NCBI Logo
GEO Logo
   NCBI > GEO > Accession DisplayHelp Not logged in | LoginHelp
GEO help: Mouse over screen elements for information.
          Go
Sample GSM11152 Query DataSets for GSM11152
Status Public on Oct 15, 2003
Title ARPE-19 cells grown on Matrigel.1
Sample type RNA
 
Source name ARPE-19 cells
Organism Homo sapiens
Extracted molecule total RNA
 
Description I. Exp Design
1. Type of experiment: Comparison of native versus cultured RPE cells
2. Experimental factors: Native RPE versus ARPE-19 cells grown on different matrices
3. How many hybridizations in exp: 21
4. If a common reference used for all the hybs: no
5. Quality control steps: three independent arrays for each condition
6. Description: The expression profile of ARPE-19 cells grown on different matrices were compared to morphologically normal native macular RPE cells that were laser capture microdissected from 3 donors.

II. Samples used, extract prep, and labeling
1. Biosource: Human donor globes from NDRI (63, 71, 74 years old) and ARPE-19 cells.
2. Manipulations: Human donor globes were cryopreserved, and morphologically normal RPE cells from the macula were laser capture micodissected. ARPE-19 cells were grown on different matrices (plastic, Matrigel, collagen I, collagen IV, laminin, and fibronectin).
3. Extract preparation: Total RNA from cells were extracted with the RNeasy kit (Qiagen) using the manufacturer’s instructions.
4. Labeling protocol: Total RNA from cells was reverse transcribed with 33P-dCTP and 33P-dATP, and second strand cDNA was labeled with 33P-dCTP and 33P-dATP.
5. No external controls were added.

III. Hybridization procedures and parameters
1. Sample, array type, batch and serial # used
2. Hybridization protocol: Hybridization was carried out using the manufacturer’s recommendations. Arrays were prehybridized with Microhyb solution containing denatured Cot-1 DNA and poly dA at 42oC for two hours. Hybridization was carried out at 42oC overnight using a hybridization oven set at 8-10 rpm. Arrays were washed twice at 50oC for 20 minutes using 2x SSC, 1%SDS and once at room temperature for 15 minutes using 0.5x SSC, 1%SDS.
IV. Measurement data and specifications of data processing
1,2. Arrays were exposed to a phosphorimaging screen for 3 days and scanned at 50 mm resolution with a BioRad FX Pro-Plus phosphorimager. TIFF images from the phosphorimager were exported into ResGen Pathways 3 software for analysis.
3. Data processing: A gene was expressed if its background subtracted intensity was greater than 1.4 fold background. The data were normalized using a simple global scaling procedure, and Cluster/Treeview and Statistical Analysis of Microarrays (SAM version 1.12) programs were used for analysis.

Keywords = retinal pigment epithelium
Keywords = ARPE-19
Keywords = macula
Keywords = extracellular matrix
 
Submission date Oct 11, 2003
Last update date Oct 28, 2005
Contact name James T Handa
E-mail(s) jthanda@jhmi.edu
Phone 410 614-5481
Fax 410 614-5471
Organization name Johns Hopkins Medical Institutes
Department Wilmer Eye Institute
Lab Michael Panitch Macular Degeneration Laboratory
Street address 600 N. Wolfe St.
City Baltimore
State/province MD
ZIP/Postal code 21287
Country USA
 
Platform ID GPL538
Series (1)
GSE741 Native versus cultured retinal pigment epithelium cells

Data table header descriptions
ID_REF
Raw Signal raw total spot intensity
Bck background intensity
VALUE raw signal intensity minus background, multiplied by normalization coefficient

Data table
ID_REF Raw Signal Bck VALUE
1 0.068660102 8.859 0.063048786
2 0.330760757 8.859 0.303729003
3 0.439810482 8.859 0.403866531
4 0.064206163 8.859 0.05895885
5 0.078546373 8.859 0.072127092
6 0.063334181 8.859 0.058158132
7 0.064234882 8.859 0.058985222
8 0.070235009 8.859 0.064494982
9 0.172222582 8.859 0.158147519
10 0 8.859 0
11 5.408235058 8.859 4.96624164
12 0.054514784 8.859 0.050059509
13 0.147783309 8.859 0.13570557
14 0 8.859 0
15 0 8.859 0
16 0 8.859 0
17 0.217816316 8.859 0.20001506
18 0.069265979 8.859 0.063605148
19 0.230742076 8.859 0.211884449
20 0 8.859 0

Total number of rows: 4132

Table truncated, full table size 115 Kbytes.




Supplementary data files not provided

| NLM | NIH | GEO Help | Disclaimer | Accessibility |
NCBI Home NCBI Search NCBI SiteMap