Entering edit mode
Davis, Wade
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350
@davis-wade-2803
Last seen 10.3 years ago
Dear Yue,
I am using your RIPSeeker package and trying to use the option
multicore=TRUE. Trying it on both windows and Linux machines, I did
not observe multiple cores being used until I first called
library(parallel) before running the code below. Also, it appears that
only 2 cores were being used on the Linux machine, and only 1 on the
windows, even though detectCores() indicated 32 cores on the Linux and
8 on the windows.
Are there any additional parameters that I need to set to increase the
number of cores being used?
Thanks,
Wade
######################################################################
##
library(ShortRead)
library(RIPSeeker)
library(parallel)
filedir<-"~/bulkdata/PI/RIP"
setwd(filedir)
bamFiles <- list.files( pattern="_2\\.bam", recursive=TRUE,
full.names=TRUE)
cNAME <- "IgG"
outDir <- file.path(filedir, "RIPSeeker_output_2")
# Parameters setting
binSize <- NULL # set to NULL to automatically determine bin size
multicore <- TRUE # use multicore
strandType <- NULL # set strand type to minus
strand
biomart <- "ENSEMBL_MART_ENSEMBL" # use archive to get
ensembl 65
biomaRt_dataset <- "mmusculus_gene_ensembl" # mouse dataset id name
goAnno <- "org.Mm.eg.db" # GO annotation database
################ run main function ripSeek to predict RIP
################
seekOut.HuR <- ripSeek(bamPath = bamFiles, cNAME = cNAME,
reverseComplement = FALSE, #genomeBuild = "mm10",
not relevant for BAM
strandType = strandType,
uniqueHit = TRUE,
assignMultihits = TRUE,
rerunWithDisambiguatedMultihits = TRUE,
binSize=binSize,
#minBinSize = minBinSize,
#maxBinSize = maxBinSize,
biomart=biomart,
host=host,
biomaRt_dataset = biomaRt_dataset,
goAnno = goAnno,
multicore=multicore,
logOddCutoff = 2,
pvalCutoff = 1,
pvalAdjCutoff = 0.2,
eFDRCutoff = 0.2,
outDir=outDir)
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