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Sample GSM899817 Query DataSets for GSM899817
Status Public on Mar 23, 2012
Title EoE patient #5_after treatment [miRNA]
Sample type RNA
 
Source name EoE patient_after treatment
Organism Homo sapiens
Characteristics age range: Pediatric patient
clinical procedure: Biopsy
disease status: After glucocorticoid steroid treatment
tissue: epithelium
histology procedure: Formalin-fixed paraffin-embedded
Extracted molecule total RNA
Extraction protocol Tissue sections (10mm) were cut and mounted onto plain glass slides. If the biopsy section contained only epithelium, the sections were scraped from the slides and RNA was extracted using the RecoverAll Total Nucleic Acid Extraction kit for FFPE tissues (Ambion). If biopsy sections contained sub-epithelium, the sections were deparaffinized, stained, dehydrated through graded alcohols using the Paradise FFPE reagent System (Applied Biosystems, Foster City, CA) and subjected to LCM within 2 hr of deparaffinization. About 20000 epithelial cells were captured on LCM Macro CapSure caps (Applied Biosystems) using the Arcturus XT LCM instrument (Applied Biosystems). Total RNA was extracted from the caps also using the RecoverAll kit as above, and subjected to analysis by the Agilent Bioanalyzer using an RNA 6000 Nano or Pico LabChip (Agilent Technologies)
Label FAM
Label protocol Five nanograms of total RNA was reverse-transcribed using the Taqman MicroRNA Reverse Transcription Kit and the Megaplex RT primer Human Pool A (Applied Biosystems). The reverse-transcribed cDNA was then pre-amplified in 12 cycles of PCR using Taqman PreAmp Master Mix and the Megaplex PreAmp primers, Human Pool A (Applied Biosystems). The cDNA’s were then diluted and loaded on to a Taqman Human miRNA Array card A (Applied Biosystems), which contains probes for 377 distinct miRNAs. The Array cards were run on an ABI HT7900 qPCR instrument.
 
Hybridization protocol n/a
Scan protocol n/a
Description Fresh bipspies were fixed right away and porcessed within the same day.
EE-5A
Data processing The normalization and all the data analysis were performed according to the manufacturers instructions of ABI HT7900.
Original Ct values were normalized based on mammalian U6 as housekeeping gene control.
Target gene signals (delta Ct) normalized to housekeeping genes; delta Ct = (Ct_Target − Ct_HKG)
The folder change of each miRNA is calculated using 2^-delta delta Ct (before/after treatment ratios).
 
Submission date Mar 22, 2012
Last update date Mar 23, 2012
Contact name Shaolei Lu
E-mail(s) [email protected]
Phone 401-444-5709
Organization name Rhode Island Hospital
Department Pathology
Street address 593 Eddy Steet
City Providence
State/province Rhode Island
ZIP/Postal code 02903
Country USA
 
Platform ID GPL13328
Series (2)
GSE36726 miRNA Profiling in mucosal biopsies of Eosinophilic Esophagitis patients pre and post glucocorticoid steroid treatment
GSE36727 MicroRNA Profiling in Mucosal Biopsies of Eosinophilic Esophagitis Patients Pre and Post Glucocorticoid Steroid Treatment and Relationship with mRNA Target Expression

Data table header descriptions
ID_REF
VALUE normalized delta Ct (against housekeeping genes).

Data table
ID_REF VALUE
1.hsa-let-7a-4373169 null
2.hsa-let-7c-4373167 8.885867
3.hsa-let-7d-4395394 12.192279
4.hsa-let-7e-4395517 8.3559
5.hsa-let-7f-4373164 null
6.hsa-let-7g-4395393 11.279723
7.hsa-miR-1-4395333 null
8.hsa-miR-9-4373285 null
9.hsa-miR-10a-4373153 12.14556
10.hsa-miR-10b-4395329 null
11.MammU6-4395470 0.247113
12.MammU6-4395470 -0.07579
13.hsa-miR-15a-4373123 null
14.hsa-miR-15b-4373122 13.651639
15.hsa-miR-16-4373121 13.73895
16.hsa-miR-17-4395419 9.191533
17.hsa-miR-18a-4395533 18.561728
18.hsa-miR-18b-4395328 null
19.hsa-miR-19a-4373099 13.78865
20.hsa-miR-19b-4373098 9.941504

Total number of rows: 384

Table truncated, full table size 12 Kbytes.




Supplementary data files not provided
Processed data included within Sample table
Processed data are available on Series record

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