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Merge pull request #31 from jfy133/nfcore-tools-update
Get latest Nfcore tools update
2 parents e607888 + c026e53 commit ea9ef95

15 files changed

Lines changed: 85 additions & 179 deletions

.github/workflows/branch.yml

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@@ -12,6 +12,7 @@ jobs:
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# PRs are only ok if coming from an nf-core dev branch
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- name: Check PRs
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run: |
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{ [[ $(git remote get-url origin) == *nf-core/eager ]] && [[ ${GITHUB_HEAD_REF} = "dev" ]]; } || [[ ${GITHUB_HEAD_REF} == "patch" ]]
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echo "HOME: ${HOME}"
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echo "GITHUB_WORKFLOW: ${GITHUB_WORKFLOW}"
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echo "GITHUB_ACTION: ${GITHUB_ACTION}"

.github/workflows/nf-core_eager.yml renamed to .github/workflows/ci.yml

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- name: Try Creating Conda env
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run: |
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conda env create --prefix nf-core-eager-2.1.0dev-d95a13feb408cc17e95d38f16a81010d --file environment.yml
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github_actions_ci:
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runs-on: ubuntu-latest
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test:
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runs-on: ubuntu-18.04
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env:
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TOWER_ACCESS_TOKEN: ${{ secrets.TOWER_ACCESS_TOKEN }}
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NXF_ANSI_LOG: 0
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strategy:
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matrix:
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endedness: ['--singleEnd', '--pairedEnd']
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# Nextflow versions: check pipeline minimum and current latest
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nxf_ver: ['19.10.0', '']
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endedness: ['--single_end', '--paired_end']
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steps:
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- uses: actions/checkout@v1
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- name: Install Nextflow
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run: |
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export NXF_VER=${{ matrix.nxf_ver }}
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wget -qO- get.nextflow.io | bash
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sudo mv nextflow /usr/local/bin/
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- name: Download image
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run: |
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docker pull nfcore/eager:dev && docker tag nfcore/eager:dev nfcore/eager:dev
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- name: Extract branch name
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shell: bash
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run: echo "::set-env name=RUN_NAME::`echo ${GITHUB_REPOSITORY//\//_}`-`echo ${GITHUB_HEAD_REF//\//@} | rev | cut -f1 -d@ | rev`-${{ github.event_name }}-`echo ${GITHUB_SHA} | cut -c1-6`"
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-preindex_ref" -profile test,docker ${{ matrix.endedness }} --bwa_index 'results/reference_genome/bwa_index/BWAIndex/Mammoth_MT_Krause.fasta' --fasta_index 'https://github.com/nf-core/test-datasets/blob/eager/reference/Mammoth/Mammoth_MT_Krause.fasta.fai'
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- name: REFERENCE Run the basic pipeline with FastA reference with `fna` extension
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-fna_ref" -profile test_fna,docker --pairedEnd
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-fna_ref" -profile test_fna,docker --paired_end
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- name: REFERENCE Test with zipped reference input
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-gz_ref" -profile test,docker --pairedEnd --fasta 'https://github.com/nf-core/test-datasets/raw/eager/reference/Mammoth/Mammoth_MT_Krause.fasta.gz'
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-gz_ref" -profile test,docker --paired_end --fasta 'https://github.com/nf-core/test-datasets/raw/eager/reference/Mammoth/Mammoth_MT_Krause.fasta.gz'
