NCBI Logo
GEO Logo
   NCBI > GEO > Accession DisplayHelp Not logged in | LoginHelp
GEO help: Mouse over screen elements for information.
          Go
Sample GSM1354 Query DataSets for GSM1354
Status Public on Feb 25, 2002
Title hsotd_4
Sample type RNA
 
Source name Drosophila melanogaster embryos
Organism Drosophila melanogaster
Extracted molecule total RNA
 
Description For overexpression of otd, the hsp-otd line 5A generated by Royet and Finkelstein was used [Royet et al.: Pattern formation in Drosophila head development: the role of the orthodenticle homeobox gene. Development 1995; 121:3561-3572.]. All fly stocks were kept on standard cornmeal/yeast/agar medium at 25°C. Embryos were collected overnight for 12 hours on grape juice plates, further kept for 4 hours at 25°C and then subjected to a 37°C heat shock for 25 min, followed by a recovery period of 25 min at 25°C before RNA isolation. Therefore, at the time of RNA isolation these embryos were at embryonic stages 10-17 [Leemans et al.: Quantitative transcript imaging in normal and heat-shocked Drosophila embryos by using high-density oligonucleotide arrays. Proc Natl Acad Sci U S A 2000; 97:12138-12143.]. Embryos younger than embryonic stage 10 were not used, since heat shock in these earlier stages results in lethality [Walter set al.: Heat shock causes the collapse of the intermediate filament cytoskeleton in Drosophila embryos. Dev Genet 1990; 11:270-279.]

Total RNA was isolated from 200 mg of embryonic tissue, using guanidinium isothiocyanate in combination with acidic phenol (pH 4.0) (fast RNA tube green kit from BIO101) in a fast prep homogenizer FP120 (BIO 101). After precipitation, the RNA was dissolved in DEPC-treated water (Ambion) and spectrophotometrically quantified using a GeneQuant RNA/DNA calculator (Pharmacia Biotech). cDNA was synthesized upon total RNA as a template, using the SuperScript Choice System for cDNA synthesis (Gibco/BRL) with a T7-(T)24 DNA primer.
This primer (5'-GGCCAGTGAATTGTAATACGACTCACTATAGGGAGGCGG-(T)24VN-3') was purified by PAGE. For first-strand cDNA synthesis, a typical 40 ul reaction contained 25 ug RNA, 200 pmol T7-(T)24 primer, 500 uM of each dNTP and 800 units reverse transcriptase (AMV Superscript II). The reaction was incubated for 1 h at 42°C. Second-strand cDNA synthesis was carried out at 18°C for 2 h in a total volume of 340 ul, using 20 units Escherichia coli DNA ligase, 80 units E. coli DNA polymerase I and 4 units RNase H in the presence of 250 uM of each dNTP. After second-strand cDNA synthesis, 0.5 ul RNase A (100 mg/ml) (Qiagen) was added and the samples were incubated at 37°C for 30 min. Thereafter, 7.5 ul proteinase K (10 mg/ml) (Sigma) was added and the samples were further incubated at 37°C for another 30 min. After cDNA synthesis was completed, samples were phenol-chloroform extracted, using Phase Lock Gel (5 Prime-3 Prime) and ethanol precipitated. Biotinylated antisense cRNA was synthesized from the dsDNA template, using T7 RNA polymerase (MEGAscript T7 Kit: Ambion.). A 20 ul reaction volume contained between 0.3-1.5 ug cDNA, 7.5 mM of both ATP and GTP, 5.6 mM of both UTP and CTP and 1.8 mM of both biotinylated Bio-16-UTP and Bio-11-CTP (ENZO diagnostics) and 2 ul 10x T7 enzyme mix. The reaction was incubated at 37°C for 8 h. Thereafter, the unincorporated NTPs were removed by running the sample over an RNeasy spin column (Qiagen). Samples were precipitated, taken up in 20 ul DEPC-treated water and spectrophotometrically quantified. Thereafter, 40 ug of the biotinylated antisense cRNA was fragmented by heating the sample to 95°C for 35 min in a volume of 25 ul, containing 40 mM tris-acetate (pH 8.1), 100 mM potassium acetate, 30 mM magnesium acetate. After the fragmentation, the samples were placed on ice.
Gene Chips were pre-hybridized with 220 ul hybridization buffer (1x MES (pH 6.7), 1 M NaCl, 0.01% Triton, 0.5 g/l acetylated BSA, 0.5 g/l sonicated herring sperm DNA) for 15 min at 45°C on a rotisserie (Heidolph) at 60 rpm. Hybridization was done in a final volume of 220 ul hybridization buffer, containing 40 g fragmented biotinylated cRNA. The samples were heated to 95°C for 5 min and briefly spun down. Hybridizations were carried out for 16 h at 45°C with mixing on a rotisserie at 60 rpm. After hybridization, the arrays were briefly rinsed with 6x SSPE-T (0.9 M NaCl, 0.06 M NaH2PO4, 6 mM EDTA, 0.01% Triton) and washed on a Fluidics station (Affymetrix). Hybridized arrays were stained with 220 ul detection solution (1x MES buffer, containing 2.5 ul streptavidin-R phycoerythrin conjugate (1 mg/ml) (Molecular Probes)) and 2.0 mg/ml acetylated BSA (Sigma) at 40°C for 15 min and washed again before being scanned.

