Description
This track shows allele statistics for 361,362 variable number tandem repeat (VNTR)
loci genotyped from Oxford Nanopore long-read whole-genome sequencing of 1,019 samples
from the
1000 Genomes
ONT Vienna project. VNTR genotyping was performed with
VAMOS,
a tool that determines the motif composition of VNTR alleles from long reads.
This is version 1.1 of the dataset.
Unlike the other STR tracks in this collection which are based on short-read sequencing
and limited to short tandem repeats (motifs of 1-6 bp), this track is derived from
long-read sequencing data, which can span much longer repeat regions. The VNTR loci
in this track have average motif lengths ranging from a few base pairs to over 100 bp,
and allele lengths up to several kilobases.
For each locus, the track shows the average repeat unit length, the number of unique
alleles observed, the range and median of repeat unit counts, and the range and median
of allele lengths in base pairs. The 1000 Genomes Vienna ONT project also produced
structural variant calls available in the
Long-Read Structural Variants track.
Display Conventions
Items are colored by expected heterozygosity, computed as
het = 1 − ∑pi2 from allele frequencies
across the 1,019 samples:
- Light gray – monomorphic (het = 0, single allele observed)
- Dark blue – nearly monomorphic (0 < het < 0.1)
- Medium blue – low diversity (het 0.1–0.3)
- Light purple – moderate diversity (het 0.3–0.5)
- Salmon – high diversity (het 0.5–0.7)
- Dark red – very high diversity (het ≥ 0.7)
- Medium gray – no allele frequency data available
Methods
The 1000 Genomes Vienna ONT project sequenced 1,019 samples from the 1000 Genomes
collection using Oxford Nanopore Technologies long-read sequencing. VNTR genotyping
was performed using
VAMOS,
which determines the motif composition of VNTR alleles by aligning long reads to
a catalog of known VNTR sites.
The analysis pipeline is available at
GitHub.
At UCSC, the summary statistics file (vamos-summary.tsv) was converted
to bigBed format using a
custom Python script.
Loci with coordinates exceeding chromosome boundaries were excluded.
Data Access
The raw data can be explored interactively with the
Table Browser or the
Data Integrator.
The data can be accessed from scripts through our
API, the track name is viennaVntr.
For automated download and analysis, the genome annotation is stored in a bigBed
file that can be downloaded from
our download server.
The file for this track is called viennaVntr.bb.
Individual regions or the whole genome annotation can be obtained using our tool
bigBedToBed, which can be compiled from the source code or downloaded as a
precompiled binary for your system. Instructions for downloading source code and
binaries can be found
here.
The tool can also be used to obtain features within a given range, e.g.
bigBedToBed http://hgdownload.soe.ucsc.edu/gbdb/hg38/strVar/viennaVntr.bb
-chrom=chr21 -start=0 -end=100000000 stdout
The original data (multisample VCF and summary statistics) can be downloaded from
the 1000 Genomes FTP server.
The VNTR site list used for genotyping is available from
Zenodo.
Credits
Thanks to the 1000 Genomes ONT Vienna consortium and the Marschall Lab at
Heinrich Heine University Düsseldorf for making this data publicly available.
References
De Coster W, Condon DE, De Baets G, Tsui A, Saeed F, Harerimana J, Amiraghdam F, Yaari R,
De Vos L, Mahfouz A et al.
Sequencing and variant calling of 1019 samples from the
1000 Genomes Project using Oxford Nanopore Technology.
bioRxiv. 2024 Dec 23;.