Resolving the Full Spectrum of Human Genome Variation using Linked-Reads

Marks, Patrick; Garcia, Sarah; Barrio, Álvaro Martínez; Belhocine, Kamila; Bernate, Jorge; Bharadwaj, Rajiv; Bjornson, Keith P.; Catalanotti, Claudia; Delaney, Josh; Fehr, Adrian; Galvin, Brendan D.; Heaton, Haynes; Herschleb, Jill; Hindson, Christopher M.; Holt, Esty; Jabara, Cassandra B.; Jett, Susanna; Keivanfar, Nikka; Kyriazopoulou-Panagiotopoulou, Sofia; Lek, Monkol; Lin, Bill K.; Lowe, Adam; Mahamdallie, Shazia; Maheshwari, Shamoni; Makarewicz, Tony; Marshall, Jamie L.; Meschi, Francesca; O'keefe, Chris; Ordonez, Heather; Patel, Pranav; Price, Andrew D.F.; Royall, Ariel; Ruark, Elise; Seal, Sheila; Schnall-Levin, Michael; Shah, Preyas; Williams, Stephen R.; Wu, Indira; Xu, Andrew Wei; Rahman, Nazneen; MacArthur, Daniel G.; Church, Deanna M.

doi:10.1101/230946

Cited by 90 publications

(158 citation statements)

References 43 publications

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“…The 10X Genomics linked-reads dataset was used to phase haplotypes as well as to identify, assemble, and phase primarily large (>30kb) SVs that include translocations (Spies et al 2017;Zheng et al 2016;Marks et al 2018). The 3kb-mate pair was used to validate the large SVs resolved from using the linked-read sequencing data and also to identify additional SVs, mostly in the medium size-range (1kb-100kb).…”

Section: Methods Overviewmentioning

confidence: 99%

“…SVs can also be assigned to specific haplotypes if the breakpoint-supporting reads contain phased SNVs or indels Marks et al 2018). Using this approach (implemented by the Long Ranger software from 10X Genomics), we identified 97 large SVs >30 kb (99% phased) (Dataset 3) and 3,473 deletions between 50 bp and 30 kb (78% phased) (Dataset 4).…”

Section: Using Linked-reads To Identify and Reconstruct Svsmentioning

confidence: 99%

“…We phased the heterozygous SNVs and indels in the HepG2 genome by performing 10X Genomics Chromium linked-read library preparation and sequencing Marks et al 2018). Post sequencing quality control analysis show that 1.49 ng or approximately 447 genomic equivalents of high molecular weight (HMW) genomic DNA fragments (mean=68 kb, 96.1% > 20 kb, 22.0% >100 kb) were partitioned .…”

Section: Resolving Haplotypesmentioning

confidence: 99%

“…Paired-end linked-reads (median insert size 396 bp, duplication rate 7.68%, Q30 Read1 78.7%, Q30 Read2 63.1%) were aligned to hg19 (alignment rate 90.4%, mean coverage 67.0x, zero coverage 0.117%) and analyzed using the Long Ranger Software (version 2.1.5) from 10x Genomics Marks et al 2018) (Pleasanton, CA, USA). Segmental duplications, reference gaps, unplaced contigs, regions with assembly issues, and highly polymorphic sites (http://cf.10xgenomics.com/supp/genome/hg19/sv_blacklist.bed, http://cf.10xgenomics.com/supp/genome/hg19/segdups.bedpe) were excluded from the analysis.…”

Section: Haplotype Phasing and Variant Calling Using 10x Genomics Linmentioning

confidence: 99%

“…HepG2 genomic DNA sample (~35 kb-80 kb) was size selected on the BluePippin instrument (Sage Science, Beverly, MA, USA) using the manufacturer's U1 Maker 30 kb High Pass protocol and then diluted to 1 ng/µl and used as input for the Chromium reagent delivery system Marks et al 2018) from 10x Genomics (Pleasanton, CA, USA) where HMW DNA fragments are partitioned into >1 million droplets, uniquely barcoded (16 bp) within each droplet, and subjected to random priming and isothermal amplification following standard manufacturer's protocol. Afterwards, the emulsion was broken, and the barcoded DNA molecules were released and converted to a Chromium linked-read library in which each library molecule retains its "HMW fragment barcode".…”

Section: X Genomics Linked-read Library and Sequencingmentioning

confidence: 99%

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Haplotype-resolved and integrated genome analysis of the cancer cell line HepG2

Zhou

Greer

Spies

et al. 2018

Preprint

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HepG2 is one of the most widely used human cell lines in biomedical research and one of the main cell lines of ENCODE. Although the functional genomic and epigenomic characteristics of HepG2 are extensively studied, its genome sequence has never been comprehensively analyzed and higher-order structural features of its genome beyond its karyotype were only cursorily known. The high degree of aneuploidy in HepG2 renders traditional genome variant analysis methods challenging and partially ineffective. Correct and complete interpretation of the extensive functional genomics data fromHepG2 requires an understanding of the cell line's genome sequence and genome structure. We performed deep whole-genome sequencing, mate-pair sequencing and linked-read sequencing to identify a wide spectrum of genome characteristics in HepG2: copy numbers of chromosomal segments, SNVs and Indels (both corrected for copynumber), phased haplotype blocks, structural variants (SVs) including complex genomic rearrangements, and novel mobile element insertions. A large number of SVs were phased, sequence assembled and experimentally validated. Several chromosomes show striking loss of heterozygosity. We re-analyzed HepG2 RNA-Seq and wholegenome bisulfite sequencing data for allele-specific expression and phased DNA methylation. We show examples where deeper insights into genomic regulatory complexity could be gained by taking knowledge of genomic structural contexts into account. Furthermore, we used the haplotype information to produce an allele-specific CRISPR targeting map. This comprehensive whole-genome analysis serves as a resource for future studies that utilize HepG2.

