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luslab-umitools | Module feature complete
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4 changed files with 49 additions and 45 deletions
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name: HISAT2
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description: Graph-based alignment of next generation sequencing reads to a population of genomes
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keywords:
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- Alignment
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- Short reads
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- graph FM Index (GFM)
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- RNA-seq
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tools:
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- fastqc:
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description: |
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HISAT2 is a fast and sensitive alignment program for mapping next-generation
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sequencing reads (whole-genome, transcriptome, and exome sequencing data)
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against the general human population (as well as against a single reference genome).
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Based on GCSA (an extension of BWT for a graph) it is designed and implemented as a
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graph FM index (GFM).
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homepage: http://daehwankimlab.github.io/hisat2/
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documentation: https://ccb.jhu.edu/software/hisat2/manual.shtml
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input:
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-
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- sample_id:
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type: string
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description: Sample identifier
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- reads:
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type: file
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description: Input FastQ file, or pair of files
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output:
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-
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- report:
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type: file
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description: mapping statistics report
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pattern: *hisat2_stats.txt
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- alignment:
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type: file
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description: alignment file in BAM format
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pattern: *hisat2.bam
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authors:
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- @FelixKrueger
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@ -17,7 +17,8 @@ process umitools_dedup {
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tuple val(sample_id), path(bai), path(bam)
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output:
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tuple val(sample_id), path(bam), emit: dedupBam
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tuple val(sample_id), path("*.dedup.bam"), emit: dedupBam
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path "*.dedup.log", emit: report
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shell:
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@ -30,16 +31,17 @@ process umitools_dedup {
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// Check main args string exists and strip whitespace
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if(params.umitools_dedup_args) {
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internal_args = params.umitools_dedup_args
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internal_args = internal_args.trim() + " "
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internal_args = internal_args.trim() + " --log=${sample_id}.dedup.log "
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args_exist = "true"
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}
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else {
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error_message = "params.umitools_dedup_args does not exist, please define to run this module."
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}
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//SHELL
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"""
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if ${args_exist}; then
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${internal_prog}${internal_args}-I $bam
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${internal_prog}${internal_args}-I $bam -S ${sample_id}.dedup.bam --output-stats=${sample_id}
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else
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echo "${error_message}" 1>&2
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exit 1
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@ -23,10 +23,6 @@ include umitools_dedup from '../main.nf'
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/* Define input channels
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--------------------------------------------------------------------------------------*/
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//fileName=`basename $bam`
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// sampleName="\${fileName%.Aligned.sortedByCoord.out.bam}"
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// umi_tools dedup --umi-separator=":" -I $bam -S \${sampleName}.dedup.bam --output-stats=\${sampleName}
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// Meta data
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testMetaDataBam = [
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['sample1', "$baseDir/input/sample1.bam"],
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44
tools/umi_tools/umi_tools.yml
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44
tools/umi_tools/umi_tools.yml
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name: umi_tools
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version: 1.0
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description: Tools for dealing with Unique Molecular Identifiers (UMIs)/Random Molecular Tags (RMTs) and single cell RNA-Seq cell barcodes.
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keywords:
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- UMI
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- RMT
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- Barcode
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tools:
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- umi_tools:
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description: |
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Tools for dealing with Unique Molecular Identifiers (UMIs)/Random Molecular Tags (RMTs) and single cell RNA-Seq cell barcodes.
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homepage: https://github.com/CGATOxford/UMI-tools
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documentation: https://umi-tools.readthedocs.io/en/latest/
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processes:
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- dedup:
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opperation: |
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Set command args to params.umitools_dedup_args
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The program will execute with the following pattern: umi_tools dedeup ARGS -I $bam -S SAMPLE_ID.dedup.bam --output-stats=SAMPLE_ID
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description: |
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Groups PCR duplicates and deduplicates reads to yield one read per group.
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Use this when you want to remove the PCR duplicates prior to any downstream analysis.
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input:
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- sample_id:
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type: string
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description: Sample identifier
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- bai:
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type: file
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description: BAM file index
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- bam:
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type: file
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description: BAM sequence file
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output:
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- dedupBam:
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type: tuple
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description: A tuple of samples id and output bam file
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pattern: *SAMPLE_ID.dedup.bam
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- report:
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type: file
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description: Log file for the umi_tools opperation
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pattern: *SAMPLE_ID.dedup.log
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authors:
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- @candiceh08
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- @chris-cheshire
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