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inst/doc/nearBynding.R
In nearBynding: Discern RNA structure proximal to protein binding
## ----setup, include = FALSE---------------------------------------------------
knitr::opts_chunk$set(
collapse = TRUE,
comment = "#>"
)
library(nearBynding)
library(Rsamtools)
## ---- echo=FALSE--------------------------------------------------------------
## test whether the local computer can run the required programs
bedtools<-suppressWarnings(system2("bedtools", "--version",
stdout = NULL, stderr = NULL)) == 0
CapR<-suppressWarnings(system2("CapR", stdout = NULL, stderr = NULL)) == 0
stereogene<-suppressWarnings(system2("Stereogene", "-h",
stdout = NULL, stderr = NULL)) == 0
## ---- eval = FALSE------------------------------------------------------------
# if(!requireNamespace("BiocManager", quietly = TRUE))
# install.packages("BiocManager")
# BiocManager::install("nearBynding")
## ---- eval=FALSE--------------------------------------------------------------
# cd CapR-master
# make
# ./CapR
## ---- eval=FALSE--------------------------------------------------------------
# cd stereogene-master
# cd src
# make
# ./stereogene -h
## -----------------------------------------------------------------------------
# load transcript list
load(system.file("extdata/transcript_list.Rda", package="nearBynding"))
# get GTF file
gtf<-system.file("extdata/Homo_sapiens.GRCh38.chr4&5.gtf",
package="nearBynding")
GenomeMappingToChainFile(genome_gtf = gtf,
out_chain_name = "test.chain",
RNA_fragment = "three_prime_utr",
transcript_list = transcript_list,
alignment = "hg38")
## -----------------------------------------------------------------------------
getChainChrSize(chain = "test.chain",
out_chr = "chr4and5_3UTR.size")
## ---- eval = FALSE------------------------------------------------------------
# ExtractTranscriptomeSequence(transcript_list = transcript_list,
# ref_genome = "Homo_sapiens.GRCh38.dna.primary_assembly.fa",
# genome_gtf = gtf,
# RNA_fragment = "three_prime_utr",
# exome_prefix = "chr4and5_3UTR")
## -----------------------------------------------------------------------------
chr4and5_3UTR.fa <- system.file("extdata/chr4and5_3UTR.fa",
package="nearBynding")
## ---- eval = CapR-------------------------------------------------------------
# runCapR(in_file = chr4and5_3UTR.fa)
## ---- eval = bedtools---------------------------------------------------------
# bam <- system.file("extdata/chr4and5.bam", package="nearBynding")
# sorted_bam<-sortBam(bam, "chr4and5_sorted")
#
# CleanBAMtoBG(in_bam = sorted_bam)
## -----------------------------------------------------------------------------
liftOverToExomicBG(input = "chr4and5_sorted.bedGraph",
chain = "test.chain",
chrom_size = "chr4and5_3UTR.size",
output_bg = "chr4and5_liftOver.bedGraph")
## -----------------------------------------------------------------------------
processCapRout(CapR_outfile = system.file("extdata/chr4and5_3UTR.out",
package="nearBynding"),
chain = "test.chain",
output_prefix = "chr4and5_3UTR",
chrom_size = "chr4and5_3UTR.size",
genome_gtf = gtf,
RNA_fragment = "three_prime_utr")
## ---- eval = stereogene-------------------------------------------------------
# runStereogeneOnCapR(protein_file = "chr4and5_liftOver.bedGraph",
# chrom_size = "chr4and5_3UTR.size",
# name_config = "chr4and5_3UTR.cfg",
# input_prefix = "chr4and5_3UTR")
## ---- echo = FALSE, eval = !stereogene, results='hide'------------------------
get_outfiles()
