| #!/bin/bash |
| set -e |
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| THREADS=$(( $(nproc) > 8 ? 8 : $(nproc) )) |
| SCRIPT_DIR="$(cd "$(dirname "${BASH_SOURCE[0]}")" && pwd)" |
| DATA="${SCRIPT_DIR}/data" |
| REF="${SCRIPT_DIR}/reference" |
| OUT="${SCRIPT_DIR}/outputs" |
| RES="${SCRIPT_DIR}/results" |
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| READS="${DATA}/barcode10.fastq.gz" |
| REFERENCE="${REF}/salmonella_ref.fna" |
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| log_step() { |
| echo "==================================================================" |
| echo "STEP: $1" |
| echo "$(date)" |
| echo "==================================================================" |
| } |
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| mkdir -p "${OUT}"/{nanoplot,filtered,assembly,mapping,polished,qc,prokka,amr} "${RES}" |
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| log_step "L1: NanoPlot read QC" |
| if [ ! -f "${OUT}/nanoplot/NanoStats.txt" ]; then |
| NanoPlot --fastq "${READS}" -o "${OUT}/nanoplot" -t ${THREADS} --plots dot |
| else echo "Skipping (exists)"; fi |
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| log_step "L2: Filtlong quality filtering" |
| if [ ! -f "${OUT}/filtered/filtered.fastq.gz" ]; then |
| filtlong --min_length 200 "${READS}" | gzip > "${OUT}/filtered/filtered.fastq.gz" |
| else echo "Skipping (exists)"; fi |
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| log_step "L3: Flye assembly" |
| if [ ! -f "${OUT}/assembly/assembly.fasta" ]; then |
| flye --nano-raw "${OUT}/filtered/filtered.fastq.gz" \ |
| --out-dir "${OUT}/assembly" \ |
| --threads ${THREADS} --genome-size 5m |
| else echo "Skipping (exists)"; fi |
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| log_step "L4: minimap2 read mapping" |
| if [ ! -f "${OUT}/mapping/reads2assembly.bam" ]; then |
| minimap2 -ax map-ont -t ${THREADS} \ |
| "${OUT}/assembly/assembly.fasta" "${OUT}/filtered/filtered.fastq.gz" \ |
| | samtools sort -@ ${THREADS} -o "${OUT}/mapping/reads2assembly.bam" |
| samtools index "${OUT}/mapping/reads2assembly.bam" |
| else echo "Skipping (exists)"; fi |
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| log_step "L5: Medaka polishing" |
| if [ ! -f "${OUT}/polished/consensus.fasta" ]; then |
| medaka_consensus -i "${OUT}/filtered/filtered.fastq.gz" \ |
| -d "${OUT}/assembly/assembly.fasta" \ |
| -o "${OUT}/polished" \ |
| -t ${THREADS} -m r1041_e82_400bps_sup_v5.0.0 2>&1 || { |
| echo "WARNING: Medaka failed with specified model, trying default" |
| medaka_consensus -i "${OUT}/filtered/filtered.fastq.gz" \ |
| -d "${OUT}/assembly/assembly.fasta" \ |
| -o "${OUT}/polished" \ |
| -t ${THREADS} 2>&1 || { |
| echo "WARNING: Medaka failed, using unpolished assembly" |
| cp "${OUT}/assembly/assembly.fasta" "${OUT}/polished/consensus.fasta" |
| } |
| } |
| else echo "Skipping (exists)"; fi |
| FINAL="${OUT}/polished/consensus.fasta" |
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| log_step "L6-LEFT: QUAST assembly QC" |
| if [ ! -f "${OUT}/qc/quast/report.tsv" ]; then |
| quast "${FINAL}" -r "${REFERENCE}" -o "${OUT}/qc/quast" -t ${THREADS} |
| else echo "Skipping (exists)"; fi |
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| log_step "L6-LEFT: BUSCO completeness" |
| if [ ! -d "${OUT}/qc/busco" ]; then |
