genomation
is a toolkit for annotation and in bulk visualization of genomic intervals (scored or unscored) over predefined regions. The genomic intervals which the package can handle can be anything with a minimal information of chromosome, start and end. The intervals could have any length and most of the time they are associated with a score. Typical examples of such data sets include aligned
reads from high-throughput sequencing (HTS) experiments, percent methylation values for CpGs (or other cytosines), locations of transcription factor binding, and so on. On the other hand, throughout the vignette we use the phrase “genomic annotation” to refer to the regions of the genome associated with a potential function which does not necessarily have a score (examples: CpG islands, genes, enhancers, promoter, exons, etc. ). These genomic annotations are usually the regions of interest, and distribution of genomic intervals over/around the annotations are can make the way for biological interpretation of the data. The pipeline for computational knowledge extraction consists of three steps: data filtering, integration of data from multiple sources or generation of predictive models and biological interpretation of produced models, which leads to novel hypotheses that can be tested in the wetlab.genomation
aims to facilitate the integration of multiple sources of genomic intervals with genomic annotation or already published experimental results.
High-throughput data which will be used to show the functonality of the genomation
are located in two places. The annotation and cap analysis of gene expression (CAGE) data comes prepared with the genomation
package, while the raw HTS data can be found in the sister package genomationData
. To install the genomation
and the complementary data package the from the Bioconductor repository, copy and paste the following lines into your R interpreter:
biocLite('genomationData')
biocLite('genomation')
The r Biocpkg(“genomationData”) vignette contains a verbose description of included files. To list the available data, type:
list.files(system.file('extdata',package='genomationData'))
## [1] "H1.Bisulfite-Seq.combined.chr21.bedGraph.gz"
## [2] "SamplesInfo.txt"
## [3] "wgEncodeBroadHistoneH1hescCtcfStdAlnRep1.chr21.bam"
## [4] "wgEncodeBroadHistoneH1hescCtcfStdAlnRep1.chr21.bam.bai"
## [5] "wgEncodeBroadHistoneH1hescCtcfStdPk.broadPeak.gz"
## [6] "wgEncodeBroadHistoneH1hescP300kat3bAlnRep1.chr21.bam"
## [7] "wgEncodeBroadHistoneH1hescP300kat3bAlnRep1.chr21.bam.bai"
## [8] "wgEncodeBroadHistoneH1hescP300kat3bPk.broadPeak.gz"
## [9] "wgEncodeBroadHistoneH1hescSuz12051317AlnRep1.chr21.bam"
## [10] "wgEncodeBroadHistoneH1hescSuz12051317AlnRep1.chr21.bam.bai"
## [11] "wgEncodeBroadHistoneH1hescSuz12051317Pk.broadPeak.gz"
## [12] "wgEncodeHaibTfbsA549Rad21V0422111RawRep1.chr21.bw"
## [13] "wgEncodeHaibTfbsH1hescRad21V0416102AlnRep1.chr21.bam"
## [14] "wgEncodeHaibTfbsH1hescRad21V0416102AlnRep1.chr21.bam.bai"
## [15] "wgEncodeHaibTfbsH1hescRad21V0416102PkRep1.broadPeak.gz"
## [16] "wgEncodeRikenCageA549CellPapAlnRep1.chr21.bam"
## [17] "wgEncodeRikenCageA549CellPapAlnRep1.chr21.bam.bai"
## [18] "wgEncodeSydhTfbsH1hescZnf143IggrabAlnRep1.chr21.bam"
## [19] "wgEncodeSydhTfbsH1hescZnf143IggrabAlnRep1.chr21.bam.bai"
## [20] "wgEncodeSydhTfbsH1hescZnf143IggrabPk.narrowPeak.gz"
To see the descriptions of the files:
sampleInfo = read.table(system.file("extdata/SamplesInfo.txt", package = "genomationData"),
header = TRUE, sep = "\t")
sampleInfo[1:5, 1:5]
## fileName dataOrigin
## 1 wgEncodeBroadHistoneH1hescCtcfStdAlnRep1.chr21.bam Encode
## 2 wgEncodeBroadHistoneH1hescP300kat3bAlnRep1.chr21.bam Encode
## 3 wgEncodeBroadHistoneH1hescSuz12051317AlnRep1.chr21.bam Encode
## 4 wgEncodeHaibTfbsH1hescRad21V0416102AlnRep1.chr21.bam Encode
## 5 wgEncodeSydhTfbsH1hescZnf143IggrabAlnRep1.chr21.bam Encode
## cellType sampleName experimentType
## 1 H1hesc Ctcf ChipSeq
## 2 H1hesc P300 ChipSeq
## 3 H1hesc Suz12 ChipSeq
## 4 H1hesc Rad21 ChipSeq
## 5 H1hesc Znf143 ChipSeq
Basic annotation data and processed experimental data can be found within the genomation
package. The data can be accesed throught the data command or located in the extdata folder.
