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Sample GSM404439 Query DataSets for GSM404439
Status Public on May 18, 2010
Title MTB strain 1254 Ctrl vs 0.5 mM DETA/NO 40min rep 1
Sample type RNA
 
Channel 1
Source name Strain: MTB strain 1254 Treatment: Control
Organism Mycobacterium tuberculosis
Characteristics strain: MTB strain 1254
treatment: Control
Extracted molecule total RNA
Extraction protocol not provided
Label Cy3
Label protocol TB-Synthesis and Labeling of cDNA SKlab 01; 1. Bring 0.5-5 ?g RNA (Typically 3 ?g) to 11 ?l and add 2 ?l (~2 mg/ml) random hexamers. 2. Heat 10 min at 65C (or 2 min at 98C), snap cool on ice. 10 rxns 20 rxns 3. Add 11?l 5.0 ?l 5X First-Strand buffer (51) (102) 2.5 ?l 100 mM DTT (25.5) (51) 2.0 ?l dNTP (5 mM A,G,C and 0.2 mM T) (20.5) (41) 1.5 ?l Cy3 or Cy5 (Typically use Cy5 for sample that should change) (15.3) (30.6) Then add 1.2-1.8 ?l Stratascript or 0.8-1.2 ?l Superscript II RTase. 4. Incubate 10m at 25C followed by 90m at 42C in PCR machine. Can freeze or leave at 4C o/n.; Protocol Type = Labeling; Performer: Kevin,,Visconti
 
