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### R code from vignette source 'isobar-ptm.Rnw'
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### code chunk number 1: init
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require(ggplot2)
dir.create(file.path("graphics"), showWarnings = FALSE)
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### code chunk number 2: load-isobar
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library(isobar) ## load the isobar package
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### code chunk number 3: isobar-ptm.Rnw:81-87 (eval = FALSE)
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## # Generate PhosphoRS XML input file based on MGF and identification file
## # massTolerance: fragment ion mass tolerance (in Da)
## # activationType: CID, HCD, or ETD
## writePhosphoRSInput("phosphors.in.xml",
## "identifications.id.csv","peaklist.mgf",
## massTolerance=0.5,activationType="CID")
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### code chunk number 4: isobar-ptm.Rnw:94-98 (eval = FALSE)
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## # Read PhosphoRS XML output file
## # simplify: if TRUE, a data.frame is returned, else a list
## # besthit.only: if TRUE, only the best localization per spectrum is returned
## readPhosphoRSOutput("phosphors.out.xml",simplify=TRUE,besthit.only=TRUE)
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### code chunk number 5: isobar-ptm.Rnw:104-107 (eval = FALSE)
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## getPhosphoRSProbabilities("identifications.id.csv","peaklist.mgf",
## massTolerance=0.5,activationType="CID",
## phosphors.cmd="java -jar phosphoRS.jar")
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### code chunk number 6: isobar-ptm.Rnw:125-140 (eval = FALSE)
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## # filterSpectraDeltaScore calls calc.delta.score
## # if no column named delta.score is present in the data frame
## # identifications below a min.delta.score are REMOVED
## ib <- readIBSpectra("identifications.id.csv","peaklist.mgf",
## annotate.spectra.f=function(...)
## filterSpectraDeltaScore(...,min.delta.score=10))
##
##
## # filterSpectraPhosphoRS calls PhosphoRS to caluclate PhosphoRS probabilities
## # identifications below a min.prob (PhosphoRS peptide isoform probability)
## # are marked to be NOT QUANTIFIED (use.for.quant=FALSE), but not removed
## ib <- readIBSpectra("identifications.id.csv","peaklist.mgf",
## annotate.spectra.f=
## function(...) filterSpectraPhosphoRS(...,min.prob=0.9,
## phosphors.cmd="java -jar PhosphoRS.jar"))
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### code chunk number 7: isobar-ptm.Rnw:161-165
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data(ib_phospho)
data(noise.model.hcd)
head(proteinGroup(ib_phospho)@peptideInfo)
10^estimateRatio(ib_phospho,noise.model.hcd,peptide="SPLSPTETFSWPDVR")
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### code chunk number 8: isobar-ptm.Rnw:170-176
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pep.n.modif <- unique(apply(fData(ib_phospho)[,c("peptide","modif")],2,cbind))
print(head(pep.n.modif))
estimateRatio(ib_phospho,noise.model.hcd,channel1="114",channel2="115",
peptide=head(pep.n.modif),combine=FALSE)[,c("lratio","variance",
"n.spectra","p.value.rat")]
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### code chunk number 9: ratiodistr
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suppressPackageStartupMessages(library(distr))
suppressPackageStartupMessages(library(ggplot2))
peptide.ratios <- peptideRatios(ib_phospho,noise.model=noise.model.hcd,
cmbn=matrix(c("114","116"),ncol=1))
lim <- max(abs(peptide.ratios$lratio),na.rm=TRUE)
peptide.distr.cauchy <- fitCauchy(peptide.ratios$lratio)
pseq <- seq(from=-lim,to=lim,length.out=1000)
ggplot() +
geom_histogram(aes(x=lratio,y=..density..),data=peptide.ratios,binwidth=0.05,
color="darkgreen",fill="white") +
geom_line(aes(x=x,y=y),color="black",
data=data.frame(x=pseq,y=d(peptide.distr.cauchy)(pseq)))
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### code chunk number 10: isobar-ptm.Rnw:233-243
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peptides <- pep.n.modif[1:5,]
orig.ratio <- estimateRatio(ib_phospho,noise.model.hcd,channel1="114",channel2="115",
peptide=peptides,combine=FALSE)[,c("lratio","variance")]
peptides.c <- cbind(peptides,correct.ratio=c(0,-1,1,2,-2))
corr.ratio <- estimateRatio(ib_phospho,noise.model.hcd,channel1="114",channel2="115",
peptide=peptides.c,combine=FALSE)[,c("lratio","variance")]
data.frame(peptides.c,orig.ratio,corr.ratio)
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### code chunk number 11: isobar-ptm.Rnw:264-266 (eval = FALSE)
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## ptm.info <- getPtmInfoFromPhosphoSitePlus(proteinGroup(ib_phospho),modif="PHOS")
## ptm.info <- getPtmInfoFromNextprot(proteinGroup(ib_phospho))
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### code chunk number 12: isobar-ptm.Rnw:268-269
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head(ptm.info)
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