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Sample GSM12195 Query DataSets for GSM12195
Status Public on Nov 25, 2003
Title 3000002603
Sample type RNA
 
Channel 1
Source name RDC-8 Thyroid knock-out (Cy5)
Organism Mus musculus
Extracted molecule total RNA
 
Channel 2
Source name C57Bl6 Thyroid Wild Type (Cy3)
Organism Mus musculus
Extracted molecule total RNA
 
 
Description I. Labelling Protocol (VIB-MAF Cy3 Labeling v1 and VIB-MAF Cy5 Labeling v1)
[1] RNA amplification by in vitro transcription
This protocol has been published in L. G. Puskás, Á. Zvara, L. Hackler Jr., and P. Van Hummelen (2002). RNA amplification results in reproducible microarray data with slight ratio bias. Biotechniques (2002) vol. 32, no. 6 p.1330-1341.
1.1 Reagents:
------------
(1) RNase Out 40U/ul (Invitrogen, 5000U, Cat. No. 10777-019),
(2) HT7T primer, HPLC purified (Eurogentec, sequence: 5 - GGCCAGTGAATTGTAATACGACTCACTATAGGGAGGCGGTTTTTTTTTT TTTTTTTTTTTTTT-3 ),
(3) Trehalose 1.7 M (Sigma, Cat. No. T-5251),
(4) 5 x first strand buffer (SuperScript II RT, Invitrogen, Cat. No. 18064-014),
(5) 0.1 M DTT (SuperScript II RT, Invitrogen, Cat. No. 18064-014),
(6) 10 mM dNTP-mix (Amersham Pharmacia Biotech, 100 mM, Cat. No. 27-2035- 01),
(7) SuperScript II RT 200U/ul (Invitrogen, 10000U, Cat. No. 18064-014),
(8) 5 x second strand buffer: 100 mM Tris-HCl (pH 6.9) (Invitrogen, Cat. No. 15714- 025 (Tris) and 1027 (HCl)), 450 mM KCl (Sigma, Cat. No. P-9541), 23 mM MgCl2 (Sigma, Cat. No. M 8266), 0.75 mM Beta-NAD+ (Sigma, Cat. No. N- 1636), 50 mM (NH4)2SO4 (Invitrogen, Cat. No. 15501-018)),
(9) E. coli DNA Ligase 10U/ul (Invitrogen, 100U, Cat. No. 18052-019),
(10) E. coli DNA Polymerase I 10U/ul (Invitrogen, 1000U, Cat. No. 18010-025),
(11) E. coli RNase H 2U/ul (Invitrogen, 120U, Cat. No. 18021-071),
(12) DEPC-water (Invitrogen, Cat. No. 10977-015),
(13) Ethanol Absolut (VWR, Cat. No. 1.08543.0250),
(14) QIAquick PCR Purification Kit (Qiagen, Cat. No 28106),
(15) NaAc 3M, pH 5.0 (Sigma, Cat. No. S-2889),
(16) AmpliScribeTM T7 Transcription Kit (Epicentre Technologies, Cat. No. AS3107),
(17) RNeasy Mini Kit (Qiagen, Cat. No 74106).
1.2 Protocol First Strand Synthesis:
-----------------------------------
(1) Mix 5 ug of total RNA (3 ul) with 1 ul of RNase Out 40U/ul.
(2) Add 1 ul of (HT7T) primer 200 ng/ul and 6 ul of 1.7 M Trehalose heated to 42C.
(3) Put on 75C for 5 minutes, chill on ice and spin down.
(4) Add 4 ul of 5 x first strand buffer, 2 ul of 0.1 M DTT, 1 ul of 10mM dNTP-mix, 1 ul of 1.7 M Trehalose and 1 ul of SuperScript II RT.
(5) Incubate at 37C for 5 minutes, at 45C for 5 minutes and then make 10 cycles of 60C for 2 minutes and 55C for 2 minutes. Go to 65C for 10 minutes and then go to 4C or chill on ice.
1.3 Protocol Second Strand Synthesis:
------------------------------------
(1) Add 33.4 ul of 5 x second strand buffer, 3.4 ul of 10 mM dNTP-mix, 1 ul of E. coli DNA Ligase (10U/ul), 4 ul of E. coli DNA Polymerase I (10U/ul), 1 ul of E. coli RNase H (2U/ul) and 103.8 ul of DEPC-water to the 20 ul of first strand mix.
(2) Incubate at 16C for 3 hours, at 65C for 10 minutes and then go to 4C or chill on ice.
(3) Purification with QIAquick PCR Purification Kit according to the manufacturers guidelines.
1.4 Protocol for In Vitro Transcription (IVT):
---------------------------------------------
(1) Add 2 ul of 10 x T7 reaction buffer (heated to 42C), 6 ul of 25 mM rNTP-mix, 2 ul of 100 mM DTT and 2 ul of AmpliScribe T7 enzyme solution to the DNA from second strand synthesis.
(2) Incubate at 37C for 3 hours, at 65C for 10 minutes and then go to 4C or chill on ice.
(3) Purification with QIAgen RNeasy Mini Kit according to the manufacturers guidelines.
(4) Check RNA concentration by OD. We recommend a 1/10 dilution in water or no dilution when using Nanodrop. Check A260/A280 ratio and determine the RNA concentration (1 OD = 40 ng/ul).
[2] Labeling
2.1 Reagents:
------------
(1) RNase Out 40U/ul (Invitrogen, 5000U, Cat. No. 10777-019),
(2) Random nonamers N9 1 ug/ul (Genset, 1862270),
(3) 5 x first strand buffer (SuperScript II RT, Invitrogen, Cat. No. 18064-014),
(4) 0.1 M DTT (SuperScript II RT, Invitrogen, Cat. No. 18064-014),
(5) 10 mM dNTP/2 mM dCTP (Amersham Pharmacia Biotech, 100 mM, Cat. No. 272050/60/70/80),
(6) CyTM-3-dCTP and CyTM-5-dCTP for microarrays (Amersham Pharmacia Biotech, 25 nmol, Cat. No. PA 53021 and PA 55021),
(7) SuperScript II RT 200U/ul (Invitrogen, 10000U, Cat. No. 18064-014),
(8) 2.5 M NaOH (Sigma, Cat. No. S-0899),
(9) MOPS (3-(N-Morpholino)propanesulfonic acid) (Sigma, Cat. No. M-8899),
(10) NaAc 3M, pH 5.0 (Sigma, Cat. No. S-2889),
(11) QIAquick PCR Purification Kit (Qiagen, Cat. No 28106).

