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Sample GSM102383 Query DataSets for GSM102383
Status Public on Dec 30, 2007
Title B. fragilis IB397 O2-b
Sample type RNA
 
Source name IB397 wild type strain stressed in oxygen
Organism Bacteroides fragilis
Characteristics Total RNA obtained from mid-logarithmic phase Anaerobic culture of B. fragilis IB397
(wild-type) grown in BHIS complex media and then stressed by shaking aerobically for 30
min
Extracted molecule total RNA
Extraction protocol For each microarray, 3 to 5 µg of cDNA was fragmented using DNaseI and then labeled with biotin-N6-ddATP using terminal transferase. Labeled cDNA samples were individually hybridized to the microarray according to the NimbleGen standard operating procedure. The arrays were then washed and labeled with a streptavidin-Cy3 complex according to the NimbleGen procedure. The microoarrays then were scanned at 5-µm resolution using an Axon 4000B.
Label Cy3
Label protocol For each microarray, 3 to 5 µg of cDNA was fragmented using DNaseI and then labeled with biotin-N6-ddATP using terminal transferase. Labeled cDNA samples were individually hybridized to the microarray according to the NimbleGen standard operating procedure. The arrays were then washed and labeled with a streptavidin-Cy3 complex according to the NimbleGen procedure. The microoarrays then were scanned at 5-µm resolution using an Axon 4000B.
 
Hybridization protocol For each microarray, 3 to 5 µg of cDNA was fragmented using DNaseI and then labeled with biotin-N6-ddATP using terminal transferase. Labeled cDNA samples were individually hybridized to the microarray according to the NimbleGen standard operating procedure. The arrays were then washed and labeled with a streptavidin-Cy3 complex according to the NimbleGen procedure. The microoarrays then were scanned at 5-µm resolution using an Axon 4000B.
Scan protocol For each microarray, 3 to 5 µg of cDNA was fragmented using DNaseI and then labeled with biotin-N6-ddATP using terminal transferase. Labeled cDNA samples were individually hybridized to the microarray according to the NimbleGen standard operating procedure. The arrays were then washed and labeled with a streptavidin-Cy3 complex according to the NimbleGen procedure. The microoarrays then were scanned at 5-µm resolution using an Axon 4000B.
Description For each microarray, 3 to 5 µg of cDNA was fragmented using DNaseI and then labeled with biotin-N6-ddATP using terminal transferase. Labeled cDNA samples were individually hybridized to the microarray according to the NimbleGen standard operating procedure. The arrays were then washed and labeled with a streptavidin-Cy3 complex according to the NimbleGen procedure. The microoarrays then were scanned at 5-µm resolution using an Axon 4000B.
Data processing data processed using quantile normalization and RMA algorithm
 
Submission date Mar 30, 2006
Last update date Feb 26, 2007
Contact name Charles Jeffrey Smith
E-mail(s) smithcha@ecu.edu
Phone 252-744-2700
Fax 252-744-3104
Organization name East Carolina University
Department Microbiology & Immunology
Street address 600 Moye Blvd.
City Greenville
State/province NC
ZIP/Postal code 27834
Country USA
 
Platform ID GPL3596
Series (1)
GSE4583 Bacteroides fragilis oxidative stress

Data table header descriptions
ID_REF
VALUE normalized gene expression value from 18 probe pairs; perfect match-mismatch

Data table
ID_REF VALUE
BFRG000100000001 427.8279718
BFRG000100000002 162.0846883
BFRG000100000003 144.4661818
BFRG000100000004 112.418059
BFRG000100000005 956.5303933
BFRG000100000006 241.6955331
BFRG000100000007 98.42309644
BFRG000100000008 65.08616476
BFRG000100000009 35.4620246
BFRG000100000010 39.00012925
BFRG000100000011 490.6984826
BFRG000100000012 59.99145013
BFRG000100000013 926.9553256
BFRG000100000014 730.0578612
BFRG000100000015 129.938667
BFRG000100000016 61.67303758
BFRG000100000017 47.19669723
BFRG000100000018 127.710559
BFRG000100000019 4042.771644
BFRG000100000020 480.3539364

Total number of rows: 4272

Table truncated, full table size 120 Kbytes.




Supplementary data files not provided

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