R/functions_scc.R
In FrietzeLabUVM/ssvQC: QC for enrichment based NGS
Defines functions
gather_metrics
harmonize_seqlengths
getReadLength
crossCorrByRle
Documented in
harmonize_seqlengths
#functions from peakrefine
crossCorrByRle = function(bam_file,
query_gr,
max_dupes = 1,
fragment_sizes = 50:300,
read_length = NULL,
include_plots = TRUE,
...){
rn = cor = NULL # reserve for data.table
if(is.null(query_gr$name)){
if(is.null(names(query_gr))){
query_gr$name = paste0("peak_", seq_along(query_gr))
}else{
query_gr$name = names(query_gr)
}
}else{
if(is.null(names(query_gr))){
names(query_gr) = query_gr$name
}else{
#both names() and $name are set, leave it alone
}
}
names(query_gr) = query_gr$name
# query_gr = resize(query_gr, 500, fix = "center")
query_gr = harmonize_seqlengths(query_gr, bam_file)
Param <- Rsamtools::ScanBamParam(which=query_gr,
what=c("flag","mapq"),
...)
temp <- GenomicAlignments::readGAlignments(bam_file,param=Param)
dt = as.data.table(temp)
if(is.null(read_length)){
read_length = getReadLength(bam_file, query_gr)
}
if(length(read_length) == 0){
read_length = NA
}
if(is.na(read_length)){
read_length = numeric()
}
fragment_sizes = sort(union(read_length, fragment_sizes))
PosCoverage <- coverage(GenomicRanges::shift(GRanges(temp[strand(temp)=="+"])), -read_length)
PosCoverage = PosCoverage[query_gr]
names(PosCoverage) = query_gr$name
NegCoverage <- coverage(GRanges(temp[strand(temp)=="-"]))
NegCoverage = NegCoverage[query_gr]
names(NegCoverage) = query_gr$name
ShiftMatCor = pbapply::pbsapply(seq_along(query_gr), simplify = FALSE, function(i){
ShiftsCorTemp <- S4Vectors::shiftApply(fragment_sizes,
PosCoverage[[i]],
NegCoverage[[i]],
cor, simplify = FALSE,
verbose = FALSE)
})
#necessary due to singleton query_gr or shift not resulting in matrix
ShiftMatCor = matrix(unlist(ShiftMatCor),
byrow = FALSE,
nrow = length(fragment_sizes),
ncol = length(query_gr))
ShiftMatCor[is.nan(ShiftMatCor)] = 0
colnames(ShiftMatCor) = query_gr$name
rownames(ShiftMatCor) = fragment_sizes
shift_dt = as.data.table(ShiftMatCor, keep.rownames = TRUE)
shift_dt[, shift := as.numeric(rn)]
shift_dt$rn = NULL
shift_dt = melt(shift_dt, id.vars = "shift",
variable.name = "id", value.name = "correlation")
return(shift_dt)
}
getReadLength = function(bam_file,
query_gr){
Param <- Rsamtools::ScanBamParam(which=sample(query_gr, min(10, length(query_gr))),
what=c("flag","mapq"))
temp <- GenomicAlignments::readGAlignments(bam_file,param=Param)
readlength=as.numeric(names(sort(table(width(temp)), decreasing = TRUE))[1])
readlength
}
#' Forces seqlengths in GRanges to be that in header of bam_file
#'
#' This is important to avoid errors while using the gr to query the bam_file.
