inst/scripts/make-data.R
In alexchwong/NxtIRFcore: Core Engine for NxtIRF: a User-Friendly Intron Retention and Alternative Splicing Analysis using the IRFinder Engine
#' Making Mappability Exclusion Region BED files from FASTA file
#'
#' Making a Mappability Region Exclusion BED file requires 3 steps.
#' 1) Generate mappability reads using `run_IRFinder_GenerateMapReads()`,
#' using the primary assembly genome FASTA as `genome.fa`
#' 2) Align `out.fa` to the corresponding genome using a genome splice-aware aligner such as STAR
#' 3) Process the aligned BAM file using `run_IRFinder_MapExclusionRegions()`
#' @examples
#' \dontrun{
#' FASTA = "/path/to/genome.fa"
#' run_IRFinder_GenerateMapReads(
#' genome.fa = FASTA,
#' out.fa = "/path/to/mappability_reads.fa",
#' read_len = 70,
#' read_stride = 10,
#' error_pos = 35
#' )
#'
#' # Now run STAR in the command line, e.g.:
#' # STAR \
#' # --genomeDir /path/to/Reference \
#' # --genomeLoad NoSharedMemory \
#' # --runThreadN 4 --outStd SAM --outSAMmode NoQS \
#' # --outSAMattributes None \
#' # --outFilterMultimapNmax 1 \
#' # --readFilesIn /path/to/mappability_reads.fa \
#' # > /path/to/genome_fragments.sam
#'
#' run_IRFinder_MapExclusionRegions(
#' bamfile = "/path/to/genome_fragments.sam",
#' output_file = "/path/to/MappabilityExclusionBED.txt",
#' threshold = 4,
#' includeCov = FALSE
#' )
#' }
NULL
#' Sample NxtSE object using the NxtIRF example reference and example bam files
#'
#' This function generates an example reference, and runs IRFinder on example
#' bam files. This object is used in downstream examples throughout
#' the documentation of all functions that use NxtSE objects as input
#' @examples
#' se = readRDS(
#' system.file("extdata", "example_NxtSE.Rds", package = "NxtIRFcore")
#' )
#' se = NxtIRF_example_NxtSE()
#' @seealso [MakeSE()]
make_example_NxtSE <- function() {
require(NxtIRFcore)
bams = NxtIRF_example_bams()
BuildReference(
fasta = chrZ_genome(), gtf = chrZ_gtf(),
reference_path = file.path(tempdir(), "Reference")
)
IRFinder(bams$path, bams$sample,
reference_path = file.path(tempdir(), "Reference"),
output_path = file.path(tempdir(), "IRFinder_output"),
overwrite = TRUE, n_threads = 1
)
expr = Find_IRFinder_Output(file.path(tempdir(), "IRFinder_output"))
CollateData(expr,
reference_path = file.path(tempdir(), "Reference"),
output_path = file.path(tempdir(), "NxtIRF_output")
)
se = MakeSE(collate_path = file.path(tempdir(), "NxtIRF_output"))
# Save COV files
file.copy(
expr$cov_file,
file.path("../extdata", basename(expr$cov_file)),
overwrite = TRUE
)
# De-identify COV files for validity:
covfile(se) <- rep("", 6)
# Convert from HDF5-linked se to in-memory se:
se <- realize_NxtSE(se)
saveRDS(se, "../extdata/example_NxtSE.Rds")
}
alexchwong/NxtIRFcore documentation built on Oct. 31, 2022, 9:14 a.m.
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#' Making Mappability Exclusion Region BED files from FASTA file
#'
#' Making a Mappability Region Exclusion BED file requires 3 steps.
#' 1) Generate mappability reads using `run_IRFinder_GenerateMapReads()`,
#' using the primary assembly genome FASTA as `genome.fa`
#' 2) Align `out.fa` to the corresponding genome using a genome splice-aware aligner such as STAR
#' 3) Process the aligned BAM file using `run_IRFinder_MapExclusionRegions()`
#' @examples
#' \dontrun{
#' FASTA = "/path/to/genome.fa"
#' run_IRFinder_GenerateMapReads(
#' genome.fa = FASTA,
#' out.fa = "/path/to/mappability_reads.fa",
#' read_len = 70,
#' read_stride = 10,
#' error_pos = 35
#' )
#'
#' # Now run STAR in the command line, e.g.:
#' # STAR \
#' # --genomeDir /path/to/Reference \
#' # --genomeLoad NoSharedMemory \
#' # --runThreadN 4 --outStd SAM --outSAMmode NoQS \
#' # --outSAMattributes None \
#' # --outFilterMultimapNmax 1 \
#' # --readFilesIn /path/to/mappability_reads.fa \
#' # > /path/to/genome_fragments.sam
#'
#' run_IRFinder_MapExclusionRegions(
#' bamfile = "/path/to/genome_fragments.sam",
#' output_file = "/path/to/MappabilityExclusionBED.txt",
#' threshold = 4,
#' includeCov = FALSE
#' )
#' }
NULL
#' Sample NxtSE object using the NxtIRF example reference and example bam files
#'
#' This function generates an example reference, and runs IRFinder on example
#' bam files. This object is used in downstream examples throughout
#' the documentation of all functions that use NxtSE objects as input
#' @examples
#' se = readRDS(
#' system.file("extdata", "example_NxtSE.Rds", package = "NxtIRFcore")
#' )
#' se = NxtIRF_example_NxtSE()
#' @seealso [MakeSE()]
make_example_NxtSE <- function() {
require(NxtIRFcore)
bams = NxtIRF_example_bams()
BuildReference(
fasta = chrZ_genome(), gtf = chrZ_gtf(),
reference_path = file.path(tempdir(), "Reference")
)
IRFinder(bams$path, bams$sample,
reference_path = file.path(tempdir(), "Reference"),
output_path = file.path(tempdir(), "IRFinder_output"),
overwrite = TRUE, n_threads = 1
)
expr = Find_IRFinder_Output(file.path(tempdir(), "IRFinder_output"))
CollateData(expr,
reference_path = file.path(tempdir(), "Reference"),
output_path = file.path(tempdir(), "NxtIRF_output")
)
se = MakeSE(collate_path = file.path(tempdir(), "NxtIRF_output"))
# Save COV files
file.copy(
expr$cov_file,
file.path("../extdata", basename(expr$cov_file)),
overwrite = TRUE
)
# De-identify COV files for validity:
covfile(se) <- rep("", 6)
# Convert from HDF5-linked se to in-memory se:
se <- realize_NxtSE(se)
saveRDS(se, "../extdata/example_NxtSE.Rds")
}
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