2.2 Cy3 labeling Protocol:
----------------------
(1) Mix 5 ug of RNA from IVT (8 ul), 0.5 ul of RNase Out 40U/ul, 5 ul spikes (not for Arabidopsis thaliana) and 2 ul of random nonamers N9 1 ug/ul.
(2) Denaturate at 70C for 10 minutes, chill on ice and add the following components: 4 ul of first strand buffer, 1 ul of 10 mM dNTP/2 mM dCTP, 2 ul of 0.1 M DTT, 1.5 ul Cy3 dCTP and 1 ul of SuperScript II RT 200U/ul.
(3) Incubate at 42C for 2.5 hours and then go to 4C or chill on ice.
(4) Denaturate the RNA template by adding 2 ul of 2.5 M NaOH, incubating at 37C for exactly 15 minutes, adding 10 ul of 2 M MOPS and putting on ice.
(5) Purification with QIAquick PCR Purification Kit according to manufacturers guidelines.

2.3 Cy5 Labeling Protocol:
----------------------
(1) Mix 5 ug of RNA from IVT (8 ul), 0.5 ul of RNase Out 40U/ul, 5 ul spikes (not for Arabidopsis thaliana) and 2 ul of random nonamers N9 1 ug/ul.
(2) Denaturate at 70C for 10 minutes, chill on ice and add the following components: 4 ul of first strand buffer, 1 ul of 10 mM dNTP/2 mM dCTP, 2 ul of 0.1 M DTT, 1.5 ul of Cy5 dCTP and 1 ul of SuperScript II RT 200U/ul.
(3) Incubate at 42C for 2.5 hours and then go to 4C or chill on ice.
(4) Denaturate the RNA template by adding 2 ul of 2.5 M NaOH, incubating at 37C for exactly 15 minutes, adding 10 ul of 2 M MOPS and putting on ice.
(5) Purification with QIAquick PCR Purification Kit according to manufacturers guidelines.

