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Sample GSM263130

Query DataSets for GSM263130

Status

Public on May 01, 2008

Title

Rhodococcus jostii RHA1 desiccated at 20% relative humidity for 12 h, replicate 2

Sample type

RNA

Channel 1

Source name

mid-exponential phase, benzoate-grown Rhodococcus jostii RHA1 desiccated (20% RH) for 12 h

Organism

Rhodococcus jostii RHA1

Characteristics

mid-exponential phase, benzoate-grown Rhodococcus jostii RHA1 desiccated (20% RH) for 12 h

Growth protocol

Grown at 30°C and 200 rpm in W minimal medium amended with 20 mM sodium benzoate.

Extracted molecule

total RNA

Extraction protocol

Cell pellets were vortexed with glass beads, hot phenol, and SDS at final concentrations of 14.3% and 0.9% (vol/vol) respectively. Debris was precipitated with acetate followed by the addition of 4.0 mL phenol-chloroform (1:1, vol/vol). Nucleic acids were precipitated with acetate plus isopropanol, treated with DNase, and purified with an RNeasy mini column (Qiagen).

Label

Cy3

Label protocol

Cy-labelled cDNA was prepared by indirect labelling. For two of the three hybridizations, the Cy3/Cy5 dyes were reversed (i.e., cDNA from the T = 12 h treatment was labelled with Cy5 rather than Cy3) to control for dye bias.

Channel 2

Source name

mid-exponential phase, benzoate-grown Rhodococcus jostii RHA1 at time zero (just after filtration onto nitrocellulose membrane)

Organism

Rhodococcus jostii RHA1

Characteristics

mid-exponential phase, benzoate-grown Rhodococcus jostii RHA1 at time zero (just after filtration onto nitrocellulose membrane)

Growth protocol

Grown at 30°C and 200 rpm in W minimal medium amended with 20 mM sodium benzoate.

Extracted molecule

total RNA

Extraction protocol

Cell pellets were vortexed with glass beads, hot phenol, and SDS at final concentrations of 14.3% and 0.9% (vol/vol) respectively. Debris was precipitated with acetate followed by the addition of 4.0 mL phenol-chloroform (1:1, vol/vol). Nucleic acids were precipitated with acetate plus isopropanol, treated with DNase, and purified with an RNeasy mini column (Qiagen).

Label

Cy5

Label protocol

Cy-labelled cDNA was prepared by indirect labelling. For two of the three hybridizations, the Cy3/Cy5 dyes were reversed (i.e., cDNA from the T = 12 h treatment was labelled with Cy5 rather than Cy3) to control for dye bias.

Hybridization protocol

The microarray slides were pre-hybridized using 5X SSC containing 0.1% SDS and 0.2% BSA for 45 minutes at 48°C and used immediately for hybridization in a GeneTac HybStation (Genomic Solution). Equal amounts of differentially labelled cDNA – 50 million pixels as measured by ImageQuant 5.2 (Molecular Dynamics) – from T = 12 h and T = 0 cells were hybridized at 42°C for 17 h with agitation using 120 uL per slide of SlideHyb#1 hybridization solution (Ambion). The post-hybridization washing consisted of 3 cycles of 20 second incubations with each of the following solutions: 2X SSC plus 0.1% SDS (medium stringency) at 42°C; 0.1X SSC plus 0.05% SDS (high stringency) at 25°C; and 0.1X SSC (low stringency) at 25°C. Lastly, the slides were dipped in 0.2X SSC and dried by centrifugation at 225 x g for 5 min at room temperature.

Scan protocol

Microarray slides were scanned with a GenePix 4000B scanner (Axon Instruments) and spot intensities were quantified using Imagene 6.0 (BioDiscovery, Inc.).

Description

none

Data processing

Expression ratios were normalized using GeneSpring version 7.2 (Silicon Genetics) by the intensity-dependent Lowess method, with 20% of the data used for smoothing. Replicate spots of the same type were combined to yield a single normalized ratio, which is output for the first ID_REF number representing that spot type.

Submission date

Feb 06, 2008

Last update date

Apr 20, 2008

Contact name

Justin Christian LeBlanc

Phone

604-822-5646

Fax

604-822-6041

Organization name

University of British Columbia

Department

Microbiology & Immunology

Lab

Dr. William W. Mohn

Street address

2350 Health Sciences Mall

City

Vancouver

State/province

British Columbia

ZIP/Postal code

V6T 1Z3

Country

Canada

Platform ID

Series (1)

Desiccation and control transcriptomes of Rhodococcus jostii RHA1

Data table header descriptions
ID_REF
VALUE	Log2 normalized ratio of means defined as CH1 divided by CH2.
CH1_SIG_MEAN	Channel 1 mean signal intensity
CH1_BKD_MEAN	Channel 1 mean background intensity
CH2_SIG_MEAN	Channel 2 mean signal intensity
CH2_BKD_MEAN	Channel 2 mean background intensity

Data table
ID_REF	VALUE	CH1_SIG_MEAN	CH1_BKD_MEAN	CH2_SIG_MEAN	CH2_BKD_MEAN
1	-0.14829021	71.82608696	66.90378007	40.97101449	39.82474227
2	-1.872534598	77.85714286	64.18654434	60.39285714	40.79456193
3		74.68	63.81939799	61.32	40.41471572
4	1.605923238	70.04	63.2541806	42.08	39.97324415
5		67.32	61.83880597	41.6	39.30447761
6		72.32	63.48669202	43.4	39.22053232
7		65.76146789	61.19123506	40.46788991	39.34661355
8		66.15625	62.61398176	39.40625	39.37993921
9		66.9375	62.16129032	39	39.48387097
10		68.28125	63.13870968	40.75	38.92258065
11		69.76	62.51735016	40.76	39.33860759
12		65.48	62.19242902	40.68	39.69716088
13		66.51111111	61.72727273	41.86666667	40.32996633
14		68.81666667	63.04719764	41.31666667	40.58702065
15		73.72	63.54180602	43.4	40.44147157
16		70.8	64.97338403	47.13559322	40.25378788
17		69.3125	65.78448276	41.59375	39.52298851
18		72.36	65.51419558	40.64	39.14826498
19		67.68888889	63.61952862	39.62222222	39.51851852
20		69.08	62.74247492	40.24	39.5819398

Total number of rows: 22080

Table truncated, full table size 1195 Kbytes.

Supplementary data files not provided

Processed data included within Sample table

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