Illumina HiSeq 2000 paired end sequencing; A study of transcriptome r... - SRA

ERX1437556: Illumina HiSeq 2000 paired end sequencing; A study of transcriptome response to salt treatment across three zones of the root in a barley landrace and malting cultivar
4 ILLUMINA (Illumina HiSeq 2000) runs: 28.8M spots, 5.8G bases, 3.8Gb downloads

Design: A study of transcriptome response to salt treatment across three zones of the root in a barley landrace and malting cultivar

Submitted by: MU (Murdoch University)

Study: A study of transcriptome response to salt treatment across three zones of the root in a barley landrace and malting cultivar

PRJEB13621 • ERP015182 • All experiments • All runs

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Paired-end RNA-Seq libraries were constructed for three root sections of the roots of barley cv. Clipper, and landrace Sahara, grown under control and salt-treated (100 mM NaCl) conditions on agar plates in quadruplicate. Experiments were conducted in a temperature-controlled growth cabinet at 17 °C in the dark. After three days of germination, seminal roots were dissected according to the following steps: A 1.5 mm long section marked ‘Zone 1’ (meristematic zone) was taken from the root tip. A second section (‘Zone 2’) was dissected from the elongation zone up to a third section, ‘Zone 3’ (maturation zone), which was excised at the point of visible root hair elongation up to 3/4 of the entire root. Four biological replicates were generated for each sample in four separate experiments totaling 48 samples. All RNA-seq libraries were constructed and paired-end sequenced (100 bp) on an Illumina HiSeq 2000 system at the Australian Genome Research Facility (Melbourne, Australia).

Sample: C100_Z3-4

SAMEA3935070 • ERS1122204 • All experiments • All runs

Organism: Hordeum vulgare

Library:

Name: C100_Z3-4

Instrument: Illumina HiSeq 2000

Strategy: RNA-Seq

Source: TRANSCRIPTOMIC

Selection: RANDOM

Layout: PAIRED

Construction protocol: Uniformly sized seeds were selected, surface-sterilised, and grown under control (nutrient medium without additional NaCl) and salt-treated (nutrient medium supplemented with 100 mM NaCl) conditions as described in (Shelden et al. 2013). After three days of germination, seminal roots were dissected, collected into 1.5 mL tubes, immediately snap-frozen in liquid nitrogen, and then stored at -80°C. Samples were dissected in the following steps: A 1.5 mm long section marked Zone 1 (meristematic zone) was taken from the root tip. The second section (Zone 2) was dissected from the elongation zone up to the third section, Zone 3 (maturation zone), which was excised at the point of visible root hair elongation up to 3/4 of the entire root. Total RNA was isolated from 50 mg root tissue using the Qiagen RNeasy kit following the manufacturer’s protocol. The RNA was analyzed for quality and concentration using a DeNovix DS-11 spectrophotometer (Wilmington, DE, USA) and an Agilent Technologies 2100 Bioanalyzer. Libraries were amplified through 13 cycles of PCR using Illumina guidelines. The Illumina TruSeq RNA Sample preparation kit v2 (Illumina Inc.) was used according to the manufacturer’s protocol. Poly(A) enrichment was used.

Spot descriptor:

1 forward101 reverse

Experiment attributes: (show all 4 attributes...) (hide...)

Experimental Factor: Clipper: genotype

Experimental Factor: NaCl: compound

Experimental Factor: 100: dose

Experimental Factor: Root maturation zone: organism part

Runs: 4 runs, 28.8M spots, 5.8G bases, 3.8Gb

Run	# of Spots	# of Bases	Size	Published
ERR1366355	7,215,942	1.4G	984.8Mb	2017-01-07
ERR1366356	7,141,814	1.4G	973.3Mb	2017-01-07
ERR1366357	7,274,602	1.5G	990.9Mb	2017-01-07
ERR1366358	7,121,652	1.4G	964.7Mb	2017-01-07

ID:: 3585482

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