II. Hybridisation Protocol (VIB-MAF Automatic hybridization v1 using Automatic Slide Processor (ASP))
A. Reagents:
-----------
(1) PolydT35 1 ug/ul (Genset),
(2) Mouse COT-1 DNA (R) 1 mg/ml (Invitrogen, 500 ug, Cat. No. 18440-016),
(3) Human COT-1 DNA (R)1 mg/ml (Invitrogen, 500 ug, Cat. No. 15279-011),
(4) Microarray hybridization buffer (Amersham Pharmacia Biotech, Cat. No. RPK0325),
(5) Formamide (Sigma, Cat. No. F-9037). Use Mouse COT DNA on Mouse slides, Human COT DNA on Human slides and no COT on Arabidopsis slides.
B. Protocol for automatic hybridization with ASP:
------------------------------------------------
(1) Make 210 ul hybridization mixture per slide with 25% probe, 25% buffer and 50% formamide.
(2) Dissolve the Cy3 and Cy5 sample together in 12 ul of polydT35, 30 ul of Mouse or Human or no (Arabidopsis) COT, water to make a total volume of 52.5 ul, 52.5 ul of Microarray 4x hybridization buffer and 105 ul formamide.
(3) Denature at 96C for 3 minutes.
(4) Keep on ice until hybridization.
(5) Inject samples in ASP.
III. Scanning Protocol (VIB-MAF scanning v1)
A. Equipment:
------------
(1) Generation III Scanner, Amersham Biosciences
(2) Scanner software: Default scanner software
B. Scanning Protocol:
--------------------
(1) Before scanning, adjust scanning parameters to: Full Slide, Cy5 PMT=550V, Cy3 PMT=550V
Keywords = Thyroid
Keywords = Adenosine Receptor 2a
Lot batch = batch 36A, RPK 0331 ; Printed 24-Sep-2001
 
Submission date Oct 23, 2003
Last update date Oct 28, 2005
Contact name Rekin's Janky
E-mail(s) Nucleomics.Bioinformatics@vib.be
Organization name VIB
Department Nucleomics Core
Street address Herestraat 49 Box 816
City Leuven
ZIP/Postal code B-3000
Country Belgium
 
Platform ID GPL556
Series (2)
GSE773 Thyroid RDC8 versus C57Bl6
GSE780 Gene Expression Profile in thyroid of Transgenic Mice over-expressing the Adenosine Receptor 2a

Data table header descriptions
ID_REF
CH1_NBC_INT Channel 1 artifact-removed density value for each spot, multiplied by its area. Pixels with values exceeding a user-defined threshold value (default is 4.0 Median of Absolute Deviations) are excluded and are replaced with estimated values, derived by interpolation from neighboring pixels. This measure removes the influence of image artifacts (e.g., dust particles) on density estimation.
CH1_PCTREPARVOL Channel 1 percent of pixels replaced with estimated values in the calculation of AR Volume.
CH1_MAD_RFU Channel 1 median of Absolute Deviation -- Median of the absolute values of deviations from the median density (i.e., the absolute values of pixel densities median density). It is a measure of the variation around the median density value of the spot.
CH1_PIXEL_SD Channel 1 deviation -- Standard deviation of the pixel density values.
CH1_SPOT_AREA Channel 1 area -- Area of the spot.
CH1_BKGD Channel 1 Background density or volume. Background volume value is adjusted to the size of spot, where applicable.
CH1_BC_INT Channel 1 Subtracted artifact removed (AR) volume value. AR Volume value of the spot, minus the background Volume value. The background value is adjusted to the size of the spot when applicable.
CH1_SN Channel 1 Signal-to-Noise Ratio -- Spot density minus Background density, divided by the SD of the Background density.
CH2_NBC_INT Channel 2 artifact-removed density value for each spot, multiplied by its area. Pixels with values exceeding a user-defined threshold value (default is 4.0 Median of Absolute Deviations) are excluded and are replaced with estimated values, derived by interpolation from neighboring pixels. This measure removes the influence of image artifacts (e.g., dust particles) on density estimation.
CH2_PCTREPARVOL Channel 2 percent of pixels replaced with estimated values in the calculation of AR Volume.
CH2_MAD_RFU Channel 2 median of Absolute Deviation -- Median of the absolute values of deviations from the median density (i.e., the absolute values of pixel densities median density). It is a measure of the variation around the median density value of the spot.
CH2_PIXEL_SD Channel 2 deviation -- Standard deviation of the pixel density values.
CH2_SPOT_AREA Channel 2 area -- Area of the spot.
CH2_BKGD Channel 2 Background density or volume. Background volume value is adjusted to the size of spot, where applicable.
CH2_BC_INT Channel 2 Subtracted artifact removed (AR) volume value. AR Volume value of the spot, minus the background Volume value. The background value is adjusted to the size of the spot when applicable.
CH2_SN Channel 2 Signal-to-Noise Ratio -- Spot density minus Background density, divided by the SD of the Background density.
BC_RATIO_LOG10 BC_RATIO_LOG10 = LOG10(CH1_BC_INT / CH2_BC_INT)
BC_TOTAL_INT_LOG10 BC_TOTAL_INT_LOG10 = LOG10(CH1_BC_INT * CH2_BC_INT)
VALUE BC_RATIO_NORM_LOG10 = LOG10 of normalized ratio from background corrected signals
NBC_RATIO_NORM_LOG10 NBC_RATIO_NORM_LOG10 = LOG10 of normalized ratio from NON background corrected signals

