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SRX15625061: Nanopore long read cDNA-PCR sequencing of recombinant 3' end
1 OXFORD_NANOPORE (MinION) run: 1.4M spots, 1.5G bases, 1.2Gb downloads

Design: Library prepared using total RNA extracted from U. maydis cells expressing a recombinant chimeric UmaTR construct. Total RNA was G/I tailed using the polyA length kit (USB). This was followed by reverse transcription using an oligo-dC reverse primer containing a 5' nanopore compatible adapter. cDNA was amplified using 1 round of nested PCR to enrich for recombinant UmaTR sequences. SQK-PCS109 PCR-cDNA library preparation kit instructions largely followed with above modifications. Subsequent steps followed according to kit. Raw reads prior to processing deposited in this entry
Submitted by: Arizona State University
Study: Identification of Ustilago maydis telomerase RNA (TR) and characterization of TR precursors
show Abstracthide Abstract
Ustilago maydis cells over-expressing 3xFLAG-UmaTERT (telomerase reverse transcriptase) lysed and immunoprecipitation (IP) performed with anti-FLAG antibodies to IP telomerase. Co-immunoprecipitated RNA extracted and subject to illumina next-generation sequencing (NGS) followed by computational screening of TR candidates from NGS data and experimental validation of top candidate. Nanopore long read sequencing libraries were generated using total RNA from wild type cells to characterize TR precursor transcripts or from recombinant Ustilago maydis cells expressing a mutated TR precursor to determine maturation mechanism of TR. For illumina library, Illumina Scriptseq v2 RNA-seq library preparation kit was used and sequenced on a Nextseq 500. For Nanopore long read libraries, PCR-cDNA sequencing kit (SQK-PCS109 - Oxford Nanopore Technologies) was used with additional nested PCR steps to enrich targets and sequenced on a minION device. All reads subject to adapter trimming and quality control using tools specific for each technology.
Sample: Nanopore-seq
SAMN28901656 • SRS13325187 • All experiments • All runs
Library:
Name: Recombinant_3'
Instrument: MinION
Strategy: RNA-Seq
Source: TRANSCRIPTOMIC
Selection: PCR
Layout: SINGLE
Runs: 1 run, 1.4M spots, 1.5G bases, 1.2Gb
Run# of Spots# of BasesSizePublished
SRR195730741,360,1791.5G1.2Gb2022-06-07

ID:
22238811

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