// Import generic module functions include { initOptions; saveFiles; getSoftwareName; getProcessName } from './functions' params.options = [:] options = initOptions(params.options) def VERSION = '2.2.0' process HISAT2_ALIGN { tag "$meta.id" label 'process_high' publishDir "${params.outdir}", mode: params.publish_dir_mode, saveAs: { filename -> saveFiles(filename:filename, options:params.options, publish_dir:getSoftwareName(task.process), meta:meta, publish_by_meta:['id']) } conda (params.enable_conda ? "bioconda::hisat2=2.2.0 bioconda::samtools=1.10" : null) if (workflow.containerEngine == 'singularity' && !params.singularity_pull_docker_container) { container "https://depot.galaxyproject.org/singularity/mulled-v2-a97e90b3b802d1da3d6958e0867610c718cb5eb1:2880dd9d8ad0a7b221d4eacda9a818e92983128d-0" } else { container "quay.io/biocontainers/mulled-v2-a97e90b3b802d1da3d6958e0867610c718cb5eb1:2880dd9d8ad0a7b221d4eacda9a818e92983128d-0" } input: tuple val(meta), path(reads) path index path splicesites output: tuple val(meta), path("*.bam"), emit: bam tuple val(meta), path("*.log"), emit: summary path "versions.yml" , emit: version tuple val(meta), path("*fastq.gz"), optional:true, emit: fastq script: def software = getSoftwareName(task.process) def prefix = options.suffix ? "${meta.id}${options.suffix}" : "${meta.id}" def strandedness = '' if (meta.strandedness == 'forward') { strandedness = meta.single_end ? '--rna-strandness F' : '--rna-strandness FR' } else if (meta.strandedness == 'reverse') { strandedness = meta.single_end ? '--rna-strandness R' : '--rna-strandness RF' } def seq_center = params.seq_center ? "--rg-id ${prefix} --rg SM:$prefix --rg CN:${params.seq_center.replaceAll('\\s','_')}" : "--rg-id ${prefix} --rg SM:$prefix" if (meta.single_end) { def unaligned = params.save_unaligned ? "--un-gz ${prefix}.unmapped.fastq.gz" : '' """ INDEX=`find -L ./ -name "*.1.ht2" | sed 's/.1.ht2//'` hisat2 \\ -x \$INDEX \\ -U $reads \\ $strandedness \\ --known-splicesite-infile $splicesites \\ --summary-file ${prefix}.hisat2.summary.log \\ --threads $task.cpus \\ $seq_center \\ $unaligned \\ $options.args \\ | samtools view -bS -F 4 -F 256 - > ${prefix}.bam cat <<-END_VERSIONS > versions.yml ${getProcessName(task.process)}: ${getSoftwareName(task.process)}: \$(echo $VERSION) END_VERSIONS """ } else { def unaligned = params.save_unaligned ? "--un-conc-gz ${prefix}.unmapped.fastq.gz" : '' """ INDEX=`find -L ./ -name "*.1.ht2" | sed 's/.1.ht2//'` hisat2 \\ -x \$INDEX \\ -1 ${reads[0]} \\ -2 ${reads[1]} \\ $strandedness \\ --known-splicesite-infile $splicesites \\ --summary-file ${prefix}.hisat2.summary.log \\ --threads $task.cpus \\ $seq_center \\ $unaligned \\ --no-mixed \\ --no-discordant \\ $options.args \\ | samtools view -bS -F 4 -F 8 -F 256 - > ${prefix}.bam if [ -f ${prefix}.unmapped.fastq.1.gz ]; then mv ${prefix}.unmapped.fastq.1.gz ${prefix}.unmapped_1.fastq.gz fi if [ -f ${prefix}.unmapped.fastq.2.gz ]; then mv ${prefix}.unmapped.fastq.2.gz ${prefix}.unmapped_2.fastq.gz fi cat <<-END_VERSIONS > versions.yml ${getProcessName(task.process)}: ${getSoftwareName(task.process)}: \$(echo $VERSION) END_VERSIONS """ } }