:08 a.m.
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Defines functions allPeptidesPlot
Documented in allPeptidesPlot
#' Create scatter plot
#'
#' This function creates a plot of all peptides that belong to a single protein
#'
#' @param .listDF list, list containing data frames of peptides for each
#' protein indexed by `Protein Group Accessions`
#' @param protein character, `Protein Group Accession` to show in the plot
#' @param max_frac numeric, total number of fractions
#' @param meanLine logical, specifies whether to plot a mean line
#' @param repPepLine logical, specifies whether to plot a representative
#' peptide line
#' @param separateLabStates logical, specifies whether label states will be
#' separated into facets
#' @param titleLabel character, what to call the plot
#' @param titleAlign character, one of the 'left', 'center'/'centre', 'right',
#' specifies alignment of the title in plot
#' @param ylabel character
#' @param xlabel character
#' @param legendLabel character
#' @param grid logical, specifies presence/absence of gridline in the plot
#' @param labelled character, label to be used for isLabel == TRUE
#' @param unlabelled character, label to be used for isLabel == FALSE
#' @param controlSample character, either labelled or unlabelled, this setting
#' will adjust coloring based on which sample is a control
#' @param textSize numeric, size of text in the plot
#' @param axisTextSize numeric, size of axis labels in the plot
#'
#' @importFrom tibble rowid_to_column
#'
#' @return plot
#' @export
#'
#' @examples
#' ##Use example peptide data set, read in and clean data
#' inputFile <- system.file("extData", "data.txt", package = "ComPrAn")
#' peptides <- peptideImport(inputFile)
#' peptides <- cleanData(peptides, fCol = "Search ID")
#' ## separate chemical modifications and labelling into separate columns
#' peptides <- splitModLab(peptides)
#' ## remove unneccessary columns, simplify rows
#' peptides <- simplifyProteins(peptides)
#' ## Pick representative peptide for each protein for both scenarios
#' peptide_index <- pickPeptide(peptides)
#'
#' ##create a plot showing all peptides of selected protein
#' protein <- "P52815"
#' max_frac <- 23
#' #default plot
#' allPeptidesPlot(peptide_index,protein, max_frac = max_frac)
#' #other plot version
#' allPeptidesPlot(peptide_index,protein, max_frac = max_frac,
#' repPepLine = TRUE, grid = FALSE, titleAlign = "center")
#' #other plot version
#' allPeptidesPlot(peptide_index,protein, max_frac = max_frac,
#' repPepLine = TRUE, meanLine = TRUE, separateLabStates =TRUE,
#' titleLabel = "GN")
allPeptidesPlot <- function(.listDF, protein, max_frac, meanLine = FALSE,
repPepLine = FALSE,separateLabStates = FALSE,grid = TRUE,titleLabel = 'all',
titleAlign = 'left',ylabel = 'Precursor Area', xlabel = 'Fraction',
legendLabel = 'Condition', labelled = "Labeled", unlabelled = "Unlabeled",
controlSample = "",textSize = 12, axisTextSize = 8){
#if controlSample specified, adjust colouring so control is always same
if (controlSample == "labelled"|controlSample == "labeled"){
col_vector_peptides <- c("TRUE" = "#ffc125", "FALSE" = "#a020f0")
}else if(controlSample == "unlabelled"|controlSample == "unlabeled"){
col_vector_peptides <- c("FALSE" = "#ffc125", "TRUE" = "#a020f0")
}
dataFrame <- .listDF[[protein]]
#Next lines: edit data frame to neccessary format before plotting
description <- dataFrame$`Protein Descriptions`[1]
#add mean and repPepValue columns to DF, keep only necessary rows
data.frame(Value = NA, Fraction = seq_len(max_frac)) %>%
spread(Fraction, "Value") -> padding
dataFrame %>%
select(Fraction, `Precursor Area`, isLabel, repPepA) %>%
rowid_to_column() %>% spread(Fraction, `Precursor Area`) %>%
merge(padding, all.x = TRUE)%>%
gather(Fraction, `Precursor Area`, -c(isLabel,repPepA,rowid))%>%
group_by(Fraction, isLabel) %>%
mutate (meanValue = mean(`Precursor Area`, na.rm = TRUE)) %>%
mutate (repPepValue = ifelse(all(is.na(`Precursor Area`)),
NA, mean(`Precursor Area`[repPepA],
na.rm=TRUE))) %>%
ungroup() -> dataFrame
dataFrame$Fraction <- as.numeric(as.character(dataFrame$Fraction))
if (meanLine | repPepLine){alphaValue <- 0.20
} else {alphaValue <- 1} #transparent dots in case of drawing a line
linetype_vector <- c('twodash', 'solid') #define linetype_vector
names(linetype_vector) <- c('mean','representative peptide')
p <- ggplot(dataFrame,aes(Fraction, `Precursor Area`, colour = isLabel)) +
geom_point(na.rm = TRUE, alpha = alphaValue) +
scale_y_log10() +
scale_x_continuous(breaks = seq_len(max_frac), limits = c(0,max_frac))+
scale_colour_manual(legendLabel, values = col_vector_peptides,
labels = c("TRUE" = labelled,
"FALSE" = unlabelled)) +
ylab (ylabel) + xlab (xlabel) +
scale_linetype_manual('Line type', values = linetype_vector)
if(grid){p<- p +theme_minimal() + #add grid
theme(panel.grid.minor = element_blank())
} else {p<- p +theme_classic()}
if (titleAlign == 'left'){adjust <- 0 #title alignment settings
} else if ((titleAlign == 'centre')|(titleAlign=='center')) {adjust <- 0.5
} else if(titleAlign == 'right'){adjust <- 1}
if (titleLabel == 'all'){
p <- p+labs(title=str_remove(str_extract(description, "^.* OS")," OS"),
subtitle = str_extract(str_remove(description," PE=.*$"), "OS=.*$"),
caption = paste('UniProt ID:', protein, sep ='')) +
theme(plot.title = element_text(hjust = adjust))
} else if (titleLabel == 'GN') {
p <- p + labs(title = str_remove(
str_extract(description, "GN=[:alnum:]*"), "GN="),
caption = paste('UniProt ID:', protein, sep ='')) +
theme(plot.title = element_text(hjust = adjust))
} else {p <- p + labs( title = titleLabel,
caption = paste('UniProt ID:', protein, sep ='')) +
theme(plot.title = element_text(hjust = adjust))}
if(meanLine) { ## add line that is a mean of all peptide values
p <- p + geom_line(aes(y=meanValue, colour = isLabel,linetype ='mean'),
size = 1, na.rm = TRUE)
}
if (repPepLine) { ## add rep pep line fir scenario A
p <- p + geom_line(aes(y = repPepValue, colour = isLabel,
linetype = 'representative peptide'),size=1, na.rm = TRUE)+
geom_point(aes(y=repPepValue,colour=isLabel),na.rm=TRUE,alpha = 1)
}
#edit title in case of a multiprotein group
if(str_detect(description,'\\|')){
p <- p + labs(title = protein,
subtitle = 'Multiple proteins group')+
theme(plot.title = element_text(hjust = adjust))
}
#make facets if one wishes to separate label states
if(separateLabStates){
p <- p + facet_wrap(isLabel ~ ., nrow =2,scales = "free_x")+
theme(strip.text = element_blank())
}
p <- p + theme(text = element_text(size = textSize), #adjust text size
axis.text=element_text(size = axisTextSize))
return (p)
}
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