Whole Genome Analyses of Chinese Population and <i>De Novo</i> Assembly of A Northern Han Genome

Du, Zhenglin; Ma, Liang; Qu, Hongzhu; Chen, Wei; Zhang, Bing; Lü, Xi; Zhai, Weibo; Sheng, Xin; Sun, Yongqiao; Li, Wenjie; Meng, Lu; Qi, Qiuhui; Ni, Yuan; Shi, Shuo; Zeng, Jingyao; Wang, Jinyue; Yang, Yadong; Liu, Qi; Hong, Yaqiang; Dong, Lili; Zhang, Zhewen; Zou, Dong; Wang, Yanqing; Song, Shuhui; Liu, Fan; Fang, Xiangdong; Chen, Hua; Liu, Xin; Xiao, Jingfa; Zeng, Changqing

doi:10.1016/j.gpb.2019.07.002

Cited by 49 publications

(47 citation statements)

References 77 publications

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“…A FADS2 -promoter SNP (rs968567) enhancing FADS2 expression was discovered [120] . A whole genome analysis of the Chinese population showed rs28456 to be associated with AA [121] . ELOVL2 and ELOVL5 maternal genetic variants were associated with PUFA levels in breast milk [89] .…”

Section: Fads and Elovl Biochemical Functionsmentioning

confidence: 99%

Polyunsaturated fatty acid biosynthesis pathway and genetics. implications for interindividual variability in prothrombotic, inflammatory conditions such as COVID-19✰,✰✰,★,★★

Kothapalli¹,

Park²,

Brenna

2020

Prostaglandins, Leukotrienes and Essential Fatty Acids

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Section: Fads and Elovl Biochemical Functionsmentioning

confidence: 99%

Polyunsaturated fatty acid biosynthesis pathway and genetics. implications for interindividual variability in prothrombotic, inflammatory conditions such as COVID-19✰,✰✰,★,★★

Kothapalli¹,

Park²,

Brenna

2020

Prostaglandins, Leukotrienes and Essential Fatty Acids

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“…Furthermore, genotyping tests for the presence of a known variant, and does not reveal the spectrum of copy number variation that exists in tandem repeat sequences. An alternative use of LRS assemblies is for population-specific references that improve SRS read mapping by adding sequences missing from the reference (Du et al 2019;Shi et al 2016) . Because missing sequences are enriched for VNTRs (Audano et al 2019) , haplotype-resolved LRS genomes may help improve alignment to VNTR regions, as well as facilitate the development of a model to discover VNTR variation by serving as a ground truth.…”

Section: Introductionmentioning

confidence: 99%

Profiling variable-number tandem repeat variation across populations using repeat-pangenome graphs

Chaisson

2020

Preprint

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Variable number tandem repeats (VNTR) are genetic loci composed of consecutive repeats of short segments of DNA, with hypervariable repeat count and composition across individuals. Many genes have coding VNTR sequences, and noncoding VNTR variants are associated with a wide spectrum of clinical disorders such as Alzheimer's disease, bipolar disorder and colorectal cancer. The identification of VNTR length and composition provides the basis for downstream analysis such as expression quantitative trait loci discovery and genome wide association studies. Disease studies that use high-throughput short read sequencing do not resolve the repeat structures of many VNTR loci because the VNTR sequence is missing from the reference or is too repetitive to map. We solve the VNTR mapping problem for short reads by representing a collection of genomes with a repeat-pangenome graph, a data structure that encodes both the population diversity and repeat structure of VNTR loci. We developed software to build a repeat-pangenome using haplotype-resolved single-molecule sequencing assemblies, and to estimate VNTR length and sequence composition based on the alignment of short read sequences to the graph. Using long-read assemblies as ground truth, we are able to determine which VNTR loci may be accurately profiled using repeat-pangenome graph analysis with short reads. This enabled measuring the global diversity of VNTR sequences in the 1000-Genomes Project, and the discovery of expression quantitative trait loci in the Genotype-Tissue Expression Project. This analysis reveals loci that have significant differences in length and repeat composition between continental populations. Furthermore, the repeat pangenome graph analysis establishes an association between previously inaccessible variation and gene expression. Taken together, these indicate that measuring VNTR sequence diversity with repeat-pangenome graphs will be a critical component of future studies on human diversity and disease.

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“…As a result of using longer reads, the assembly result is better than the 30× dataset assembly obtained using the nanopore sequencing platform by Jain et al (2018), which comprised 2886 contigs with an N50 contig size of 3 Mb. Summary statistics for the sequencing and assembly of five reference genomes, including three existing individual Chinese reference genomes (Wang et al 2008;Shi et al 2016;Du et al 2019), were listed in Table 1. We aligned the assembled contigs to the GRCh38 reference, and then created chromosomes plot illustrating the contiguity of the nanopore assembly (the Cytogenetic band is background on the right, Fig.…”

Section: De Novo Assembly Of Nanopore Readsmentioning

confidence: 99%

De novo genome assembly of a Han Chinese male and genome-wide detection of structural variants using Oxford Nanopore sequencing

et al. 2020

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Advances in third-generation sequencing technologies provide an opportunity to investigate the complex organizational structure of the genome and unravel the genetic mechanisms of disease and physiological traits. Here we report the sequencing and de novo assembly of a healthy male northern Han Chinese genome and detection of structural variants using only nanopore sequencing data. We performed de novo assembly after filtering the raw data. Then, we aligned the assembled contigs to the human reference genome, and visualized chromosomes plot, which illustrated the contiguity of the nanopore assembly. Additionally, genomic structural variants were detected using a structure variation detection tool with long-read sequencing data. Median coverage depth was 30-fold and the read N50 was 27,136 bp. 96.51% of reads had at least one alignment to the human reference genome. The final assembled genome was 2.85 GB in size, with an N50 contig size of 5.4 MB. We identified 20,085 structural variants. Third-generation sequencing technologies have many advantages in de novo whole-genome assembly and detection of structural variants. Our results provide reference data for disease research, and can be used as a novel population-specific dataset of structural variants to support the efficient development of personalized precision medicine.

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Whole Genome Analyses of Chinese Population and De Novo Assembly of A Northern Han Genome

Cited by 49 publications

References 77 publications

Polyunsaturated fatty acid biosynthesis pathway and genetics. implications for interindividual variability in prothrombotic, inflammatory conditions such as COVID-19✰,✰✰,★,★★

Polyunsaturated fatty acid biosynthesis pathway and genetics. implications for interindividual variability in prothrombotic, inflammatory conditions such as COVID-19✰,✰✰,★,★★

Profiling variable-number tandem repeat variation across populations using repeat-pangenome graphs

De novo genome assembly of a Han Chinese male and genome-wide detection of structural variants using Oxford Nanopore sequencing

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