Workflow Type: Galaxy
Frozen
This workflow take as input a collection of paired fastq. It will remove bad quality and adapters with cutadapt. Map with Bowtie2 end-to-end. Will remove reads on MT and unconcordant pairs and pairs with mapping quality below 30 and PCR duplicates. Will compute the pile-up on 5' +- 100bp. Will call peaks and count the number of reads falling in the 1kb region centered on the summit. Will plot the number of reads for each fragment length.
Inputs
ID | Name | Description | Type |
---|---|---|---|
PE fastq input | PE fastq input | Should be a paired collection with ATAC-seq fastqs |
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effective_genome_size | effective_genome_size | Used by macs2:\nH. sapiens: 2700000000, M. musculus: 1870000000, D. melanogaster: 120000000, C. elegans: 90000000 |
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reference_genome | reference_genome | reference_genome |
|
Steps
ID | Name | Description |
---|---|---|
3 | Cutadapt (remove adapter + bad quality bases) | toolshed.g2.bx.psu.edu/repos/lparsons/cutadapt/cutadapt/4.0+galaxy0 |
4 | Bowtie2 map on reference | toolshed.g2.bx.psu.edu/repos/devteam/bowtie2/bowtie2/2.4.5+galaxy1 |
5 | filter MAPQ30 concordant pairs and not mitochondrial pairs | toolshed.g2.bx.psu.edu/repos/devteam/bamtools_filter/bamFilter/2.5.1+galaxy0 |
6 | Get number of reads per chromosome | toolshed.g2.bx.psu.edu/repos/devteam/samtools_idxstats/samtools_idxstats/2.0.4 |
7 | remove PCR duplicates | toolshed.g2.bx.psu.edu/repos/devteam/picard/picard_MarkDuplicates/2.18.2.3 |
8 | reads in chrM/MT for multiQC | toolshed.g2.bx.psu.edu/repos/bgruening/text_processing/tp_awk_tool/1.1.2 |
9 | convert BAM to BED to improve peak calling | toolshed.g2.bx.psu.edu/repos/iuc/bedtools/bedtools_bamtobed/2.30.0+galaxy2 |
10 | Compute fragment length histogram | toolshed.g2.bx.psu.edu/repos/iuc/pe_histogram/pe_histogram/1.0.1 |
11 | number of reads | toolshed.g2.bx.psu.edu/repos/iuc/samtools_view/samtools_view/1.15.1+galaxy0 |
12 | Call Peak with MACS2 | toolshed.g2.bx.psu.edu/repos/iuc/macs2/macs2_callpeak/2.2.7.1+galaxy0 |
13 | get summits +/-500kb | toolshed.g2.bx.psu.edu/repos/iuc/bedtools/bedtools_slopbed/2.30.0+galaxy1 |
14 | summary of MACS2 | toolshed.g2.bx.psu.edu/repos/bgruening/text_processing/tp_grep_tool/1.1.1 |
15 | Bigwig from MACS2 | wig_to_bigWig |
16 | Merge summits +/-500kb | toolshed.g2.bx.psu.edu/repos/iuc/bedtools/bedtools_mergebed/2.30.0 |
17 | Compute coverage on summits +/-500kb | toolshed.g2.bx.psu.edu/repos/iuc/bedtools/bedtools_coveragebed/2.30.0 |
18 | number of reads in peaks | toolshed.g2.bx.psu.edu/repos/bgruening/text_processing/tp_awk_tool/1.1.2 |
19 | Combine number of reads in peaks with total number of reads | cat1 |
20 | reads in peaks multiQC | toolshed.g2.bx.psu.edu/repos/bgruening/text_processing/tp_awk_tool/1.1.2 |
21 | MultiQC | toolshed.g2.bx.psu.edu/repos/iuc/multiqc/multiqc/1.11+galaxy0 |
Outputs
ID | Name | Description | Type |
---|---|---|---|
mapping stats | mapping stats | n/a |
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MarkDuplicates metrics | MarkDuplicates metrics | n/a |
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BAM filtered rmDup | BAM filtered rmDup | n/a |
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histogram of fragment length | histogram of fragment length | n/a |
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MACS2 narrowPeak | MACS2 narrowPeak | n/a |
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MACS2 report | MACS2 report | n/a |
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Coverage from MACS2 (bigwig) | Coverage from MACS2 (bigwig) | n/a |
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1kb around summits | 1kb around summits | n/a |
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Nb of reads in summits +-500bp | Nb of reads in summits +-500bp | n/a |
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MultiQC on input dataset(s): Stats | MultiQC on input dataset(s): Stats | n/a |
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MultiQC webpage | MultiQC webpage | n/a |
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Version History
Version 1 (earliest) Created 23rd Nov 2022 at 10:41 by Finn Bacall
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Frozen
Version-1
938dbc5
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Created: 23rd Nov 2022 at 10:41
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