library(genomation)
data(cage)
data(cpgi)
list.files(system.file("extdata", package = "genomation"))
One of larger hindrances in computational genomics stems from the myriad of formats that are used to store the data. Although some formats have been selected as de facto standards for specific kind of biological data (e.g. BAM, VCF), almost all publications come with supplementary tables that do not have the same structure, but hold similar information. The tables usually have a tabular format, contain the locationof elements in genomic coordinates and various metadata colums. genomation
contais functions to read genomic intervals and genomic annotation provided they are in a tabular format. These functions will read the data from flat files into GRanges or GRangesList objects.
readGeneric is the workhorse of the genomation
package. It is a function developed specifically for input of genomic data in tabular formats, and their conversion to a GRanges object. By default, the function persumes that the file is a standard .bed file containing columns chr, start, end.
library(genomation)
tab.file1 = system.file("extdata/tab1.bed", package = "genomation")
readGeneric(tab.file1, header = TRUE)
## GRanges object with 6 ranges and 0 metadata columns:
## seqnames ranges strand
## <Rle> <IRanges> <Rle>
## [1] chr21 [9437272, 9439473] *
## [2] chr21 [9483485, 9484663] *
## [3] chr21 [9647866, 9648116] *
## [4] chr21 [9708935, 9709231] *
## [5] chr21 [9825442, 9826296] *
## [6] chr21 [9909011, 9909218] *
## -------
## seqinfo: 1 sequence from an unspecified genome; no seqlengths
If the file contains meta data columns (as in extended bed format), it is possible to read all or some of the additional columns. To select columns which you want to read in, use the meta.col argument
readGeneric(tab.file1, header = TRUE, keep.all.metadata = TRUE)
## GRanges object with 6 ranges and 3 metadata columns:
## seqnames ranges strand | cpgNum gcNum perCpg
## <Rle> <IRanges> <Rle> | <integer> <integer> <numeric>
## [1] chr21 [9437272, 9439473] * | 285 1426 25.9
## [2] chr21 [9483485, 9484663] * | 165 818 28
## [3] chr21 [9647866, 9648116] * | 18 168 14.4
## [4] chr21 [9708935, 9709231] * | 31 218 20.9
## [5] chr21 [9825442, 9826296] * | 120 568 28.1
## [6] chr21 [9909011, 9909218] * | 20 143 19.3
## -------
## seqinfo: 1 sequence from an unspecified genome; no seqlengths
readGeneric(tab.file1, header = TRUE, meta.col = list(CpGnum = 4))
## GRanges object with 6 ranges and 1 metadata column:
## seqnames ranges strand | CpGnum
## <Rle> <IRanges> <Rle> | <integer>
## [1] chr21 [9437272, 9439473] * | 285
## [2] chr21 [9483485, 9484663] * | 165
## [3] chr21 [9647866, 9648116] * | 18
## [4] chr21 [9708935, 9709231] * | 31
## [5] chr21 [9825442, 9826296] * | 120
## [6] chr21 [9909011, 9909218] * | 20
## -------
## seqinfo: 1 sequence from an unspecified genome; no seqlengths
If the file contains header, the function will automatically recognize the columns using the header names.
