R/fcts_mass.R
In pkrog/biodb: biodb, a library and a development framework for connecting to chemical and biological databases
Defines functions
compareSpectra
calcDistance
simplifySpectrum
simplifySpectrum <- function(spec) {
if(length(spec) == 0){
return(NA_real_)
}
if (nrow(spec) == 0)
return(NA_real_)
# Get mz vals
mz.vals <- NULL
for (mzcol in c('mz', 'peak.mz', 'peak.mztheo', 'peak.mzexp'))
if (mzcol %in% colnames(spec)) {
mz.vals <- spec[, mzcol]
break
}
if (is.null(mz.vals))
stop("Cannot find MZ values.")
int.vals <- NULL
for (int.col in c('rel.int', 'peak.relative.intensity'))
if (int.col %in% colnames(spec)) {
int.vals <- spec[, int.col]
break
}
if (is.null(int.vals)) {
for (int.col in c('int', 'peak.intensity'))
if (int.col %in% colnames(spec)) {
int.vals <- spec[, int.col,]
int.vals <- int.vals * 100 / max(int.vals)
break
}
}
if (is.null(int.vals))
stop("Cannot find intensity values.")
spec <- data.frame(mz=mz.vals, int=int.vals)
colnames(spec) <- c('peak.mz', 'peak.relative.intensity')
return(spec)
}
calcDistance <- function(spec1, spec2, npmin=2, fun=c("wcosine"),
params=list()) {
#fun <- match.arg(fun)
#Spec are always normalized in percentage
spec1 <- simplifySpectrum(spec1)
spec2 <- simplifySpectrum(spec2)
if(any(is.na(spec1)) || any(is.na(spec2)))
return(list(matched=numeric(0),similarity=0))
params$mz1 <- as.numeric(spec1[, 'peak.mz'])
params$mz2 <- as.numeric(spec2[, 'peak.mz'])
params$int1 <- as.numeric(spec1[, 'peak.relative.intensity'])
params$int2 <- as.numeric(spec2[, 'peak.relative.intensity'])
res <- do.call(fun, args=params)
if (sum(res$matched != -1) < npmin)
return(list(matched=res$matched, similarity=0))
list(matched=res$matched,
similarity=res$measure)
}
compareSpectra <- function(spec, libspec, npmin=2, fun="wcosine",
params=list()) {
###The returned sim list is not ordered
res <- data.frame(score=numeric(0))
# Create one result column for each input spectrum peak
if ( ! is.null(spec)) {
peak.cols <- paste('peak', seq(nrow(spec)), sep='.')
for (p in peak.cols)
res[[p]] <- integer(0)
}
if ( ! is.null(libspec) && ! is.null(spec) && length(libspec) > 0
&& nrow(spec) > 0) {
# `spec` is supposed to be already normalized.
vall <- lapply(libspec, calcDistance, spec1=spec, npmin=npmin,
params=params, fun=fun)
# The list is ordered with the chosen metric.
sim <- vapply(vall, '[[', i="similarity", FUN.VALUE=1)
matched <- lapply(vall, '[[', i="matched")
res[seq_len(length(sim)), 'score'] <- sim
for (i in seq_len(length(matched)))
res[i, peak.cols] <- matched[[i]]
}
return(res)
}
pkrog/biodb documentation built on Nov. 29, 2022, 4:24 a.m.
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Defines functions compareSpectra calcDistance simplifySpectrum
simplifySpectrum <- function(spec) {
if(length(spec) == 0){
return(NA_real_)
}
if (nrow(spec) == 0)
return(NA_real_)
# Get mz vals
mz.vals <- NULL
for (mzcol in c('mz', 'peak.mz', 'peak.mztheo', 'peak.mzexp'))
if (mzcol %in% colnames(spec)) {
mz.vals <- spec[, mzcol]
break
}
if (is.null(mz.vals))
stop("Cannot find MZ values.")
int.vals <- NULL
for (int.col in c('rel.int', 'peak.relative.intensity'))
if (int.col %in% colnames(spec)) {
int.vals <- spec[, int.col]
break
}
if (is.null(int.vals)) {
for (int.col in c('int', 'peak.intensity'))
if (int.col %in% colnames(spec)) {
int.vals <- spec[, int.col,]
int.vals <- int.vals * 100 / max(int.vals)
break
}
}
if (is.null(int.vals))
stop("Cannot find intensity values.")
spec <- data.frame(mz=mz.vals, int=int.vals)
colnames(spec) <- c('peak.mz', 'peak.relative.intensity')
return(spec)
}
calcDistance <- function(spec1, spec2, npmin=2, fun=c("wcosine"),
params=list()) {
#fun <- match.arg(fun)
#Spec are always normalized in percentage
spec1 <- simplifySpectrum(spec1)
spec2 <- simplifySpectrum(spec2)
if(any(is.na(spec1)) || any(is.na(spec2)))
return(list(matched=numeric(0),similarity=0))
params$mz1 <- as.numeric(spec1[, 'peak.mz'])
params$mz2 <- as.numeric(spec2[, 'peak.mz'])
params$int1 <- as.numeric(spec1[, 'peak.relative.intensity'])
params$int2 <- as.numeric(spec2[, 'peak.relative.intensity'])
res <- do.call(fun, args=params)
if (sum(res$matched != -1) < npmin)
return(list(matched=res$matched, similarity=0))
list(matched=res$matched,
similarity=res$measure)
}
compareSpectra <- function(spec, libspec, npmin=2, fun="wcosine",
params=list()) {
###The returned sim list is not ordered
res <- data.frame(score=numeric(0))
# Create one result column for each input spectrum peak
if ( ! is.null(spec)) {
peak.cols <- paste('peak', seq(nrow(spec)), sep='.')
for (p in peak.cols)
res[[p]] <- integer(0)
}
if ( ! is.null(libspec) && ! is.null(spec) && length(libspec) > 0
&& nrow(spec) > 0) {
# `spec` is supposed to be already normalized.
vall <- lapply(libspec, calcDistance, spec1=spec, npmin=npmin,
params=params, fun=fun)
# The list is ordered with the chosen metric.
sim <- vapply(vall, '[[', i="similarity", FUN.VALUE=1)
matched <- lapply(vall, '[[', i="matched")
res[seq_len(length(sim)), 'score'] <- sim
for (i in seq_len(length(matched)))
res[i, peak.cols] <- matched[[i]]
}
return(res)
}
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