nPhase is a command line ploidy agnostic phasing pipeline and algorithm which phases samples of any ploidy with sequence alignment of long and short read data to a reference sequence.
Project description
nPhase
Ploidy agnostic phasing pipeline and algorithm
nPhase is a ploidy agnostic tool developed in python which predicts the haplotypes of a sample that was sequenced by both long and short reads by aligning them to a reference. It should work with any ploidy.
Quick-start
If you have bioconda you can install nPhase by running the following commands in your terminal:
conda create -n polyploidPhasing python=3.8
conda activate polyploidPhasing
conda install -c oakheart nphase
Then you can phase your data with the following command:
nphase pipeline --sampleName Individual_1 --reference /path/to/Individual_referenceGenome.fasta
--R1 /path/to/Individual_1_shortReads_R1.fastq.gz --R2 /path/to/Individual_1_shortReads_R2.fastq.gz
--longReads /path/to/Individual_1_longReads.fastq.gz --longReadPlatform [ont|pacbio]
--output /path/to/outputFolder --threads 8
Once you've phased your data, you can use our automated cleaning method on the raw results with the following command:
nphase cleaning --sampleName Cleaning_1 --resultFolder /path/to/outputFolder/Individual_1
--longReads /path/to/Individual_1_longReads.fastq.gz --threads 8
Installation
With bioconda
Install bioconda and set the correct channels by following the first two steps here: https://bioconda.github.io/user/install.html
Then you can create a new environment and install nPhase with the following commands:
conda create -n polyploidPhasing python=3.8
conda activate polyploidPhasing
conda install -c oakheart nphase
Without bioconda
Pre-requisites
You will have to install the following software before nPhase:
*Currently, installing samtools v1.10 or higher will cause an error to occur due to a bug in the way ngmlr handles MAPQ scores.
Installation via PyPI
You can now install nPhase via
pip install -U nPhase
Usage
nphase pipeline or algorithm
There are two main ways to run nPhase:
nphase pipeline
will run the entire pipeline from start to finish and requires the following inputs:
nphase pipeline --sampleName SAMPLE_NAME --reference REFERENCE --output OUTPUT_FOLDER --longReads LONG_READ_FILE
--longReadPlatform {ont,pacbio} --R1 SHORT_READ_FILE_R1 --R2 SHORT_READ_FILE_R2 --threads 8
Optional parameters are described in Parameters.
nphase algorithm
will only run the phasing algorithm, it requires inputs generated by nphase pipeline
. This is useful if you want to test different paramaters on your dataset after having generated the pre-processed files once. Here are the inputs required by nphase algorithm
:
nphase algorithm --sampleName SAMPLE_NAME --reference REFERENCE --output OUTPUT_FOLDER --longReads LONG_READ_FILE
--contextDepth CONTEXT_DEPTHS_FILE --processedLongReads VALIDATED_SNP_ASSIGNMENTS_FILE
Optional parameters are described in Parameters.
nphase partial
Alternatively, if you already mapped your short reads to a reference, or your long reads, or already variant called your mapped short reads, you can try to use
nphase partial
which will run only the parts of the pipeline that you need to run. So for example if you provide it with a vcf file, then it will only try to map the long reads. If you provide it with mapped short reads and mapped long reads, it will only variant call the short reads, etc. This is not recommended since I can't control what you input but it can save people time or allow for more creative uses of nPhase.
