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Sample GSM189571 Query DataSets for GSM189571
Status Public on May 17, 2007
Title Fig 5A: YAC-2 (A17392) chem RNA
Sample type RNA
 
Channel 1
Source name F1 12/6/5 RNA
Organism Saccharomyces cerevisiae
Characteristics Strain Name : wt (A11311)
Biomaterial provider Maitreya Dunham, Dunham Lab, Princeton University
Extracted molecule total RNA
Extraction protocol Description : Filters were incubated for 1 hour at 65oC in lysis buffer (10 mM EDTA, 0.5% SDS, and 10 mM Tris, pH 7.5) and acid phenol. The aqueous phase was further extracted twice with an equal volume of chloroform using phase lock gel (Eppendorf). Total RNA was then ethanol precipitated and further purified over RNeasy columns (Qiagen). RNA quality was checked using the Bioanalyzer RNA Nano kit.
Label Cy3
Label protocol Description : 325 ng was used for microarray labeling with the Agilent Low RNA Input Fluorescent Linear Amplification Kit. Reactions were performed as directed except using half the recommended reaction volume and one quarter the recommended Cy-CTP amount. Dye incorporation and yield were measured with a Nanodrop spectrophotometer.
 
Channel 2
Source name F13 11/19/6 RNA
Organism Saccharomyces cerevisiae
Characteristics Strain Name : YAC-2 (A17392)
Biomaterial provider Maitreya Dunham, Dunham Lab, Princeton University
Growth protocol Description : ATR Sixfors fermenters were modified for use as chemostats. Chemostat cultures were run at 30oC at a working volume of 300 mls, mixed at 400 rpm, and sparged at 5 standard liters per minute with humidified and filter-sterilized air. The dilution rate was set to 0.17 volumes/hour. Cultures were run in phosphate limited minimal defined medium containing the following (per liter): 100 mg calcium chloride, 100 mg sodium chloride, 500 mg magnesium sulfate, 5 g ammonium sulfate, 1 g potassium chloride, 500 mg boric acid, 40 mg copper sulfate, 100 mg potassium iodide, 200 mg ferric chloride, 400 mg manganese sulfate, 200 mg sodium molybdate, 400 mg zinc sulfate, 1 mg biotin, 200 mg calcium pantothenate, 1 mg folic acid, 1 mg inositol, 200 mg niacin, 100 mg p-aminobenzoic acid, 200 mg pyridoxine, 100 mg riboflavin, 200 mg thiamine, 50 mg adenine, 50 mg tryptophan, 20 mg uracil, 100 mg lysine, 20 mg methionine, 100 mg leucine, 100 mg G418, and 5 g glucose. Chemostats were inoculated with 1 ml overnight culture grown in chemostat media. Cultures were maintained in batch for 24 hours, at which time the media flow was switched on. Cultures were sampled daily for cell density by Coulter count, klett, and absorbance, and were considered to be in steady state when all parameters measurements were the same for two consecutive measurements, which occurred 4 days after inoculation for all cultures. 100 ml of cultures were harvested by vacuum filtration, flash-frozen in liquid nitrogen, and stored at ?80oC until RNA extraction.
Extracted molecule total RNA
Extraction protocol Description : Filters were incubated for 1 hour at 65oC in lysis buffer (10 mM EDTA, 0.5% SDS, and 10 mM Tris, pH 7.5) and acid phenol. The aqueous phase was further extracted twice with an equal volume of chloroform using phase lock gel (Eppendorf). Total RNA was then ethanol precipitated and further purified over RNeasy columns (Qiagen). RNA quality was checked using the Bioanalyzer RNA Nano kit.
Label Cy5
Label protocol Description : 325 ng was used for microarray labeling with the Agilent Low RNA Input Fluorescent Linear Amplification Kit. Reactions were performed as directed except using half the recommended reaction volume and one quarter the recommended Cy-CTP amount. Dye incorporation and yield were measured with a Nanodrop spectrophotometer.
 
 
Hybridization protocol Description : Equal masses of differentially labeled control and sample cRNA were combined such that each sample contained at least 2.5 pmol dye. Samples were mixed with control targets, fragmented, combined with hybridization buffer, and applied to a microarray consisting of 60mer probes for each yeast open reading frame (Agilent). Microarrays were rotated at 60?C for 17 hours in a hybridization oven (Agilent). Arrays were then washed according to the Agilent SSPE wash protocol, and scanned on an Agilent scanner.
Scan protocol Pixel Size : 10
Scan Date : 2006-11-22
Scan Time : 13:31:44
Scanner Make : Agilent Technologies Scanner
Scanner Model : G2505B
Scanning software : ChipScan
Scanning software version : A.7.0.1
Description former name: YAC 11.1, AA YAC-2 (A17392) P-lim
Data processing Extraction Software : Agilent Feature Extractor
Extraction Software Version : A.7.5.1
Datafile type : Agilent result file
 
Submission date May 15, 2007
Last update date May 16, 2007
Contact name Maitreya J. Dunham
E-mail(s) maitreya@uw.edu
Phone 206-543-2338
Organization name University of Washington
Department Genome Sciences
Lab Dunham Lab
Street address Foege Building, S403B, Box 355065
City Seattle
State/province WA
ZIP/Postal code 98195-5065
Country USA
 
Platform ID GPL2883
Series (1)
GSE7812 Effects of aneuploidy on cellular physiology and cell division in haploid yeast.

Data table header descriptions
ID_REF Uniquely identifies feature/spot in array layout.
VALUE log(base 2) (R_PROCESSED_SIGNAL/G_PROCESSED_SIGNAL)
R_PROCESSED_SIGNAL The propagated feature signal in the red channel, used for computation of log ratio
G_PROCESSED_SIGNAL The propagated feature signal in the green channel, used for computation of log ratio
R_MEAN_SIGNAL Mean foreground intensity Ch 2.
G_MEAN_SIGNAL Mean foreground intensity Ch 1.

Data table
ID_REF VALUE R_PROCESSED_SIGNAL G_PROCESSED_SIGNAL R_MEAN_SIGNAL G_MEAN_SIGNAL
1 -6.644 232.4888 32181.01 53.64407 6607.136
2 0 22.96007 17.05567 24.90323 26.87097
3 -.6 1215.726 1842.279 171.1379 405.0172
4 -.392 361.0669 473.9429 68.58333 123.8333
5 .132 1301.899 1188.222 181.4138 270.431
6 .213 75.85571 65.43287 35.9 37.55
7 -.364 34.90011 44.92399 30.60345 33.55172
8 1.622 995.4571 323.4153 143.8727 92.72727
9 .174 1875.946 1662.54 250.9483 367.1379
10 .483 6579.313 4707.909 822.0175 984.7368
11 -.313 3690.766 4584.31 471.7091 961.3273
12 -.916 1957.412 3693.576 261.9273 781.0545
13 -.416 128.3526 171.2823 42.34426 58.83607
14 .328 14096.26 11228.76 1764.695 2270.034
15 1.469 93.36405 33.73612 38.68966 31.82759
16 .41 3256.412 2450.093 418.7667 526.6833
17 5.518 650.8865 14.20442 111.8814 27.94915
18 -.102 4702.176 5048.389 594.4259 1055.759
19 -.511 5933.66 8454.966 747.1356 1741.559
20 -.294 61.17484 75.02826 34.46552 39.75862

Total number of rows: 10789

Table truncated, full table size 478 Kbytes.




Supplementary file Size Download File type/resource
GSM189571.txt.gz 2.4 Mb (ftp)(http) TXT
Processed data included within Sample table

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