Comparative Benchmarking of Optical Genome Mapping and Chromosomal Microarray Reveals High Technological Concordance in CNV Identification and Additional Structural Variant Refinement

Hayk Barseghyan; Andy Wing Chun Pang; Benjamin Clifford; Moises A Serrano; Alka Chaubey; Alex R Hastie

doi:10.3390/genes14101868

Comparative Benchmarking of Optical Genome Mapping and Chromosomal Microarray Reveals High Technological Concordance in CNV Identification and Additional Structural Variant Refinement

Genes (Basel). 2023 Sep 26;14(10):1868. doi: 10.3390/genes14101868.

Authors

Hayk Barseghyan^{1

2

3}, Andy Wing Chun Pang¹, Benjamin Clifford¹, Moises A Serrano⁴, Alka Chaubey¹, Alex R Hastie¹

Affiliations

¹ Bionano, San Diego, CA 92121, USA.
² Center for Genetic Medicine Research, Children's National Hospital, Washington, DC 20010, USA.
³ Genomics and Precision Medicine, School of Medicine and Health Sciences, George Washington University, Washington, DC 20037, USA.
⁴ Bionano Laboratories, Salt Lake City, UT 84109, USA.

Abstract

The recommended practice for individuals suspected of a genetic etiology for disorders including unexplained developmental delay/intellectual disability (DD/ID), autism spectrum disorders (ASD), and multiple congenital anomalies (MCA) involves a genetic testing workflow including chromosomal microarray (CMA), Fragile-X testing, karyotype analysis, and/or sequencing-based gene panels. Since genomic imbalances are often found to be causative, CMA is recommended as first tier testing for many indications. Optical genome mapping (OGM) is an emerging next generation cytogenomic technique that can detect not only copy number variants (CNVs), triploidy and absence of heterozygosity (AOH) like CMA, but can also define the location of duplications, and detect other structural variants (SVs), including balanced rearrangements and repeat expansions/contractions. This study compares OGM to CMA for clinically reported genomic variants, some of these samples also have structural characterization by fluorescence in situ hybridization (FISH). OGM was performed on IRB approved, de-identified specimens from 55 individuals with genomic abnormalities previously identified by CMA (61 clinically reported abnormalities). SVs identified by OGM were filtered by a control database to remove polymorphic variants and against an established gene list to prioritize clinically relevant findings before comparing with CMA and FISH results. OGM results showed 100% concordance with CMA findings for pathogenic variants and 98% concordant for all pathogenic/likely pathogenic/variants of uncertain significance (VUS), while also providing additional insight into the genomic structure of abnormalities that CMA was unable to provide. OGM demonstrates equivalent performance to CMA for CNV and AOH detection, enhanced by its ability to determine the structure of the genome. This work adds to an increasing body of evidence on the analytical validity and ability to detect clinically relevant abnormalities identified by CMA. Moreover, OGM identifies translocations, structures of duplications and complex CNVs intractable by CMA, yielding additional clinical utility.

Keywords: AOH; CMA; CNVs; OGM; SVs; Saphyr; absence of heterozygosity; aneuploidy; chromosomal microarray; optical genome mapping; triploidy.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Benchmarking*
Child
Chromosome Mapping
Developmental Disabilities* / diagnosis
Developmental Disabilities* / genetics
Humans
In Situ Hybridization, Fluorescence
Karyotype

Grants and funding

This study was funded in part by Bionano.