PING_nucleosome_positions: Nucleosome positions detected by the PING software using...
In ArnaudDroitLab/consensusSeekeR: Detection of consensus regions inside a group of experiences using genomic positions and genomic ranges
Description
Usage
Format
References
See Also
Examples
Description
Nucleosome positions detected by the PING software using
syntetic reads generated using a normal distribution with a variance
of 20 for regions chr1:10000-15000.
Usage
1
Format
A GRanges containing one entry per detected
nucleosome. The surronding ranges associated to those nucleosomes are in
the dataset PING_nucleosome_positions.
References
Sangsoon W, Zhang X, Sauteraud R, Robert F and Gottardo R. 2013.
PING 2.0: An R/Bioconductor package for nucleosome positioning using
next-generation sequencing data. Bioinformatics 29 (16): 2049-50.
See Also
-
PING_nucleosome_ranges the associate
genomic ranges dataset.
-
findConsensusPeakRegions for extracting regions
sharing nucleosomes from more than one experiment.
Examples
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## Loading datasets
data(PING_nucleosome_positions)
data(PING_nucleosome_ranges)
data(NOrMAL_nucleosome_positions)
data(NOrMAL_nucleosome_ranges)
data(NucPosSimulator_nucleosome_positions)
data(NucPosSimulator_nucleosome_ranges)
## Assigning experiment name to each row of the dataset.
## Position and range datasets from the same sofware must
## have identical names.
names(PING_nucleosome_positions) <- rep("PING",
length(PING_nucleosome_positions))
names(PING_nucleosome_ranges) <- rep("PING",
length(PING_nucleosome_ranges))
names(NOrMAL_nucleosome_positions) <-rep("NOrMAL",
length(NOrMAL_nucleosome_positions))
names(NOrMAL_nucleosome_ranges) <- rep("NOrMAL",
length(NOrMAL_nucleosome_ranges))
names(NucPosSimulator_nucleosome_positions) <-rep("NucPosSimulator",
length(NucPosSimulator_nucleosome_positions))
names(NucPosSimulator_nucleosome_ranges) <- rep("NucPosSimulator",
length(NucPosSimulator_nucleosome_ranges))
## Calculating consensus regions for chromosome 1
## with a default region size of 20 bp (2 * extendingSize).
## The consensus regions are not resized to fit genomic ranges of the
## included nucleosomes.
## Nucleosomes from at least 2 software must be present in a region to
## be retained as a consensus region.
chrList <- Seqinfo(c("chr1"), c(249250621), NA)
findConsensusPeakRegions(
narrowPeaks = c(PING_nucleosome_ranges,
NOrMAL_nucleosome_ranges,
NucPosSimulator_nucleosome_ranges),
peaks = c(PING_nucleosome_positions,
NOrMAL_nucleosome_positions,
NucPosSimulator_nucleosome_positions),
chrInfo = chrList,
extendingSize = 10,
expandToFitPeakRegion = FALSE,
shrinkToFitPeakRegion = FALSE,
minNbrExp = 3,
nbrThreads = 1)
ArnaudDroitLab/consensusSeekeR documentation built on Feb. 6, 2020, 6:45 p.m.
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Description Usage Format References See Also Examples
Description
Nucleosome positions detected by the PING software using syntetic reads generated using a normal distribution with a variance of 20 for regions chr1:10000-15000.
Usage
1 |
Format
A GRanges containing one entry per detected
nucleosome. The surronding ranges associated to those nucleosomes are in
the dataset PING_nucleosome_positions.
References
Sangsoon W, Zhang X, Sauteraud R, Robert F and Gottardo R. 2013. PING 2.0: An R/Bioconductor package for nucleosome positioning using next-generation sequencing data. Bioinformatics 29 (16): 2049-50.
See Also
-
PING_nucleosome_rangesthe associate genomic ranges dataset. -
findConsensusPeakRegionsfor extracting regions sharing nucleosomes from more than one experiment.
Examples
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40 41 42 43 44 | ## Loading datasets
data(PING_nucleosome_positions)
data(PING_nucleosome_ranges)
data(NOrMAL_nucleosome_positions)
data(NOrMAL_nucleosome_ranges)
data(NucPosSimulator_nucleosome_positions)
data(NucPosSimulator_nucleosome_ranges)
## Assigning experiment name to each row of the dataset.
## Position and range datasets from the same sofware must
## have identical names.
names(PING_nucleosome_positions) <- rep("PING",
length(PING_nucleosome_positions))
names(PING_nucleosome_ranges) <- rep("PING",
length(PING_nucleosome_ranges))
names(NOrMAL_nucleosome_positions) <-rep("NOrMAL",
length(NOrMAL_nucleosome_positions))
names(NOrMAL_nucleosome_ranges) <- rep("NOrMAL",
length(NOrMAL_nucleosome_ranges))
names(NucPosSimulator_nucleosome_positions) <-rep("NucPosSimulator",
length(NucPosSimulator_nucleosome_positions))
names(NucPosSimulator_nucleosome_ranges) <- rep("NucPosSimulator",
length(NucPosSimulator_nucleosome_ranges))
## Calculating consensus regions for chromosome 1
## with a default region size of 20 bp (2 * extendingSize).
## The consensus regions are not resized to fit genomic ranges of the
## included nucleosomes.
## Nucleosomes from at least 2 software must be present in a region to
## be retained as a consensus region.
chrList <- Seqinfo(c("chr1"), c(249250621), NA)
findConsensusPeakRegions(
narrowPeaks = c(PING_nucleosome_ranges,
NOrMAL_nucleosome_ranges,
NucPosSimulator_nucleosome_ranges),
peaks = c(PING_nucleosome_positions,
NOrMAL_nucleosome_positions,
NucPosSimulator_nucleosome_positions),
chrInfo = chrList,
extendingSize = 10,
expandToFitPeakRegion = FALSE,
shrinkToFitPeakRegion = FALSE,
minNbrExp = 3,
nbrThreads = 1)
|
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