NCBI Logo
GEO Logo
   NCBI > GEO > Accession DisplayHelp Not logged in | LoginHelp
GEO help: Mouse over screen elements for information.
          Go
Sample GSM141425 Query DataSets for GSM141425
Status Public on Dec 19, 2006
Title STROMA_NOR_2
Sample type RNA
 
Channel 1
Source name STROMA_NOR_2
Organism Homo sapiens
Characteristics Normal Stroma - Organ Donor Sample 2
Extracted molecule total RNA
Extraction protocol Laser Capture Microdissection (LCM) was performed from frozen tissue sections with the SL Microtest device using µCUT software MMI). Approximately 10,000 cells were captured for each sample. Serial sections were used if cells could not be obtained from a single section. Total RNA was isolated from captured cells with the RNAqueous Micro kit (Ambion) and treated with DNAse I according to the manufacturer's instructions. RNA quantification was perfomed using Ribogreen (Molecular Probes).
Label Cy5
Label protocol Total RNA (~10ng) in a volume of 25 µl was converted into an OmniPlex WTA cDNA library and amplified by WTA PCR using reagents and protocols according to the beta-commercial TransPlex WTA kit (Rubicon Genomics, Ann Arbor, MI). For each sample, a single 10 µl aliquot of the WTA cDNA library was amplified by WTA PCR and products were purified. Four or five 5 ng aliquots of product were subjected to a second WTA PCR amplification in the presence of amino-allyl dUTP for post amplification labeling and products were pooled before proceeding with the hybridization. Yields after all WTA PCR amplifications were between 2 to 5 ?g per reaction. For all WTA amplified cDNA samples with amino-allyl dUTP incorporated (10-20 ?g), nuclease free water was added to 500 ?l, the sample was transferred to a Microcon YM-30 filter, and centrifuged at 13,000 rcf at RT for 12 minutes. The spin column was inverted in a new collection tube and centrifuged at 13,000 rcf for 2 min at RT. The amount of sample was measured and the volume was adjusted to 5 ?l with nuclease free water. For labeling, 5 ?l of 1 M sodium bicarbonate (pH 9.0) was added and allowed to incubate at RT for 15 min. Nine ?l of anhydrous DMSO were added to Mono Reactive Cy3 and Cy5 dye packs (Amersham, Buckinghamshire, England), mixed thoroughly, and 1 ?l of the proper dye was added to each sample. The labeling mixture was incubated in the dark at RT for 1 hour. The reaction was stopped by the addition of 9 ?l of 4 M Hydroxylamine for 15 min. For each labeling mixture, RNase free water was added to 100 ?l, 500 ?l of PB buffer was added and Cy3 and Cy5 mixtures were added to separate Qiaquick (Qiagen, Valencia, CA) spin columns and centrifuged at 13,000 rcf. Columns were washed twice with 700 ?l of buffer PE, and centrifuged dry at 13,000 rcf for 2 min. To elute, 60 ?l of EB buffer was placed on the column, incubated for 5 min and centrifuged at 13,000 rcf for 1 min. The Cy3 labeled and Cy5 labeled cDNA for each hybridization were mixed and 1.5 ?l were used for analysis on a ND-1000 spectrophotometer.
 
Channel 2
Source name CPP
Organism Homo sapiens
Characteristics Clontech Prostate Pool
Extracted molecule total RNA
Extraction protocol commercially-obtained
Label Cy3
Label protocol Total RNA (~10ng) in a volume of 25 µl was converted into an OmniPlex WTA cDNA library and amplified by WTA PCR using reagents and protocols according to the beta-commercial TransPlex WTA kit (Rubicon Genomics, Ann Arbor, MI). For each sample, a single 10 µl aliquot of the WTA cDNA library was amplified by WTA PCR and products were purified. Four or five 5 ng aliquots of product were subjected to a second WTA PCR amplification in the presence of amino-allyl dUTP for post amplification labeling and products were pooled before proceeding with the hybridization. Yields after all WTA PCR amplifications were between 2 to 5 ?g per reaction. For all WTA amplified cDNA samples with amino-allyl dUTP incorporated (10-20 ?g), nuclease free water was added to 500 ?l, the sample was transferred to a Microcon YM-30 filter, and centrifuged at 13,000 rcf at RT for 12 minutes. The spin column was inverted in a new collection tube and centrifuged at 13,000 rcf for 2 min at RT. The amount of sample was measured and the volume was adjusted to 5 ?l with nuclease free water. For labeling, 5 ?l of 1 M sodium bicarbonate (pH 9.0) was added and allowed to incubate at RT for 15 min. Nine ?l of anhydrous DMSO were added to Mono Reactive Cy3 and Cy5 dye packs (Amersham, Buckinghamshire, England), mixed thoroughly, and 1 ?l of the proper dye was added to each sample. The labeling mixture was incubated in the dark at RT for 1 hour. The reaction was stopped by the addition of 9 ?l of 4 M Hydroxylamine for 15 min. For each labeling mixture, RNase free water was added to 100 ?l, 500 ?l of PB buffer was added and Cy3 and Cy5 mixtures were added to separate Qiaquick (Qiagen, Valencia, CA) spin columns and centrifuged at 13,000 rcf. Columns were washed twice with 700 ?l of buffer PE, and centrifuged dry at 13,000 rcf for 2 min. To elute, 60 ?l of EB buffer was placed on the column, incubated for 5 min and centrifuged at 13,000 rcf for 1 min. The Cy3 labeled and Cy5 labeled cDNA for each hybridization were mixed and 1.5 ?l were used for analysis on a ND-1000 spectrophotometer.
 
