#Assembly Improvement
Take in an assembly in FASTA format, reads in FASTQ format, and make the assembly better by scaffolding and gap filling.
Instructions for installing the software can be found in INSTALL.md.
improve_assembly
The improve_assembly script is the main script for the repository. The usage is:
Usage: improve_assembly [options] -a <FASTA> -f <FASTQ> -r <FASTQ> -s <EXEC> -g <EXEC>
Given an assembly in FASTA format and paired ended reads in FASTQ format, output a scaffolded and gapfilled assembly.
Required:
-a STR assembly FASTA(.gz) file
-f STR forward reads FASTQ(.gz) file
-r STR reverse reads FASTQ(.gz) file
-s STR path to SSPACE executable
-g STR path to GapFiller executable
Options:
-c STR reference FASTA(.gz) file
-i INT insert size [250]
-b STR path to abacas.pl executable
-o STR output directory [.]
-l INT Minimum final contig length [300]
-p INT Only filter if this percentage of bases left [95]
-d debug output []
-h print this message and exit
To scaffold and gap fill an assembly you run:
improve_assembly -a contigs.fa -f 123_1.fastq -r 123_2.fastq
This will output files for each stage in the script, with the various processes performed in the filename. The final filename in this case is scaffolds.scaffolded.gapfilled.length_filtered.sorted.fa.
A reference genome can be used to additionally orientate and order the contigs using ABACAS. This is useful for when you have a close by high quality reference sequence.
improve_assembly -a contigs.fa -f 123_1.fastq -r 123_2.fastq -c my_reference.fa
The input files can be optionally gzipped.
improve_assembly -a contigs.fa.gz -f 123_1.fastq.gz -r 123_2.fastq.gz
The insert size (fragment size) should ideally be set to the actual insert size. Be aware that the insert size you ask for can often differ from the actual insert size achieved in the lab. It is assumed that most of the reads will fall within 30% of the insert size given. To change it use -i:
improve_assembly -a contigs.fa -f 123_1.fastq -r 123_2.fastq -i 500
Small contigs are filtered out at the end (default 300 bases).
improve_assembly -a contigs.fa -f 123_1.fastq -r 123_2.fastq -l 500
The filtering step is only run if the size of the assembly is at least 95% of the input size. This can be changed using -p:
improve_assembly -a contigs.fa -f 123_1.fastq -r 123_2.fastq -p 95
The output directory for the results can be set using -o.
improve_assembly -a contigs.fa -f 123_1.fastq -r 123_2.fastq -o my_directory
descaffold_assembly
Given a FASTA file, break up each sequence where there is a gap.
Usage: descaffold_assembly -a <FASTA>
diginorm_with_khmer
A wrapper script around the khmer normalize-by-median.py script. This is useful where you have uneven coverage. For example in certain virus sequencing experiments, there can be 10,000X coverage however different parts of the genome may have been amplified so the actual coverage can have massive peaks and troughs.
Usage: diginorm_with_khmer [options] -i <FASTQ>
Required:
-i STR input FASTQ(.gz) file of shuffled reads
Options:
-c INT target median coverage [2]
-k INT length of kmer to be used, higher numbers require more RAM [31]
-n INT number of hashes [4]
-m FLOAT minimum hash size. [2.5e8]
-o STR output directory [.]
-z STR output filename [digitally_normalised.fastq.gz]
-e STR path to normalize-by-median.py
-py STR python executable [python-2.7]
-d debug output []
-h print this message and exit
fastq_tools
This script has some useful utilities for analysing a shuffled paired ended FASTQ file. We know they are available in other applications but to minimise dependancies we reimplemented them and have exposed them here for completeness sake.
