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FastQ Screen works with E coli paired-end test file
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3 changed files with 38 additions and 3 deletions
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@ -9,7 +9,9 @@ process FASTQ_SCREEN {
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input:
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tuple val(name), path(reads)
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val (outputdir)
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val (fastq_screen_args)
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// fastq_screen_args are best passed in to the workflow in the following manner:
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// --fastq_screen_args="--subset 200000 --force"
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val (fastq_screen_args)
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val (verbose)
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output:
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@ -21,8 +23,9 @@ process FASTQ_SCREEN {
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mode: "link", overwrite: true
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script:
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fastq_screen_args = fastq_screen_args.replaceAll(/'/,"")
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println(name)
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println(reads)
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println(outputdir)
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if (verbose){
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println ("[MODULE] FASTQ SCREEN ARGS: "+ fastq_screen_args)
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}
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30
tools/fastq_screen/test/main.nf
Executable file
30
tools/fastq_screen/test/main.nf
Executable file
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@ -0,0 +1,30 @@
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#!/usr/bin/env nextflow
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nextflow.preview.dsl = 2
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params.outdir = "."
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params.fastq_screen_args = ''
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// fastq_screen_args are best passed in to the workflow in the following manner:
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// --fastq_screen_args="--subset 200000 --force"
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params.verbose = false
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if (params.verbose){
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println ("[WORKFLOW] FASTQ SCREEN ARGS ARE: " + params.fastq_screen_args)
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}
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// TODO: include '../../../nf-core/module_testing/check_process_outputs.nf'
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include '../main.nf'
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// Define input channels
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ch_read_files = Channel
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.fromFilePairs('../../../test-datasets/Ecoli*{1,2}.fastq.gz',size:-1)
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// .view() // to check whether the input channel works
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// Run the workflow
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workflow {
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main:
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FASTQ_SCREEN(ch_read_files, params.outdir, params.fastq_screen_args, params.verbose)
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// TODO .check_output()
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}
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2
tools/fastq_screen/test/nextflow.config
Normal file
2
tools/fastq_screen/test/nextflow.config
Normal file
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@ -0,0 +1,2 @@
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// docker.enabled = true
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params.outdir = './results'
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