 
Hybridization protocol For hybridization, 40 ug of human Cot-1 DNA (Invitrogen, Carlsbad, CA) was added to 120 ?l of labeled cDNA, the probe was transferred to a Microcon YM-30 filter and centrifuged at 13,000 rcf for 6 min at RT. The spin column was inverted in a new collection tube and centrifuged at 13,000 rcf for 2 min at RT. The eluted probe volume was adjusted to 18.6 ?l with nuclease free water and the following were added: 4 ?l of yeast tRNA (10 ?g/?l, Invitrogen, Carlsbad, CA), 4.9 ?l of 20X SSC and 0.84 ?l of 10% SDS. The probe was denatured at 100 Co for 3 min and centrifuged at 13,000 rcf for 45 sec. The probe was added directly to the microarray and a cover slip was added. Slides were hybridized overnight in DIE-TECH 1 or 5 slide hybridization chambers in a 65 Co water bath. After hybridization, cover slips were removed by incubation in 2x SSC / 0.05% SDS. Slides were then washed in 2x SSC / 0.05% SDS for 5 min and 0.2x SSC / 0.05% SDS for five minutes. Slides were then washed in 0.2x SSC for 10 sec and centrifuged dry at 500 rpm for 5 min.
Scan protocol Microarrays were scanned using a GenePix 4000B scanner (Axon Instruments, Union City, CA).
Description See MIAME checklist, included in the Supplementary Methods, for additional information
Data processing Images were gridded and spots were quantified using GenePix Pro 4.0 software (Axon Instruments, Union City, CA). For all hybridizations, the log2 normalized Median of Ratios (as described below) was used.
 
Submission date Oct 21, 2006
Last update date Jul 22, 2008
Contact name Scott Tomlins
E-mail(s) [email protected]
Phone 734-615-1417
Organization name University of Michigan
Department Pathology
Lab Chinnaiyan Lab
Street address 1400 E. Medical Center Dr., 5410 CCGC
City Ann Arbor
State/province MI
ZIP/Postal code 48109
Country USA
 
Platform ID GPL2013
Series (1)
GSE6099 Integrative Molecular Concepts Modeling of Prostate Cancer Progression