Channel 2
Source name Strain: MTB strain 1254 Treatment: 0.5 mM DETA/NO for 40min
Organism Mycobacterium tuberculosis
Characteristics strain: MTB strain 1254
treatment: 0.5 mM DETA/NO for 40min
Growth protocol Growth Conditions; Parameters that describe the conditions under which the biological sample was grown or propagated; Protocol Type = Growth Conditions; Parameter Starting OD = 0.15; Parameter Elapsed Time = 40 min; Parameter Growth Temperature = 37oC; Parameter Culture Synchrony = Unsynchronized; Parameter Growth Vessel Volume = 250 ml; Parameter Media = Middlebrook 7H9 supplemented with albumin-dextrose complex (ADC) and 0.01% Tween 80; Performer: Kevin,,Visconti
Extracted molecule total RNA
Extraction protocol not provided
TB-RNA Isolation and Purification SKlab 01; 1. Centrifuge 20-30 ml of early- to mid-log culture (O.D. 0.1-0.2) 4 min at 3700 rpm, at RT-37C. Pipette off supernatant and immediately freeze on dry ice and store at ?80C. 2. Add 1 ml Trizol (Gibco-BRL) to each of 4-8 pellets, suspend first pellet by vortexing,while other pellets are still frozen. Add suspension to 0.4 ml glass beads in a 2 ml screw cap tube. 3. Shake 30s at maximum speed in bead beater. Suspend next pellet and add to glass beads. Apply next sample to bead beater. Repeat bead beating two more times with each sample.Continue to periodically invert samples for at least 5 min in Trizol. 4. Centrifuge samples 45s at max speed, remove Trizol solution to a 2 ml screw cap tube containing half of the Heavy Phase Lock Gel I, supplied by 5 Prime 3 Prime, Inc. in 1.5 ml tubes and transferred with sterile stick to 2 ml tubes, and 300 ?l Chloroform:isoamyl alcohol (24:1). Invert rapidly for 15s, and continue inverting periodically for 2 min.a 5. Centrifuge 5-10m, remove aqueous layer (540 ?l) and add to a 1.5 ml tube containing 270 ?l isopropanol then add 270 ?l high salt solution (0.8M Na Citrate, 1.2M NaCl). Invert several times and spray with Staphene and remove from the P3. Typically ppted at 4C O/N. 6. Centrifuge 10m at 4C and remove isopropanol. Add 1 ml 75% EtOHb, invert several times and centrifuge 5m. 7. Remove EtOH by aspiration. Then, dry under vacuum for 2 min [Do not over dry]. 8. Suspend RNA in 90 ml RNase free water (don?t suspend in DNaseI buffer), may need to heat 10m at 55-60C to dissolve RNA. (Optional: obtain RNA concentration) 9. Add 10 ?l 10X DNaseI buffer to RNA (use no more than 80 ?g RNA) and add 4 ?l DNaseI (Ambion). Incubate 30m at 37C. Qiagen RNeasy purification. 1. Add 350 ?l RLT buffer (add 10 ?l BME to 1 ml RLT before using) and vortex. Add 260 ?l 95% EtOH (or 250 ?l 100% EtOH) to each sample and vortex. 2. Add to RNeasy spin column, centrifuge 15s, transfer column to a new 2 ml collection tube. Add 500 ?l RPE, centrifuge 15s, discard flow-through, add 500 ?l additional RPE and centrifuge 2m. If column still wet on sides, remove wash solution from tube and spin 1m to dry. 3. Transfer to a 1.5 ml collection tube, elute with 40 ?l RNase free water, centrifuge 1m. 4. Determine RNA concentration with A260/A280 readings. Dilute 1 ?l in 199 ?l TE. [200(dilution factor)x 40 ?g/A260x A260 = ?g/ml]. 5. Run 1 ?l RNA on 2% Agarose TAE gel. Run gel 45m at 100 volts. aIf Phase Lock Gel is not used, decrease Chloroform:isoamyl alcohol to 200?l. The yield will be less. Be careful not to remove any of the interface layer. bUsing 100% EtOH should be avoided in all steps of preparation of RNA intended for array analysis. Instead use 95% EtOH in preparation of solutions. Benzene contamination may fluoresce. cInstead of using the RNeasy purification, the DNaseI can be inactivated at 65-70C for 15m and then EtOH precipitated. The RNeasy purification may not be necessary in all applications. We find the purification gives more consistent results and is less time consuming, compared to precipitation. In addition, other purifications can be used. Note: The RNeasy column will remove much of the small tRNA and degraded RNA.; Protocol Type = Extract preparation; Performer: Kevin,,Visconti
Label Cy5
Label protocol TB-Slide Preparation SKlab 01; 1. Prepare NaOH-ethanol solution ? dissolve NaOH in ddH2O 70 g / 280 mL 175 g / 700mL 200 g / 800 mL ? stir until completely dissolved ? add 95% ethanol 420 mL 1050 mL 1200mL ? stir until completely mixed ? if solution remains cloudy, add water until clear 2. Place slides in metal slide racks (30 slides/rack). Do not use defective slides. 3. Soak slides in the NaOH:EtOH:ddH2O solution for 2 hours with gentle rotation. 4. Rinse extensively with dH2O: ? rinse each unit (slide/rack/container) vigorously with dH2O for 5 min ? place slide racks in a large clean glass container, and tilt the container slightly for constant water flow. ? wash under running water for 30 minutes. ? do not allow the slides to dry at any time. It is critical to remove all traces of NaOH:EtOH. 5. Prepare poly-L-lysine solution in plastic container. ? 100 mL tissue culture PBS 800 mL Milli-Q water 100 mL poly-L-Lysine ? We bring up the volume to about 1050 mL with Milli-Q water in order to submerge 3 racks of slides. ? Mix well and split into 3 plastic containers. 6. Soak the slides in lysine solution for 45 min with shaking. Be sure to use a plastic container, because poly-L-lysine adheres to glass. Poly-L-Lysine solution may be reused. Keep the other slide filled racks in dH2O, while the first 3 are being coated. 7. After the lysine coating, rinse the slides by gently plunging up and down in 2 different changes of water. Spin dry 5' at 600 rpm. Place paper towels below rack to absorb liquid. 8. Store slides in a dessicator for 3 weeks prior to use. Slides that are older than 3 months may result in faint printing and higher background. Be sure to clean racks and containers thoroughly after each use. Built-up poly-L-Lysine on the sides of the containers may cause problems.; Protocol Type = Treatment; Performer: Kevin,,Visconti
Labeling - Channel 2; Methods for labeling extracted molecules that are used in hybridizations and scanned in Channel 2 (red); Protocol Type = Labeling; Parameter Amount of extract labeled = 1.5ug of total RNA; Parameter Type of label = Cy5; Performer: Kevin,,Visconti
 
 
Hybridization protocol not provided
Scan protocol GenePix
Description Image: http://smd.stanford.edu/MicroArray/gifs/2001-08/19041.gif
Data processing VALUE is Log (base 2) of the ratio of the mean of Channel 2 (usually 635 nm) to Channel 1 (usually 532 nm)
 
