Alignment to all pre-2019 bacteria from ENA on standard desktop and laptops computers. Phylign uses phylogenetically compressed assemblies and their k-mer indexes to align batches of queries to them by Minimap 2, all within only several hours.
- 1. Introduction
- 2. Requirements
- 3. Installation
- 4. Usage
- 5. Additional information
- 6. License
- 7. Contacts
The central idea behind Phylign, enabling alignment locally at such a large scale, is phylogenetic compression (paper) - a technique based on using estimated evolutionary history to guide compression and search of large genome collections using existing algorithms and data structures.
In short, input data are reorganized according to the topology of the estimated phylogenies, which makes data highly locally compressible even using basic techniques. Existing software packages for compression, indexing, and search
- in this case XZ, COBS, and Minimap2 - are then used as low-level tools. The resulting performance gains come from a wide range of benefits of phylogenetic compression, including easy parallelization, small memory requirements, small database size, better memory locality, and better branch prediction.
For more information about phylogenetic compression and the implementation details of Phylign, see the corresponding paper (including its supplementary material and visit the associated website.
K. Břinda, L. Lima, S. Pignotti, N. Quinones-Olvera, K. Salikhov, R. Chikhi, G. Kucherov, Z. Iqbal, and M. Baym. Efficient and Robust Search of Microbial Genomes via Phylogenetic Compression. bioRxiv 2023.04.15.536996, 2023. https://doi.org/10.1101/2023.04.15.536996
Phylign requires a standard desktop or laptop computer with an *nix system, and it can also run on a cluster. The minimal hardware requirements are 12 GB RAM and approximately 120 GB of disk space (102 GB for the database and a margin for intermediate files).
Phylign is implemented as a Snakemake pipeline, using the Conda system to manage non-standard dependencies. Ensure you have Conda installed with the following packages:
- GNU Time (on Linux present by default; on OS X, install with
brew install gnu-time
). - Python (>=3.7)
- Snakemake (>=6.2.0)
- Mamba (>= 0.20.0) - optional, but recommended
Additionally, Phylign uses standard Unix tools like GNU Make, cURL, XZ Utils, and GNU Gzip. These tools are typically included in standard *nix installations. However, in minimal setups (e.g., virtualization, continuous integration), you might need to install them using the corresponding package managers.
Make sure you have Conda and GNU Time installed. On Linux:
sudo apt-get install conda
On OS X (using Homebrew):
brew install conda
brew install gnu-time
Install Python (>=3.7), Snakemake (>=6.2.0), and Mamba (optional but recommended) using Conda:
conda install -y -c bioconda -c conda-forge \
"python>=3.7" "snakemake>=6.2.0" "mamba>=0.20.0"
Clone the Phylign repository from GitHub and navigate into the directory:
git clone https://github.com/karel-brinda/phylign
cd phylign
Run the following command to ensure the pipeline works for sample queries and 3 batches (this will also install all additional dependencies using Conda):
make test
Make sure the test returns 0 (success) and that you see the expected output message:
Success! Test run produced the expected output.
Download all phylogenetically compressed assemblies and COBS k-mer indexes for the 661k-HQ collection by:
make download
The downloaded files will be located in the asms/
and cobs/
directories.
Notes:
- The compressed assemblies comprise all the genomes from the 661k collection.The COBS indexes comprise only those genomes that passed quality control.
Remove the default test files or your old files in the input/
directory and
copy or symlink (recommended) your query files. The supported input formats are
FASTA and FASTQ, possibly gzipped. All query files will be preprocessed and
merged together.
Notes:
- All query names have to be unique among all query files.
- Queries should not contain non-ACGT characters. All non-
ACGT
characters in your query sequences will be translated toA
.
Edit the config.yaml
file for your desired search. All
available options are documented directly there.
Run make clean
to clean intermediate files from the previous runs. This
includes COBS matching files, alignment files, and various reports.
Simply run make
, which will execute Snakemake with the corresponding
parameters. If you want to run the pipeline step by step, run make match
followed by make map
.
Check the output files in output/
(for more info about formats, see
5c) File formats).
If the results do not correspond to what you expected and you need to re-adjust
your search parameters, go to Step 2. If only the mapping part is affected by
the changes, you proceed more rapidly by manually removing the files in
intermediate/05_map
and output/
and running directly make map
.
Phylign is executed via GNU Make, which handles all parameters and passes them to Snakemake.
Here's a list of all implemented commands (to be executed as make {command}
):
####################
# General commands #
####################
all Run everything (the default rule)
test Quick test using 3 batches
help Print help messages
clean Clean intermediate search files
cleanall Clean all generated and downloaded files
##################
# Pipeline steps #
##################
conda Create the conda environments
download Download the assemblies and COBS indexes
download_asms Download only the assemblies
download_cobs Download only the COBS indexes
match Match queries using COBS (queries -> candidates)
map Map candidates to assemblies (candidates -> alignments)
#############
# Reporting #
#############
config Print configuration without comments
report Generate Snakemake report
###########
# Cluster #
###########
cluster_slurm Submit to a SLURM cluster
cluster_lsf Submit to LSF cluster
cluster_lsf_test Submit the test pipeline to LSF cluster
##################
# For developers #
##################
format Reformat Python and Snakemake files
checkformat Check source code format
Note: make format
requires
YAPF and
Snakefmt, which can be installed by
conda install -c conda-forge -c bioconda yapf snakefmt
.
asms/
,cobs/
Downloaded assemblies and COBS indexesinput/
Queries, to be provided within one or more FASTA/FASTQ files, possibly gzipped (.fa
)intermediate/
Intermediate files00_queries_preprocessed/
Preprocessed queries01_queries_merged/
Merged queries02_cobs_decompressed/
Decompressed COBS indexes (temporary, used only in the disk mode is used)03_match/
COBS matches04_filter/
Filtered candidates05_map/
Minimap2 alignments
logs/
Logs and benchmarksoutput/
The resulting files (in a headerless SAM format)
Input files: FASTA or FASTQ files possibly compressed by gzipped. The files
are searched in the input/
directory, as files with the following suffixes:
.fa
, .fasta
, .fq
, .fastq
(possibly with .gz
at the end).
Output files:
output/{name}.sam_summary.gz
: output alignments in a headerless SAM formatoutput/{name}.sam_summary.stats
: statistics about your computed alignments in TSV
SAM headers are omitted as all search experiments
generate hits across large numbers of assemblies (many
of them being spurious). As a result, SAM headers then
dominate the outputs. Nevertheless, we note that, in
principle, the SAM headers can always be recreated from the
FASTA files in asms/
, although this functionality is not
currently implemented.
Running on a cluster is much faster as the jobs produced by this pipeline are quite light and usually start running as soon as they are scheduled.
For LSF clusters:
- Test if the pipeline is working on a LSF cluster:
make cluster_lsf_test
; - Configure you queries and run the full pipeline:
make cluster_lsf
;
- Swapping if the number of queries too high. If the number of queries is too high (e.g., 10M Illumina reads), the auxiliary Python scripts start to use too much memory, which may result in swapping. Try to keep the number of queries moderate and ideally their names short.
- No support for ambiguous characters in queries. Queries are expected to be over the ACGT alphabet. All non-ACGT characters in queries are first converted to A.
- Too many reported hits. When queries have too many equally good hits in the database, even if the threshold on the maximum number of hits is chosen low – for instance 10 – the program will take top 10 + ties, which can be a huge number (especially for short sequences).