Here are the use cases of nphase partial
:
You have mapped long reads and a vcf file of your short reads:
nphase partial --sampleName SAMPLE_NAME --reference REFERENCE --output OUTPUT_FOLDER --longReads LONG_READ_FILE
--vcf VCF_FILE --mappedLongReads MAPPED_LONG_READ_FILE --threads 8
You have mapped long reads and mapped short reads, but not vcf:
nphase partial --sampleName SAMPLE_NAME --reference REFERENCE --output OUTPUT_FOLDER --longReads LONG_READ_FILE
--mappedLongReads MAPPED_LONG_READ_FILE --mappedShortReads MAPPED_SHORT_READ_FILE --threads 8
You have mapped long reads, but no mapped short reads and no vcf:
nphase partial --sampleName SAMPLE_NAME --reference REFERENCE --output OUTPUT_FOLDER --longReads LONG_READ_FILE
--mappedLongReads MAPPED_LONG_READ_FILE --R1 SHORT_READ_FILE_R1 --R2 SHORT_READ_FILE_R2 --threads 8
You have a short read vcf, but no mapped long reads:
nphase partial --sampleName SAMPLE_NAME --reference REFERENCE --output OUTPUT_FOLDER --longReads LONG_READ_FILE
--vcf VCF_FILE --longReadPlatform {ont,pacbio} --threads 8
You have mapped short reads, but no mapped long reads and no vcf:
nphase partial --sampleName SAMPLE_NAME --reference REFERENCE --output OUTPUT_FOLDER --longReads LONG_READ_FILE
--mappedShortReads MAPPED_SHORT_READ_FILE --longReadPlatform {ont,pacbio} --threads 8
Parameters
nPhase pipeline or algorithm
nphase pipeline [-h] [--version] [--threads [THREADS]] [--maxID [MAXID]] [--minOvl [MINOVL]] [--minSim [MINSIM]] [--minLen [MINLEN]] --sampleName SAMPLE_NAME
--reference REFERENCE --output OUTPUT_FOLDER --longReads LONG_READ_FILE --longReadPlatform {ont,pacbio} --R1 SHORT_READ_FILE_R1 --R2
SHORT_READ_FILE_R2
or
nphase algorithm [-h] [--threads [THREADS]] [--maxID [MAXID]] [--minOvl [MINOVL]] [--minSim [MINSIM]] [--minLen [MINLEN]] --sampleName SAMPLE_NAME
--reference REFERENCE --output OUTPUT_FOLDER --longReads LONG_READ_FILE --contextDepth CONTEXT_DEPTHS_FILE --processedLongReads
VALIDATED_SNP_ASSIGNMENTS_FILE
positional arguments:
pipeline Run the entire nPhase pipeline on your sample
algorithm Only run the nPhase algorithm. NOTE: This will require files generated by running the pipeline mode
arguments always required:
--sampleName STRAINNAME
Name of your sample, ex: "Individual_1"
--reference REFERENCE
Path to fasta file of reference genome to align to, ex: /home/reference/Individual_reference.fasta
--output OUTPUTFOLDER
Path to output folder, ex: /home/phased/
--longReads LONGREADFILE
Path to long read FastQ file, ex: /home/longReads/Individual_1.fastq.gz
additional arguments required by nphase pipeline:
--longReadPlatform {ont,pacbio}
Long read platform, must be 'ont' or 'pacbio'
--R1 SHORTREADFILE_R1
Path to paired end short read FastQ file #1, ex: /home/shortReads/Individual_1_R1.fastq.gz
--R2 SHORTREADFILE_R2
Path to paired end short read FastQ file #2, ex: /home/shortReads/Individual_1_R2.fastq.gz
additional arguments required by nphase algorithm:
--contextDepth CONTEXTDEPTHSFILE
Path to context depths file, ex: /home/phased/Individual_1/Overlaps/Individual_1.contextDepths.tsv
--processedLongReads VALIDATEDSNPASSIGNMENTSFILE
Path to validated long read SNPs, ex:
/home/phased/Individual_1/VariantCalls/longReads/Individual_1.hetPositions.SNPxLongReads.validated.tsv
additional arguments potentially required by nphase partial:
--mappedShortReads MAPPEDSHORTREADS
Path to mapped, sorted short read file in BAM format, ex: /home/phased/Individual_1/Mapped/shortReads/Individual_1.final.bam
--vcf VCFFILE Path to VCF file (must be generated with GATK --ploidy=2), ex:/home/phased/Individual_1/VariantCalls/shortReads/Individual.vcf
--mappedLongReads MAPPEDLONGREADS
Path to mapped long read file in SAM format and should be filtered to keep split reads (flag 260), ex: /home/phased/Individual_1/Mapped/longReads/Individual_1.sorted.sam
--longReadPlatform {ont,pacbio}
Long read platform, must be 'ont' or 'pacbio'
--R1 SHORTREADFILE_R1
Path to paired end short read FastQ file #1, ex: /home/shortReads/Individual_1_R1.fastq.gz
--R2 SHORTREADFILE_R2
Path to paired end short read FastQ file #2, ex: /home/shortReads/Individual_1_R2.fastq.gz
optional arguments:
-h, --help show this help message and exit
--version show program's version number and exit
--threads [THREADS] Number of threads to use on some steps, default 8
