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Non-redundant pangenome assemblies from multiple genomes or bins

Project description

SuperPang: non-redundant pangenome assemblies from multiple genomes or bins

Check our paper: Puente-Sánchez F, Hoetzinger M, Buck M and Bertilsson S. Exploring intra-species diversity through non-redundant pangenome assemblies Molecular Ecology Resources (2023) DOI: 10.1111/1755-0998.13826

... but note that performance is now better (3x less memory usage, 20% faster execution time) than when we first benchmarked Superpang.

Installation

Requires graph-tool, speedict, mOTUlizer v0.2.4, minimap2 and mappy. The easiest way to get it running is using conda.

# Install into a new conda environment
conda create -n SuperPang -c conda-forge -c bioconda -c fpusan superpang
# Check that it works for you!
conda activate SuperPang
test-SuperPang.py

Usage

SuperPang.py --fasta <genome1.fasta> <genome2.fasta> <genomeN.fasta> --checkm <check_results> --output-dir <output_directory>

Input files and choice of parameters

  • The input genomes can be genomes from isolates, MAGs (Metagenome-Assembled Genomes) or SAGs (Single-cell Assembled Genomes).
  • The input genomes can have different qualities, for normal usage we recommend that you provide completeness estimates for each input genome through the -q/--checkm parameter.
  • If you are certain that all your input genomes are complete, you can use the --assume-complete flag or manually tweak the -a/--genome-assignment-threshold and -x/--default-completeness parameters instead of providing a file with completeness estimates.
  • The default parameter values in SuperPang assume that all of the input genomes come from the same species (ANI>=0.95). This can be controlled by changing the values of the -i/--identity_threshold and -b/--bubble-identity-threshold to the expected ANI. However SuperPang has currently only been tested in species-level clusters.

Arguments

  • -f/--fasta: Input fasta files with the sequences for each bin/genome, or a single file containing the path to one input fasta file per line.
  • -q/--checkm: CheckM output for the bins. This can be the STDOUT of running checkm on all the fasta files passed in --fasta, or a tab-delimited file ended with a .tsv extension, in the form genome1 percent_completeness. Genome names should not contain the file extension (e.g. .fna). If empty, completeness will be estimated by mOTUpan but this may lead to wrong estimations for very incomplete genomes.
  • -i/--identity_threshold: Identity threshold (fraction) to initiate correction with minimap2. Values of 1 or higher will skip the correction step entirely. Default 0.95.
  • -m/--mismatch-size-threshold: Maximum contiguous mismatch size that will be corrected. Default 100.
  • -g/--indel-size-threshold: Maximum contiguous indel size that will be corrected. Default 100.
  • -r/--correction-repeats: Maximum iterations for sequence correction. Default 20.
  • -n/--correction-repeats-min: Minimum iterations for sequence correction. Default 5.
  • -k/--ksize: Kmer-size. Default 301.
  • -l/--minlen: Scaffold length cutoff. Default 0 (no cutoff).
  • -c/--mincov: Scaffold coverage cutoff. Default 0 (no cutoff).
  • -b/--bubble-identity-threshold: Minimum identity (matches / length) required to remove a bubble in the sequence graph. Default 0.95.
  • -a/--genome-assignment-threshold. Fraction of shared kmers required to assign a contig to an input genome (0 means a single shared kmer is enough) (DEPRECATED).
  • -x/--default-completeness: Default genome completeness to assume if a CheckM output is not provided with --checkm. Default 70.
  • -t/--threads: Number of processors to use. Default 1.
  • -o/--output: Output directory. Default output.
  • -d/--temp-dir: Directory for temp files. Default tmp.
  • -u/--header-prefix: Prefix to be added to output sequence names. No prefix is added by default.
  • --assume-complete: Assume that the input genomes are complete (--default-completeness 99).
  • --lowmem: Use disk storages instead of memory when possible, reduces memory usage at the cost of execution time.
  • --minimap2-path: Path to the minimap2 executable. Default minimap2.
  • --keep-intermediate: Keep intermediate files.
  • --keep-temporary: Keep temporary files.
  • --verbose-mOTUpan: Print out mOTUpan logs.
  • --nice-headers: Removes semicolons from non-branching-path names.
  • --output-as-file-prefix: Use the output dir name also as a prefix for output file names.
  • --force-overwrite: Write results even if the output directory already exists.
  • --debug: Run additional sanity checks (increases execution time).

Output

  • assembly.fasta: contigs.
  • assembly.info: core/auxiliary and path information for each contig.
  • NBPs.fasta: non-branching paths.
  • NBPs.core.fasta: non-branching paths deemed to belong to the core genome of the species by mOTUpan.
  • NBPs.accessory.fasta: non-branching paths deemed to belong to the accessory genome of the species.
  • NBP2origins.tsv: tab-separated file with the non-branching path IDs, a comma-separated list of the input sequences in which that NBP was deemed present, a comma-separated list of the input genomes in which that NBP was deemed present, and the number of input genomes in which that NBP was deemed present.
  • graph.fastg: assembly graph in a format compatible with bandage.
  • graph.NBP2origins.csv: file with similar structure as NBP2origins.tsv, formatted for use together with the "Load CSV file" option in Bandage. This allows using the information in the file as node labels in Bandage.
  • params.tsv: parameters used in the run.

About

SuperPang is developed by Fernando Puente-Sánchez (Sveriges lantbruksuniversitet). Feel free to open an issue or reach out for support fernando.puente.sanchez@slu.se.

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