Rapid detection of structural variation in a human genome using nanochannel-based genome mapping technology

Hongzhi Cao; Alex R Hastie; Dandan Cao; Ernest T Lam; Yuhui Sun; Haodong Huang; Xiao Liu; Liya Lin; Warren Andrews; Saki Chan; Shujia Huang; Xin Tong; Michael Requa; Thomas Anantharaman; Anders Krogh; Huanming Yang; Han Cao; Xun Xu

doi:10.1186/2047-217X-3-34

Rapid detection of structural variation in a human genome using nanochannel-based genome mapping technology

Gigascience. 2014 Dec 30;3(1):34. doi: 10.1186/2047-217X-3-34. eCollection 2014.

Authors

Hongzhi Cao¹, Alex R Hastie², Dandan Cao³, Ernest T Lam², Yuhui Sun⁴, Haodong Huang⁴, Xiao Liu⁵, Liya Lin⁴, Warren Andrews², Saki Chan², Shujia Huang⁴, Xin Tong⁶, Michael Requa², Thomas Anantharaman², Anders Krogh⁷, Huanming Yang³, Han Cao², Xun Xu³

Affiliations

¹ BGI-Shenzhen, Shenzhen, 518083 China ; Shenzhen Key Laboratory of Transomics Biotechnologies, Shenzhen, 518083 China ; Department of Biology, University of Copenhagen, Copenhagen, 2200 Denmark.
² BioNano Genomics, San Diego, California 92121 USA.
³ BGI-Shenzhen, Shenzhen, 518083 China ; Shenzhen Key Laboratory of Transomics Biotechnologies, Shenzhen, 518083 China.
⁴ BGI-Shenzhen, Shenzhen, 518083 China ; School of Bioscience and Biotechnology, South China University of Technology, Guangzhou, 511400 China.
⁵ BGI-Shenzhen, Shenzhen, 518083 China ; Department of Biology, University of Copenhagen, Copenhagen, 2200 Denmark.
⁶ BGI-Shenzhen, Shenzhen, 518083 China.
⁷ Department of Biology, University of Copenhagen, Copenhagen, 2200 Denmark.

Abstract

Background: Structural variants (SVs) are less common than single nucleotide polymorphisms and indels in the population, but collectively account for a significant fraction of genetic polymorphism and diseases. Base pair differences arising from SVs are on a much higher order (>100 fold) than point mutations; however, none of the current detection methods are comprehensive, and currently available methodologies are incapable of providing sufficient resolution and unambiguous information across complex regions in the human genome. To address these challenges, we applied a high-throughput, cost-effective genome mapping technology to comprehensively discover genome-wide SVs and characterize complex regions of the YH genome using long single molecules (>150 kb) in a global fashion.

Results: Utilizing nanochannel-based genome mapping technology, we obtained 708 insertions/deletions and 17 inversions larger than 1 kb. Excluding the 59 SVs (54 insertions/deletions, 5 inversions) that overlap with N-base gaps in the reference assembly hg19, 666 non-gap SVs remained, and 396 of them (60%) were verified by paired-end data from whole-genome sequencing-based re-sequencing or de novo assembly sequence from fosmid data. Of the remaining 270 SVs, 260 are insertions and 213 overlap known SVs in the Database of Genomic Variants. Overall, 609 out of 666 (90%) variants were supported by experimental orthogonal methods or historical evidence in public databases. At the same time, genome mapping also provides valuable information for complex regions with haplotypes in a straightforward fashion. In addition, with long single-molecule labeling patterns, exogenous viral sequences were mapped on a whole-genome scale, and sample heterogeneity was analyzed at a new level.

Conclusion: Our study highlights genome mapping technology as a comprehensive and cost-effective method for detecting structural variation and studying complex regions in the human genome, as well as deciphering viral integration into the host genome.

Keywords: Epstein-Barr virus (EBV) integration; Genome mapping; Repeat units; Structural variation.