The data was normalized against the mean of the total sums of Avg Diff values across all 16 arrays used in this study.
 
Submission date Feb 21, 2002
Last update date Oct 28, 2005
Contact name Thomas Loop
E-mail(s) thomas.loop@unibas.ch
Phone +41612671616
URL http://www.unibas.ch/dib/zoologie/research/neuro.html
Organization name University of Basel
Department Institute of Zoology
Lab Reichert Lab
Street address Klingelbergstrasse 50
City Basel
ZIP/Postal code CH-4056
Country Switzerland
 
Platform ID GPL70
Series (1)
GSE32 Heatshock otd / OTX2

Data table header descriptions
ID_REF
Experiment Name
Positive Number of positive probe pairs
Negative Number of negative probe pairs
Pairs Number of probe set specific probe pairs on the array
Pairs Used
Pairs InAvg Trimmed probe pair set
Pos Fraction
Log Avg
Pos/Neg
VALUE Average Difference Intensity
ABS_CALL Whether a probe set is present, marginal, or absent

Data table
ID_REF Experiment Name Positive Negative Pairs Pairs Used Pairs InAvg Pos Fraction Log Avg Pos/Neg VALUE ABS_CALL
AFFX-BioC-5_at hsotd-4 11 2 20 20 18 0.55 2.92 5.5 515 P
AFFX-BioDn-5_at hsotd-4 16 3 20 20 19 0.8 4.07 5.3 773 P
AFFX-BioDn-3_at hsotd-4 13 3 20 20 19 0.65 4.39 4.3 2619 P
AFFX-CreX-5_at hsotd-4 18 0 20 20 20 0.9 7.49 Undef 6585 P
AFFX-CreX-3_at hsotd-4 18 0 20 20 20 0.9 7.42 Undef 8841 P
AFFX-DapX-M_at hsotd-4 8 2 20 20 18 0.4 1.61 4 110 P
AFFX-LysX-3_at hsotd-4 7 0 20 20 20 0.35 1.52 Undef 153 P
DMGADPH1-1_at hsotd-4 12 1 14 14 13 0.86 4.36 12 2433 P
DMGADPH1-2_at hsotd-4 8 1 14 14 13 0.57 3.11 8 3609 P
DMGADPH1-3_at hsotd-4 11 0 14 14 13 0.79 4.01 Undef 2984 P
DMRAC2A-1_at hsotd-4 10 1 14 14 13 0.71 3.67 10 1419 P
DMRAC2A-2_at hsotd-4 11 0 14 14 14 0.79 4.43 Undef 2343 P
DMRAC2A-3_at hsotd-4 9 0 14 14 13 0.64 3.06 Undef 1172 P
DMRP49-1_at hsotd-4 14 0 14 14 14 1 6.97 Undef 23364 P
DMRP49-2_at hsotd-4 11 0 14 14 14 0.79 4.14 Undef 18715 P
DMRP49-3_i_at hsotd-4 12 1 13 13 13 0.92 5.68 12 18384 P
DMRP49-3_r_at hsotd-4 10 2 14 14 14 0.71 3.95 5 15764 P
DMU62892-1_at hsotd-4 9 0 14 14 13 0.64 3.26 Undef 263 P
DMU62892-3_at hsotd-4 14 0 14 14 14 1 8.44 Undef 10996 P
A10_at hsotd-4 6 0 14 14 13 0.43 1.01 Undef 1091 P

Total number of rows: 14090

Table truncated, full table size 711 Kbytes.




Supplementary data files not provided

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