| busco -i "${FINAL}" -o busco --out_path "${OUT}/qc" \ |
| -l bacteria_odb10 -m genome -c ${THREADS} --force |
| else echo "Skipping (exists)"; fi |
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| log_step "L6-RIGHT: Prokka annotation" |
| if [ ! -f "${OUT}/prokka/SALM.gff" ]; then |
| prokka "${FINAL}" --outdir "${OUT}/prokka" --prefix SALM \ |
| --cpus ${THREADS} --kingdom Bacteria --genus Salmonella --force |
| else echo "Skipping (exists)"; fi |
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| log_step "L6-RIGHT: abricate AMR detection" |
| if [ ! -f "${OUT}/amr/abricate_card.tsv" ]; then |
| abricate "${FINAL}" --db card --minid 80 --mincov 60 > "${OUT}/amr/abricate_card.tsv" |
| else echo "Skipping (exists)"; fi |
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| log_step "L7-MERGE: Building results" |
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| MEAN_LEN=$(grep "Mean read length" "${OUT}/nanoplot/NanoStats.txt" | awk '{print $NF}' | tr -d ',') |
| MEAN_QUAL=$(grep "Mean read quality" "${OUT}/nanoplot/NanoStats.txt" | awk '{print $NF}') |
| TOTAL_BASES=$(grep "Total bases" "${OUT}/nanoplot/NanoStats.txt" | awk '{print $NF}' | tr -d ',') |
| NUM_READS=$(grep "Number of reads" "${OUT}/nanoplot/NanoStats.txt" | head -1 | awk '{print $NF}' | tr -d ',') |
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| TOTAL_LEN=$(grep "^Total length" "${OUT}/qc/quast/report.tsv" | head -1 | cut -f2) |
| NUM_CONTIGS=$(grep "^# contigs " "${OUT}/qc/quast/report.tsv" | head -1 | cut -f2) |
| N50=$(grep "^N50" "${OUT}/qc/quast/report.tsv" | cut -f2) |
| GC=$(grep "^GC" "${OUT}/qc/quast/report.tsv" | cut -f2) |
| LARGEST=$(grep "^Largest contig" "${OUT}/qc/quast/report.tsv" | cut -f2) |
| GENOME_FRAC=$(grep "^Genome fraction" "${OUT}/qc/quast/report.tsv" | cut -f2) |
| MISASSEMBLIES=$(grep "^# misassemblies" "${OUT}/qc/quast/report.tsv" | cut -f2) |
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| BUSCO_SUM=$(grep "C:" "${OUT}/qc/busco/short_summary.specific.bacteria_odb10.busco.txt" 2>/dev/null \ |
| | head -1 | sed 's/^[[:space:]]*//;s/[[:space:]]*$//' || echo "N/A") |
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| CDS=$(grep "^CDS" "${OUT}/prokka/SALM.txt" | awk '{print $2}') |
| TRNA=$(grep "^tRNA" "${OUT}/prokka/SALM.txt" | awk '{print $2}') |
| RRNA=$(grep "^rRNA" "${OUT}/prokka/SALM.txt" | awk '{print $2}') |
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| AMR_COUNT=$(tail -n +2 "${OUT}/amr/abricate_card.tsv" 2>/dev/null | wc -l | tr -d ' ') |
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| cat > "${RES}/longread_assembly_report.csv" << CSVEOF |
| metric,value |
| num_reads,${NUM_READS} |
| mean_read_length,${MEAN_LEN} |
| mean_read_quality,${MEAN_QUAL} |
| total_bases,${TOTAL_BASES} |
| assembly_length,${TOTAL_LEN} |
| num_contigs,${NUM_CONTIGS} |
| n50,${N50} |
| gc_content,${GC} |
| largest_contig,${LARGEST} |
| genome_fraction,${GENOME_FRAC} |
| misassemblies,${MISASSEMBLIES} |
| completeness,${BUSCO_SUM} |
| cds_count,${CDS} |
| trna_count,${TRNA} |
| rrna_count,${RRNA} |
| amr_genes,${AMR_COUNT} |
| CSVEOF |
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| echo "" |
| echo "=== Pipeline complete ===" |
| cat "${RES}/longread_assembly_report.csv" |
| echo "" |
| ls -lh "${RES}/" |
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