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Sample GSM351854 Query DataSets for GSM351854
Status Public on Dec 11, 2009
Title Osmostress._4
Sample type RNA
 
Source name Before Lysis the cells were in contact with 0.5M NaCl for 20 min.
Organism Mycoplasmoides pneumoniae M129
Characteristics Strain M129
whole organism
Growth protocol Bacterial Strains and culture conditions: Mycoplasma pneumoniae is grown in 150 cm2 tissue culture flasks with 50mL of modified Hayflick medium with the following composition. The basic medium consisted of 18.4g of PPLO broth, 29.8g of HEPES,10 g glucose, 5mL of 0.5% phenol red, and 35mL of 2N NaOH per liter. Horse serum and penicillin were included to a final concentration of 20% and 100 U/mL, respectively.
Extracted molecule total RNA
Extraction protocol After growth , surface-attached cells are washed once with phosphate-buffered saline (PBS; 0.15M NaCl, 10mM sodium phosphate, pH 7.4) and immediately lysed in the cultivation flask by adding RLT buffer from the QiagenTM RNeasy Plus Mini Kit (Cat. Num. 74134). This isolation method is used for RNA extraction as it removes most RNAs smaller than 200 bases, thus preventing the synthesis of cDNA from tRNA. For cell lysis, 2mL of RLT buffer in presence of 20μL β-mercaptoethanol was used per cultivation flask. The purification is done according the manufacturers protocol.
Label Cy5
Label protocol 9μg of total RNA were used so as to carry out the reverse transcription using SuperScriptTM Indirect cDNA Labeling System from Invitrogen. This kit was used according manufacturer indication but two modifications were introduced in the protocol. Reverse transcription was carried out at 37ºC instead of 46ºC and the set of random hexamers (2uL of 2.5ug/uL) was used instead of polyT 20mers.
 
Hybridization protocol Hybridization and Scanning (Axon GenePix 4000) has been carried out in the Genomic Core Facility of EMBL-Heidelberg.
Scan protocol Hybridization and Scanning (Axon GenePix 4000) has been carried out in the Genomic Core Facility of EMBL-Heidelberg.
Description 2007-03-22_MP-59_0635.gpr
Data processing After background subtraction quantile (Boltad 2003) normalization was done using the bioconductor package marray (Yang 2005)
 
Submission date Dec 17, 2008
Last update date Dec 17, 2008
Contact name Marc Güell
E-mail(s) [email protected]
Organization name Centre for Genomic Regulation
Department Systems Biology
Lab Design of Biological Systems
Street address C/ Dr.Aiguader 88
City Barcelona
ZIP/Postal code 08003
Country Spain
 
Platform ID GPL7822
Series (2)
GSE14015 Mycoplasma pneumoniae expression profiling
GSE14019 Transcriptome/Expression analysis in Mycoplasma pneumoniae

Data table header descriptions
ID_REF
VALUE log2 transformed quantile normalized intensities

Data table
ID_REF VALUE
MPN001|dnaN(+) 12.42272079
MPN002|xdj1(+) 10.71838767
MPN003|gyrB(+) 12.2171512
MPN004|gyrA(+) 10.45266515
MPN005|serS(+) 10.10803905
MPN006|-(+) 9.660613616
MPN007|holB(+) 10.33952948
MPN008|trmE(+) 7.387979084
MPN009|yabD(+) 6.033316342
MPN010|-(+)
MPN011|-(-) 9.069198317
MPN012|-(-) 10.04123143
MPN013|-(+) 13.13682721
MPN014|dnaE(+) 11.34885448
MPN015|-(-) 10.27001699
MPN016|rimK(-) 7.284765037
MPN017|mtd1(-) 7.673888761
MPN018|pmd1(+) 10.72570315
MPN019|msbA(+) 10.50757239
MPN020|yb95(+) 11.35585289

Total number of rows: 688

Table truncated, full table size 17 Kbytes.




Supplementary file Size Download File type/resource
GSM351854.gpr.gz 158.0 Kb (ftp)(http) GPR
Processed data included within Sample table

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