Ultralow-input single-tube linked-read library method enables short-read second-generation sequencing systems to routinely generate highly accurate and …

Z Chen, L Pham, TC Wu, G Mo, Y Xia… - Genome …, 2020 - genome.cshlp.org
Z Chen, L Pham, TC Wu, G Mo, Y Xia, PL Chang, D Porter, T Phan, H Che, H Tran, V Bansal
Genome research, 2020genome.cshlp.org
Long-range sequencing information is required for haplotype phasing, de novo assembly,
and structural variation detection. Current long-read sequencing technologies can provide
valuable long-range information but at a high cost with low accuracy and high DNA input
requirements. We have developed a single-tube Transposase Enzyme Linked Long-read
Sequencing (TELL-seq) technology, which enables a low-cost, high-accuracy, and high-
throughput short-read second-generation sequencer to generate over 100 kb of long-range …
Long-range sequencing information is required for haplotype phasing, de novo assembly, and structural variation detection. Current long-read sequencing technologies can provide valuable long-range information but at a high cost with low accuracy and high DNA input requirements. We have developed a single-tube Transposase Enzyme Linked Long-read Sequencing (TELL-seq) technology, which enables a low-cost, high-accuracy, and high-throughput short-read second-generation sequencer to generate over 100 kb of long-range sequencing information with as little as 0.1 ng input material. In a PCR tube, millions of clonally barcoded beads are used to uniquely barcode long DNA molecules in an open bulk reaction without dilution and compartmentation. The barcoded linked-reads are used to successfully assemble genomes ranging from microbes to human. These linked-reads also generate megabase-long phased blocks and provide a cost-effective tool for detecting structural variants in a genome, which are important to identify compound heterozygosity in recessive Mendelian diseases and discover genetic drivers and diagnostic biomarkers in cancers.
genome.cshlp.org
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