#'
#' @param gr GRanges
#' @param bam_file bam_file
#'
#' @return GRanges with seqlengths matching bam_file
#' @import Rsamtools GenomeInfoDb
#' @examples
#' peak_files = dir(system.file("extdata", package = "seqqc"), pattern = "Peak$", full.names = TRUE)
#' peak_grs = seqsetvis::easyLoad_narrowPeak(peak_files)
#' query_gr = resize(seqsetvis::ssvOverlapIntervalSets(peak_grs), 6e2, fix = "center")
#'
#' bam_files = dir(system.file("extdata", package = "seqqc"), pattern = "^M.+bam$", full.names = TRUE)
#'
#' query_gr.harmonized = seqqc:::harmonize_seqlengths(query_gr, bam_files[1])
#' seqlengths(query_gr.harmonized)
#'
harmonize_seqlengths = function(gr, bam_file){
chr_lengths = Rsamtools::scanBamHeader(bam_file)[[1]]$targets
GenomeInfoDb::seqlengths(gr) = chr_lengths[names(GenomeInfoDb::seqlengths(gr))]
too_long = end(gr) > GenomeInfoDb::seqlengths(gr)[as.character(seqnames(gr))]
if(any(too_long)){
message(sum(too_long), " region shifted for extending beyond seqlengths")
fix_gr = gr[too_long]
shift_by = -(end(fix_gr) - GenomeInfoDb::seqlengths(fix_gr)[as.character(seqnames(fix_gr))])
gr[too_long] = GenomicRanges::shift(fix_gr, shift_by)
}
too_short = start(gr) < 1
if(any(too_short)){
message(sum(too_short), " region shifted for starting before seqlengths")
fix_gr = gr[too_short]
shift_by = 1 - start(fix_gr)
gr[too_short] = GenomicRanges::shift(fix_gr, shift_by)
}
gr
}
gather_metrics = function(peak_strand_corr, read_length = NULL){
correlation = id = NULL
max_dt = peak_strand_corr[, list(shift = shift[which.max(correlation)], correlation = max(correlation)), by = list(id)]
# if(is.null(read_length)){
# fl = round(.my_mode(max_dt[shift != min(shift, na.rm = TRUE) & shift != max(shift, na.rm = TRUE)]$shift, na.rm = TRUE))
# }else{
# fl = round(.my_mode(max_dt[shift != read_length][shift != min(shift, na.rm = TRUE) & shift != max(shift, na.rm = TRUE)]$shift, na.rm = TRUE))
# }
flex_frag_corrs = max_dt[, list(shift, id, correlation)]
average_corr = peak_strand_corr[, list(correlation = mean(correlation)), list(shift)]
fl = average_corr[, shift[which.max(correlation)[1]]]
stable_frag_corrs = peak_strand_corr[shift == fl]
if(!is.null(read_length)){
read_corrs = peak_strand_corr[shift == read_length]
out = list(
read_length = read_length,
fragment_length = fl,
read_correlation = read_corrs,
flex_fragment_correlation = flex_frag_corrs,
stable_fragment_correlation = stable_frag_corrs,
full_correlation_results = peak_strand_corr,
average_correlation = average_corr)
}else{
read_corrs = copy(flex_frag_corrs)
read_corrs$shift = NA
read_corrs$correlation = NA
out = list(
read_length = NA,
fragment_length = fl,
read_correlation = read_corrs,
flex_fragment_correlation = flex_frag_corrs,
stable_fragment_correlation = stable_frag_corrs,
full_correlation_results = peak_strand_corr,
average_correlation = average_corr)
}
out
}
FrietzeLabUVM/ssvQC documentation built on March 25, 2024, 12:24 a.m.
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Defines functions gather_metrics harmonize_seqlengths getReadLength crossCorrByRle
Documented in harmonize_seqlengths
#functions from peakrefine
crossCorrByRle = function(bam_file,
query_gr,
max_dupes = 1,
fragment_sizes = 50:300,
read_length = NULL,
include_plots = TRUE,
...){
rn = cor = NULL # reserve for data.table
if(is.null(query_gr$name)){
if(is.null(names(query_gr))){
query_gr$name = paste0("peak_", seq_along(query_gr))
}else{
query_gr$name = names(query_gr)
}
}else{
if(is.null(names(query_gr))){
names(query_gr) = query_gr$name
}else{
#both names() and $name are set, leave it alone
}
}
names(query_gr) = query_gr$name
# query_gr = resize(query_gr, 500, fix = "center")
query_gr = harmonize_seqlengths(query_gr, bam_file)
Param <- Rsamtools::ScanBamParam(which=query_gr,
what=c("flag","mapq"),
...)
temp <- GenomicAlignments::readGAlignments(bam_file,param=Param)
dt = as.data.table(temp)
if(is.null(read_length)){
read_length = getReadLength(bam_file, query_gr)
}
if(length(read_length) == 0){
read_length = NA
}
if(is.na(read_length)){
read_length = numeric()
}
fragment_sizes = sort(union(read_length, fragment_sizes))
PosCoverage <- coverage(GenomicRanges::shift(GRanges(temp[strand(temp)=="+"])), -read_length)
PosCoverage = PosCoverage[query_gr]
names(PosCoverage) = query_gr$name
NegCoverage <- coverage(GRanges(temp[strand(temp)=="-"]))
NegCoverage = NegCoverage[query_gr]
names(NegCoverage) = query_gr$name
ShiftMatCor = pbapply::pbsapply(seq_along(query_gr), simplify = FALSE, function(i){
ShiftsCorTemp <- S4Vectors::shiftApply(fragment_sizes,
PosCoverage[[i]],
NegCoverage[[i]],
cor, simplify = FALSE,
verbose = FALSE)
})
#necessary due to singleton query_gr or shift not resulting in matrix
ShiftMatCor = matrix(unlist(ShiftMatCor),
byrow = FALSE,
nrow = length(fragment_sizes),
ncol = length(query_gr))
ShiftMatCor[is.nan(ShiftMatCor)] = 0
colnames(ShiftMatCor) = query_gr$name
rownames(ShiftMatCor) = fragment_sizes
shift_dt = as.data.table(ShiftMatCor, keep.rownames = TRUE)
shift_dt[, shift := as.numeric(rn)]
shift_dt$rn = NULL
shift_dt = melt(shift_dt, id.vars = "shift",
variable.name = "id", value.name = "correlation")
return(shift_dt)
}
getReadLength = function(bam_file,
query_gr){
Param <- Rsamtools::ScanBamParam(which=sample(query_gr, min(10, length(query_gr))),
what=c("flag","mapq"))
temp <- GenomicAlignments::readGAlignments(bam_file,param=Param)
readlength=as.numeric(names(sort(table(width(temp)), decreasing = TRUE))[1])
readlength
}
#' Forces seqlengths in GRanges to be that in header of bam_file
#'
#' This is important to avoid errors while using the gr to query the bam_file.