Data table header descriptions
ID_REF
X the X-coordinate in um of the center of the feature indicator associated with the feature, where (0,0) is the top left of the image
Y the Y-coordinate in um of the center of the feature-indicator associated with the feature, where (0,0) is the top left of the image
Dia. the diameter in um of the feature indicator
F635.Median median feature pixel intensity at wavelength 1 (635 nm, Cy5)
F635.Mean mean feature pixel intensity at wavelength 1
F635.SD standard deviation of the feature pixel intensity at wavelength 1
B635.Median median feature background intensity at wavelength 1
B635.Mean mean feature background intensity at wavelength 1
B635.SD standard deviation of the feature background intenstiy at wavelength 1
X....B635.1SD percentage of feature pixels with intensities more than one standard deviation above the background pixel intensity, at wavelength 1
X....B635.2SD the percentage of fetaure pixels with intensities more than two standard deviations above the background pixel intensity, at wavelength 1
F635...Sat. the perentage of feature pixels at wavelength 1 that are saturated
F532.Median median feature pixel intensity at wavelength 2 (532 nm, Cy3)
F532.Mean mean featur pixel intensity at wavelength 2
F532.SD standard deviation of feature pixel intensity at wavelength 2
B532.Median medain feature backgroudn intensity at wavelength 2
B532.Mean mean feature background intensity at wavelength 2
B532.SD standard deviation of the feature background intensity at wavelength 2
X....B532.1SD the percentage of feature pixels with intensities more than one standard deviation above the background pixel intensity, at wavelength 2
X....B532.2SD the percentage of feature pixels with intensities more than two standard deviations above the backroudnn pixel intensity, at wavelength 2
F532...Sat. the percentage of feature pixels at wavelength 2 that are saturated
Ratio.of.Medians..635.532. the ratio of the median intensities of each feature for each wavelength, with the median background subtracted
Ratio.of.Means..635.532. the ratio of the arithmetic mean intesnties of each feature for each wavelength, with the median background subtracted
Median.of.Ratios..635.532. the median of pixel by pixel ratios of pixel intensities, with the median backgroudn subtracted
Mean.of.Ratios..635.532. the arithemetic mean of the pixel by pixel ratios of pixel intensities, with the median background subtracted
Ratios.SD..635.532. the standard deviation of pixel intensity ratios
Rgn.Ratio..635.532. the regression ratio
Rgn.R. the coefficient of determination for the current regression value
F.Pixels the total number of feature pixels
B.Pixels the total number of background pixels
Sum.of.Medians the sum of hte median intensities for each wavelength, with the median background subtracted
Sum.of.Means the sum of the arithemetic mean intensities for each wavelength, with the median background subtracted
Log.Ratio..635.532. log (base 2) transform of the ratio of the medians
F635.Median...B635 the median feature pixel intenisty at wavelength 1 with the median background subtracted
F532.Median...B532 the median feature pixel intensity at wavelgnth 2 with the emdian background subtracted
F635.Mean...B635 the mean feature pixel intensity at wavelength 1 with the median background subtracted
F532.Mean...B532 the mean feature pixel inentisy at wavelength 2 with the median background subtracted
Flags 0 = unflagged; negative values indicate unalignend features flagged by GenePix or areas of obvious defects and were not used for data analysis
VALUE Normalized, log2-transformed Median of Ratios (635/532)

