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Recurrent neural network for predicting absence of heterozygosity from low pass WGS with ultra-low depth. | LitMetric

AI Article Synopsis

  • The study introduces CNVseq-AOH, a new method that detects absence of heterozygosity (AOH) using ultra-low coverage whole genome sequencing (LP-WGS), which is lower than typical methods, by integrating population-based data and advanced algorithms like recurrent neural networks (RNN).
  • The CNVseq-AOH method demonstrated high accuracy in identifying AOH regions, achieving concordance rates of 96.23% for autosomes and discovering additional AOHs when tested on genomic data from 409 samples from the 1000 Genomes Project.
  • In clinical trials, CNVseq-AOH successfully identified all known AOH regions in six patients, showcasing its potential as a

Article Abstract

Background: The absence of heterozygosity (AOH) is a kind of genomic change characterized by a long contiguous region of homozygous alleles in a chromosome, which may cause human genetic disorders. However, no method of low-pass whole genome sequencing (LP-WGS) has been reported for the detection of AOH in a low-pass setting of less than onefold. We developed a method, termed CNVseq-AOH, for predicting the absence of heterozygosity using LP-WGS with ultra-low sequencing data, which overcomes the sparse nature of typical LP-WGS data by combing population-based haplotype information, adjustable sliding windows, and recurrent neural network (RNN). We tested the feasibility of CNVseq-AOH for the detection of AOH in 409 cases (11 AOH regions for model training and 863 AOH regions for validation) from the 1000 Genomes Project (1KGP). AOH detection using CNVseq-AOH was also performed on 6 clinical cases with previously ascertained AOHs by whole exome sequencing (WES).

Results: Using SNP-based microarray results as reference (AOHs detected by CNVseq-AOH with at least a 50% overlap with the AOHs detected by chromosomal microarray analysis), 409 samples (863 AOH regions) in the 1KGP were used for concordant analysis. For 784 AOHs on autosomes and 79 AOHs on the X chromosome, CNVseq-AOH can predict AOHs with a concordant rate of 96.23% and 59.49% respectively based on the analysis of 0.1-fold LP-WGS data, which is far lower than the current standard in the field. Using 0.1-fold LP-WGS data, CNVseq-AOH revealed 5 additional AOHs (larger than 10 Mb in size) in the 409 samples. We further analyzed AOHs larger than 10 Mb, which is recommended for reporting the possibility of UPD. For the 291 AOH regions larger than 10 Mb, CNVseq-AOH can predict AOHs with a concordant rate of 99.66% with only 0.1-fold LP-WGS data. In the 6 clinical cases, CNVseq-AOH revealed all 15 known AOH regions.

Conclusions: Here we reported a method for analyzing LP-WGS data to accurately identify regions of AOH, which possesses great potential to improve genetic testing of AOH.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11092001PMC
http://dx.doi.org/10.1186/s12864-024-10400-4DOI Listing

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