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Sample GSM868401 Query DataSets for GSM868401
Status Public on Jan 01, 2015
Title Sample 45, replicate 3
Sample type RNA
 
Source name Sample 45, replicate 3
Organism Yarrowia lipolytica
Characteristics sampling time (h): 161.58
n/c ratio (moln / cmol): 0.0421
Treatment protocol Samples have been collected from the bioreactor directly through the sampling septum. For each time point, a volume equivalent to ca. 300 mg dry cell weight was harvested, frozen in liquid nitrogen, and further stored at -80°C until extraction.
Growth protocol Precultivations for chemostat were carried out on a 5-ml tube of YPD medium at 28 °C for 16 h at 100 rpm. The culture in growth phase was transferred into a 1-l Erlenmeyer flask containing 170 ml of mineral medium at pH 5.6 prepared as follows (all compounds are expressed in gl-1): (NH4)2SO4, 3.5; KH2PO4, 6; MgSO4, 2; EDTA, 0.0375; ZnSO4∙7H2O, 0.0281; MnCl2∙4H2O, 0.0025; CoCl2∙6H2O, 0.00075; CuSO4∙5H2O, 0.00075; Na2MoSO4∙2H2O, 0.00005; CaCl2∙2H2O, 0.0125; FeSO4∙7H2O, 0.00875; H3BO3, 0.0025; D-biotin, 0.00025; D-L-panthotenic acid, 0.001; nicotinic acid, 0.001; my0-inositol, 0.00625; thiamin, 0.001; pyridoxine, 0.001; para-aminobenzoic acid, 0.0002. Glucose was added to a final concentration of 18 gl-1 with chloramphenicol at 10 mgl-1. After 16 h of growth at 28°C and 100 rpm, 170 ml of the broth were used to inoculate 1.7 l of the same mineral medium in a 3-l bioreactor. Chemostat and D-Stat experiments were performed in a 3-l stirred tank bioreactor with a working volume of 1.5 l using the Biostat B. Braun Biotech International (Sartorius AG , Germany) with the acquisition software MFCS/win 2.0. The temperature was regulated at 28°C and the pH at 5.6 by the in-line addition of 5 M NaOH. The fermentation started in batch under full aerobic conditions. The Dissolved Oxygen was maintained above 20% of saturation by modulating the air flow rate or the stirring rate in order to avoid oxygen limitation. 11 h after inoculation, when the glucose was totally consumed, continuous cultivation was started. For chemostat cultivation, the bioreactor was continuously fed with the mineral medium (except (NH4)2SO4) supplemented with 23 gl-1 glucose at 0.108 lh-1. The bioreactor was fed with a second reservoir containing 60 gl-1 (NH4)2SO4 at 0.0117 lh-1 corresponding to a N/C ratio of 0.129 molN.Cmol-1. The working dilution rate was 0.08 h-1. When the steady state was reached after 5 residence times (ד= 1/D), the D-Stat was set up. The feeding rate of the mineral medium supplemented with glucose was maintained constant at 0.120 lh-1 while the (NH4)2SO4 feeding rate followed a linear and smooth decrease from 0.0117 lh-1 to 0.0003 lh-1 for 50 h (deceleration factor : 0.00015 h-2) corresponding to a decrease in the N/C ratio from 0.129 to 0.0028 molNCmol-1. All other parameters were maintained unchanged.
Extracted molecule total RNA
Extraction protocol Frozen samples were treated by mechanical disruption, using a bead beater (Microdismenbrator, Braun, Germany) and a tungsten bead (Ø ~ 7 mm), for 2 min at 2600 rpm. After disruption, the resulting cell powder was recovered and further processed for RNA purification using the RNEasy Midi Kit (Qiagen, The Netherlands), according to the manufacturer's instruction.
Label Cy3
Label protocol Samples were treated with the Low Input Quick Amp labelling kit (Agilent, USA), according to manufacturer's protocol.
 
Hybridization protocol Hybridization was performed according to Agilent's general protocol (http://www.chem.agilent.com/Library/usermanuals/Public/G4140-90040_GeneExpression_One-color_v6.5.pdf)
Scan protocol Scanning was performed using a INNOSCAN 900 Microarray Scanner (INNOPSYS, France). Images were further treated using Mapix v5.5.0 (Innopsys, France).
Description Sample 45, replicate 3
Data processing Raw transcriptomic data were filtered and normalized using the R software and the Limma package of the Bioconductor library. Local background estimates were corrected using the “normexp + offset” method, using an offset value of 10. A « scale » normalization method was applied to normalize background substracted data between arrays.
 
Submission date Jan 31, 2012
Last update date Jan 01, 2015
Contact name Nicolas Morin
E-mail(s) nmorin@grignon.inra.fr
Organization name INRA
Department UMR 1319 Micalis
Lab Biologie Intégrative du Métabolisme Lipidique Microbien
Street address Av. Lucien Bretignières
City Thiverval-Grignon
ZIP/Postal code F-78850
Country France
 
Platform ID GPL15177
Series (2)
GSE35445 Yarrowia lipolytica biolipid production during D-stat setup. [Part 1]
GSE35447 Yarrowia lipolytica biolipid production during D-stat setup.

Data table header descriptions
ID_REF
VALUE log2(fluorescence), based on background substracted, normalized data.

Data table
ID_REF VALUE
Cereb_01 5.03398948074697
Cereb_02 4.87114234851224
Cereb_03 5.14904885098317
HCHer_01 8.69735523946358
HCHer_02 5.46045649194271
HCHer_03 6.45843443725691
huEpo_01 5.81929447581042
huEpo_02 4.52661464278021
huGAA_01 4.94579651373308
huGAA_02 5.96101801072515
huGAA_03 6.76714819789526
huGM-CSF_01 5.65100345424379
huGM-CSF_02 4.70913866315205
huGM-CSF_03 5.32717036032097
huIDS_01 7.48584655825983
huIDS_02 6.99956562113853
huIDS_03 6.53901221527239
LCHER_01 6.99517809163307
LCHER_02 3.32679505732243
LCHER_03 6.0900561638548

Total number of rows: 14322

Table truncated, full table size 427 Kbytes.




Supplementary file Size Download File type/resource
GSM868401_45_r3.txt.gz 1.4 Mb (ftp)(http) TXT
Processed data included within Sample table

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