GSM2492113: sIEC1 mRNA; Gasterosteus aculeatus; RNA-Seq - SRA

SRX2564542: GSM2492113: sIEC1 mRNA; Gasterosteus aculeatus; RNA-Seq
1 ILLUMINA (Illumina HiSeq 2000) run: 106.3M spots, 10.6G bases, 6Gb downloads

Submitted by: NCBI (GEO)

Study: Genomic dissection of conserved transcriptional regulation in intestinal epithelial cells [Stickleback]

PRJNA374873 • SRP099849 • All experiments • All runs

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We profiled genome-wide accesssible chromatin data and RNA-seq from four species (zebrafish, stickleback, mouse, and human) to identify commonly regulated genes and regulatory metods in intestinal epithelial cells (IECs). We identify a group genes that are commonly expressed in IECs and genes that are commonly expressed along the length of the intestine in fish and mammals. Using accessible chromatin data we identified enriched transcription factor binding site motifs In IECs and sites that are commonly accessible in IECs in all species. Finally, we confirm the ability for these regions from multiple species to drive conserved expression in IECs using a zebrafish reporter assay. Overall design: Examination of expression levels and chromatin accessibility in intestinal epithelaial cells in stickleback

Sample: sIEC1 mRNA

SAMN06339225 • SRS1981202 • All experiments • All runs

Organism: Gasterosteus aculeatus

Library:

Instrument: Illumina HiSeq 2000

Strategy: RNA-Seq

Source: TRANSCRIPTOMIC

Selection: cDNA

Layout: PAIRED

Construction protocol: To isolate stickleback IECs, intestines were dissected, splayed, and washed extensively with ice-cold 1x PBS with care taken to remove as much intestine associated fascia, adipocytes, and blood vessels as possible. Three washed intestines were transferred into dissociation reagent 1 (DR1; 30 mM EDTA, 1.5 mM DTT, 0.5x Complete protease inhibitors (Roche), in 1x PBS) for 15 minutes on ice. Segments were transferred to Dissociation Reagent 2 (DR2; 30 mM EDTA, 0.5x Complete protease inhibitors (Roche), in PBS) and moderately shaken by hand for 5 minutes until most epithelial cells were isolated in the suspension. Intestinal lamina propria was removed and 8 ml of cold 1x PBS was added to the cells on ice. Cells were pelleted at 500 x G at 4°C, washed once with 13 ml of cold 1X PBS, and re-suspended in 0.5 ml cold 1x PBS. A 0.4 ml fraction was used for FAIRE, and 0.1 ml fraction was reserved for RNA extraction. Isolated IECs were placed in TRIzol Reagent for RNA extraction.freshly isolated intestinal epithelial cells were directly fixed for 5-10 minutes in 10 ml of 1-3% w/v Formaldehyde solution (in 1x PBS) at room temperature and gentle rocking. Glycine (2.5M) was added to a final concentration of 125 mM to quench the formaldehyde. Cells were pelleted at 600 x G and washed three times in cold 1x PBS without dissociating the pellet. Fixed and washed cell pellets were flash frozen and stored at -80°C. Cells were lysed in 2 ml Lysis Buffer A (10 mMTris-HCl (pH8.0), 2% (vol/vol) Triton X-100, 1% SDS, 100 mM NaCl and 1 mM EDTA) and sonicated using a Branson Sonifier 450D equipped with a microtip for 6-13 cycles (1 second burst, 0.5 second pause, for 30 seconds/cycle at 70% intensity) allowing samples to cool on ice for 1 minute between cycles. RNA-seq: Total RNA was submitted and library construction was performed by Duke Sequencing and Genomic Technologies Shared Resources. FAIRE-seq: FAIRE-seq libraries were prepared using the TruSeq kit with 100ng of FAIRE DNA according to manufacturer's protocols and sequenced by UNC High Through-put Sequencing Core.

Experiment attributes:

GEO Accession: GSM2492113

Links:

NCBI link: NCBI Entrez (gds)

Runs: 1 run, 106.3M spots, 10.6G bases, 6Gb

Run	# of Spots	# of Bases	Size	Published
SRR5259811	106,326,278	10.6G	6Gb	2017-05-03

ID:: 3706934

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