Usage: fastq_tools [options] -i <FASTQ>
Required:
-i STR input FASTQ(.gz) file of shuffled reads
-t STR task to be run (kmer/coverage/split/histogram)
Options:
-g INT genome size of the coverage task []
-h print this message and exit
Calculate 66% and 90% of median read length as minimum and maximum kmer sizes for use when runnning VelvetOptimiser:
fastq_tools -i input.fastq -t kmer
To calculate the coverage of a genome:
fastq_tools -i input.fastq -t coverage -g 5000000
To split a shuffled paired ended FASTQ file into 2 FASTQ files, one containing the forward reads and another containing the reverse reads. At the end of each read name /1 (forward) or /2 (reverse) is appended:
fastq_tools -i input.fastq -t split
To produce a histogram (histogram.png) of the read lengths found in the FASTQ file. This is useful for after you have trimmed the reads to get an indication of whats left:
fastq_tools -i input.fastq -t histogram
fill_gaps_with_gapfiller
Given an assembly in FASTA format and paired ended reads in FASTQ format, iteratively fill in gaps with GapFiller. Initially a high level of read coverage is required to close a gap, which decreases with subsequent iterations. The means that bases with the highest level of evidence are filled in first, reducing the possiblity of errors.
Usage: fill_gaps_with_gapfiller [options] -a <FASTA> -f <FASTQ> -r <FASTQ> -g <EXEC>
Take in an assembly in FASTA format and reads in FASTQ format, then iteratively fill in the gaps with GapFiller.
Required:
-a STR assembly FASTA(.gz) file
-f STR forward reads FASTQ(.gz) file
-r STR reverse reads FASTQ(.gz) file
-g STR path to GapFiller executable
Options:
-i INT insert size [250]
-t INT number of threads [1]
-o STR output directory [.]
-d debug output []
-h print this message and exit
order_contigs_with_abacas
A wrapper script around ABACAS for ordering contigs against a reference.
Usage: order_contigs_with_abacas -a <FASTA> -c <FASTA>
Take in an assembly and a reference in FASTA format and order the contigs.
Required:
-a STR assembly FASTA(.gz) file
-c STR reference genome FASTA(.gz) file
Options:
-b STR ABACAS executable [abacas.pl]
-h print this message and exit
read_correction_with_sga
A wrapper script around SGA read correction which sets some common defaults.
Usage: read_correction_with_sga [options] -f <FASTQ> -r <FASTQ> -s <EXEC>
Takes in FASTQ files and produces read corrected fastq files using SGA.
Required:
-f STR forward reads FASTQ(.gz) file
-r STR reverse reads FASTQ(.gz) file
-s STR path to SGA executable
Options:
-m INT minimum read length [66]
-q trim reads using BWT trimming algorithm
-a STR indexing algorithm to use (ropebwt/sais) [ropebwt]
-t INT number of threads [1]
-o STR output directory [.]
-h INT kmer threshold [5]
-k INT length of kmer to be used [41]
-z STR output filename [_sga_error_corrected.fastq.gz]
-d debug output []
remove_primers_with_quasr
A wrapper script around QUASR.
rename_contigs
Rename all sequences in a FASTA file with a common base name and a sequential number.
Usage: rename_contigs [options]
Given an assembly, rename the contigs iteratively
Required:
-a STR assembly FASTA(.gz) file
-b STR basename for sequences
Options:
-h print this message and exit
scaffold_with_sspace
A script to iteratively run scaffold an assembly using paired ended reads using SSPACE. Multiple iterations of scaffolding are run, begining where there is the highest level of read pair evidence linking together 2 contigs. It then outputs the scaffolded assembly in FASTA format.
Usage: scaffold_with_sspace [options] -a <FASTA> -f <FASTQ> -r <FASTQ> -s <EXEC>
Take in an assembly in FASTA format and reads in FASTQ format, then iteratively scaffold with SSPACE.
Required:
-a STR assembly FASTA(.gz) file
-f STR forward reads FASTQ(.gz) file
-r STR reverse reads FASTQ(.gz) file
-s STR path to SSPACE executable
Options:
-i INT insert size [250]
-t INT number of threads [1]
-o STR output directory [.]
-d debug output []
-h print this message and exit