smoove
simplifies and speeds calling and genotyping SVs for short reads. It also improves specificity by removing many
spurious alignment signals that are indicative of low-level noise and often contribute to spurious calls.
There is a blog-post describing smoove
in more detail here
It both supports small cohorts in a single command, and population-level calling with 4 total steps, 2 of which are parallel by sample.
There is a table on the precision and recall of smoove and duphold (which is used by smoove)here
It requires:
- lumpy and lumpy_filter
- samtools: for CRAM support
- gsort: to sort final VCF
- bgzip+tabix: to compress and index final VCF
And optionally (but all highly recommended):
- svtyper: to genotypes SVs
- svtools: required for large cohorts
- mosdepth: remove high coverage regions.
- bcftools: version 1.5 or higher for VCF indexing and filtering.
- duphold: to annotate depth changes within events and at the break-points.
Running smoove
without any arguments will show which of these are found so they can be added to the PATH as needed.
smoove
will:
- parallelize calls to
lumpy_filter
to extract split and discordant reads required by lumpy - further filter
lumpy_filter
calls to remove high-coverage, spurious regions and user-specified chroms like 'hs37d5'; it will also remove reads that we've found are likely spurious signals. after this, it will remove singleton reads (where the mate was removed by one of the previous filters) from the discordant bams. This makeslumpy
much faster and less memory-hungry. - calculate per-sample metrics for mean, standard deviation, and distribution of insert size as required by lumpy.
- stream output of lumpy directly into multiple svtyper processes for parallel-by-region genotyping while lumpy is still running.
- sort, compress, and index final VCF.
you can get smoove
and all dependencies via (a large) docker image:
docker pull brentp/smoove
docker run -it brentp/smoove smoove -h
Or, you can download a smoove
binary from here: https://github.com/brentp/smoove/releases
When run without any arguments, smoove
will show you which of it's dependencies it can find
so you can adjust your $PATH and install accordingly.
for small cohorts it's possible to get a jointly-called, genotyped VCF in a single command.
smoove call -x --name my-cohort --exclude $bed --fasta $reference_fasta -p $threads --genotype /path/to/*.bam
output will go to ./my-cohort-smoove.genotyped.vcf.gz
the --exclude $bed
is highly recommended as it can be used to ignore reads that overlap problematic regions.
A good set of regions for GRCh37 is here.
And for hg38 here
For population-level calling (large cohorts) the steps are:
- For each sample, call genotypes:
smoove call --outdir results-smoove/ --exclude $bed --name $sample --fasta $reference_fasta -p 1 --genotype /path/to/$sample.bam
For large cohorts, it's better to parallelize across samples rather than using a large $threads per sample. smoove
can only
parallelize up to 2 or 3 threads on a single-sample and it's most efficient to use 1 thread.
output will go to `results-smoove/$sample-smoove.genotyped.vcf.gz``
- Get the union of sites across all samples (this can parallelize this across as many CPUs or machines as needed):
# this will create ./merged.sites.vcf.gz
smoove merge --name merged -f $reference_fasta --outdir ./ results-smoove/*.genotyped.vcf.gz
- genotype each sample at those sites (this can parallelize this across as many CPUs or machines as needed) and run duphold to add depth annotations.
smoove genotype -d -x -p 1 --name $sample-joint --outdir results-genotped/ --fasta $reference_fasta --vcf merged.sites.vcf.gz /path/to/$sample.$bam
- paste all the single sample VCFs with the same number of variants to get a single, squared, joint-called file.
smoove paste --name $cohort results-genotyped/*.vcf.gz
- (optional) annotate the variants with exons, UTRs that overlap from a GFF and annotate high-quality heterozygotes:
smoove annotate --gff Homo_sapiens.GRCh37.82.gff3.gz $cohort.smoove.square.vcf.gz | bgzip -c > $cohort.smoove.square.anno.vcf.gz
This adds a SHQ
(Smoove Het Quality) tag to every sample format) a value of 4 is a high quality call and the value of 1 is low quality. -1 is non-het.
It also adds a MSHQ
for Mean SHQ to the INFO field which is the mean SHQ score across all heterozygous samples for that variant.
As a first pass, users can look for variants with MSHQ > 3. If you added duphold annotations, it's also
useful to check deletions with DHFFC < 0.7
and duplications with DHFFC > 1.25
.
-
A panic with a message like
Segmentation fault (core dumped) | bcftools view -O z -c 1 -o
is likely to mean you have an old version of bcftools. see #10 -
smoove
will write to the system TMPDIR. For large cohorts, make sure to set this to something with a lot of space. e.g.export TMPDIR=/path/to/big
-
smoove
requires recent version oflumpy
andlumpy_filter
so build those from source or get the most recent bioconda version.