readGeneric(tab.file1, header = TRUE, keep.all.metadata = TRUE)
## GRanges object with 6 ranges and 3 metadata columns:
## seqnames ranges strand | cpgNum gcNum perCpg
## <Rle> <IRanges> <Rle> | <integer> <integer> <numeric>
## [1] chr21 [9437272, 9439473] * | 285 1426 25.9
## [2] chr21 [9483485, 9484663] * | 165 818 28
## [3] chr21 [9647866, 9648116] * | 18 168 14.4
## [4] chr21 [9708935, 9709231] * | 31 218 20.9
## [5] chr21 [9825442, 9826296] * | 120 568 28.1
## [6] chr21 [9909011, 9909218] * | 20 143 19.3
## -------
## seqinfo: 1 sequence from an unspecified genome; no seqlengths
If the files have permutted columns, such that the first three do not represent chromosome, start and end, you can select an arbitrary set of columns using the chr, start and end arguments.
tab.file2 = system.file("extdata/tab2.bed", package = "genomation")
readGeneric(tab.file2, chr = 3, start = 2, end = 1)
## GRanges object with 6 ranges and 0 metadata columns:
## seqnames ranges strand
## <Rle> <IRanges> <Rle>
## [1] chr21 [9437272, 9439473] *
## [2] chr21 [9483485, 9484663] *
## [3] chr21 [9647866, 9648116] *
## [4] chr21 [9708935, 9709231] *
## [5] chr21 [9825442, 9826296] *
## [6] chr21 [9909011, 9909218] *
## -------
## seqinfo: 1 sequence from an unspecified genome; no seqlengths
readGeneric function can easily be extended to read almost any kind of biological data. As an example we have provided convenience functions to read the Encode narrowPeak and broadPeak formats, and gtf formatted files.
gff.file = system.file("extdata/chr21.refseq.hg19.gtf", package = "genomation")
gff = gffToGRanges(gff.file)
head(gff)
## GRanges object with 6 ranges and 6 metadata columns:
## seqnames ranges strand | source type score
## <Rle> <IRanges> <Rle> | <factor> <factor> <numeric>
## [1] chr21 [9825832, 9826011] + | hg19_refGene exon 0
## [2] chr21 [9826203, 9826263] + | hg19_refGene exon 0
## [3] chr21 [9907189, 9907492] - | hg19_refGene exon 0
## [4] chr21 [9909047, 9909277] - | hg19_refGene exon 0
## [5] chr21 [9966322, 9966380] - | hg19_refGene exon 0
## [6] chr21 [9968516, 9968593] - | hg19_refGene exon 0
## phase gene_id transcript_id
## <integer> <character> <character>
## [1] <NA> NR_037421 NR_037421
## [2] <NA> NR_037458 NR_037458
## [3] <NA> NR_038328 NR_038328
## [4] <NA> NR_038328 NR_038328
## [5] <NA> NR_038328 NR_038328
## [6] <NA> NR_038328 NR_038328
## -------
## seqinfo: 1 sequence from an unspecified genome; no seqlengths
In order to split the last column of the gff file, use the split.group=TRUE argument.
gff = gffToGRanges(gff.file, split.group = TRUE)
head(gff)
There are specific functions to read genomic annotation from flat bed files. readFeatureFlank is a convenience function used to get the ranges flanking the set of interest. As an example, it could be used to get the CpG island shores, which have been shown to harbour condition specific differential methylation.
# reading genes stored as a BED files
cpgi.file = system.file("extdata/chr21.CpGi.hg19.bed", package = "genomation")
cpgi.flanks = readFeatureFlank(cpgi.file)
head(cpgi.flanks$flanks)
## GRanges object with 6 ranges and 0 metadata columns:
## seqnames ranges strand
## <Rle> <IRanges> <Rle>
## [1] chr21 [9823442, 9825441] *
## [2] chr21 [9826297, 9828296] *
## [3] chr21 [9907011, 9909010] *
## [4] chr21 [9909219, 9911218] *
## [5] chr21 [9966264, 9968263] *
## [6] chr21 [9968621, 9970620] *
## -------
## seqinfo: 1 sequence from an unspecified genome; no seqlengths
A standard step in a computational genomics experiment is visualization of average enrichment over a certain predefined set of ranges, such as mean coverage of a certain histone modification around a transcription factor binding site, or visualization of histone positions around transcription start sites.
ScoreMatrix and ScoreMatrixBin are functions used to extract data over predefined windows.
