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Sample GSM1360854 Query DataSets for GSM1360854
Status Public on Apr 07, 2014
Title sputum_111
Sample type RNA
 
Source name sputum
Organism Homo sapiens
Characteristics cluster assignment: TEA_3
Treatment protocol Sputum cell pellets were processed using the All-in-One purification kit (Norgen Biotek, Thorhold, CAN), checked on an Agilent bioanalyzer and, if needed, treated again to remove DNA contamination (Qiagen, Gaithersberg, MD).
Growth protocol Sputum induction was performed with hypertonic saline, as previously described. Simply, by using a microscope, mucus plugs (cellular parts) from the sputum sample were dissected, separated and collected from aqueous compartments. Processing of the collected cellular part was done by mixing with 1 X Sputolysin Reagent (Calbiochem, cat# 560000) at a ratio of 1:4 (weight:volume), followed by vortexings at high speed for 30 seconds and low speed for 15 min, adding equal volume of PBS and a cell strainer filtration. Total cell count, viability, and differential, were determined by hemocytometer, trypan blue exclusion, and Wright-Geimsa stain, respectively. After centrifuged at 3,500 x g for 5 min, cell pellets were lysed in lysis solution of All-in-One Purification Kit (Product# 24200, Norgen Biotek Co, Thorhold, CAN) and stored at -80C until use.
Extracted molecule total RNA
Extraction protocol 10 ng of sputum RNA was amplified using the WT-Ovation Pico RNA amplification System (NuGen, San Carlos, CA) and processed per Affymetrix protocols. Total RNA from the blood was isolated using a column-based system (total-RNA kit, Norgen) and if needed, DNA contamination was removed using a DNA clear kit (Qiagen). Hemoglobin reduction of blood samples was used to remove hemoglobin gene transcripts (GLOBINclear Kit, Ambion, Austin, TX) and samples were checked by Agilent bioanalyzer.
Label biotin
Label protocol Purified RNA from the sputum or blood was processed for gene expression using the Affymetrix HuGene 1.0 ST gene arrays following manufacturer’s protocols.
 
Hybridization protocol See manufacturer's protocol
Scan protocol See manufacturer's protocol
Description Gene expression from sputum
Data processing RMA was used to background correct, quantile normalize and summarize the gene expression levels across all arrays. Blood and sputum arrays were processed separately. Principal component analysis (PCA) was used to visualize the data and remove outliers. The batch effect was adjusted using Combat and the RIN number was adjusted using linear regression model.
 
Submission date Apr 01, 2014
Last update date Apr 07, 2014
Contact name Geoffrey L. Chupp
E-mail(s) [email protected]
Organization name Section of Pulmonary, Critical Care and Sleep Medicine
Department Department of Internal Medicine
Street address 300 Cedar St, S441
City New Haven
ZIP/Postal code 06520
Country USA
 
Platform ID GPL6244
Series (1)
GSE56396 Non-invasive Analysis of the Airway Transcriptome Discriminates Clinical Phenotypes of Asthma

Data table header descriptions
ID_REF
VALUE Quantile normalized log2 intensity values that were adjusted for batch effect and RIN number

Data table
ID_REF VALUE
7896740 3.000774876
7896742 7.923205777
7896744 3.710611847
7896750 3.966656844
7896754 3.063806083
7896756 4.465616131
7896759 4.779442289
7896761 6.16473619
7896779 6.063568366
7896798 6.869665717
7896817 6.156858331
7896822 5.591678789
7896859 5.133896963
7896861 3.745025072
7896863 5.234113672
7896865 6.481028641
7896878 5.907066217
7896882 6.192244099
7896908 6.221478183
7896917 5.064808407

Total number of rows: 22148

Table truncated, full table size 430 Kbytes.




Supplementary file Size Download File type/resource
GSM1360854_SAMPLE_111.CEL.gz 4.0 Mb (ftp)(http) CEL
Processed data included within Sample table

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