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Sample GSM1722824 Query DataSets for GSM1722824
Status Public on Aug 08, 2015
Title LightMelanocytes_6h_KCM-_rep3
Sample type RNA
 
Source name LightMelanocytes_6h_KCM-_rep3
Organism Homo sapiens
Characteristics tissue: skin
cell type: epidermal keratinocytes
pigmentation level: light
media: KCM-
hours post irradiation: 6
Treatment protocol Keratinocyte supernatants were harvested from both non-irradiated (hereinafter KCM-) and irradiated keratinocytes (24 hours after treatment) (hereinafter KCM+) and kept frozen at -80ºC until use. Subconfluent melanocyte cultures were cultivated in Medium 254 supplemented with HMGS and KCM+ or KCM- Medium in a proportion 1:1. The following day they were irradiated with 75 mJ/cm2 of UVB, and harvested at 6, 12 and 24 hours post irradiation. We used non-irradiated control cultures that were covered by aluminium foil during irradiation (Fig 1).
Growth protocol Human epidermal keratinocytes were cultured in EpiLife Medium supplemented with human keratinocyte growth supplement (HKGS). Human epidermal melanocytes were cultivated in Medium 254 supplemented with 1% human melanocyte growth supplement (HMGS). All the cell lines were maintained in an incubator under an atmosphere of 5% CO2 at 37ºC. Media were refreshed every two days.
Extracted molecule total RNA
Extraction protocol RNA extraction kit from Ambion
Label Cy3
Label protocol 100 ng RNA were labelled with the Low input Quick Amp Labeling kit, one color (Agilent)
 
Hybridization protocol The hybridization step was performed using SureHyb hybridization chamber (Agilent Technologies) and 600 ng of labeled cRNA samples, for 17 hours at 65ºC and 10,000 rpms in an hybridization oven. Microarrays were stabilized with ozone-barrier slide covers (Agilent).
Scan protocol Image processing of the microarrays was performed by using Agilent Feature Extraction software v10.7.3.1.
Data processing Raw data were processed with GeneSpring GX software v11.5.1 (Agilent). Feature extraction flags were transformed as follows: if feature was not positive and significant, not uniform, not well above background or was a population outlier: compromised; if feature was saturated: not detected. our data were subjected to a DDHF (Data-Driven Haar-Fisz) transformation for variance stabilization with the R package DDHFm (Motakis et al, 2006). Data were transformed to log base 2 and normalized following the quantile method (Bolstad et al, 2003). Flag spot information in data files was used to filter probe sets. Entities in which more than 50% of samples in 1 out of any 7 conditions (0h, 6h KCM-, 12h KCM-, 24h KCM, 6h KCM+, 12h KCM+ and 24h KCM+) had “detected” flags were maintained for the analysis.
 
Submission date Jun 25, 2015
Last update date Aug 09, 2015
Contact name Saioa Lopez
E-mail(s) [email protected]
Organization name UCL
Street address Gower Street
City London
ZIP/Postal code WC1E 6BT
Country United Kingdom
 
Platform ID GPL14550
Series (1)
GSE70280 Comparison of the Transcriptional Profiles of Melanocytes from Dark and Light Skinned Individuals under Basal Conditions and Following Ultraviolet-B Irradiation

Data table header descriptions
ID_REF
VALUE Normalized signal after variance stabilization

Data table
ID_REF VALUE
A_19_P00315452 11.04982217
A_19_P00315459 11.04610966
A_19_P00315482 11.04601047
A_19_P00315504 11.0435959
A_19_P00315506 11.04323021
A_19_P00315523 11.05081503
A_19_P00315526 11.04885187
A_19_P00315527 11.04762719
A_19_P00315529 11.04414978
A_19_P00315532 11.04565201
A_19_P00315533 11.04452418
A_19_P00315538 11.04411695
A_19_P00315543 11.04502788
A_19_P00315550 11.04963234
A_19_P00315551 11.04777458
A_19_P00315554 11.04891078
A_19_P00315558 11.04450057
A_19_P00315560 11.04355697
A_19_P00315561 11.0432208
A_19_P00315571 11.04717863

Total number of rows: 26493

Table truncated, full table size 655 Kbytes.




Supplementary file Size Download File type/resource
GSM1722824_L_3.6C.txt.gz 3.1 Mb (ftp)(http) TXT
Processed data included within Sample table

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