"samtools faidx" compatible FASTA indexing in pure python
Project description
Description
Samtools provides a function “faidx” (FAsta InDeX), which creates a small flat index file “.fai” allowing for fast random access to any subsequence in the indexed fasta, while loading a minimal amount of the file in to memory.
Pyfaidx provides an interface for creating and using this index for fast random access of DNA subsequences from huge fasta files in a “pythonic” manner. Indexing speed is comparable to samtools, and in some cases sequence retrieval is much faster (benchmark). For example:
>>> from pyfaidx import Fasta
>>> genes = Fasta('tests/data/genes.fasta')
>>> genes
Fasta("tests/data/genes.fasta")
Acts like a dictionary.
>>> genes.keys() ['NR_104215.1',
'KF435150.1', 'NM_001282548.1', 'NM_001282549.1', 'XM_005249644.1',
'NM_001282543.1', 'NR_104216.1', 'XM_005265508.1', 'XR_241079.1',
'AB821309.1', 'XM_005249645.1', 'XR_241081.1', 'XM_005249643.1',
'XM_005249642.1', 'NM_001282545.1', 'NR_104212.1', 'XR_241080.1',
'XM_005265507.1', 'KF435149.1', 'NM_000465.3']
>>> genes['NM_001282543.1'][200:230]
NM_001282543.1:201-230
CTCGTTCCGCGCCCGCCATGGAACCGGATG
>>> genes['NM_001282543.1'][200:230].seq
'CTCGTTCCGCGCCCGCCATGGAACCGGATG'
>>> genes['NM_001282543.1'][200:230].name
'NM_001282543.1:201-230'
>>> genes['NM_001282543.1'][200:230].start
201
>>> genes['NM_001282543.1'][200:230].end
230
Slices just like a string:
>>> genes['NM_001282543.1'][200:230][:10]
NM_001282543.1:201-210
CTCGTTCCGC
>>> genes['NM_001282543.1'][200:230][::-1]
NM_001282543.1:230-201
GTAGGCCAAGGTACCGCCCGCGCCTTGCTC
>>> genes['NM_001282543.1'][200:230][::3]
NM_001282543.1:201-230
CGCCCCTACA
Complements and reverse complements just like DNA
>>> genes['NM_001282543.1'][200:230].complement
NM_001282543.1 (complement):201-230
GAGCAAGGCGCGGGCGGTACCTTGGCCTAC
>>> genes['NM_001282543.1'][200:230]
NM_001282543.1 (complement):230-201
CATCCGGTTCCATGGCGGGCGCGGAACGAG
It also provides a command-line script:
cli script: faidx
$ faidx tests/data/genes.fasta NM_001282543.1:201-210 NM_001282543.1:300-320
>NM_001282543.1:201-210
CTCGTTCCGC
>NM_001282543.1:300-320
GTAATTGTGTAAGTGACTGCA
Same syntax as samtools faidx
A lower-level Faidx class is also available:
>>> from pyfaidx import Faidx
>>> fa = Faidx('T7.fa')
>>> fa.build('T7.fa', 'T7.fa.fai')
>>> fa.index
{'EM_PHG:V01146': {'lenc': 60, 'lenb': 61, 'rlen': 39937, 'offset': 40571}, 'EM_PHG:GU071091': {'lenc': 60, 'lenb': 61, 'rlen': 39778, 'offset': 74}}
>>> fa.fetch('EM_PHG:V01146', 1, 10)
EM_PHG:V01146
TCTCACAGTG
>>> fa.fetch('EM_PHG:V01146', 100, 120)
>EM_PHG:V01146
GGTTGGGGATGACCCTTGGGT
If the FASTA file is not indexed, when Faidx is initialized the build method will automatically run, producing “filename.fa.fai” where “filename.fa” is the original FASTA file.
Start and end coordinates are 1-based.
Installation
This package is tested under Python 3.3, 3.2, 2.7, 2.6, and pypy.
pip install pyfaidx or python setup.py install
CLI Usage
“samtools faidx” compatible FASTA indexing in pure python.
usage: faidx [-h] [-n] fasta [regions [regions ...]] Fetch sequence from faidx-indexed FASTA positional arguments: fasta FASTA file regions space separated regions of sequence to fetch e.g. chr1:1-1000 optional arguments: -h, --help show this help message and exit -n, --name print sequence names
Acknowledgements
This project is freely licensed by the author, Matthew Shirley, and was completed under the mentorship and financial support of Drs. Sarah Wheelan and Vasan Yegnasubramanian at the Sidney Kimmel Comprehensive Cancer Center in the Department of Oncology.
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