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Sample GSM1327321

Query DataSets for GSM1327321

Status

Public on May 15, 2015

Title

H1 shCtrl

Sample type

genomic

Source name

H1 ESCs

Organism

Homo sapiens

Characteristics

shRNA: stable control (scramble) shRNA

Treatment protocol

Pluripotent stem cells were differentiated as previously described (Kurian et al, 2012). Briefly, undifferentiated human ES/iPS cells were freshly split on to matrigel-coated plates, making sure the sub-colonies were of small size (~300-500 cells /colony). Cells were differentiated using the chemically defined mesodermal induction media (MIM) (DMEM:F12, 15mg/ml stem cell grade BSA (MP biomedicals), 17.5µg/ml Human Insulin, (SAFC bioscience), 275 µg/ml Human holo transferrin (Sigma Aldrich), 20ng/ml bFGF (Hymanzyme), 50ng/ml Human VEGF-165 aa (Humanzyme), 25ng/ml human BMP4 (Stemgent), 450µM monothioglycerol (Sigma Aldrich), 2.25mM each L-Glutamine and Nonn-essential amino acids (Invitrogen).

Growth protocol

Human ES cells, H1 (WA1, WiCell), (passage 25-40) were cultured in chemically defined hES/hiPS growth media, mTeSR on growth factor reduced matrigel (BD biosciences) coated plates. Briefly, 70-80% confluent hES/hiPS cells were treated with dispase (Invitrogen) for 7 minutes at 37¡C and the colonies were dispersed to small clusters and lifted carefully using a 5ml glass pipette, at a ratio of ~1:6. Human Umbilical Vein Endothelial Cells (HUVEC) were purchased from Promocell and cultivated in EBM medium supplemented with EGM singlequots (Lonza). iPS/ES-derived endothelial cells were cultivated in EGM-2 bullet kit (Lonza). All the endothelial cells were grown on collagen I coated plates (BD biosciences). All cell lines were maintained in an incubator (37¡C, 5% CO2) with media changes every day (hES/hiPS) or every second day (HUVEC).

Extracted molecule

genomic DNA

Extraction protocol

genomic DNA was extracted and purified from samples using Qiagen DNeasy Kit according to standard instructions

Label

Cy5 and Cy3

Label protocol

Standard Illumina Protocol

Hybridization protocol

bisulphite converted DNA was amplified, fragmented and hybridised to Illumina 450K Infinium Methylation Arrays using standard Illumina protocol

Scan protocol

Arrays were imaged using BeadArray Reader using standard recommended Illumina scanner setting

Description

H1 cells with stable control (scramble) shRNA

Data processing

Illumina GenomeStudio

Submission date

Feb 13, 2014

Last update date

May 15, 2015

Contact name

Christopher Benner

E-mail(s)

cbenner@ucsd.edu

Organization name

University of California, San Diego (UCSD)

Department

Medicine

Street address

9500 Gilman Dr. MC 0640

City

La Jolla

State/province

California

ZIP/Postal code

92093-0640

Country

USA

Platform ID

GPL13534

Series (2)

GSE54966	Transcriptomic analysis reveals novel long non-coding RNAs critical for vertebrate development [Illumina]
GSE54969	Transcriptomic analysis reveals novel long non-coding RNAs critical for vertebrate development

Data table header descriptions
ID_REF
VALUE	Average Beta
Detection Pval

Data table
ID_REF	VALUE	Detection Pval
cg00000029	0.50397	0
cg00000108	0.79752	0
cg00000109	0.67981	0
cg00000165	0.17244	0
cg00000236	0.64039	0
cg00000289	0.48941	0
cg00000292	0.71471	0
cg00000321	0.22416	0
cg00000363	0.10152	0
cg00000622	0.03578	0
cg00000658	0.61049	0
cg00000714	0.16569	0
cg00000721	0.70425	0
cg00000734	0.07704	0
cg00000769	0.10162	0
cg00000807	0.61094	0
cg00000884	0.57608	0
cg00000905	0.19466	0
cg00000924	0.41044	0
cg00000948	0.71031	0

Total number of rows: 485577

Table truncated, full table size 9912 Kbytes.

Supplementary data files not provided

Processed data included within Sample table