--maxID [MAXID] MaxID parameter, determines how different two clusters must be to prevent them from merging. Default 0.05
--minOvl [MINOVL] minOvl parameter, determines the minimal percentage of overlap required to allow a merge between two clusters that have fewer than
100 heterozygous SNPs in common. Default 0.1
--minSim [MINSIM] minSim parameter, determines the minimal percentage of similarity required to allow a merge between two clusters. Default 0.01
--minLen [MINLEN] minLen parameter, any cluster based on fewer than N reads will not be output. Default 0
nPhase cleaning
nPhase cleaning [-h] [--version] --sampleName STRAINNAME --longReads LONGREADFILE --resultFolder PHASINGRESULT [--filterPct [PERCENTKEPT]]
[--fillGaps [DEDUPLICATE]] [--filterFirst [FFBOOL]] [--setMaxDiscordance [MAXDISCORDANCE]
optional arguments:
-h, --help show this help message and exit
--version show program's version number and exit
required arguments:
--sampleName STRAINNAME
Name of your sample, ex: "Individual_1"
--longReads LONGREADFILE
Path to long read FastQ file, ex: /home/longReads/Individual_1.fastq.gz
--resultFolder PHASINGRESULT
Path to output folder, ex: /home/nphaseResults/Individual_1/
--filterPct [PERCENTKEPT]
Percentage of results to filter out. Default 2.0
--fillGaps [DEDUPLICATE]
Attempt to fill gaps by redistributing reads from most covered cluster. Set to 0 to disable this step. Default 1
--filterFirst [FFBOOL]
Perform the filtering step before the merging step. Set to 1 to enable. Default 0
--setMaxDiscordance [MAXDISCORDANCE]
If this is set higher than 0, use this percentage as the stopping rule for merging instead of using the mean discordance of raw
results. Inputting 6.8 means 6.8% discordance max allowed. Default 0
Outputs
All files will be named with the prefix "SAMPLE_NAME_minOvl_minSim_maxID", which we will shorten to $prefix in this section.
-
One fastQ file per predicted haplotig in OUTPUT_FOLDER/Phased/FastQ/
-
Three plots in OUTPUT_FOLDER/Phased/Plots/:
- $prefix_coverageVis.{png|svg|pdf}: Coverage of each haplotig plotted against your reference genome
- $prefix_discordanceVis.{png|svg|pdf}: Violin plot for each haplotig showing the distribution of allele frequency within the haplotig. Values around 0.5 here are a sign that two distinct haplotypes were erroneously merged into one
- $prefix_phasedVis.{png|svg|pdf}: Displays the haplotigs along the genome
-
Six tab-separated value (.tsv) files in OUTPUT_FOLDER/Phased/:
- $prefix_variants.tsv: For each haplotig, the haplotig name, chromosome, position, base
- $prefix_clusterReadNames.tsv: For each haplotig, the names of reads that comprise it
- $prefix_phasedDataFull.tsv: For each haplotig, the position, chromosome, y position of each phased SNP. Raw data, not used to generate the phasedVis plot.
- $prefix_discordanceVis.tsv: For each haplotig, the haplotig name, chromosome, position, base, frequency, coverage. Used to generate the discordanceVis plot.
- $prefixD_phasedDataSimple.tsv: For each haplotig, the start position, stop position, chromosome, y position. Used to generate the phasedVis plot.
- $prefix_covVis.tsv: For each haplotig, the haplotig name, chromosome, 5kb window, mean coverage for the window
Paper
If you use nPhase in your work or if you're interested in better understanding how nPhase works, please cite/read the following publication: nPhase: An accurate and contiguous phasing method for polyploids
Media
Online lightning talk I gave about nPhase for an Oxford Nanopore event [5:44]: link
Recommendations
Current recommendations for default parameters are at least 20X coverage per haplotype (so 3*20=60X for a triploid) and a heterozygosity level of at least 0.4% (average of 1 heterozygous SNP every 250 bp).
It is currently untested on pacbio data so if you have a pacbio dataset (with a known ground truth) please contact me (raise an issue on github or email me), especially if you have errors.
There is an example dataset on this github, in the example folder, which you can test nPhase on. It contains a reference sequence, short reads and long reads. The result should look like a triploid and it should run quickly.
Contact me
email: omaroakheart@gmail.com
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