Description Usage Arguments Value Author(s) References Examples
View source: R/factorFootprints.R
Aggregate ATAC-seq footprint for a given motif generated over binding sites within the genome.
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 | factorFootprints(
bamfiles,
index = bamfiles,
pfm,
genome,
min.score = "95%",
bindingSites,
seqlev = paste0("chr", c(1:22, "X", "Y")),
upstream = 100,
downstream = 100,
maxSiteNum = 1e+06,
anchor = "cut site",
group = "strand",
...
)
|
bamfiles |
A vector of characters indicates the file names of bams. All the bamfiles will be pulled together. |
index |
The names of the index file of the 'BAM' file being processed; This is given without the '.bai' extension. |
pfm |
A Position frequency Matrix represented as a numeric matrix with row names A, C, G and T. |
genome |
An object of BSgenome. |
min.score |
The minimum score for counting a match. Can be given as a character string containing a percentage (e.g. "95 score or as a single number. See matchPWM. |
bindingSites |
A object of GRanges indicates candidate binding sites (eg. the output of fimo). The GRanges object must have score column in the metadata column. |
seqlev |
A vector of characters indicates the sequence levels. |
upstream, downstream |
numeric(1) or integer(1). Upstream and downstream of the binding region for aggregate ATAC-seq footprint. |
maxSiteNum |
numeric(1). Maximal number of predicted binding sites. if predicted binding sites is more than this number, top maxSiteNum binding sites will be used. |
anchor |
"cut site" or "fragment center". If "fragment center" is used, the input bamfiles must be paired-end. |
group |
Group information for the bamfiles. Default by strand. Otherwise, a factor or vector of characters with same length of bamfiles. The group is limited to 2 groups. |
... |
xlab, legTitle, xlim or ylim could be used by plotFootprints |
an invisible list of matrixes with the signals for plot. It includes: - signal mean values of coverage for positive strand and negative strand in feature regions - spearman.correlation spearman correlations of cleavage counts in the highest 10-nucleotide-window and binding prediction score. - bindingSites predicted binding sites.
Jianhong Ou, Julie Zhu
Chen, K., Xi, Y., Pan, X., Li, Z., Kaestner, K., Tyler, J., Dent, S., He, X. and Li, W., 2013. DANPOS: dynamic analysis of nucleosome position and occupancy by sequencing. Genome research, 23(2), pp.341-351.
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 | bamfile <- system.file("extdata", "GL1.bam",
package="ATACseqQC")
library(MotifDb)
CTCF <- query(MotifDb, c("CTCF"))
CTCF <- as.list(CTCF)
library(BSgenome.Hsapiens.UCSC.hg19)
factorFootprints(bamfile, pfm=CTCF[[1]],
genome=Hsapiens,
min.score="95%", seqlev="chr1",
upstream=100, downstream=100)
##### Using user defined binding sites #####
bds <- readRDS(system.file("extdata", "jolma2013.motifs.bindingList.95.rds",
package="ATACseqQC"))
bindingSites <- bds[["Hsapiens-jolma2013-CTCF"]]
seqlev <- "chr1" #seqlevels(bindingSites)
bindingSites <- bindingSites[seqnames(bindingSites) %in% seqlev]
seqlevels(bindingSites) <- seqlev
seqinfo(bindingSites) <- seqinfo(Hsapiens)[seqlev]
factorFootprints(bamfile, pfm=CTCF[[1]],
genome=Hsapiens, seqlev=seqlev,
upstream=100, downstream=100)
|
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