name: bio-genome-assembly-metagenome-assembly
description: Metagenome assembly from long reads using metaFlye and metaSPAdes with binning strategies. Use when reconstructing genomes from microbial communities, recovering metagenome-assembled genomes (MAGs), or resolving strain-level variation in complex samples.
tool_type: cli
primary_tool: metaFlye
measurable_outcome: Execute skill workflow successfully with valid output within 15 minutes.
allowed-tools:
- read_file
- run_shell_command
Metagenome Assembly
Overview
Metagenome assembly reconstructs genomes from mixed microbial communities. Long reads enable recovery of complete circular genomes and resolution of strain-level differences.
metaFlye (Long Reads)
# ONT metagenome assembly
flye --nano-raw reads.fastq.gz \
--meta \
--out-dir flye_meta \
--threads 32
# PacBio HiFi metagenome
flye --pacbio-hifi reads.hifi.fastq.gz \
--meta \
--out-dir flye_meta_hifi \
--threads 32
# Key output files:
# assembly.fasta - assembled contigs
# assembly_graph.gfa - assembly graph
# assembly_info.txt - contig statistics
metaSPAdes (Short Reads)
# Illumina paired-end metagenome
metaspades.py -1 R1.fastq.gz -2 R2.fastq.gz \
-o spades_meta \
-t 32 \
-m 500
# With multiple libraries
metaspades.py \
--pe1-1 lib1_R1.fq.gz --pe1-2 lib1_R2.fq.gz \
--pe2-1 lib2_R1.fq.gz --pe2-2 lib2_R2.fq.gz \
-o spades_meta -t 32
Hybrid Assembly
# Combine short and long reads
flye --nano-raw ont_reads.fastq.gz \
--meta \
--out-dir flye_hybrid \
--threads 32
# Polish with short reads
pilon --genome flye_hybrid/assembly.fasta \
--frags short_reads.bam \
--output polished \
--threads 16
Key Parameters
metaFlye
| Parameter |
Description |
| --meta |
Metagenome mode (handles uneven coverage) |
| --min-overlap |
Minimum overlap for assembly (default: auto) |
| --genome-size |
Estimated total size (optional for meta) |
| --iterations |
Polishing iterations (default: 1) |
| --keep-haplotypes |
Preserve strain variants |
metaSPAdes
| Parameter |
Description |
| -m |
Memory limit in GB |
| --only-assembler |
Skip error correction |
| -k |
K-mer sizes (auto-selected by default) |
| --phred-offset |
Quality encoding (33 or 64) |
Binning Workflow
# Step 1: Map reads back to assembly
minimap2 -ax map-ont -t 32 assembly.fasta reads.fastq.gz | \
samtools sort -o mapped.bam -
# Step 2: Generate depth file
jgi_summarize_bam_contig_depths --outputDepth depth.txt mapped.bam
# Step 3: Bin with MetaBAT2
metabat2 -i assembly.fasta -a depth.txt -o bins/bin -t 32
# Step 4: Assess bin quality with CheckM2
checkm2 predict --input bins/ --output-directory checkm2_out -x fa --threads 32
SemiBin2 (Deep Learning Binning)
# Single-sample binning
SemiBin2 single_easy_bin \
-i assembly.fasta \
-b mapped.bam \
-o semibin_out \
--environment global
# Multi-sample binning (better for time-series)
SemiBin2 multi_easy_bin \
-i assembly.fasta \
-b sample1.bam sample2.bam sample3.bam \
-o semibin_multi
Quality Assessment
# Assembly stats
seqkit stats assembly.fasta
# CheckM2 for bin completeness
checkm2 predict -i bins/ -o checkm2_out -x fa -t 32
# GTDB-Tk for taxonomic classification
gtdbtk classify_wf --genome_dir bins/ --out_dir gtdbtk_out --cpus 32
# QUAST for assembly metrics
metaquast.py -o metaquast_out assembly.fasta -t 32
Circular Genome Detection
# Flye marks circular contigs in assembly_info.txt
grep "Y" flye_meta/assembly_info.txt | cut -f1 > circular_contigs.txt
# Extract circular contigs
seqkit grep -f circular_contigs.txt assembly.fasta > circular_genomes.fasta
Python Pipeline
import subprocess
from pathlib import Path
import pandas as pd
def run_metaflye(reads, output_dir, read_type='nano-raw', threads=32):
cmd = ['flye', f'--{read_type}', reads, '--meta', '--out-dir', output_dir, '--threads', str(threads)]
subprocess.run(cmd, check=True)
return Path(output_dir) / 'assembly.fasta'
def run_binning(assembly, bam, output_dir, threads=32):
depth_file = Path(output_dir) / 'depth.txt'
subprocess.run(['jgi_summarize_bam_contig_depths', '--outputDepth', str(depth_file), bam], check=True)
bins_dir = Path(output_dir) / 'bins'
bins_dir.mkdir(exist_ok=True)
subprocess.run(['metabat2', '-i', assembly, '-a', str(depth_file), '-o', str(bins_dir / 'bin'), '-t', str(threads)], check=True)
return bins_dir
def assess_bins(bins_dir, output_dir, threads=32):
subprocess.run(['checkm2', 'predict', '--input', str(bins_dir), '--output-directory', output_dir, '-x', 'fa', '--threads', str(threads)], check=True)
results = pd.read_csv(Path(output_dir) / 'quality_report.tsv', sep='\t')
high_quality = results[(results['Completeness'] > 90) & (results['Contamination'] < 5)]
return high_quality
# Example workflow
assembly = run_metaflye('ont_reads.fq.gz', 'flye_out')
bins = run_binning(str(assembly), 'mapped.bam', 'binning_out')
hq_bins = assess_bins(bins, 'checkm2_out')
print(f'High-quality MAGs: {len(hq_bins)}')
Expected Outputs
| Metric |
Good Assembly |
| N50 |
>50 kb |
| Largest contig |
>1 Mb |
| HQ MAGs (>90% complete, <5% contam) |
Varies by sample |
| Circular genomes |
Sample dependent |
Troubleshooting
| Issue |
Solution |
| Few long contigs |
Increase read depth or length |
| High chimeric rate |
Use --keep-haplotypes in Flye |
| Poor binning |
Add more samples for differential coverage |
| Missing taxa |
Check read QC; consider targeted enrichment |
Related Skills
- genome-assembly/contamination-detection - CheckM2/GUNC
- metagenomics/taxonomic-profiling - Kraken2/Bracken
- metagenomics/functional-profiling - HUMAnN
- long-read-sequencing/read-qc - Input quality control
By