FastEAR - Fast(er) Extraction of Alignment Regions

• Last modified: mån nov 21, 2022 01:20
• Sign: JN

Description

Shell (bash) scripts for extracting regions from a fasta-formatted nucleotide alignment based on the description of ranges in a partitions file.

The scripts act as a wrapper for the main software that performs the extraction: faidx. GNU parallel is used for doing the extraction in parallel.

The string in the first column of the partitions file will be used as the stem of the output file name, and the suffix .fas will be added (for example: Apa.fas). The output file will contain all fasta entries in the input fasta file, but only with the sequence positions as specified in the partitions file.

Note that only the first string (without white-space characters!) in the fasta headers will be used in the output.

Currently two versions of the script is provided, differing in which version of faidx used (see Requirements and Installation).

Update: A script using bedtools for extraction is also provided (see Requirements and Installation).

Usage

$ ./fastear_<version>.sh fasta.fas partitions.txt

Example:

$ ./fastear_samtools-1.10.sh data/fasta.fas data/partitions.txt

Example partitions file

Apa = 1-100
Bpa = 101-200
Cpa = 201-300
Dpa = 301-400
Epa = 401-484

Requirements and Installation

Make sure to install GNU parallel, and faidx. For faidx, I tried both the python version, pyfaidx (https://pypi.org/project/pyfaidx), and the original version from samtools (https://github.com/samtools/samtools). Samtools v1.10 is available from, e.g., Ubuntu Linux repositories:

$ sudo apt install samtools

The syntax for samtools faidx have changed between minor samtools versions, and there are two versions of the fastear-script supplied; one for samtools v1.7, and one for v1.10 (or above. Last tested with v1.15).

In addition, if one wishes to use the "bedtools"-version, then bedtools needs to be installed (tested using v2.27). For example (on ubuntu):

$ sudo apt install bedtools

Finally, put the fastear-script(s) in your PATH (e.g., cp fastear_*.sh ~/bin/).

Timings

From a fasta file with 146 sequences, each with length 6,180,000 bp, we extracted 4,818 alignments (on a GNU/Linux system with two Intel Xeon Silver 4214 CPU @ 2.20GHz, 48 cores in total):

Using GNU parallel

#  fastear pyfaidx v.0.5.8 parallel
$ time fastear_pyfaidx.sh data.fas partitions.txt
real    0m47,499s
user    16m44,924s
sys     3m8,175s

# fastear samtools faidx v.1.7 parallel
$ time fastear_samtools-1.7.sh data.fas partitions.txt
real    0m19,714s
user    1m43,326s
sys     1m18,667s

# fastear samtools faidx v.1.10 parallel
$ time fastear_samtools-1.10.sh data.fas partitions.txt
real    0m20,172s
user    1m31,063s
sys     1m12,016s

# fastear bamtools parallel
$ time fastear_bedtools.sh data.fas partitions.txt
real    0m19,784s
user    1m3,445s
sys     0m53,333s

Using a "while read"-loop over the partitions file

#  fastear pyfaidx v.0.5.8 serial
$ time fastear_pyfaidx.serial.sh data.fas partitions.txt
real    11m16,616s
user    9m50,814s
sys     2m11,124s

# fastear samtools faidx v.1.7 serial
$ time fastear_samtools-1.7.serial.sh data.fas partitions.txt
real    2m2,562s
user    1m33,131s
sys     0m53,938s

# fastear samtools faidx v.1.10 serial
$ time fastear_samtools-1.10.serial.sh data.fas partitions.txt
real    1m47,825s
user    1m18,883s
sys     0m52,152s

Disclaimer

Currently in beta version, with minimal error checking. Caveat emptor!

License and Copyright

Copyright (C) 2020, 2021, 2022 Johan Nylander <johan.nylander@nrm.se>. Distributed under terms of the MIT license.