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SRX16745140: GSM6422268: OS152, nuclei, m6dA methylated, rep6; Homo sapiens; OTHER
1 PACBIO_SMRT (Sequel II) run: 19.7M spots, 33.6G bases, 8Gb downloads

External Id: GSM6422268_r1
Submitted by: Ramani Lab, Gladstone Institute for Data Science & Biotechnology, Gladstone Institutes / UCSF
Study: Direct transposition of native DNA for sensitive multimodal single-molecule sequencing I
show Abstracthide Abstract
Concurrent readout of sequence and base modifications from long unamplified DNA templates by PacBio single-molecule sequencing requires large amounts of input material. Here we adapt Tn5 transposition to introduce hairpin oligonucleotides and fragment (tagment) limiting quantities of DNA for generating PacBio-compatible circular molecules. We developed two methods that implement tagmentation and use 90–99% less input than current protocols: (1) single-molecule real-time sequencing by tagmentation (SMRT-Tag), which allows detection of genetic variation and CpG methylation; and (2) single-molecule adenine-methylated oligonucleosome sequencing assay by tagmentation (SAMOSA-Tag), which uses exogenous adenine methylation to add a third channel for probing chromatin accessibility. SMRT-Tag of 40?ng or more human DNA (approximately 7,000 cell equivalents) yielded data comparable to gold standard whole-genome and bisulfite sequencing. SAMOSA-Tag of 30,000–50,000 nuclei resolved single-fiber chromatin structure, CTCF binding and DNA methylation in patient-derived prostate cancer xenografts and uncovered metastasis-associated global epigenome disorganization. Tagmentation thus promises to enable sensitive, scalable and multimodal single-molecule genomics for diverse basic and clinical applications. Overall design: Chromatin profiling with m6dA methyltransferase footprinting of the OS152 osteosarcoma cell line, followed by transposase-mediated PCR-free library construction in situ (SAMOSA-Tag) and single molecule sequencing.
Sample: OS152, nuclei, m6dA methylated, rep6
SAMN30072545 • SRS14372816 • All experiments • All runs
Organism: Homo sapiens
Library:
Name: GSM6422268
Instrument: Sequel II
Strategy: OTHER
Source: GENOMIC
Selection: other
Layout: SINGLE
Construction protocol: Tagmented nuclei were pre-treated with 10uL RNaseA at 37°C for 15 minutes, then purified with 2.5uL Proteinase K (20mg/mL), 2.5uL 10% SDS, and 2.5uL 0.5mM EDTA at 60°C for 1-2 hours with continuous shaking at 1000 rpm. DNA was extracted with 2x SPRI bead cleanup. Tagmented fragments were gap-repaired using Phusion DNA polymerase and Taq Ligase, or T4 DNA polymerase and Ampligase, at 37ºC for 1hr, digested with Exonuclease III at 37ºC for 1hr, then cleaned up using Ampure PB. Library quality was assessed with Qubit 1x High Sensitivity DNA Assay and Agilent Bioanalyzer High Sensitivity DNA kit.
Runs: 1 run, 19.7M spots, 33.6G bases, 8Gb
Run# of Spots# of BasesSizePublished
SRR2072468919,671,48333.6G8Gb2022-08-08

ID:
23499798

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