Submission date May 18, 2009
Last update date May 18, 2009
Contact name Martin I Voskuil
E-mail(s) martin.voskuil@ucdenver.edu
Phone 303-724-4219
Organization name University of Colorado Denver
Department Microbiology
Lab Voskuil Lab
Street address 12800 E. 19th Ave
City Aurora
State/province CO
ZIP/Postal code 80045
Country USA
 
Platform ID GPL8561
Series (1)
GSE16146 The response of Mycobacterium tuberculosis to reactive oxygen and nitrogen species

Data table header descriptions
ID_REF ID_REF
CH1I_MEAN Uncorrected Cy3 mean pixel intensity.; Type: integer; Scale: linear_scale; Channel: Cy3 Channel
CH2I_MEAN Uncorrected Cy3 mean pixel intensity.; Type: integer; Scale: linear_scale; Channel: Cy5 channel
CH1B_MEDIAN Median intensities of background pixels of Cy3.; Type: integer; Scale: linear_scale; Channel: Cy3 Channel
CH2B_MEDIAN Median intensities of background pixels of Cy3.; Type: integer; Scale: linear_scale; Channel: Cy5 channel
CH1D_MEAN The mean feature pixel intensity with the median background subtracted (channel 1).; Type: integer; Scale: linear_scale; Channel: Cy3 Channel
CH2D_MEAN The mean feature pixel intensity with the median background subtracted (channel 2).; Type: integer; Scale: linear_scale; Channel: Cy5 channel
CH1B_MEAN Mean intensities of background pixels of Cy3.; Type: integer; Scale: linear_scale; Background
CH2B_MEAN Mean intensities of background pixels of Cy5.; Type: integer; Scale: linear_scale; Background
PERGTBCH1I_1SD The percentage of feature pixels with intensities more than one standard deviation above the background pixel intensity, at wavelength 532 nm.; Type: integer; Scale: linear_scale
PERGTBCH2I_1SD The percentage of feature pixels with intensities more than one standard deviation above the background pixel intensity, at wavelength 635 nm.; Type: integer; Scale: linear_scale
PIX_RAT2_MEDIAN Contains median of Ch2PI-CH2B/Ch1PI-CH1B where Ch1PI & Ch2PI represent single pixel intensities.; Type: float; Scale: linear_scale
TOT_SPIX Count of the number of pixels in the spot.; Type: integer; Scale: linear_scale
TOT_BPIX Number of background pixels.; Type: integer; Scale: linear_scale
REGR The regression ratio of every pixel in a 2-feature-diameter circle around the center of the feature.; Type: float; Scale: linear_scale
CORR The correlation between channel1 (Cy3) & Channel 2 (Cy5) pixels within the spot, and is a useful quality control parameter. Generally, high values imply better fit & good spot quality.; Type: float; Scale: linear_scale
TOP Box top: int(((centerX - radius) - Xoffset) / pixelSize).; Type: integer; Scale: linear_scale
BOT Box bottom: int(((centerX + radius) - Xoffset) / pixelSize).; Type: integer; Scale: linear_scale
LEFT Box left: int(((centerY - radius) - yoffset) / pixelSize).; Type: integer; Scale: linear_scale
RIGHT Box right: int(((centerY + radius) - yoffset) / pixelSize); Type: integer; Scale: linear_scale
FLAG User defined spot flag (default 0).; Type: integer; Scale: linear_scale
CH2IN_MEAN Normalized value of mean Channel 2 (usually 635 nm) intensity (CH2I_MEAN/Normalization factor).; Type: integer; Scale: linear_scale; Channel: Cy5 channel
CH2BN_MEDIAN Normalized value of median Channel 2 (usually 635 nm) background (CH2B_MEDIAN/Normalization factor).; Type: integer; Scale: linear_scale; Channel: Cy5 channel; Background
CH2DN_MEAN Normalized value of mean Channel 2 (usually 635 nm) intensity with normalized background subtracted (CH2IN_MEAN - CH2BN_MEDIAN).; Type: integer; Scale: linear_scale; Channel: Cy5 channel
RAT2N_MEAN Type: float; Scale: linear_scale
RAT1N_MEAN Ratio of the means of Channel 1 (usually 532 nm) intensity to normalized Channel 2 (usually 635 nm) intensity with median background subtracted (CH1D_MEAN/CH2DN_MEAN). Channel 1/Channel 2 ratio normalized or Green/Red ratio normalized.; Type: float; Scale: linear_scale
VALUE Log (base 2) of the ratio of the mean of Channel 2 (usually 635 nm) to Channel 1 (usually 532 nm) [log (base 2) (RAT2N_MEAN)].; Type: float; Scale: log_base_2

