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Sample GSM679379 Query DataSets for GSM679379
Status Public on May 20, 2011
Title lung_adenocarcinoma_13
Sample type RNA
 
Channel 1
Source name Lung adenocarcinoma case ID 13
Organism Homo sapiens
Characteristics gender: Male
age: 85 y
tissue: Lung adenocarcinoma
disease: Lung adenocarcinoma
Extracted molecule total RNA
Extraction protocol Total RNA was isolated from blood collected and stored in PAXgene Blood RNA tubes using a PAXgene Blood RNA isolation kit at the University of Pennsylvania as per the protocol suggested by the manufacturer (Qiagen®, Valencia, CA, USA). The human universal reference RNA was made by pooling contents of FirstChoice total RNA panel that is made of RNA from different tissues of multiple individuals (Ambion®, Austin, TX, USA; catalog no. AM6000.
Label Hy3
Label protocol RNA was labeled by Exiqon®, Vedbaek, Denmark using the miRCURY LNA microRNA Power labeling kit. Five hundred ng of RNA, as quantified using Bioanalyzer (Agilent®, Santa Clara, CA, USA), was used per labeling reaction with the Hy3 dye. A human universal reference RNA, made by pooling contents of FirstChoice total RNA panel (Ambion®, Austin, TX, USA; catalog no. AM6000), was similarly labeled with the Hy5 dye. Synthetic small RNAs were spiked-in to the RNA samples before labeling as per the kit protocol.
 
Channel 2
Source name Human universal reference RNA from Ambion®
Organism Homo sapiens
Characteristics sample type: universal reference RNA was made by pooling contents of FirstChoice total RNA panel that is made of RNA from different tissues of multiple individuals, Ambion, Austin, TX, USA; catalog no. AM6000
gender: Mixed
Extracted molecule total RNA
Extraction protocol Total RNA was isolated from blood collected and stored in PAXgene Blood RNA tubes using a PAXgene Blood RNA isolation kit at the University of Pennsylvania as per the protocol suggested by the manufacturer (Qiagen®, Valencia, CA, USA). The human universal reference RNA was made by pooling contents of FirstChoice total RNA panel that is made of RNA from different tissues of multiple individuals (Ambion®, Austin, TX, USA; catalog no. AM6000.
Label Hy5
Label protocol RNA was labeled by Exiqon®, Vedbaek, Denmark using the miRCURY LNA microRNA Power labeling kit. Five hundred ng of RNA, as quantified using Bioanalyzer (Agilent®, Santa Clara, CA, USA), was used per labeling reaction with the Hy3 dye. A human universal reference RNA, made by pooling contents of FirstChoice total RNA panel (Ambion®, Austin, TX, USA; catalog no. AM6000), was similarly labeled with the Hy5 dye. Synthetic small RNAs were spiked-in to the RNA samples before labeling as per the kit protocol.
 
 
Hybridization protocol Hybridization of the mix of Hy3-labeled sample and Hy5-labeled reference RNAs to the arrays at 56 ºC for 16 hours followed by washing was performed by Exiqon® (Vedbaek, Denmark) on an HS Pro instrument (Tecan®, Männedorf, Switzerland). The 5th generation miRCURY LNA microRNA arrays (Exiqon®, Vedbaek,Denmark) that were used have approx. 1891 locked nucleic acid oligonucleotide probes on quadruplicate 105 µM-sized probe-spots to detect 74%, 72% and 68% of the 1223, 1055 and 680 human, mouse and rat microRNAs, respectively, of miRbase v.16.
Scan protocol Arrays were scanned, after hybridization and washing, using the G2505B scanning system (Agilent®, Santa Clara, CA, USA) by Exiqon® (Vedbaek, Denmark).
Description Hy3 and Hy5 are Cy3- and Cy5-like dyes, respectively.
Data processing Data processing was done in R (version 2.12.1) using the limma (version 3.4.5) Bioconductor package. The 'normexp' method with offset=10 was used for background-correction, and followed with within-array global 'loess' normalization, with span=1/3 and values from probe-spots with flag-values >1 ignored, and then, between-array 'Rquantile' normalization. For probe-set summarization, the median of the values from multiple spots was used when the ratio of the maximum and minimum values was > 1.5; else, the mean was used. The ratios of the summarized normalized Hy3/Hy5 (test/reference) signal-intensities were log2-transformed.
 
Submission date Feb 24, 2011
Last update date May 20, 2011
Contact name Santosh Kumar Patnaik
Phone 716-8458364
Organization name Roswell Park Comprehensive Cancer Center
Department Thoracic Surgery
Street address Elm and Carlton Streets
City Buffalo
State/province NY
ZIP/Postal code 14263
Country USA
 
Platform ID GPL11432
Series (1)
GSE27486 Whole blood microRNA expression profiles in human non-small cell lung adenocarcinoma

Data table header descriptions
ID_REF
VALUE log2-transformed ratio of summarized loess- and Rquantile-normalized Hy3/Hy5 (test/reference) signal-intensities

Data table
ID_REF VALUE
-1 -0.888765986
1100 0.938581093
4040 0.004816098
4390 1.081555668
4610 -1.590329824
4700 -1.799870769
5250 0.1212403
5730 -1.035640293
5740 -1.715532946
6880 0.126133776
9938 -0.238208316
10138 0.309536816
10306 0.057137392
10899 -0.470350935
10901 -0.139276493
10902 -0.379574003
10903 -0.342434346
10904 -1.030515335
10905 -0.410838682
10906 0.065044538

Total number of rows: 2026

Table truncated, full table size 36 Kbytes.




Supplementary file Size Download File type/resource
GSM679379_0_Exiqon_14223631_S01_Hy5.txt.gz 783.6 Kb (ftp)(http) TXT
GSM679379_1_Exiqon_14223631_S01_Hy3.txt.gz 880.3 Kb (ftp)(http) TXT
Processed data included within Sample table

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