NCBI Logo
GEO Logo
   NCBI > GEO > Accession DisplayHelp Not logged in | LoginHelp
GEO help: Mouse over screen elements for information.
          Go
Sample GSM141360 Query DataSets for GSM141360
Status Public on Dec 19, 2006
Title MET_HR_4
Sample type RNA
 
Channel 1
Source name MET_HR_4
Organism Homo sapiens
Characteristics Metastatic Prostate Carcinoma - Hormone Refractory Sample 4
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 20, 2006
Last update date Jul 22, 2008
Contact name Scott Tomlins
E-mail(s) tomlinss@med.umich.edu
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 1450 18770 80 981 1109 695 300 334 151 76 71 0 1616 1490 838 1269 1284 196 59 50 0 1.963 3.661 1.569 1.054 3.609 0.965 0.627 52 274 1028 1030 0.973 681 347 809 221 0 null
Hs6-1-2-1 1590 18770 90 1317 1444 818 322 360 167 92 82 0 1716 1724 829 1298 1305 198 65 53 0 2.38 2.634 1.656 1.751 2.695 1.166 0.677 52 338 1413 1548 1.251 995 418 1122 426 0 null
Hs6-1-3-1 1780 18760 100 402 435 175 318 364 179 33 10 0 954 918 427 1322 1308 198 3 0 0 -0.228 -0.29 0.132 0.279 7.738 0.176 0.072 80 447 -284 -287 Error 84 -368 117 -404 -50 null
Hs6-1-4-1 1940 18760 120 1170 1210 570 313 361 214 90 80 0 1798 1832 669 1335 1307 230 65 50 0 1.851 1.805 1.501 1.731 1.893 1.132 0.722 120 610 1320 1394 0.888 857 463 897 497 0 null
Hs6-1-5-1 2130 18760 100 654 770 424 337 389 237 60 36 0 1259 1286 564 1378 1402 243 27 20 0 -2.664 -4.707 1.565 1.414 5.007 0.924 0.397 80 397 198 341 Error 317 -119 433 -92 -50 null
Hs6-1-6-1 2300 18760 120 1744 1827 1059 378 499 394 85 70 0 2761 2782 1527 1412 1467 334 78 65 0 1.013 1.058 0.974 0.875 2.464 0.813 0.904 120 566 2715 2819 0.018 1366 1349 1449 1370 0 0.08667
Hs6-1-7-1 2470 18760 120 9003 9796 5521 449 562 374 95 94 0 9022 9789 5392 1442 1510 366 93 92 0 1.128 1.12 1.103 1.129 1.412 1.076 0.99 120 534 16134 17694 0.174 8554 7580 9347 8347 0 0.1771
Hs6-1-8-1 2640 18750 110 2553 2691 1481 550 623 354 83 78 0 3295 3195 1664 1516 1521 387 77 73 0 1.126 1.275 1.136 1.027 2.043 1.025 0.918 80 502 3782 3820 0.171 2003 1779 2141 1679 0 0.01481
Hs6-1-9-1 2820 18750 110 4762 5180 2754 506 513 184 92 90 0 5386 5744 2932 1434 1407 267 88 87 0 1.077 1.084 1.056 1.04 1.48 1.011 0.974 80 536 8208 8984 0.107 4256 3952 4674 4310 0 0.05933
Hs6-1-10-1 3000 18750 100 1514 1575 742 464 476 167 86 83 0 1935 1853 856 1406 1379 258 60 51 0 1.985 2.485 1.554 1.478 3.213 1.216 0.761 80 462 1579 1558 0.989 1050 529 1111 447 0 0.1091
Hs6-1-11-1 3170 18750 110 2073 2223 1302 429 439 149 85 82 0 2857 3131 1780 1379 1351 245 81 77 0 1.112 1.024 0.894 0.771 2.447 0.842 0.93 80 509 3122 3546 0.154 1644 1478 1794 1752 0 -0.1164
Hs6-1-12-1 3340 18760 110 1309 1363 726 411 446 179 83 78 0 1824 1734 920 1388 1360 264 57 43 0 2.06 2.751 1.382 1.137 3.141 1.019 0.703 80 498 1334 1298 1.042 898 436 952 346 0 null
Hs6-1-13-1 3510 18750 110 3975 4312 2449 421 514 377 90 88 0 3891 4083 2185 1402 1426 300 85 83 0 1.428 1.451 1.364 1.293 1.862 1.295 0.956 80 546 6043 6572 0.514 3554 2489 3891 2681 0 0.08278
Hs6-1-14-1 3700 18750 110 2841 3110 1891 396 503 422 87 81 0 2933 3076 1752 1335 1350 400 77 72 0 1.53 1.559 1.468 1.423 1.926 1.274 0.924 80 576 4043 4455 0.614 2445 1598 2714 1741 0 0.1776
Hs6-1-15-1 3900 18760 70 1490 1659 702 386 497 414 96 65 0 2159 2214 863 1248 1274 488 75 46 0 1.212 1.318 1.17 1.46 2.127 0.883 0.809 32 220 2015 2239 0.277 1104 911 1273 966 0 null
Hs6-1-16-1 4050 18750 100 1262 1325 868 359 397 196 75 71 0 1543 1554 995 1319 1287 393 43 36 0 4.031 4.111 1.477 1.036 4.184 0.955 0.636 80 472 1127 1201 2.011 903 224 966 235 0 null
Hs6-1-17-1 4220 18760 110 3255 3417 2032 363 397 180 91 91 0 2939 3219 1789 1344 1353 216 85 78 0 1.813 1.629 1.525 1.517 2.143 1.359 0.933 80 464 4487 4929 0.859 2892 1595 3054 1875 0 0.1907
Hs6-1-18-1 4390 18750 110 1127 1223 590 351 376 160 86 85 0 1734 1674 781 1305 1303 183 58 52 0 1.809 2.363 1.357 1.185 2.993 1.084 0.671 80 500 1205 1241 0.855 776 429 872 369 0 null
Hs6-1-19-1 4580 18750 130 5442 6250 3811 355 387 190 94 93 0 5063 5882 3319 1287 1281 188 91 91 0 1.347 1.283 1.252 1.206 1.691 1.217 0.973 120 668 8863 10490 0.430 5087 3776 5895 4595 0 0.2089
Hs6-1-20-1 4750 18750 110 3472 4529 3290 447 499 243 86 85 0 2509 3466 2380 1352 1370 256 80 80 0 2.615 1.931 1.73 1.545 3.083 1.564 0.941 80 476 4182 6196 1.387 3025 1157 4082 2114 0 0.3482

Total number of rows: 20000

Table truncated, full table size 3745 Kbytes.




Supplementary file Size Download File type/resource
GSM141360.gpr.gz 2.1 Mb (ftp)(http) GPR
Processed data included within Sample table

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