ScoreMatrix is used when all of the windows have the same width, such as a designated area around the transcription start site, while the ScoreMatrixBin is designed for use with windows of unequal width (e.g. enrichment of methylation over exons).
Both functions have 2 main arguments: target and windows. target is the data that we want to extract, while the windows represents the regions over which we want to see the enrichment. The target data can be in 3 forms: a GRanges, a RLeList or a path to an indexed .bam file. The windows must be GRanges object.
As an example we will extract the density of cage tags around the promoters on the human chromosome 21.
data(cage)
data(promoters)
sm = ScoreMatrix(target = cage, windows = promoters)
sm
## scoreMatrix with dims: 1055 2001
ScoreMatrixBin function has an additional bin.num argument which specifies the number of bins that will represent each windot window
(ie. it converts windows of unequal width into ones of equal width.). By default, the binning function is set to mean.
data(cage)
gff.file = system.file("extdata/chr21.refseq.hg19.gtf", package = "genomation")
exons = gffToGRanges(gff.file, filter = "exon")
sm = ScoreMatrixBin(target = cage, windows = exons, bin.num = 50)
sm
Running ScoreMatrixBin with bin.num=50 on a set of exons warned us that some of the exons are shorter than 50 bp and were thus removed from the set before binning. The rownames of the resulting ScoreMatrix object correspond to the ranges that were used to construct the windows (e.g. row name 10 means that the 10th element in the target GRanges object was used to extract the data). If a certain rowname is not present in the ScoreMatrix object, that means that the corresponding range was filtered out (e.g. the range could have been on a chromosome that was not present in the target).
To simultaneously work on multiple files you can use the ScoreMatrixList function. The function also has 2 obligatory arguments targets and windows. While the windows is the same as in ScoreMatrix, the targets argument contains results from multiple experiments. It can be in one of the three formats: a list of RleLists, a list of GRanges (or a GRangesList object), or a character vector designating a set of .bam or .bigWig files.
data(promoters)
data(cpgi)
data(cage)
cage$tpm = NULL
targets = list(cage = cage, cpgi = cpgi)
sm = ScoreMatrixList(targets = targets, windows = promoters, bin.num = 50)
## working on cage
## working on cpgi
sm
## scoreMatrixlist of length:2
## 1. scoreMatrix with dims: 1055 50
## 2. scoreMatrix with dims: 1055 50
If all of the windows have the same width ScoreMatrixList will use the ScoreMatrix function. That can be overridden by explicitly specifying the bin.num argument, as we did in the example.
There are 2 basic modes of visualization of enrichment over windows: either as a heatmap, or as a histogram. heatMatrix, plotMeta and multiHeatMatrix are functions for visualization of ScoreMatrix and ScoreMatrixList objects.
We will plot the distribution of CAGE tags around promoters on human chr21.
data(cage)
data(promoters)
sm = ScoreMatrix(target = cage, windows = promoters)
heatMatrix(sm, xcoords = c(-1000, 1000))
plotMeta(sm, xcoords = c(-1000, 1000))
The heatMatrix function can also take a list of numeric vectors designating row names, or a factor variable that represent our annotation over the windows.
library(GenomicRanges)
data(cage)
data(promoters)
data(cpgi)
sm = ScoreMatrix(target = cage, windows = promoters, strand.aware = TRUE)
cpg.ind = which(countOverlaps(promoters, cpgi) > 0)
nocpg.ind = which(countOverlaps(promoters, cpgi) == 0)
heatMatrix(sm, xcoords = c(-1000, 1000), group = list(CpGi = cpg.ind, noCpGi = nocpg.ind))
Because the enrichment in windows can have a high dynamic range, it is sometimes convenient to scale the matrix before plotting.
sm.scaled = scaleScoreMatrix(sm)
heatMatrix(sm.scaled, xcoords = c(-1000, 1000), group = list(CpGi = cpg.ind,
noCpGi = nocpg.ind))
Several experiments can be plotted in a side by side fashion using a combination of ScoreMatrixList and multiHeatMatrix.
cage$tpm = NULL
targets = list(cage = cage, cpgi = cpgi)
sml = ScoreMatrixList(targets = targets, windows = promoters, bin.num = 50,
strand.aware = TRUE)
multiHeatMatrix(sml, xcoords = c(-1000, 1000))
We can put the clustering function clustfun to see whether there are any patterns present in the data.
multiHeatMatrix(sml, xcoords = c(-1000, 1000), clustfun = function(x) kmeans(x,
centers = 2)$cluster)
More advance usage of the ScoreMatrix family of functions and their visualtization can be found in the specific use-cases at the end of the vignette.
