Structural variant caller using low-depth long reads
Project description
NanoVar - Structural variant caller using low-depth long-read sequencing
NanoVar is a genomic structural variant (SV) caller that utilizes low-depth long-read sequencing such as Oxford Nanopore Technologies (ONT). It characterizes SVs with high accuracy and speed using only 4x depth sequencing for homozygous SVs and 8x depth for heterozygous SVs. NanoVar reduces sequencing cost and computational requirements which makes it compatible with large cohort SV-association studies or routine clinical SV investigations.
Basic capabilities
- Performs long-read mapping (Minimap2 and HS-BLASTN) and SV discovery in a single rapid pipeline.
- Accurately characterizes SVs using long sequencing reads (High SV recall and precision in simulation datasets, overall F1 score >0.9)
- Characterizes six classes of SVs including novel-sequence insertion, deletion, inversion, tandem duplication, sequence transposition and translocation.
- Requires 4x and 8x sequencing depth for detecting homozygous and heterozygous SVs respectively.
- Rapid computational speed (Takes <3 hours to map and analyze 12 gigabases datasets (4x) using 24 CPU threads)
- Approximates SV genotype
Getting Started
Quick run
nanovar [Options] -t 24 -f hg38 sample.fq/sample.bam ref.fa working_dir
Parameter | Argument | Comment |
---|---|---|
-t |
num_threads | Indicate number of CPU threads to use |
-f (Optional) |
gap_file (Optional) | Choose built-in gap BED file or specify own file to exclude gap regions in the reference genome. Built-in gap files include: hg19, hg38 and mm10 |
- | sample.fq/sample.bam | Input long-read FASTA/FASTQ file or mapped BAM file |
- | ref.fa | Input reference genome in FASTA format |
- | working_dir | Specify working directory |
Output
Output file | Comment |
---|---|
${sample}.nanovar.pass.vcf | Final VCF filtered output file (1-based) |
${sample}.nanovar.pass.report.html | HTML report showing run summary and statistics |
For more information, see wiki.
Operating system:
- Linux (x86_64 architecture, tested in Ubuntu 14.04, 16.04, 18.04)
Installation:
There are three ways to install NanoVar:
Option 1: Conda (Recommended)
# Installing from bioconda automatically installs all dependencies
conda install -c bioconda nanovar
Option 2: Pip (See dependencies below)
# Installing from PyPI requires own installation of dependencies, see below
pip install nanovar
Option 3: GitHub (See dependencies below)
# Installing from GitHub requires own installation of dependencies, see below
git clone https://github.com/cytham/nanovar.git
cd nanovar
pip install .
Installation of dependencies
- bedtools >=2.26.0
- samtools >=1.3.0
- minimap2 >=2.17
- makeblastdb and windowmasker
- hs-blastn
Please make sure each executable binary is in PATH.
1. bedtools
Please visit here for instructions to install.
2. samtools
Please visit here for instructions to install.
3. minimap2
Please visit here for instructions to install.
4. makeblastdb and windowmasker
# Download NCBI-BLAST v2.3.0+ from NCBI FTP server
wget ftp://ftp.ncbi.nlm.nih.gov/blast/executables/blast+/2.3.0/ncbi-blast-2.3.0+-x64-linux.tar.gz
# Extract tar.gz
tar zxf ncbi-blast-2.3.0+-x64-linux.tar.gz
# Copy makeblastdb and windowmasker binaries to PATH (e.g. ~/bin)
cp ncbi-blast-2.3.0+/bin/makeblastdb ~/bin && cp ncbi-blast-2.3.0+/bin/windowmasker ~/bin
5. hs-blastn
# Download and compile
git clone https://github.com/chenying2016/queries.git
cd queries/hs-blastn-src/
make
# Copy hs-blastn binary to path (e.g. ~/bin)
cp hs-blastn ~/bin
Documentation
See wiki for more information.
Versioning
See CHANGELOG
Citation
If you use NanoVar, please cite:
Tham, CY., Tirado-Magallanes, R., Goh, Y. et al. NanoVar: accurate characterization of patients’ genomic structural variants using low-depth nanopore sequencing. Genome Biol. 21, 56 (2020). https://doi.org/10.1186/s13059-020-01968-7
Authors
- Tham Cheng Yong - cytham
- Roberto Tirado Magallanes - rtmag
- Touati Benoukraf - benoukraflab
License
This project is licensed under GNU General Public License - see LICENSE.txt for details.
Simulation datasets and scripts used in the manuscript
SV simulation datasets used in the manuscript can be downloaded here. Scripts used for simulation dataset generation and tool performance comparison are available here.
Although NanoVar is provided with a universal model and threshold score, instructions required for building a custom neural-network model is available here.
Limitations
-
The inaccurate basecalling of large homopolymer or low complexity DNA regions may result in the false determination of deletion SVs. We advise the use of up-to-date ONT basecallers such as Guppy to minimize this possibility.
-
For BND SVs, NanoVar is unable to calculate the actual number of SV-opposing reads (normal reads) at the novel adjacency as there are two breakends from distant locations. It is not clear whether the novel adjacency is derived from both or either breakends, in cases of balanced and unbalanced variants, and therefore its not possible to know which breakend location(s) to consider for counting normal reads. Currently, NanoVar approximates the normal read count by the minimum count from either breakend location. Although this helps in capturing unbalanced BNDs, it might lead to some false positives.
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