## ---- eval = FALSE------------------------------------------------------------
# runStereogene(track_files = c("chr4and5_3UTR_stem_liftOver.bedGraph",
# "chr4and5_liftOver.bedGraph"),
# name_config = "chr4and5_3UTR.cfg")
## ---- eval = stereogene-------------------------------------------------------
# visualizeCapRStereogene(CapR_prefix = "chr4and5_3UTR",
# protein_file = "chr4and5_liftOver",
# heatmap = TRUE,
# out_file = "all_contexts_heatmap",
# x_lim = c(-500, 500))
# visualizeCapRStereogene(CapR_prefix = "chr4and5_3UTR",
# protein_file = "chr4and5_liftOver",
# x_lim = c(-500, 500),
# out_file = "all_contexts_line",
# y_lim = c(-18, 22))
## ---- fig.show='hold', echo = FALSE, out.width = '50%'------------------------
knitr::include_graphics("all_contexts_heatmap.jpeg")
knitr::include_graphics("all_contexts_line.pdf")
## ---- eval = stereogene-------------------------------------------------------
# visualizeStereogene(context_file = "chr4and5_3UTR_stem_liftOver",
# protein_file = "chr4and5_liftOver",
# out_file = "stem_line",
# x_lim = c(-500, 500))
# visualizeStereogene(context_file = "chr4and5_3UTR_stem_liftOver",
# protein_file = "chr4and5_liftOver",
# heatmap = TRUE,
# out_file = "stem_heatmap",
# x_lim = c(-500, 500))
## ---- fig.show='hold', echo = FALSE, out.width = '50%'------------------------
knitr::include_graphics("stem_heatmap.jpeg")
knitr::include_graphics("stem_line.pdf")
## -----------------------------------------------------------------------------
bindingContextDistance(RNA_context = "chr4and5_3UTR_stem_liftOver",
protein_file = "chr4and5_liftOver",
RNA_context_2 = "chr4and5_3UTR_hairpin_liftOver")
## -----------------------------------------------------------------------------
bindingContextDistance(RNA_context = "chr4and5_3UTR_internal_liftOver",
protein_file = "chr4and5_liftOver",
RNA_context_2 = "chr4and5_3UTR_hairpin_liftOver")
## -----------------------------------------------------------------------------
sessionInfo()
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nearBynding documentation built on Nov. 8, 2020, 8:15 p.m.
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## ----setup, include = FALSE---------------------------------------------------
knitr::opts_chunk$set(
collapse = TRUE,
comment = "#>"
)
library(nearBynding)
library(Rsamtools)
## ---- echo=FALSE--------------------------------------------------------------
## test whether the local computer can run the required programs
bedtools<-suppressWarnings(system2("bedtools", "--version",
stdout = NULL, stderr = NULL)) == 0
CapR<-suppressWarnings(system2("CapR", stdout = NULL, stderr = NULL)) == 0
stereogene<-suppressWarnings(system2("Stereogene", "-h",
stdout = NULL, stderr = NULL)) == 0
## ---- eval = FALSE------------------------------------------------------------
# if(!requireNamespace("BiocManager", quietly = TRUE))
# install.packages("BiocManager")
# BiocManager::install("nearBynding")
## ---- eval=FALSE--------------------------------------------------------------
# cd CapR-master
# make
# ./CapR
## ---- eval=FALSE--------------------------------------------------------------
# cd stereogene-master
# cd src
# make
# ./stereogene -h
## -----------------------------------------------------------------------------
# load transcript list
load(system.file("extdata/transcript_list.Rda", package="nearBynding"))
# get GTF file
gtf<-system.file("extdata/Homo_sapiens.GRCh38.chr4&5.gtf",
package="nearBynding")
GenomeMappingToChainFile(genome_gtf = gtf,
out_chain_name = "test.chain",
RNA_fragment = "three_prime_utr",
transcript_list = transcript_list,
alignment = "hg38")
## -----------------------------------------------------------------------------
getChainChrSize(chain = "test.chain",
out_chr = "chr4and5_3UTR.size")
## ---- eval = FALSE------------------------------------------------------------
# ExtractTranscriptomeSequence(transcript_list = transcript_list,
# ref_genome = "Homo_sapiens.GRCh38.dna.primary_assembly.fa",
# genome_gtf = gtf,
# RNA_fragment = "three_prime_utr",
# exome_prefix = "chr4and5_3UTR")
## -----------------------------------------------------------------------------
chr4and5_3UTR.fa <- system.file("extdata/chr4and5_3UTR.fa",
