NCBI Logo
GEO Logo
   NCBI > GEO > Accession DisplayHelp Not logged in | LoginHelp
GEO help: Mouse over screen elements for information.
          Go
Sample GSM3243100 Query DataSets for GSM3243100
Status Public on Dec 10, 2018
Title Ecoli_MG1655_T0_rep3
Sample type RNA
 
Source name Ecoli_MG1655_T0
Organism Escherichia coli str. K-12 substr. MG1655
Characteristics genotype/variation: wild type
sampling time point: before rifampicin addition
repetition: repetition 3
Treatment protocol Three hours after the stationary phase of growth was reached, samples were collected for transcriptomic analysis; this time point was also the reference time point (T0) for the half-life determination procedure. Subsequently, rifampicin (500 µg.mL-1) was added to inhibit the initiation of transcription, and cells were harvested at three different time points after this addition. Cultures were performed in triplicate. Samples were taken at either at 0’, 2’, 8’ and 15’, or 0’, 5’, 10’ and 18’ or 0’, 3’, 12’ and 30’ min after rifampicin addition. Samples were immediately frozen in liquid nitrogen upon collection.
Growth protocol The laboratory strain E. coli K12 MG1655 and two mutant strains E. coli MG1655(Δrnr) and E. coli MG1655(Δpnp) were grown in baffled flasks in LB medium at 37 °C and 180 rpm. Initial pH was set to 7. All cultures were inoculated at OD 0.1 from overnight pre-cultures performed in similar conditions. Biomass was estimated from absorbance at 600 nm. Cultures were performed in triplicate.
Extracted molecule total RNA
Extraction protocol After thawing and centrifugation steps, total RNA was extracted with TRIZOL® Reagent (Ambion) according to the manufacturer’s instructions. DNA contamination was eliminated with Turbo DNase kit (Ambion). Total RNA concentration and integrity were measured using a Nanodrop® spectrophotometer and Agilent BioAnalyzer, respectively. Total RNA extraction profiles were checked to be similar for all the three tested strains.
Label Cy3
Label protocol According to manufacturer instructions, 1 µg of cDNA was labeled using one color DNA labeling kit
 
Hybridization protocol According to manufacturer instructions, 2 µg of labeled cDNA were hybridized onto E. coli K-12 gene expression arrays (Nimblegen, Roche) during 17 h at 42 °C.
Scan protocol Arrays were later washed and scanned using MS200 Microarray Scanner (Nimblegen, Roche). Pictures were analyzed with DEVA 1.2.1 software.
Description the cells were in stationary phase, the sampling was performed just before rifampicin addition. It is the third of three biological replicates used in this experiment, each from separate cultures.
SAMPLE 9
Data processing Raw probe intensities ( .pair files three replicates for each strain before and after transcription arrest by rifampicin addition) were processed and analyzed with R computing environment using the affy and limma package of Bioconductor. Twelve arrays (three reference T0 samples, and nine time points after addition of rifampicin) were used. Only a normalization between arrays according to an invariant probeset intensities was performed. For each strain, a set of probes in the background for which the ranks were roughly invariant across all twelve arrays was selected. The median value of the invariant probe set intensities in each condition was used as a scaling factor for normalization between the three strains. After normalization, the intensity of a transcript was calculated by a RMA-summarization procedure [Irizarry et al, 2003, Biostatistics 4(2): 249-264] within each condition.
After normalization, in each array, transcript-specific intensity was computed as the median value of the 16 targeting probe intensities.
 
Submission date Jul 03, 2018
Last update date Dec 10, 2018
Contact name Laurence Girbal
E-mail(s) girbal@insa-toulouse.fr
Phone 33 5 61 55 97 24
Organization name TBI
Street address 135 avenue de rangueil
City Toulouse
ZIP/Postal code 31077
Country France
 
Platform ID GPL14649
Series (2)
GSE116576 Exoribonucleases coordinate degradation and expression of mRNAs in Escherichia coli at the stationary phase [stabilome]
GSE116652 Exoribonucleases coordinate degradation and expression of mRNAs in Escherichia coli at the stationary phase
Relations
Reanalyzed by GSM3243129

Data table header descriptions
ID_REF
VALUE processed

Data table
ID_REF VALUE
b0001071000000001 3.434966692
b0002071000000002 3.917487044
b0003071000000003 15.40437603
b0004071000000004 2.73700738
b0005071000000005 1.571691662
b0006071000000006 1.651934101
b0007071000000007 3.269457662
b0008071000000008 6.840727701
b0009071000000009 3.04041016
b0010071000000010 1.910417294
b0011071000000011 1.528680932
b0013071000000012 1.262503821
b0014071000000013 74.21037304
b0015071000000014 46.70122375
b0016071000000015 6.964447642
b0018071000000016 1.589348175
b0019071000000018 8.97547259
b0020071000000019 2.660970882
b0021071000000020 2.133105553
b0022071000000021 4.563690212

Total number of rows: 4254

Table truncated, full table size 124 Kbytes.




Supplementary file Size Download File type/resource
GSM3243100_Ecoli_MG1655_T0_rep3.pair.gz 1.1 Mb (ftp)(http) PAIR
Processed data included within Sample table

| NLM | NIH | GEO Help | Disclaimer | Accessibility |
NCBI Home NCBI Search NCBI SiteMap