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- name: FASTP Test fastp complexity filtering
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-fastp" -profile test,docker --pairedEnd --complexity_filter
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- name: ADAPTERREMOVAL Test skip pairedEnd collapsing
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-fastp" -profile test,docker --paired_end --complexity_filter
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- name: ADAPTERREMOVAL Test skip paired end collapsing
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-skip_collapse" -profile test,docker --pairedEnd --skip_collapse
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- name: ADAPTERREMOVAL Test pairedEnd collapsing but no trimming
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-skip_collapse" -profile test,docker --paired_end --skip_collapse
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- name: ADAPTERREMOVAL Test paired end collapsing but no trimming
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-pretrim" -profile test_pretrim,docker --pairedEnd --skip_trim
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-pretrim" -profile test_pretrim,docker --paired_end --skip_trim
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- name: ADAPTERREMOVAL Run the basic pipeline with paired end data without adapterRemoval
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-skip_adapterremoval" -profile test,docker --pairedEnd --skip_adapterremoval
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-skip_adapterremoval" -profile test,docker --paired_end --skip_adapterremoval
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- name: ADAPTERREMOVAL Run the basic pipeline with preserve5p end option
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-preserve5p" -profile test,docker --pairedEnd --preserve5p
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-preserve5p" -profile test,docker --paired_end --preserve5p
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- name: ADAPTERREMOVAL Run the basic pipeline with merged only option
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-mergedonly" -profile test,docker --pairedEnd --mergedonly
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-mergedonly" -profile test,docker --paired_end --mergedonly
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- name: ADAPTERREMOVAL Run the basic pipeline with preserve5p end and merged reads only options
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-preserve5p_mergedonly" -profile test,docker --pairedEnd --preserve5p --mergedonly
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-preserve5p_mergedonly" -profile test,docker --paired_end --preserve5p --mergedonly
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- name: MAPPER_CIRCULARMAPPER Test running with CircularMapper
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-circularmapper" -profile test,docker --pairedEnd --mapper 'circularmapper' --circulartarget 'NC_007596.2'
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-circularmapper" -profile test,docker --paired_end --mapper 'circularmapper' --circulartarget 'NC_007596.2'
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- name: MAPPER_BWAMEM Test running with BWA Mem
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-bwa_mem" -profile test,docker --pairedEnd --mapper 'bwamem'
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-bwa_mem" -profile test,docker --paired_end --mapper 'bwamem'
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- name: STRIP_FASTQ Run the basic pipeline with output unmapped reads as fastq
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-stripfastq" -profile test,docker --pairedEnd --strip_input_fastq
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-stripfastq" -profile test,docker --paired_end --strip_input_fastq
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- name: BAM_FILTERING Run basic mapping pipeline with mapping quality filtering, and unmapped export
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-unmapped_export" -profile test,docker --pairedEnd --run_bam_filtering --bam_mapping_quality_threshold 37 --bam_discard_umapped --bam_unmapped_type 'fastq'
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-unmapped_export" -profile test,docker --paired_end --run_bam_filtering --bam_mapping_quality_threshold 37 --bam_discard_umapped --bam_unmapped_type 'fastq'
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- name: GENOTYPING_HC Test running GATK HaplotypeCaller
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-haplotypercaller" -profile test_fna,docker --pairedEnd --dedupper 'dedup' --run_genotyping --genotyping_tool 'hc' --gatk_out_mode 'EMIT_ALL_SITES' --gatk_hc_emitrefconf 'BP_RESOLUTION'
