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ERX987748: MinION sequencing
1 OXFORD_NANOPORE (MinION) run: 2,535 spots, 20.3M bases, 14.5Mb downloads

Design: Other
Submitted by: Genome Institute of Singapore
Study: Sequencing of E. Coli UTI89 using Oxford Nanopore MinION
show Abstracthide Abstract
Genomic DNA was extracted from Escherichia coli UTI89 using the QIAamp® DNA mini kit (Qiagen). 1µg of the extracted DNA was then sheared in a total volume of 80µl using a Covaris g-TUBE according to the manufacturer’s instructions with centrifugation for 1min at 6000rpm. Sheared DNA was end repaired and A-tailed using the GeneRead™ DNA Library Prep I Kit from Qiagen according to the manufacturer’s protocol. The reaction was purified using 1X volume of Agencourt Ampure XP beads and eluted in 30µl nuclease-free water. Subsequent steps of DNA sequencing library preparation were carried out using Oxford Nanopore’s MinION Genomic DNA Sequencing Kit (SQK-MAP003) according to the manufacturer’s recommended protocol, including the addition of purified BSA (NEB) to Agencourt Ampure XP beads and Elution buffer. Immediately prior to sequencing, 12µl of the DNA library was combined with 134µl EP buffer and 4µl Fuel Mix and mixed by inversion 10 times. The flow cell was primed by washing with two aliquots of 150µl of EP buffer, with ten minutes in between washes. 150µl of the prepared DNA Library was then loaded onto the flow cell and the Genomic DNA 48 hour sequencing run program was selected. Fresh sample was loaded onto the flow cell at 12 hour intervals throughout the run.
Sample: UTI89-nanopore
SAMEA3447616 • ERS745225 • All experiments • All runs
Library:
Name: uti89
Instrument: MinION
Strategy: OTHER
Source: GENOMIC
Selection: unspecified
Layout: SINGLE
Construction protocol: Other
Runs: 1 run, 2,535 spots, 20.3M bases, 14.5Mb
Run# of Spots# of BasesSizePublished
ERR9084932,53520.3M14.5Mb2015-06-10

ID:
1530350

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