sahirbhatnagar/methyl_annotate.R

## methyl_annotate.R
methyl.annotate <- function(file, thresholdp=1e-3, thresholdq=1e-1, tissue){

    DT <- fread(file)
    setnames(DT, c("V1","V2","V3","V4","V5"), c("probe","pvalue","z","sd","effect"))

    # use this to get CHR and BP, then merge with betareg results
    probe.info <- hm450[DT[["probe"]]]
    f <- data.table::data.table(probe=names(probe.info),CHR=as.data.frame(probe.info@seqnames)$value,
                    BP=as.numeric(probe.info@elementMetadata$probeStart))
    data.table::setkey(f,probe)

    # get nearest Transcription start sites
    TSS <- data.table::data.table(FDb.InfiniumMethylation.hg19::getNearestTSS(probe.info), keep.rownames=TRUE)
    data.table::setkey(TSS,rn)

    # change names to merge in with DT
    data.table::setnames(TSS, c("queryHits","subjectHits","distance","nearestGeneSymbol","nearestTranscript"),
             c("TSSqueryHits","TSSsubjectHits","TSSdistance","TSSnearestGeneSymbol","TSSnearestTranscript"))

    # get nearest genes
    Transcript <- data.table::data.table(FDb.InfiniumMethylation.hg19::getNearestTranscript(probe.info), keep.rownames=TRUE)
    data.table::setkey(Transcript,rn)

#     DT[,c("significant.p","lower95","upper95","tissue"):=
#            list(pvalue<=thresholdp,effect+qnorm(0.025)*sd,effect+qnorm(0.975)*sd,tissue),]

    set(DT,i=NULL, j="significant.p", value=DT[["pvalue"]]<=thresholdp)
    set(DT,i=NULL, j="lower95", value=DT[["effect"]]+qnorm(0.025)*DT[["sd"]])
    set(DT,i=NULL, j="upper95", value=DT[["effect"]]+qnorm(0.975)*DT[["sd"]])

    setkey(DT,probe)

    # Merge all tables
    DT <- DT[f][Transcript][TSS]

    set(DT, i=NULL, j="CHR.num", value=as.numeric(sub("chr","", DT[["CHR"]])))

    # significant probes based on pvalue threshold
    probenames.p <- DT[significant.p==TRUE][,c("probe","CHR.num","BP","effect","sd","nearestGeneSymbol","distance","TSSnearestGeneSymbol","TSSdistance"),with=F]

    # GRanges object for significant hits based on p value
    probenames.p.granges <- hm450[probenames.p[["probe"]]]

    # q-value
    qobj <- qvalue::qvalue(DT[["pvalue"]])
    set(DT, i=NULL, j="qvalue",value=qobj$qvalues)
    DT[,"significant.q":=qvalue<=thresholdq]

    # significant probes based on qvalue threshold
    probenames.q <- DT[significant.q==TRUE][,c("probe","CHR.num","BP","effect","sd","nearestGeneSymbol","distance","TSSnearestGeneSymbol","TSSdistance"),with=F]

    # GRanges object for significant hits based on q value
    probenames.q.granges <- hm450[probenames.q[["probe"]]]

    return(list(results=DT, significantp=probenames.p, significantq=probenames.q,
                sigpGranges=probenames.p.granges,sigqGranges=probenames.q.granges))

}
	methyl.annotate <- function(file, thresholdp=1e-3, thresholdq=1e-1, tissue){

	DT <- fread(file)
	setnames(DT, c("V1","V2","V3","V4","V5"), c("probe","pvalue","z","sd","effect"))

	# use this to get CHR and BP, then merge with betareg results
	probe.info <- hm450[DT[["probe"]]]
	f <- data.table::data.table(probe=names(probe.info),CHR=as.data.frame(probe.info@seqnames)$value,
	BP=as.numeric(probe.info@elementMetadata$probeStart))
	data.table::setkey(f,probe)

	# get nearest Transcription start sites
	TSS <- data.table::data.table(FDb.InfiniumMethylation.hg19::getNearestTSS(probe.info), keep.rownames=TRUE)
	data.table::setkey(TSS,rn)

	# change names to merge in with DT
	data.table::setnames(TSS, c("queryHits","subjectHits","distance","nearestGeneSymbol","nearestTranscript"),
	c("TSSqueryHits","TSSsubjectHits","TSSdistance","TSSnearestGeneSymbol","TSSnearestTranscript"))

	# get nearest genes
	Transcript <- data.table::data.table(FDb.InfiniumMethylation.hg19::getNearestTranscript(probe.info), keep.rownames=TRUE)
	data.table::setkey(Transcript,rn)

	# DT[,c("significant.p","lower95","upper95","tissue"):=
	# list(pvalue<=thresholdp,effect+qnorm(0.025)sd,effect+qnorm(0.975)sd,tissue),]

	set(DT,i=NULL, j="significant.p", value=DT[["pvalue"]]<=thresholdp)
	set(DT,i=NULL, j="lower95", value=DT[["effect"]]+qnorm(0.025)*DT[["sd"]])
	set(DT,i=NULL, j="upper95", value=DT[["effect"]]+qnorm(0.975)*DT[["sd"]])

	setkey(DT,probe)

	# Merge all tables
	DT <- DT[f][Transcript][TSS]

	set(DT, i=NULL, j="CHR.num", value=as.numeric(sub("chr","", DT[["CHR"]])))

	# significant probes based on pvalue threshold
	probenames.p <- DT[significant.p==TRUE][,c("probe","CHR.num","BP","effect","sd","nearestGeneSymbol","distance","TSSnearestGeneSymbol","TSSdistance"),with=F]

	# GRanges object for significant hits based on p value
	probenames.p.granges <- hm450[probenames.p[["probe"]]]

	# q-value
	qobj <- qvalue::qvalue(DT[["pvalue"]])
	set(DT, i=NULL, j="qvalue",value=qobj$qvalues)
	DT[,"significant.q":=qvalue<=thresholdq]

	# significant probes based on qvalue threshold
	probenames.q <- DT[significant.q==TRUE][,c("probe","CHR.num","BP","effect","sd","nearestGeneSymbol","distance","TSSnearestGeneSymbol","TSSdistance"),with=F]

	# GRanges object for significant hits based on q value
	probenames.q.granges <- hm450[probenames.q[["probe"]]]

	return(list(results=DT, significantp=probenames.p, significantq=probenames.q,
	sigpGranges=probenames.p.granges,sigqGranges=probenames.q.granges))

	}