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-haplotypercaller" -profile test_fna,docker --paired_end --dedupper 'dedup' --run_genotyping --genotyping_tool 'hc' --gatk_out_mode 'EMIT_ALL_SITES' --gatk_hc_emitrefconf 'BP_RESOLUTION'
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- name: GENOTYPING_FB Test running FreeBayes
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-freebayes" -profile test,docker --pairedEnd --dedupper 'dedup' --run_genotyping --genotyping_tool 'freebayes'
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-freebayes" -profile test,docker --paired_end --dedupper 'dedup' --run_genotyping --genotyping_tool 'freebayes'
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- name: SKIPPING Test checking all skip steps work i.e. input bam, skipping straight to genotyping
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-skipping_logic" -profile test_bam,docker --bam --singleEnd --skip_fastqc --skip_adapterremoval --skip_mapping --skip_deduplication --skip_qualimap --skip_preseq --skip_damage_calculation --run_genotyping --genotyping_tool 'freebayes'
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-skipping_logic" -profile test_bam,docker --bam --single_end --skip_fastqc --skip_adapterremoval --skip_mapping --skip_deduplication --skip_qualimap --skip_preseq --skip_damage_calculation --run_genotyping --genotyping_tool 'freebayes'
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#- name: TRIM_BAM/PMD/GENOTYPING_UG/MULTIVCFANALYZER Test running PMDTools, TrimBam, GATK UnifiedGenotyper and MultiVCFAnalyzer
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# run: |
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# nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-pmd_trimbam_gatkUG_MVA" -profile test,docker --pairedEnd --dedupper 'dedup' --run_trim_bam --run_pmdtools --run_genotyping --genotyping_source 'trimmed' --genotyping_tool 'ug' --gatk_out_mode 'EMIT_ALL_SITES' --gatk_ug_genotype_model 'SNP' --run_multivcfanalyzer
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# nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-pmd_trimbam_gatkUG_MVA" -profile test,docker --paired_end --dedupper 'dedup' --run_trim_bam --run_pmdtools --run_genotyping --genotyping_source 'trimmed' --genotyping_tool 'ug' --gatk_out_mode 'EMIT_ALL_SITES' --gatk_ug_genotype_model 'SNP' --run_multivcfanalyzer
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#- name: GENOTYPING_UG/PMD/MULTIVCFANALYZER Test running GATK UnifiedGenotyper and MultiVCFAnalyzer, additional VCFS
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# run: |
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# nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-MVA_additionalvcfs" -profile test,docker --pairedEnd --dedupper 'dedup' --run_genotyping --genotyping_tool 'ug' --gatk_out_mode 'EMIT_ALL_SITES' --gatk_ug_genotype_model 'SNP' --run_multivcfanalyzer --additional_vcf_files 'https://raw.githubusercontent.com/nf-core/test-datasets/eager/testdata/Mammoth/vcf/JK2772_CATCAGTGAGTAGA_L008_R1_001.fastq.gz.tengrand.fq.combined.fq.mapped_rmdup.bam.unifiedgenotyper.vcf.gz' --write_allele_frequencies
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# nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-MVA_additionalvcfs" -profile test,docker --paired_end --dedupper 'dedup' --run_genotyping --genotyping_tool 'ug' --gatk_out_mode 'EMIT_ALL_SITES' --gatk_ug_genotype_model 'SNP' --run_multivcfanalyzer --additional_vcf_files 'https://raw.githubusercontent.com/nf-core/test-datasets/eager/testdata/Mammoth/vcf/JK2772_CATCAGTGAGTAGA_L008_R1_001.fastq.gz.tengrand.fq.combined.fq.mapped_rmdup.bam.unifiedgenotyper.vcf.gz' --write_allele_frequencies
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#- name: VCF2Genome Run basic pipeline with GATK unifiedgenotyper and run VCF2Genome
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# run: |
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# nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-vcf2genome" -profile test,docker --pairedEnd --dedupper 'dedup' --run_genotyping --genotyping_tool 'ug' --genotyping_source 'raw' --gatk_out_mode 'EMIT_ALL_SITES' --gatk_ug_genotype_model 'SNP' --run_vcf2genome
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# nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-vcf2genome" -profile test,docker --paired_end --dedupper 'dedup' --run_genotyping --genotyping_tool 'ug' --genotyping_source 'raw' --gatk_out_mode 'EMIT_ALL_SITES' --gatk_ug_genotype_model 'SNP' --run_vcf2genome
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- name: BAM_INPUT Run the basic pipeline with the bam input profile, skip AdapterRemoval as no convertBam