#'
#' @param gr GRanges
#' @param bam_file bam_file
#'
#' @return GRanges with seqlengths matching bam_file
#' @import Rsamtools GenomeInfoDb
#' @examples
#' peak_files = dir(system.file("extdata", package = "seqqc"), pattern = "Peak$", full.names = TRUE)
#' peak_grs = seqsetvis::easyLoad_narrowPeak(peak_files)
#' query_gr = resize(seqsetvis::ssvOverlapIntervalSets(peak_grs), 6e2, fix = "center")
#'
#' bam_files = dir(system.file("extdata", package = "seqqc"), pattern = "^M.+bam$", full.names = TRUE)
#'
#' query_gr.harmonized = seqqc:::harmonize_seqlengths(query_gr, bam_files[1])
#' seqlengths(query_gr.harmonized)
#'
harmonize_seqlengths = function(gr, bam_file){
chr_lengths = Rsamtools::scanBamHeader(bam_file)[[1]]$targets
GenomeInfoDb::seqlengths(gr) = chr_lengths[names(GenomeInfoDb::seqlengths(gr))]
too_long = end(gr) > GenomeInfoDb::seqlengths(gr)[as.character(seqnames(gr))]
if(any(too_long)){
message(sum(too_long), " region shifted for extending beyond seqlengths")
fix_gr = gr[too_long]
shift_by = -(end(fix_gr) - GenomeInfoDb::seqlengths(fix_gr)[as.character(seqnames(fix_gr))])
gr[too_long] = GenomicRanges::shift(fix_gr, shift_by)
}
too_short = start(gr) < 1
if(any(too_short)){
message(sum(too_short), " region shifted for starting before seqlengths")
fix_gr = gr[too_short]
shift_by = 1 - start(fix_gr)
gr[too_short] = GenomicRanges::shift(fix_gr, shift_by)
}
gr
}
gather_metrics = function(peak_strand_corr, read_length = NULL){
correlation = id = NULL
max_dt = peak_strand_corr[, list(shift = shift[which.max(correlation)], correlation = max(correlation)), by = list(id)]
# if(is.null(read_length)){
# fl = round(.my_mode(max_dt[shift != min(shift, na.rm = TRUE) & shift != max(shift, na.rm = TRUE)]$shift, na.rm = TRUE))
# }else{
# fl = round(.my_mode(max_dt[shift != read_length][shift != min(shift, na.rm = TRUE) & shift != max(shift, na.rm = TRUE)]$shift, na.rm = TRUE))
# }
flex_frag_corrs = max_dt[, list(shift, id, correlation)]
average_corr = peak_strand_corr[, list(correlation = mean(correlation)), list(shift)]
fl = average_corr[, shift[which.max(correlation)[1]]]
stable_frag_corrs = peak_strand_corr[shift == fl]
if(!is.null(read_length)){
read_corrs = peak_strand_corr[shift == read_length]
out = list(
read_length = read_length,
fragment_length = fl,
read_correlation = read_corrs,
flex_fragment_correlation = flex_frag_corrs,
stable_fragment_correlation = stable_frag_corrs,
full_correlation_results = peak_strand_corr,
average_correlation = average_corr)
}else{
read_corrs = copy(flex_frag_corrs)
read_corrs$shift = NA
read_corrs$correlation = NA
out = list(
read_length = NA,
fragment_length = fl,
read_correlation = read_corrs,
flex_fragment_correlation = flex_frag_corrs,
stable_fragment_correlation = stable_frag_corrs,
full_correlation_results = peak_strand_corr,
average_correlation = average_corr)
}
out
}
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