AI Article Synopsis

  • Tandem repeat (TR) variation is linked to gene expression and rare genetic diseases, and there's a demand for better tools to analyze these variations across genomes.
  • The Tandem Repeat Genotyping Tool (TRGT) is introduced as a computational method designed to determine consensus sequences and methylation levels of TRs using PacBio HiFi sequencing data.
  • TRGT demonstrated high accuracy with a 98.38% Mendelian concordance and successfully identified known repeat expansions and their methylation status in samples, while also providing access to a database of TR sequences and methylation levels from 100 genomes.

Article Abstract

Tandem repeat (TR) variation is associated with gene expression changes and numerous rare monogenic diseases. Although long-read sequencing provides accurate full-length sequences and methylation of TRs, there is still a need for computational methods to profile TRs across the genome. Here we introduce the Tandem Repeat Genotyping Tool (TRGT) and an accompanying TR database. TRGT determines the consensus sequences and methylation levels of specified TRs from PacBio HiFi sequencing data. It also reports reads that support each repeat allele. These reads can be subsequently visualized with a companion TR visualization tool. Assessing 937,122 TRs, TRGT showed a Mendelian concordance of 98.38%, allowing a single repeat unit difference. In six samples with known repeat expansions, TRGT detected all expansions while also identifying methylation signals and mosaicism and providing finer repeat length resolution than existing methods. Additionally, we released a database with allele sequences and methylation levels for 937,122 TRs across 100 genomes.

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Source
http://dx.doi.org/10.1038/s41587-023-02057-3DOI Listing

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