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-baminput_noConvertBam" -profile test_bam,docker --bam --skip_adapterremoval --run_convertbam
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for i in index0.idx ref.db ref.idx ref.inf table0.db table0.idx taxonomy.idx taxonomy.map taxonomy.tre; do wget https://github.com/nf-core/test-datasets/raw/eager/databases/malt/"$i" -P databases/malt/; done
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- name: METAGENOMIC Run the basic pipeline but with unmapped reads going into MALT
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-malt" -profile test,docker --pairedEnd --run_bam_filtering --bam_discard_unmapped --bam_unmapped_type 'fastq' --run_metagenomic_screening --database "/home/runner/work/eager/eager/databases/malt/"
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-malt" -profile test,docker --paired_end --run_bam_filtering --bam_discard_unmapped --bam_unmapped_type 'fastq' --run_metagenomic_screening --database "/home/runner/work/eager/eager/databases/malt/"
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- name: MALTEXTRACT Download resource files
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run: |
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mkdir -p databases/maltextract
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for i in ncbi.tre ncbi.map; do wget https://github.com/rhuebler/HOPS/raw/0.33/Resources/"$i" -P databases/maltextract/; done
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- name: MALTEXTRACT Basic with MALT plus MaltExtract
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-maltextract" -profile test,docker --pairedEnd --run_bam_filtering --bam_discard_unmapped --bam_unmapped_type 'fastq' --run_metagenomic_screening --metagenomic_tool 'malt' --database "/home/runner/work/eager/eager/databases/malt" --run_maltextract --maltextract_ncbifiles "/home/runner/work/eager/eager/databases/maltextract/" --maltextract_taxon_list 'https://raw.githubusercontent.com/nf-core/test-datasets/eager/testdata/Mammoth/maltextract/MaltExtract_list.txt'
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-maltextract" -profile test,docker --paired_end --run_bam_filtering --bam_discard_unmapped --bam_unmapped_type 'fastq' --run_metagenomic_screening --metagenomic_tool 'malt' --database "/home/runner/work/eager/eager/databases/malt" --run_maltextract --maltextract_ncbifiles "/home/runner/work/eager/eager/databases/maltextract/" --maltextract_taxon_list 'https://raw.githubusercontent.com/nf-core/test-datasets/eager/testdata/Mammoth/maltextract/MaltExtract_list.txt'
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- name: SEXDETERMINATION Run the basic pipeline with the bam input profile, but don't convert BAM, skip everything but sex determination
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-sexdeterrmine" -profile test_humanbam,docker --bam --skip_fastqc --skip_adapterremoval --skip_mapping --skip_deduplication --skip_qualimap --singleEnd --run_sexdeterrmine
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-sexdeterrmine" -profile test_humanbam,docker --bam --skip_fastqc --skip_adapterremoval --skip_mapping --skip_deduplication --skip_qualimap --single_end --run_sexdeterrmine
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- name: NUCLEAR CONTAMINATION Run basic pipeline with bam input profile, but don't convert BAM, skip everything but nuclear contamination estimation
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-nuclear_contamination" -profile test_humanbam,docker --bam --skip_fastqc --skip_adapterremoval --skip_mapping --skip_deduplication --skip_qualimap --singleEnd --run_nuclear_contamination
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-nuclear_contamination" -profile test_humanbam,docker --bam --skip_fastqc --skip_adapterremoval --skip_mapping --skip_deduplication --skip_qualimap --single_end --run_nuclear_contamination
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- name: MTNUCRATIO Run basic pipeline with bam input profile, but don't convert BAM, skip everything but nmtnucratio
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run: |
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-mtnucratio" -profile test_humanbam,docker --bam --skip_fastqc --skip_adapterremoval --skip_mapping --skip_deduplication --skip_qualimap --singleEnd --skip_preseq --skip_damage_calculation --run_mtnucratio
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nextflow run ${GITHUB_WORKSPACE} "$TOWER" -name "$RUN_NAME-mtnucratio" -profile test_humanbam,docker --bam --skip_fastqc --skip_adapterremoval --skip_mapping --skip_deduplication --skip_qualimap --single_end --skip_preseq --skip_damage_calculation --run_mtnucratio

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