Collection of Python libraries to parse bioinformatics files, or perform computation related to assembly, annotation, and comparative genomics.
Authors | Haibao Tang (tanghaibao) |
Vivek Krishnakumar (vivekkrish) | |
Xingtan Zhang (tangerzhang) | |
Won Cheol Yim (wyim-pgl) | |
[email protected] | |
License | BSD |
Tip
JCVI is now published in iMeta!
Tang et al. (2024) JCVI: A Versatile Toolkit for Comparative Genomics Analysis. iMeta
Following modules are available as generic Bioinformatics handling methods.
algorithms
apps
formats
Currently supports .ace
format (phrap, cap3, etc.), .agp
(goldenpath), .bed
format, .blast
output, .btab
format,
.coords
format (nucmer
output), .fasta
format, .fastq
format, .fpc
format, .gff
format, obo
format (ontology),
.psl
format (UCSC blat, GMAP, etc.), .posmap
format (Celera
assembler output), .sam
format (read mapping), .contig
format (TIGR assembly format), etc.
graphics
utils
Then there are modules that contain domain-specific methods.
assembly
annotation
compara
Please visit wiki for full-fledged applications.
Following are a list of third-party python packages that are used by some routines in the library. These dependencies are not mandatory since they are only used by a few modules.
There are other Python modules here and there in various scripts. The
best way is to install them via pip install
when you see
ImportError
.
The easiest way is to install it via PyPI:
pip install jcvi
To install the development version:
pip install git+git://github.com/tanghaibao/jcvi.git
Alternatively, if you want to install manually:
cd ~/code # or any directory of your choice
git clone git://github.com/tanghaibao/jcvi.git
pip install -e .
In addition, a few module might ask for locations of external programs,
if the extended cannot be found in your PATH
. The external programs
that are often used are:
Most of the scripts in this package contains multiple actions. To use
the fasta
example:
Usage:
python -m jcvi.formats.fasta ACTION
Available ACTIONs:
clean | Remove irregular chars in FASTA seqs
diff | Check if two fasta records contain same information
extract | Given fasta file and seq id, retrieve the sequence in fasta format
fastq | Combine fasta and qual to create fastq file
filter | Filter the records by size
format | Trim accession id to the first space or switch id based on 2-column mapping file
fromtab | Convert 2-column sequence file to FASTA format
gaps | Print out a list of gap sizes within sequences
gc | Plot G+C content distribution
identical | Given 2 fasta files, find all exactly identical records
ids | Generate a list of headers
info | Run `sequence_info` on fasta files
ispcr | Reformat paired primers into isPcr query format
join | Concatenate a list of seqs and add gaps in between
longestorf | Find longest orf for CDS fasta
pair | Sort paired reads to .pairs, rest to .fragments
pairinplace | Starting from fragment.fasta, find if adjacent records can form pairs
pool | Pool a bunch of fastafiles together and add prefix
qual | Generate dummy .qual file based on FASTA file
random | Randomly take some records
sequin | Generate a gapped fasta file for sequin submission
simulate | Simulate random fasta file for testing
some | Include or exclude a list of records (also performs on .qual file if available)
sort | Sort the records by IDs, sizes, etc.
summary | Report the real no of bases and N's in fasta files
tidy | Normalize gap sizes and remove small components in fasta
translate | Translate CDS to proteins
trim | Given a cross_match screened fasta, trim the sequence
trimsplit | Split sequences at lower-cased letters
uniq | Remove records that are the same
Then you need to use one action, you can just do:
python -m jcvi.formats.fasta extract
This will tell you the options and arguments it expects.
Feel free to check out other scripts in the package, it is not just for FASTA.