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Sample GSM552558 Query DataSets for GSM552558
Status Public on Jul 06, 2010
Title RNA2_v_gDNA
Sample type mixed
 
Channel 1
Source name Total_RNA_2
Organism Naumovozyma castellii
Characteristics strain: NRRL Y-12630
Treatment protocol 50 ml of the culture were transferred to a 50 ml conical and spun down immediately. The isolated cell pellets were then placed in liquid nitrogen, stored at -80°C, and were later archived in RNAlater for future RNA extraction.
Growth protocol Overnight cultures for each species were grown in 450ml of media at 220 RPM in a New Brunswick Scientific air-shaker at 30°C until reaching mid log-phase.
Extracted molecule total RNA
Extraction protocol Qiagen Yeast RNA extraction
Label Cy3
Label protocol Indirect total RNA labeling
 
Channel 2
Source name Genomic_DNA
Organism Naumovozyma castellii
Characteristics strain: NRRL Y-12630
Treatment protocol 50 ml of the culture were transferred to a 50 ml conical and spun down immediately. The isolated cell pellets were then placed in liquid nitrogen, stored at -80°C, and were later archived in RNAlater for future RNA extraction.
Growth protocol Overnight cultures for each species were grown in 450ml of media at 220 RPM in a New Brunswick Scientific air-shaker at 30°C until reaching mid log-phase.
Extracted molecule genomic DNA
Extraction protocol Genomic DNA was isolated using Genomic-tip 500/G (Qiagen) using the provided protocol for yeast. DNA samples were sheared using Covaris sonicator to 500-1000 bp fragments, as verified using DNA 7500 and DNA 12000 kit for the Bioanalyzer 2100 (Agilent).
Label Cy5
Label protocol Genomic DNA samples were labeled with Cy5 using a modification of the protocol developed by Joe Derisi (UCSF) and Rosetta Inpharmatics (Kirkland, WA) that can be obtained at www.microarrays.org.
 
 
Hybridization protocol Standard Agilent protocols for Agilent Custom Oligo Microarray 8x15K G4427A
Scan protocol Arrays were scanned using an Agilent scanner and analyzed with Agilent’s feature extraction software version 10.5.1.1.
Description 252035310009_200812171241_S01_GE2-v5_10_Apr08_1_2
Data processing For each probe, the median signal intensities were background subtracted for both channels and combined by taking the log2 of the Cy3 to Cy5 channel ratio. To estimate the absolute expression values for each gene, we took the median of the log2 ratios across all probes. The experiments were highly reproducible; most biological replicates correlated at R = 0.99 and replicates with R < 0.95 were removed.
 
Submission date Jun 08, 2010
Last update date Jun 10, 2010
Contact name Alex M Tsankov
E-mail(s) atsankov@mit.edu
Phone 6172532442
Fax 6172532442
Organization name MIT
Street address 155 Bay State
City Boston
State/province MA
ZIP/Postal code 02215
Country USA
 
Platform ID GPL10501
Series (2)
GSE21960 The role of nucleosome positioning in the evolution of gene regulation
GSE22200 Absolute expression level of Saccharomyces castellii genes

Data table header descriptions
ID_REF
VALUE Median log2 Cy3/Cy5 ratio values across the probe set

Data table
ID_REF VALUE
10001 -1.986936997
10002 -6.684218356
10003 -1.056710111
10004 -4.600270867
10005 0.216035767
10006 0.142019005
10007 -5.921087786
10008 -2.619453819
10009 -4.102156374
10010 -0.567728672
10011 -1.943901452
10012 -1.314056808
10013 -1.266392407
10014 -0.611007305
10015 0.277051821
10016 -0.034121076
10017 -1.590561771
10018 -2.455934916
10019 -2.069222807
10020 -2.927768291

Total number of rows: 5688

Table truncated, full table size 104 Kbytes.




Supplementary file Size Download File type/resource
GSM552558.txt.gz 3.4 Mb (ftp)(http) TXT
Processed data included within Sample table

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