package="nearBynding")
## ---- eval = CapR-------------------------------------------------------------
# runCapR(in_file = chr4and5_3UTR.fa)
## ---- eval = bedtools---------------------------------------------------------
# bam <- system.file("extdata/chr4and5.bam", package="nearBynding")
# sorted_bam<-sortBam(bam, "chr4and5_sorted")
#
# CleanBAMtoBG(in_bam = sorted_bam)
## -----------------------------------------------------------------------------
liftOverToExomicBG(input = "chr4and5_sorted.bedGraph",
chain = "test.chain",
chrom_size = "chr4and5_3UTR.size",
output_bg = "chr4and5_liftOver.bedGraph")
## -----------------------------------------------------------------------------
processCapRout(CapR_outfile = system.file("extdata/chr4and5_3UTR.out",
package="nearBynding"),
chain = "test.chain",
output_prefix = "chr4and5_3UTR",
chrom_size = "chr4and5_3UTR.size",
genome_gtf = gtf,
RNA_fragment = "three_prime_utr")
## ---- eval = stereogene-------------------------------------------------------
# runStereogeneOnCapR(protein_file = "chr4and5_liftOver.bedGraph",
# chrom_size = "chr4and5_3UTR.size",
# name_config = "chr4and5_3UTR.cfg",
# input_prefix = "chr4and5_3UTR")
## ---- echo = FALSE, eval = !stereogene, results='hide'------------------------
get_outfiles()
## ---- eval = FALSE------------------------------------------------------------
# runStereogene(track_files = c("chr4and5_3UTR_stem_liftOver.bedGraph",
# "chr4and5_liftOver.bedGraph"),
# name_config = "chr4and5_3UTR.cfg")
## ---- eval = stereogene-------------------------------------------------------
# visualizeCapRStereogene(CapR_prefix = "chr4and5_3UTR",
# protein_file = "chr4and5_liftOver",
# heatmap = TRUE,
# out_file = "all_contexts_heatmap",
# x_lim = c(-500, 500))
# visualizeCapRStereogene(CapR_prefix = "chr4and5_3UTR",
# protein_file = "chr4and5_liftOver",
# x_lim = c(-500, 500),
# out_file = "all_contexts_line",
# y_lim = c(-18, 22))
## ---- fig.show='hold', echo = FALSE, out.width = '50%'------------------------
knitr::include_graphics("all_contexts_heatmap.jpeg")
knitr::include_graphics("all_contexts_line.pdf")
## ---- eval = stereogene-------------------------------------------------------
# visualizeStereogene(context_file = "chr4and5_3UTR_stem_liftOver",
# protein_file = "chr4and5_liftOver",
# out_file = "stem_line",
# x_lim = c(-500, 500))
# visualizeStereogene(context_file = "chr4and5_3UTR_stem_liftOver",
# protein_file = "chr4and5_liftOver",
# heatmap = TRUE,
# out_file = "stem_heatmap",
# x_lim = c(-500, 500))
## ---- fig.show='hold', echo = FALSE, out.width = '50%'------------------------
knitr::include_graphics("stem_heatmap.jpeg")
knitr::include_graphics("stem_line.pdf")
## -----------------------------------------------------------------------------
bindingContextDistance(RNA_context = "chr4and5_3UTR_stem_liftOver",
protein_file = "chr4and5_liftOver",
RNA_context_2 = "chr4and5_3UTR_hairpin_liftOver")
## -----------------------------------------------------------------------------
bindingContextDistance(RNA_context = "chr4and5_3UTR_internal_liftOver",
protein_file = "chr4and5_liftOver",
RNA_context_2 = "chr4and5_3UTR_hairpin_liftOver")
## -----------------------------------------------------------------------------
sessionInfo()
Try the nearBynding package in your browser
Any scripts or data that you put into this service are public.
R Package Documentation
Browse R Packages
We want your feedback!
Note that we can't provide technical support on individual packages. You should contact the package authors for that.
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