Data table
ID_REF CH1I_MEAN CH2I_MEAN CH1B_MEDIAN CH2B_MEDIAN CH1D_MEAN CH2D_MEAN CH1B_MEAN CH2B_MEAN PERGTBCH1I_1SD PERGTBCH2I_1SD PIX_RAT2_MEDIAN TOT_SPIX TOT_BPIX REGR CORR TOP BOT LEFT RIGHT FLAG CH2IN_MEAN CH2BN_MEDIAN CH2DN_MEAN RAT2N_MEAN RAT1N_MEAN VALUE
1 2761 2944 1209 1112 1552 1832 1307 1180 58 60 1.014 137 1429 .791 .675 126 139 156 169 0 4529 1711 2818 1.816 .551 .861
2 2717 2569 1249 1062 1468 1507 1341 1158 50 53 .778 137 1390 .625 .609 125 138 178 191 0 3952 1634 2318 1.579 .633 .659
3 1819 1827 1229 1098 590 729 1305 1154 29 39 1.148 137 1409 .59 .571 125 138 200 213 0 2811 1689 1122 1.901 .526 .927
4 1693 1669 1196 1134 497 535 1268 1194 26 28 .849 137 1398 .491 .504 125 138 223 236 0 2568 1745 823 1.656 .604 .728
5 1540 1562 1184 1139 356 423 1243 1191 21 22 1.141 137 1386 .417 .39 125 138 245 258 0 2403 1752 651 1.828 .547 .87
6 1615 1419 1187 1105 428 314 1244 1158 27 20 .743 137 1381 .486 .462 125 138 268 281 0 2183 1700 483 1.129 .886 .175
7 1559 1475 1198 1083 361 392 1248 1152 25 23 .886 137 1379 .58 .524 125 138 290 303 0 2269 1666 603 1.671 .599 .74
8 1619 1436 1183 1082 436 354 1234 1154 26 27 .82 137 1390 .401 .446 125 138 313 326 0 2209 1665 545 1.249 .801 .321
9 1577 1405 1141 1038 436 367 1194 1101 28 31 .881 137 1390 .379 .431 125 138 335 348 0 2162 1597 565 1.295 .772 .373
10 15573 19537 1028 951 14545 18586 1133 1004 78 79 1.175 177 1360 1.101 .838 123 138 359 374 0 30057 1463 28594 1.966 .509 .975
11 10376 13825 1077 965 9299 12860 1213 1033 73 79 1.251 177 1331 1.165 .818 123 138 381 396 0 21269 1485 19785 2.128 .47 1.089
12 8971 11295 1144 1045 7827 10250 1282 1182 71 77 1.279 177 1335 1.131 .859 123 138 404 419 0 17377 1608 15769 2.015 .496 1.011
13 1588 1451 1084 1001 504 450 1181 1145 29 31 .867 137 1321 .56 .439 124 137 425 438 0 2232 1540 692 1.374 .728 .458
14 1552 1531 1075 1002 477 529 1127 1060 27 30 1.118 137 1333 .53 .502 124 137 448 461 0 2355 1542 814 1.706 .586 .771
15 1573 1391 1117 1037 456 354 1157 1099 26 24 .799 137 1349 .383 .476 124 137 470 483 0 2140 1595 545 1.194 .837 .256
16 1442 1498 1122 1023 320 475 1197 1111 22 23 .856 137 1340 .574 .369 124 137 492 505 0 2305 1574 731 2.284 .438 1.191
17 3114 3728 1159 1024 1955 2704 1217 1089 55 80 1.627 137 1368 .832 .703 124 137 515 528 0 5735 1575 4160 2.128 .47 1.089
18 3580 5004 1154 1019 2426 3985 1221 1124 71 92 1.601 137 1402 1.072 .73 124 137 537 550 0 7698 1568 6131 2.527 .396 1.337
19 8437 9722 1130 1021 7307 8701 1313 1202 88 94 1.131 137 1456 1.028 .902 123 136 560 573 0 14957 1571 13386 1.832 .546 .873
20 1618 1764 1149 1092 469 672 1231 1140 27 31 1.225 137 1394 .559 .456 148 161 155 168 0 2714 1680 1034 2.204 .454 1.14

Total number of rows: 5760

Table truncated, full table size 714 Kbytes.




Supplementary data files not provided
Processed data included within Sample table

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