Data table
ID_REF CH1_NBC_INT CH1_PCTREPARVOL CH1_MAD_RFU CH1_PIXEL_SD CH1_SPOT_AREA CH1_BKGD CH1_BC_INT CH1_SN CH2_NBC_INT CH2_PCTREPARVOL CH2_MAD_RFU CH2_PIXEL_SD CH2_SPOT_AREA CH2_BKGD CH2_BC_INT CH2_SN BC_RATIO_LOG10 BC_TOTAL_INT_LOG10 VALUE NBC_RATIO_NORM_LOG10
1 34350.4477 16.041 0.185 0.603 29300 14332.124 20018.324 7.301 69229.642 2.73 0.173 0.278 29300 56431.424 12798.218 2.598 0.194278211 8.408577218
2 36308.6613 0 0.265 0.34 29300 14800.375 21508.286 7.928 88156.3837 0 0.359 0.483 29300 57864.46 30291.923 5.365 -0.148721041 8.813932647
3 1795038.234 7.509 6.801 12.752 29300 15174.394 1779863.841 632.098 711561.2755 9.556 3.016 7.083 29300 57300.428 654260.847 100.243 0.434635849 12.06613771
4 1202650.995 1.365 5.398 10.665 29300 14275.892 1188375.103 446.592 503754.885 4.096 2.356 5.383 29300 58715.814 445039.071 61.007 0.426555404 11.72335168
5 158790.3698 1.024 0.713 1.444 29300 14657.599 144132.771 59.401 131196.7511 0.341 0.443 0.88 29300 58516.619 72680.132 10.988 0.297347029 10.02017844
6 142010.2106 2.73 0.886 1.463 29300 14986.735 127023.475 52.506 127157.0359 4.778 0.32 0.741 29300 56963.203 70193.833 14.392 0.257585032 9.950182948
7 90587.2934 0 0.395 0.543 29300 15832.949 74754.344 26.895 99524.9242 1.024 0.231 0.432 29300 56571.127 42953.798 8.051 0.240634864 9.506638005
8 26978.4314 0.683 0.104 0.153 29300 16055.577 10922.855 3.899 94141.3911 0.341 0.221 0.391 29300 60466.084 33675.307 4.663 -0.488975395 8.565647732
9 117352.7877 15.017 0.624 2.207 29300 15641.27 101711.517 31.336 110489.5168 1.024 0.265 0.58 29300 61452.837 49036.68 7.746 0.316849073 9.697891191
10 188327.6429 0 0.976 1.95 29300 15523.999 172803.644 52.988 286194.7059 2.73 1.258 2.846 29300 55458.647 230736.059 42.785 -0.125562574 10.60066837
11 696489.0052 23.549 4.304 12.59 29300 14010.296 682478.709 227.597 122807.232 3.072 0.554 1.027 29300 53428.91 69378.322 13.337 0.992865316 10.6753129
12 41649.5049 0 0.221 0.294 29300 12600.727 29048.778 9.98 105299.1089 0 0.28 0.473 29300 52589.97 52709.139 10.397 -0.258758055 9.18501379
13 31545.603 1.024 0.175 0.257 29300 14261.862 17283.741 6.073 61015.5308 2.389 0.136 0.211 29300 50667.088 10348.443 2.144 0.222762738 8.252512762
14 59949.4091 0 0.317 0.51 29300 15494.722 44454.687 18.993 93754.4005 0.341 0.334 0.536 29300 47362.634 46391.766 8.399 -0.018523348 9.314358462
15 35778.5748 0 0.124 0.214 29300 15818.159 19960.416 3.979 64272.7739 0 0.271 0.39 29300 45113.31 19159.464 3.504 0.017786233 8.582552943
16 17057.3032 3.072 0.068 0.109 29300 15773.844 1283.46 0.256 44754.9841 1.706 0.128 0.204 29300 46776.116 0 0
17 43723.9018 0 0.215 0.326 29300 15305.005 28418.897 12.057 69436.4643 0.341 0.194 0.309 29300 44392.208 25044.256 3.653 0.054899084 8.852315352
18 14933.0088 6.826 0.058 0.597 29300 14529.806 403.203 0.177 41838.6235 3.413 0.103 1.158 29300 41254.931 583.693 0.132 -0.16066073 5.37170824
19 13109.69 4.096 0.058 0.363 29300 13336.861 0 0 39067.2525 5.802 0.095 0.635 29300 39577.265 0 0
20 13765.4089 0.341 0.054 0.078 29300 13282.618 482.791 0.016 40000.0576 5.119 0.091 0.168 29300 40470.869 0 0

Total number of rows: 9216

Table truncated, full table size 1521 Kbytes.




Supplementary data files not provided

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