Workflow Type: Galaxy

CUT&RUN (and CUT&TAG) Workflow

Inputs dataset

  • The workflow needs a single input which is a list of dataset pairs of fastqsanger.

Inputs values

  • adapter sequences: this depends on the library preparation. Usually CUT&RUN is Truseq and CUT&TAG is Nextera. If you don't know, use FastQC to determine if it is Truseq or Nextera
  • reference_genome: this field will be adapted to the genomes available for bowtie2
  • effective_genome_size: this is used by macs2 and may be entered manually (indications are provided for heavily used genomes)

Processing

  • The workflow will remove illumina adapters and low quality bases and filter out any read smaller than 15bp
  • The filtered reads are mapped with bowtie2 allowing dovetail and fragment length up to 1kb
  • The BAM is filtered to keep only MAPQ30 and concordant pairs
  • The PCR duplicates are removed with Picard
  • The BAM is converted to BED to enable macs2 to take both pairs into account
  • The peaks are called with macs2 which at the same time generates a coverage file.
  • The coverage file is converted to bigwig
  • A multiQC is run to have an overview of the QC

Warning

  • The coverage output is not normalized.

Inputs

ID Name Description Type
PE fastq input PE fastq input Should be a paired collection with CUT and RUN fastqs
  • File[]
adapter_forward adapter_forward Please use: For R1: - For TrueSeq (CUT and RUN): GATCGGAAGAGCACACGTCTGAACTCCAGTCAC or AGATCGGAAGAGCACACGTCTGAACTCCAGTCAC - For Nextera (CUT and TAG): CTGTCTCTTATACACATCTCCGAGCCCACGAGAC
  • string
adapter_reverse adapter_reverse Please use: For R2: - For TruSeq (CUT and RUN): GATCGGAAGAGCGTCGTGTAGGGAAAGAGTGT or AGATCGGAAGAGCGTCGTGTAGGGAAAGAGTGT - For Nextera (CUT and TAG): CTGTCTCTTATACACATCTGACGCTGCCGACGA
  • string
effective_genome_size effective_genome_size Used by MACS2: H. sapiens: 2700000000, M. musculus: 1870000000, D. melanogaster: 120000000, C. elegans: 90000000
  • int
reference_genome reference_genome reference_genome
  • string

Steps

ID Name Description
5 Cutadapt (remove adapter + bad quality bases) toolshed.g2.bx.psu.edu/repos/lparsons/cutadapt/cutadapt/4.0+galaxy1
6 Bowtie2 map on reference toolshed.g2.bx.psu.edu/repos/devteam/bowtie2/bowtie2/2.5.0+galaxy0
7 filter MAPQ30 concordant pairs toolshed.g2.bx.psu.edu/repos/devteam/samtool_filter2/samtool_filter2/1.8+galaxy1
8 remove PCR duplicates toolshed.g2.bx.psu.edu/repos/devteam/picard/picard_MarkDuplicates/2.18.2.3
9 convert BAM to BED to improve peak calling toolshed.g2.bx.psu.edu/repos/iuc/bedtools/bedtools_bamtobed/2.30.0+galaxy2
10 Call Peaks with MACS2 toolshed.g2.bx.psu.edu/repos/iuc/macs2/macs2_callpeak/2.2.7.1+galaxy0
11 summary of MACS2 toolshed.g2.bx.psu.edu/repos/bgruening/text_processing/tp_grep_tool/1.1.1
12 Bigwig from MACS2 wig_to_bigWig
13 MultiQC toolshed.g2.bx.psu.edu/repos/iuc/multiqc/multiqc/1.11+galaxy0

Outputs

ID Name Description Type
Mapping stats Mapping stats n/a
  • File
MarkDuplicates metrics MarkDuplicates metrics n/a
  • File
BAM filtered rmDup BAM filtered rmDup n/a
  • File
MACS2 peaks xls MACS2 peaks xls n/a
  • File
MACS2 summits MACS2 summits n/a
  • File
MACS2 narrowPeak MACS2 narrowPeak n/a
  • File
MACS2 report MACS2 report n/a
  • File
Coverage from MACS2 (bigwig) Coverage from MACS2 (bigwig) n/a
  • File
MultiQC webpage MultiQC webpage n/a
  • File
MultiQC on input dataset(s): Stats MultiQC on input dataset(s): Stats n/a
  • File

Version History

v0.13 (latest) Created 7th Oct 2024 at 16:33 by WorkflowHub Bot

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v0.1 (earliest) Created 20th Oct 2022 at 03:01 by WorkflowHub Bot

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help Creators and Submitter
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  • Lucille Delisle
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Created: 20th Oct 2022 at 03:01

Last updated: 21st Jan 2023 at 03:01

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