Searching for correlation between sets of genomic intervals is a standard exploratory method in computational genomics. It is usually done by looking at the overlap between 2 or more sets of ranges and calculating various overlap statistics. genomation
contains two sets of functions for annotation of ranges: the first one is used to facilitate the general annotation of any sets of ranges, while the second one is used to annotate a given feature with gene structures (promoter, exon, intron).
Firstly, we will select the broadPeak files from the genomatonData
package, and read in the peaks for the Ctcf transcription factor
library(genomationData)
genomationDataPath = system.file("extdata", package = "genomationData")
sampleInfo = read.table(file.path(genomationDataPath, "SamplesInfo.txt"), header = TRUE,
sep = "\t", stringsAsFactors = FALSE)
peak.files = list.files(genomationDataPath, full.names = TRUE, pattern = "broadPeak")
names(peak.files) = sampleInfo$sampleName[match(basename(peak.files), sampleInfo$fileName)]
ctcf.peaks = readBroadPeak(peak.files["Ctcf"])
Now we will annotate the human the Ctcf binding sites using the CpG islands. Because the CpG islands are restricted to chromosomes 21 and 22, we will set the intersect.chr = TRUE, which will limit the analysis only to the chromosomes that are present in both data sets.
data(cpgi)
peak.annot = annotateWithFeature(ctcf.peaks, cpgi, intersect.chr = TRUE)
## intersecting chromosomes...
peak.annot
## summary of target set annotation with feature annotation:
## Rows in target set: 3964
## ----------------------------
## percentage of target elements overlapping with features:
## cpgi other
## 7.62 92.38
##
## percentage of feature elements overlapping with target:
## [1] 36.94
##
The output of the annotateWithFeature function shows three types of information: The total number of elements in the target dataset, the percentage of target dataset that overlaps with the feature dataset. And the percentage of the feature elements that overlap the target.
To find the distribution of our designated intervals around gene structures, we will first read the transcript features from a file using the readTranscriptFeatures function. readTranscriptFeatures reads a bed12 formatted file and parses the coordinates into a GRangesList containing four elements: exons, introns. promoters and transcription start sites (TSSes).
bed.file = system.file("extdata/chr21.refseq.hg19.bed", package = "genomation")
gene.parts = readTranscriptFeatures(bed.file)
## Reading the table...
## Calculating intron coordinates...
## Calculating exon coordinates...
## Calculating TSS coordinates...
## Calculating promoter coordinates...
## Outputting the final GRangesList...
annotateWithGeneParts will give us the overlap statistics between our CTCF peaks and gene structures. We will again use the intersect.chr=TRUE to limit the analysis.
ctcf.annot = annotateWithGeneParts(ctcf.peaks, gene.parts, intersect.chr = TRUE)
## intersecting chromosomes...
ctcf.annot
## Summary of target set annotation with genic parts
## Rows in target set: 1681
## -----------------------
## percentage of target features overlapping with annotation:
## promoter exon intron intergenic
## 9.58 13.50 47.65 47.17
##
## percentage of target features overlapping with annotation:
## (with promoter > exon > intron precedence):
## promoter exon intron intergenic
## 9.58 7.91 35.34 47.17
##
## percentage of annotation boundaries with feature overlap:
## promoter exon intron
## 38.36 15.40 29.33
##
## summary of distances to the nearest TSS:
## Min. 1st Qu. Median Mean 3rd Qu. Max.
## 0 7977 28470 66060 74690 1195000
##
annotateWithGeneParts can also take a set of feature ranges as an argument. We will use the readGeneric function to load all of the broadPeak files in the genomationData
, which we will then annotate.
