Skip to content

bixBeta/singularity-gg02

BranchesTags

Folders and files

NameName
Last commit message
Last commit date

Latest commit

 

History

7 Commits
discovery-scripts
discovery-scripts
 
 
3.4.sh
3.4.sh
 
 
Broccoli.sorted.gff
Broccoli.sorted.gff
 
 
README.md
README.md
 
 
archive.sh
archive.sh
 
 
atacQC.R
atacQC.R
 
 
atacQC_v2.R
atacQC_v2.R
 
 
atacqc__DEV.R
atacqc__DEV.R
 
 
bacterial.index.sh
bacterial.index.sh
 
 
bam2fastq.sh
bam2fastq.sh
 
 
bedGraphs.sh
bedGraphs.sh
 
 
beta6.sh
beta6.sh
 
 
beta7.sh
beta7.sh
 
 
cdsFix
cdsFix
 
 
cellRanger2.sh
cellRanger2.sh
 
 
cellranger-atac.sh
cellranger-atac.sh
 
 
countMatrix.sh
countMatrix.sh
 
 
firstBase_readLength.sh
firstBase_readLength.sh
 
 
fq.screen.sh
fq.screen.sh
 
 
geneSwitch.R
geneSwitch.R
 
 
getMatrix.sh
getMatrix.sh
 
 
gff.Hash.Aegl5.0 txt
gff.Hash.Aegl5.0 txt
 
 
html.atacQC.sh
html.atacQC.sh
 
 
insert.sh
insert.sh
 
 
knit.atacQC.R
knit.atacQC.R
 
 
my.fastq.conf
my.fastq.conf
 
 
nameCheck.sh
nameCheck.sh
 
 
nova-cellRanger.sh
nova-cellRanger.sh
 
 
novo.download.sh
novo.download.sh
 
 
processCounts.sh
processCounts.sh
 
 
processFeatureCounts.sh
processFeatureCounts.sh
 
 
qc.atac.Rmd
qc.atac.Rmd
 
 
server.sh
server.sh
 
 
smRNA_beta5.sh
smRNA_beta5.sh
 
 
starIndex.sh
starIndex.sh
 
 
starMono.sh
starMono.sh
 
 
starMono2.sh
starMono2.sh
 
 
starSolo.sh
starSolo.sh
 
 
trim.sh
trim.sh
 
 
trimSmall.sh
trimSmall.sh
 
 

Repository files navigation

GG02

development envir for gg02 biohpc

beta6.sh <- RNA-seq workflow

Dependencies:

  • trim_galore: version 0.6 or above (should be in path on biohpc)
  • multiqc: install multiqc using the following command: pip install --user multiqc
  • STAR: version 2.7.0e or above (add to path export PATH=/programs/STAR:$PATH)
  • RSeQC: version 2.61 (add to path using this guideline biohpc)

3.4.sh <- ATAC-seq workflow

Usage:

nohup bash 3.4.sh "[-h arg] [-p arg] [-d args] [-t arg] [-g arg] [-q arg]" > 3.4.log &

Params Description:

"[-h] --> Display Help"
"[-p] --> Project Identifier Number"
"[-d] --> Comma Spearated Values for Delimiter and Field <delim,field or default> default: _,5 "
"[-t] --> Trimming <nextseq or nova>;"
"[-g] --> Reference Genome <mm10 or hg38>"
"[-q] --> Execute atacQC.R script <yes>"
  • Create a folder named fastqs and add all the PE fastq files to this folder
  • Run the 3.4.sh script from the same dir as the fastqs directory
.
├── **3.4.sh**
├── dedup-BAMS
│   ├── PIN.FRIP.multiqc.report_data
│   ├── atacQC.out
│   ├── featureCounts
│   ├── peaks.OUT
│   └── tagDirs
├── fastQC
├── **fastqs**
├── primary-BAMS
├── trimmed_fastqs
└── TrimQC_stats

Tools needed:

  1. trim_galore
  2. fastqc
  3. bwa
  4. samtools
  5. picard tools
  6. homer suite (w/ human and mouse genome config)
  7. macs2
  8. featureCounts (rsubread)
  9. multiqc

About

No description, website, or topics provided.

Resources

Readme
Activity

Stars

0 stars

Watchers

1 watching

Forks

0 forks
Report repository

Releases

No releases published

Packages

No packages published

Languages