Data table
ID_REF X Y Dia. F635.Median F635.Mean F635.SD B635.Median B635.Mean B635.SD X....B635.1SD X....B635.2SD F635...Sat. F532.Median F532.Mean F532.SD B532.Median B532.Mean B532.SD X....B532.1SD X....B532.2SD F532...Sat. Ratio.of.Medians..635.532. Ratio.of.Means..635.532. Median.of.Ratios..635.532. Mean.of.Ratios..635.532. Ratios.SD..635.532. Rgn.Ratio..635.532. Rgn.R. F.Pixels B.Pixels Sum.of.Medians Sum.of.Means Log.Ratio..635.532. F635.Median...B635 F532.Median...B532 F635.Mean...B635 F532.Mean...B532 Flags VALUE
Hs6-1-1-1 1510 18650 110 1085 1162 735 223 235 93 80 76 0 1240 1147 713 989 969 173 58 42 0 3.434 5.943 1.938 1.256 4.549 1.461 0.637 80 506 1113 1097 1.780 862 251 939 158 0 null
Hs6-1-2-1 1660 18640 110 1487 1393 867 213 221 73 85 80 0 1843 1566 898 969 961 154 67 65 0 1.458 1.977 1.282 0.958 4.716 1.289 0.778 80 469 2148 1777 0.544 1274 874 1180 597 0 -0.1803
Hs6-1-3-1 1820 18650 60 491 506 311 213 243 132 59 53 0 1217 889 559 853 877 171 56 53 0 0.764 8.139 0.794 0.487 3.175 0.498 0.367 32 176 642 329 -0.389 278 364 293 36 0 null
Hs6-1-4-1 2020 18640 120 1445 1678 1142 217 235 112 86 81 0 1438 1491 844 992 983 175 69 56 0 2.753 2.928 2.1 1.883 2.771 1.824 0.765 120 677 1674 1960 1.461 1228 446 1461 499 0 0.7549
Hs6-1-5-1 2210 18640 90 840 828 528 218 235 118 69 65 0 1388 1133 734 912 927 167 59 57 0 1.307 2.76 1.107 0.57 5.084 0.882 0.658 52 326 1098 831 0.386 622 476 610 221 0 null
Hs6-1-6-1 2350 18640 110 1655 1539 958 229 261 189 78 73 0 2821 2509 1628 970 980 237 71 66 0 0.77 0.851 0.664 0.626 3.153 0.69 0.903 80 485 3277 2849 -0.376 1426 1851 1310 1539 0 -0.3179
Hs6-1-7-1 2530 18640 110 11954 11154 6876 269 333 317 98 93 0 10956 10091 6174 997 1017 263 88 86 0 1.173 1.197 1.164 1.303 1.761 1.175 0.967 80 524 21644 19979 0.231 11685 9959 10885 9094 0 0.3134
Hs6-1-8-1 2710 18640 110 4791 3635 2507 297 354 290 76 72 0 4318 3333 2229 987 1020 302 71 67 0 1.349 1.423 1.266 1 2.441 1.26 0.944 80 505 7825 5684 0.432 4494 3331 3338 2346 0 0.3263
Hs6-1-9-1 2890 18640 120 4388 4182 2706 300 321 137 88 83 0 4767 4370 2721 1015 1018 301 76 75 0 1.09 1.157 1.059 0.937 2.482 1.057 0.942 120 593 7840 7237 0.124 4088 3752 3882 3355 0 0.08314
Hs6-1-10-1 3070 18650 110 2009 1640 1075 305 323 139 72 72 0 2153 1707 1119 991 1021 276 60 57 0 1.466 1.865 1.274 0.753 3.109 1.175 0.837 80 458 2866 2051 0.552 1704 1162 1335 716 0 0.06191
Hs6-1-11-1 3240 18640 110 2237 1873 1212 319 327 131 78 75 0 2899 2567 1674 1051 1064 254 67 63 0 1.038 1.025 0.837 0.706 2.427 0.848 0.889 80 523 3766 3070 0.054 1918 1848 1554 1516 0 -0.08382
Hs6-1-12-1 3430 18640 100 1460 1578 1062 308 334 187 78 75 0 1730 1798 1212 1123 1101 279 55 51 0 1.898 1.881 1.182 0.801 3.724 1.067 0.828 80 474 1759 1945 0.924 1152 607 1270 675 0 -0.004745
Hs6-1-13-1 3610 18650 110 1715 1695 1065 298 332 180 81 78 0 2294 2316 1494 1111 1084 270 72 66 0 1.198 1.159 0.906 0.816 3.297 0.833 0.841 80 484 2600 2602 0.260 1417 1183 1397 1205 0 -0.5215
Hs6-1-14-1 3770 18640 110 2016 2062 1452 295 312 114 86 81 0 2191 2343 1679 1135 1091 202 63 62 0 1.63 1.463 1.069 0.9 2.737 1.029 0.861 80 463 2777 2975 0.705 1721 1056 1767 1208 0 -0.2182
Hs6-1-15-1 3940 18650 130 997 1119 683 311 333 141 76 74 0 1523 1575 952 1120 1090 211 60 50 0 1.702 1.776 0.992 0.754 3.659 0.848 0.714 120 603 1089 1263 0.767 686 403 808 455 0 null
Hs6-1-16-1 4120 18640 110 721 749 573 290 319 149 61 56 0 949 1187 1027 1102 1064 271 46 38 0 -2.817 5.4 0.693 0.451 2.97 0.603 0.63 80 471 278 544 Error 431 -153 459 85 0 null
Hs6-1-17-1 4290 18650 120 2227 2147 1325 242 269 145 89 85 0 2207 2236 1274 988 977 239 75 71 0 1.628 1.526 1.312 1.111 3.631 1.034 0.585 120 590 3204 3153 0.703 1985 1219 1905 1248 0 0.01964
Hs6-1-18-1 4490 18650 110 1193 1071 602 214 237 141 82 76 0 1510 1320 746 896 903 175 62 57 0 1.594 2.021 1.298 0.929 4.209 1.074 0.725 80 474 1593 1281 0.673 979 614 857 424 0 -0.08792
Hs6-1-19-1 4650 18650 120 3990 3476 2142 243 265 110 85 84 0 4545 3994 2418 956 936 163 81 80 0 1.044 1.064 0.984 0.963 2.704 0.961 0.898 120 500 7336 6271 0.062 3747 3589 3233 3038 0 -0.1383
Hs6-1-20-1 4810 18640 110 2804 2515 1571 275 307 142 85 80 0 2962 2726 1734 963 960 192 72 68 0 1.265 1.271 1.07 1.111 2.564 1.079 0.879 80 474 4528 4003 0.339 2529 1999 2240 1763 0 -0.2671

Total number of rows: 20000

Table truncated, full table size 3714 Kbytes.




Supplementary file Size Download File type/resource
GSM141425.gpr.gz 2.0 Mb (ftp)(http) GPR
Processed data included within Sample table

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