peaks = GRangesList(lapply(peak.files, readGeneric))
names(peaks) = names(peak.files)
annot.list = annotateWithGeneParts(peaks, gene.parts, intersect.chr = TRUE)
## Working on: Ctcf
## intersecting chromosomes...
## Working on: P300
## intersecting chromosomes...
## Working on: Suz12
## intersecting chromosomes...
## Working on: Rad21
## intersecting chromosomes...
Gene annotation of multiple feature objects can be visualized in a form of a heatmap, where rows represent samples, columns the gene structure, and the value is the percentage of overlap given by priority. If cluster=TRUE, then the function will use hierarhical clustering to order the heatmap.
plotGeneAnnotation(annot.list)
plotGeneAnnotation(annot.list, cluster = TRUE)
genomation
packageThe genomation
package provides generalizable functions for genomic data analysis and visualization. Below we will demonstrate the functionality on specific use cases
We will visualize the binding profiles of 6 transcription factors around the Ctcf binding sites.
In the fist step we will select the *.bam files containing mapped reads.
genomationDataPath = system.file("extdata", package = "genomationData")
bam.files = list.files(genomationDataPath, full.names = TRUE, pattern = "bam$")
bam.files = bam.files[!grepl("Cage", bam.files)]
Firstly, we will read in the Ctcf peaks, filter regions from human chromosome 21, and order them by their signal values. In the end we will resize all ranges to have a uniform width of 500 bases, fixed on the center of the peak.
ctcf.peaks = readBroadPeak(file.path(genomationDataPath, "wgEncodeBroadHistoneH1hescCtcfStdPk.broadPeak.gz"))
ctcf.peaks = ctcf.peaks[seqnames(ctcf.peaks) == "chr21"]
ctcf.peaks = ctcf.peaks[order(-ctcf.peaks$signalValue)]
ctcf.peaks = resize(ctcf.peaks, width = 1000, fix = "center")
In order to extract the coverage values of all transcription factors around chipseq peaks, we will use the ScoreMatrixList function. ScoreMatrixList assign names to each element of the list based on the names of the bam files. We will use the names of the files to find the corresponding names of each sample in the SamplesInfo.txt. Using the heatmapProfile on our ScoreMatrixList, we can plot the underlying signal side by side.
sml = ScoreMatrixList(bam.files, ctcf.peaks, bin.num = 50, type = "bam")
sampleInfo = read.table(system.file("extdata/SamplesInfo.txt", package = "genomationData"),
header = TRUE, sep = "\t")
names(sml) = sampleInfo$sampleName[match(names(sml), sampleInfo$fileName)]
multiHeatMatrix(sml, xcoords = c(-500, 500), col = c("lightgray", "blue"))
Because of the large range of signal values in chipseq peaks, the heatmapProfile will not show the true extent of colocalization. To get around this, it is advisable to independently scale the rows of each element in the ScoreMatrixList.
sml.scaled = scaleScoreMatrixList(sml)
multiHeatMatrix(sml.scaled, xcoords = c(-500, 500), col = c("lightgray", "blue"))
In the first step we will read all peak files into a GRanges list. We will use the SamplesInfo file from the genomationData
to get he names of the samples. Four of the peak files are in the Encode broadPeak format, while one is in the narrowPeak. To read the files, we will use the readGeneric function. It enables us to select from the files only columns of interest. As the last step, we will restrict ourselves to peaks that are located on chromosome 21 and have width 100 and 1000 bp
genomationDataPath = system.file("extdata", package = "genomationData")
sampleInfo = read.table(file.path(genomationDataPath, "SamplesInfo.txt"), header = TRUE,
sep = "\t", stringsAsFactors = FALSE)
peak.files = list.files(genomationDataPath, full.names = TRUE, pattern = "Peak.gz$")
peaks = list()
for (i in 1:length(peak.files)) {
file = peak.files[i]
name = sampleInfo$sampleName[match(basename(file), sampleInfo$fileName)]
message(name)
peaks[[name]] = readGeneric(file, meta.col = list(score = 5))
}
## Ctcf
## P300
## Suz12
## Rad21
## Znf143
peaks = GRangesList(peaks)
peaks = peaks[seqnames(peaks) == "chr21" & width(peaks) < 1000 & width(peaks) >
100]
To find the combination of binding sites we will use the findFeatureComb function. It takes a granges list object, finds the union of the ranges and designates each range by the combination of overlaps from the original set. By default, the returned ranges will have a numeric class meta data column, which designates the correponding combination. If you are interested in the names of the TF which make the combinations, put the use.names=TRUE.
