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Sample GSM1527364 Query DataSets for GSM1527364
Status Public on Apr 05, 2015
Title AGM WSS-indo 6hrs rep2
Sample type RNA
 
Source name AGM WSS-indo 6hrs rep2
Organism Mus musculus
Characteristics strain: C57BL/6J
developmental stage: E10.5
tissue: AGM
duration of fluid flow: 6 hours
force: 5 dyne/cm^2
drug: indomethacin
Treatment protocol Microfluidics consisted of IBIDI VI^0.4 channel slides in line with a recirculating medium system driven by a single Harvard Apparatus PHD ULTRA 4400 with Remote syringe pump, 0.27 PSI crack pressure check valves (Qosina), and female luer lock three-way stop cocks (Qosina). After 6 to 8 hours of incubation, non-adherent cells were washed away and cells were cultured for 6 or 36 hours in static/low-flow conditions (0.0001 dyne/cm^2) or in the presence of WSS (5 dyne/cm^2).
Growth protocol Embryos from C57BL/6J timed pregnancies were microdissected for isolation of E10.5 AGM regions. Tissues were dissociated by treatment with Accutase (STEMCELL Technologies) at room temperature with gentle agitation for 20 minutes. Cells were resuspended in M5300 Myelocult medium (STEMCELL Technologies) enriched with HEPES (Invitrogen, 12.5 ml 1M HEPES/500 ml of Myelocult medium), non-Essential Amino Acids (Gibco), Sodium Pyruvate (Gibco), Penicillin 10 units/ml (Lonza) and Streptomycin 10 µg/ml (Lonza) without addition of hydrocortisone.
Extracted molecule total RNA
Extraction protocol Cells were directly lysed on microfluidic slides with RLT lysis buffer. Total RNA was immediately extracted with the QIAGEN RNeasy kit.
Label biotin
Label protocol Biotinylated cRNA were prepared with the Ambion MessageAmp kit for Illumina arrays
 
Hybridization protocol Standard Illumina hybridization protocol
Scan protocol Standard Illumina scanning protocol
Description -
Data processing Raw signals of all the build-in controls were checked as quality control for the performance of the arrays. Sample-independent controls were used to check: a. Hybridization (control molecules at low, medium and high concentrations); b. Signal generation (background, noise, biotin labeling and hybridization at high and low stringency). Housekeeping genes were used as sample-dependent controls. Background was subtracted and arrays were quantile normalized.
 
Submission date Oct 17, 2014
Last update date Apr 05, 2015
Contact name Pamela L Wenzel
Organization name University of Texas Health Science Center at Houston
Department Integrative Biology & Pharmacology
Lab Pamela Wenzel
Street address 6431 Fannin St, MSB 4.130
City Houston
State/province TX
ZIP/Postal code 77030
Country USA
 
Platform ID GPL17543
Series (1)
GSE62463 Effects of shear stress on cells of the aorta-gonad-mesonephros (AGM)

Data table header descriptions
ID_REF
VALUE All data processing, including quantile normalization and background correction, were performed using GenomeStudio software (Illumina, Inc.).
Detection Pval

Data table
ID_REF VALUE Detection Pval
ILMN_2417611 4.2 0.23932
ILMN_2762289 15.3 0.05556
ILMN_2896528 2288.8 0
ILMN_2721178 717.8 0
ILMN_2458837 -11.1 0.93269
ILMN_3033922 481.4 0
ILMN_3092673 2184.4 0
ILMN_1230777 1587.7 0
ILMN_1246069 2933.7 0
ILMN_1232042 -4.6 0.65491
ILMN_1243193 1186.3 0
ILMN_2524361 11.8 0.07906
ILMN_1242440 4.7 0.22543
ILMN_1233188 14.1 0.06197
ILMN_2543688 148.9 0
ILMN_1259789 58.6 0
ILMN_2816356 30.7 0.00855
ILMN_1224596 89.2 0
ILMN_1233643 33.3 0.00641
ILMN_2808939 929.8 0

Total number of rows: 45281

Table truncated, full table size 1060 Kbytes.




Supplementary file Size Download File type/resource
GSM1527364_9700842050_E_Grn.idat.gz 2.1 Mb (ftp)(http) IDAT
Processed data included within Sample table

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