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Sample GSM21898 Query DataSets for GSM21898
Status Public on Apr 29, 2004
Title Matrigel induced differentiation of HBC-3 cells , time 5-B days
Sample type RNA
 
Channel 1
Source name HBC-3 cells after 5 day of differentiation
Organism Mus musculus
Extracted molecule total RNA
 
Channel 2
Source name HBC-3 cells control
Organism Mus musculus
Extracted molecule total RNA
 
 
Description HBC-3 cells were maintained as previously described (Rogler,L.E.,Am.J. Path. 150:591-602). Cells grown for microarray analysis were stripped of their STON+ feeder layer by trypsinization and replating on plastic in HBM
Undifferentiated cells were harvested the next A.M. for preparation of total RNA. Twenty 10cm plates were used to obtain sufficient quantities of undifferentiated reference total RNA. Total RNAs were prepared using Qiagen RNeasy maxi kit. The quality of each RNA preparation was determined using an Agilent 2100 Bioanalyzer. Five microgram aliquots of total RNA from undifferentiated HBC-3 cells were used to generate amplified RNA (aRNA) using the Ambion Message Amp Kit (cat.# 1750). The quality of the aRNA was determined using an Agilent Bioanalyzer. Amplified RNAs were stored as 5ug aliquots under 100% Ethanol at -80oC.
Cy 3 and Cy5 labeled targets were synthesized using a modified version of the AECOM functional Genomics facility protocol (http://microarray1k.aecom.yu.edu/) as previously described (Plescia et al, 2001,Differentiation 68:254-269). Cy3 and Cy5 labeled targets were prepared using 5 ug of aRNA using random primers and Superscript reverse transcriptase (Invitrogen)
Cy3 labeled target prepared from undifferentiated HBC-3 cells provided the reference sample for all comparisons. The precipitated targets were then resuspended in hybridization buffer as previously described and applied to a microarray. Arrays were hybridized at 50oC for 20 hours. Washing was carried out as described at (http://microarray1k.aecom.yu.edu/
Cy3 and Cy5 labeled targets were synthesized using a modified version of the AECOM functional Genomics facility protocol (http://microarray1k.aecom.yu.edu/) as previously described (Plescia et al, 2001,Differentiation 68:254-269). Cy3 and Cy5 labeled targets were prepared using 5 ug of aRNA using random primers and Superscript reverse transcriptase (Invitrogen).). The purified Cy5 labeled targets were repared from aRNA made from HBC-3 cells treated with Matrigel for 5 day (to induce bile duct differentiation).Cy3 reference target and a Cy5 target prepared from an RNA isolated from cells at one of the time points of Matrigel treatment were combined and precipitated. The precipitated targets were then resuspended in hybridization buffer as previously described and applied to a microarray. Arrays were hybridized at 50oC for 20 hours. Washing was carried out as described at (http://microarray1k.aecom.yu.edu/). "
In vitro bile ductular differentiation of HBC-3 cells was performed as previously described (Rogler,L.E.,Am.J. Path. 150:591-602) Cells grown for microarray analysis were stripped of their STON+ feeder layer by trypsinization and on a 1mm Matrigel cushion (differentiated). Cells undergoing Matrigel induced differentiation were harvested at 1 day of Matrigel treatment for preparation of total RNA. Ten 10 cm plates were harvested for each time point to obtain total RNA sufficient for several target preparations at each time point. Five microgram aliquots of total RNA from undifferentiated HBC-3 or Matrigel treated HBC-3 cells were used to generate amplified RNA (aRNA) using the Ambion Message Amp Kit (cat.# 1750). The quality of the aRNA was determined using an Agilent Bioanalyzer. Amplified RNAs were stored as 5ug aliquots under 100% Ethanol at -80oC.
Following hybridization and washing, the arrays were scanned for Cy3 and y5 florescence using a scanner Genepix 3.0 scanner (Axon Instruments Inc., Union City, CA). The signal intensity of a spot was considered to be significant if the signal intensity was greater by 200 units of the background for that spot and if it was not flagged as ""not found"" by GenePix software. These data were normalized using the Lowess implementation included in BASE. Following filtration and normalization, the ratio of red and green fluorescence, (RAT) was quantified for each qualified gene. The RAT values were then Log transformed and the LOG2 of the RAT is presented in the data table."
Keywords = HBC-3 cells, murine hepatoblast cells, matrigel
 
Submission date Apr 27, 2004
Last update date May 27, 2005
Contact name Leslie Rogler
E-mail(s) [email protected]
Phone 718 430 3651
Organization name Albert Einstein College of Medicine
Department Liver Research Center/ Department of Medicine
Street address 1300 Morris Park Ave
City New York
State/province NY
ZIP/Postal code 10461
Country USA
 
Platform ID GPL1205
Series (1)
GSE1348 HBC-3 matrigel differentiation

Data table header descriptions
ID_REF
VALUE Normalized log2 ratio of medians after background substraction
dia spot diameter
FCh1Median Channel 1 median intensity
BCh1Median Channel 1 median background intensity
FCh2Median Channel 2 median intensity
BCh2Median Channel 2 median background intensity

Data table
ID_REF VALUE dia FCh1Median BCh1Median FCh2Median BCh2Median
2 0.15244498 110 677 82 740 73
3 2.51746008 90 1252 81 351 73
4 0.4548072 120 1223 97 1144 76
5 -0.42342644 110 2529 91 3894 74
7 -0.01990867 120 1754 95 2108 75
8 -0.99102773 130 257 101 533 78
11 0.29008591 110 474 102 508 78
14 -0.25845516 140 2744 99 3902 76
15 -0.02618638 120 189 95 171 90
16 -0.01620885 160 17591 109 19235 84
42 0.03138901 150 21846 135 23161 137
23936 -0.25454813 140 20953 148 26420 94
17 0.10364089 80 11887 158 11458 161
18 -0.0604232 140 10537 111 12720 78
20 0.27844293 160 1351 101 1371 68
21 -0.25698157 100 576 106 828 72
22 -2.32967186 110 459 105 2116 69
30 -0.59024915 120 646 89 1084 74
33 -1.06533835 130 2068 99 3768 76
35 -1.07570742 120 886 110 1047 76

Total number of rows: 12328

Table truncated, full table size 449 Kbytes.




Supplementary data files not provided

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