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Section: Methods Overviewmentioning

confidence: 99%

Section: Using Linked-reads To Identify and Reconstruct Svsmentioning

confidence: 99%

Section: Resolving Haplotypesmentioning

confidence: 99%

Section: Haplotype Phasing and Variant Calling Using 10x Genomics Linmentioning

confidence: 99%

Section: X Genomics Linked-read Library and Sequencingmentioning

confidence: 99%

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Haplotype-resolved and integrated genome analysis of the cancer cell line HepG2

Zhou

Greer

Spies

et al. 2018

Preprint

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Genome sequencing in cytogenetics: Comparison of short‐read and linked‐read approaches for germline structural variant detection and characterization

Uguen

Jubin

Duffourd

et al. 2020

Molec Gen & Gen Med

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Background Structural variants (SVs) include copy number variants (CNVs) and apparently balanced chromosomal rearrangements (ABCRs). Genome sequencing (GS) enables SV detection at base‐pair resolution, but the use of short‐read sequencing is limited by repetitive sequences, and long‐read approaches are not yet validated for diagnosis. Recently, 10X Genomics proposed Chromium, a technology providing linked‐reads to reconstruct long DNA fragments and which could represent a good alternative. No study has compared short‐read to linked‐read technologies to detect SVs in a constitutional diagnostic setting yet. The aim of this work was to determine whether the 10X Genomics technology enables better detection and comprehension of SVs than short‐read WGS. Methods We included 13 patients carrying various SVs. Whole genome analyses were performed using paired‐end HiSeq X sequencing with (linked‐read strategy) or without (short‐read strategy) Chromium library preparation. Two different bioinformatic pipelines were used: Variants are called using BreakDancer for short‐read strategy and LongRanger for long‐read strategy. Variant interpretations were first blinded. Results The short‐read strategy allowed diagnosis of known SV in 10/13 patients. After unblinding, the linked‐read strategy identified 10/13 SVs, including one (patient 7) missed by the short‐read strategy. Conclusion In conclusion, regarding the results of this study, 10X Genomics solution did not improve the detection and characterization of SV.

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Structural variants in the barley gene pool: precision and sensitivity to detect them using short-read sequencing and their association with gene expression and phenotypic variation

Weisweiler

Arlt

et al. 2022

Theor Appl Genet

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Key message Structural variants (SV) of 23 barley inbreds, detected by the best combination of SV callers based on short-read sequencing, were associated with genome-wide and gene-specific gene expression and, thus, were evaluated to predict agronomic traits. Abstract In human genetics, several studies have shown that phenotypic variation is more likely to be caused by structural variants (SV) than by single nucleotide variants. However, accurate while cost-efficient discovery of SV in complex genomes remains challenging. The objectives of our study were to (i) facilitate SV discovery studies by benchmarking SV callers and their combinations with respect to their sensitivity and precision to detect SV in the barley genome, (ii) characterize the occurrence and distribution of SV clusters in the genomes of 23 barley inbreds that are the parents of a unique resource for mapping quantitative traits, the double round robin population, (iii) quantify the association of SV clusters with transcript abundance, and (iv) evaluate the use of SV clusters for the prediction of phenotypic traits. In our computer simulations based on a sequencing coverage of 25x, a sensitivity > 70% and precision > 95% was observed for all combinations of SV types and SV length categories if the best combination of SV callers was used. We observed a significant (P < 0.05) association of gene-associated SV clusters with global gene-specific gene expression. Furthermore, about 9% of all SV clusters that were within 5 kb of a gene were significantly (P < 0.05) associated with the gene expression of the corresponding gene. The prediction ability of SV clusters was higher compared to that of single-nucleotide polymorphisms from an array across the seven studied phenotypic traits. These findings suggest the usefulness of exploiting SV information when fine mapping and cloning the causal genes underlying quantitative traits as well as the high potential of using SV clusters for the prediction of phenotypes in diverse germplasm sets.

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Resolving the Full Spectrum of Human Genome Variation using Linked-Reads

Cited by 90 publications

References 43 publications

Haplotype-resolved and integrated genome analysis of the cancer cell line HepG2

Haplotype-resolved and integrated genome analysis of the cancer cell line HepG2

Genome sequencing in cytogenetics: Comparison of short‐read and linked‐read approaches for germline structural variant detection and characterization

Structural variants in the barley gene pool: precision and sensitivity to detect them using short-read sequencing and their association with gene expression and phenotypic variation

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