tf.comb = findFeatureComb(peaks, width = 1000)
To visualize the results, we will plot the enricment of resulting regions. Before doing that we will order the regions by their class argument.
tf.comb = tf.comb[order(tf.comb$class)]
bam.files = list.files(genomationDataPath, full.names = TRUE, pattern = "bam$")
bam.files = bam.files[!grepl("Cage", bam.files)]
sml = ScoreMatrixList(bam.files, tf.comb, bin.num = 20, type = "bam")
names(sml) = sampleInfo$sampleName[match(names(sml), sampleInfo$fileName)]
sml.scaled = scaleScoreMatrixList(sml)
multiHeatMatrix(sml.scaled, xcoords = c(-500, 500), col = c("lightgray", "blue"))
The plot shows perfectly how misleading the peak calling process can be. Although the plots show that CTFC, Rad21 and Znf143 have almost perfect colozalization, peak callers have trouble identifying peaks in regions with lower enrichments and as a result, we get different statistics when using overlaps.
We can also use data from AnnotationHub since it can return data as GRanges object. Below we download CpG island and DNAse peak locations from AnnotationHub and get a scoreMatrix on the CpG islands.
library(AnnotationHub)
ah = AnnotationHub()
# retrieve CpG island data from annotationHub
cpgi_query <- query(ah, c("CpG Islands", "UCSC", "hg19"))
cpgi <- ah[[names(cpgi_query)]]
dnase_query <- query(ah, c("wgEncodeOpenChromDnase8988tPk.narrowPeak.gz", "UCSC",
"hg19"))
dnaseP <- ah[[names(dnase_query)]]
sm = ScoreMatrixBin(target = dnaseP, windows = cpgi, strand.aware = FALSE)
sessionInfo()
## R version 3.3.0 (2016-05-03)
## Platform: x86_64-apple-darwin13.4.0 (64-bit)
## Running under: OS X 10.11.5 (El Capitan)
##
## locale:
## [1] en_US.UTF-8/en_US.UTF-8/en_US.UTF-8/C/en_US.UTF-8/en_US.UTF-8
##
## attached base packages:
## [1] stats4 parallel grid stats graphics grDevices utils
## [8] datasets methods base
##
## other attached packages:
## [1] GenomicRanges_1.24.2 GenomeInfoDb_1.8.1 IRanges_2.6.1
## [4] S4Vectors_0.10.2 BiocGenerics_0.18.0 genomationData_1.4.2
## [7] genomation_1.5.4 knitr_1.13.1
##
## loaded via a namespace (and not attached):
## [1] Rcpp_0.12.5 formatR_1.4
## [3] plyr_1.8.4 XVector_0.12.0
## [5] bitops_1.0-6 tools_3.3.0
## [7] zlibbioc_1.18.0 digest_0.6.9
## [9] evaluate_0.9 gtable_0.2.0
## [11] BSgenome_1.40.1 gridBase_0.4-7
## [13] yaml_2.1.13 rtracklayer_1.32.1
## [15] stringr_1.0.0 Biostrings_2.40.2
## [17] Biobase_2.32.0 data.table_1.9.6
## [19] impute_1.46.0 plotrix_3.6-2
## [21] XML_3.98-1.4 BiocParallel_1.6.2
## [23] seqPattern_1.4.0 rmarkdown_0.9.6
## [25] reshape2_1.4.1 readr_0.2.2
## [27] ggplot2_2.1.0 magrittr_1.5
## [29] matrixStats_0.50.2 Rsamtools_1.24.0
## [31] scales_0.4.0 htmltools_0.3.5
## [33] GenomicAlignments_1.8.4 SummarizedExperiment_1.2.3
## [35] colorspace_1.2-6 KernSmooth_2.23-15
## [37] stringi_1.1.1 RCurl_1.95-4.8
## [39] munsell_0.4.3 chron_2.3-47