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Sample GSM461232 Query DataSets for GSM461232
Status Public on Apr 08, 2010
Title SYNW1019_mutant_bsy89280d0054_rep5
Sample type RNA
 
Channel 1
Source name ptrA mutant MO7r-synw1019-p5
Organism Parasynechococcus marenigrum WH 8102
Characteristics strain: ptrA mutant
Biomaterial provider Martin Ostrowski
Growth protocol Cells were grown in 1 liter of artificial seawater (SOW) containing 4.5 millimolar NaNO3, 90 micromolar Na2PO4, 100 micromolar NH4Cl, 13.4 micromolar Na2EDTA, 10 micromolar Na2CO3, and 10 micromolar phosphate to just after onset of phosphatase activity in wild-type WH8102 (~125-150 hours after inoculation).
Extracted molecule total RNA
Extraction protocol RNA was extracted from one litre of harvested exponential phase cells using Trizol (Invitrogen) according to the manufacturer's recommendation. RNA was resuspended in 100 microliters DEPC-treated water. RNA was digested twice with DNase I (Qiagen) using an RNeasy Mini Kit (Qiagen) according to the manufacturer's instructions. RNA yield and purity were determined by measuring optical density spectrophotometrically at 260 and 280 nm. RNA was stored at -80 degrees C.
Label Cy3
Label protocol Make spike-in control pools from RNA amplified from cloned Arabidopsis thaliana genes (cab, ltp4, rca, rbcL, ltp6, rcp1, nac, xcp2, prk, and tim) using the MegaScript Kit (Ambion) by combining for Cy5 pool:
5.2 microliters 20.3 ng/microliter cab RNA;
12.5 microliters 16.839 ng/microliter ltp4 RNA;
18.6 microliters 22.634 ng/microliter rca RNA;
41.8 microliters 15.068 ng/microliter rbcL RNA;
4.7 microliters 13.279 ng/microliter ltp6 RNA;
11.8 microliters 21.313 ng/microliter rcp1 RNA;
40.7 microliters 23.23 ng/microliter nac RNA;
4.6 microliters 18.177 ng/microliter xcp2 RNA;
14.7 microliters 11.436 ng/microliter prk RNA;
18.9 microliters 11.084 ng/microliter tim RNA;
826.5 microliters water.
And for Cy3 pool:
5.2 microliters 20.3 ng/microliter cab RNA;
12.5 microliters 16.839 ng/microliter ltp4 RNA;
18.6 microliters 22.634 ng/microliter rca RNA;
41.8 microliters 15.068 ng/microliter rbcL RNA;
1.6 microliters 13.279 ng/microliter ltp6 RNA;
3.9 microliters 21.313 ng/microliter rcp1 RNA;
13.6 microliters 23.23 ng/microliter nac RNA;
13.9 microliters 18.177 ng/microliter xcp2 RNA;
44.1 microliters 11.436 ng/microliter prk RNA;
56.8 microliters 11.084 ng/microliter tim RNA;
788.1 microliters water.
To label RNA sample combine:
4 micrograms RNA;
2 microliters 3 mg/mL random hexamers (Invitrogen);
2 microliters arabidopsis spike-in control RNA;
DEPC water to a final volume to 17.5 microliters.
Mix and incubated at 70 degrees C for 10 minutes.
Snap-freeze in dry ice/ethanol for 30 seconds and centrifuged for 1 minute at approximately 16,000g.
Add:
6 microliters 5X Superscript II buffer (Invitrogen);
3 microliters 0.1 M dithiothreitol;
1.2 microliters aminoallyl-dNTP mix containing 12.5 mM dATP, 12.5 mM dCTP, 12.5 mM dGTP, 4.16 mM dTTP, and 8.33 mM aadUTP;
2 microliters SuperScript II (Invitrogen).
Mix and incubated overnight at 42 degrees C.
Add:
10 microliters 1 M NaOH;
10 microliters 0.5 M EDTA.
Incubate for 15 minutes at 65 degrees C.
Add:
25 microliters 1 M Tris pH 7.4;
400 microliters PB buffer (Qiagen).
Apply sample to QIAquick column (Qiagen).
Centrifuge for 1 minute at 15,000g.
Wash with 750 microliters phosphate wash buffer (84.25 mL 95% EtOH + 15.25 mL water + 0.5 mL 1 M KPO4 pH 8.5 solution made by combining 0.5 mL 1M KH2PO4 with 9.5 mL 1M K2HPO4).
Centrifuge for 1 minute at 15,000g.
Repeat wash.
Empty collection tube and centrifuge for 1 minute at 15,000g.
Transfer column to fresh tube.
Add 30 microliters phosphate elution buffer (4 mM KPO4 solution made by diluting 1 M KPO4 pH 8.5 solution).
Incubate for 1 minute.
Centrifuge for 1 minute at 15,000g.
Repeat elution for a final volume of 60 microliters.
Dry sample using a speed vac.
Resuspend cDNA in 4.5 microliters 0.1 M carbonate buffer (1 M Na2CO3 buffer pH 9.0 diluted 1:10 with water).
Allow the sample to resuspend for 15 minutes at room temperature.
Add 4.5 microliters NHS-Cy (Amersham) resuspended in 73 microliters DMSO.
Incubate for 1 hour at room temperature in the dark.
Add 4.5 microliters 4 M hydroxylamine.
Incubate for 15 minutes at room temperature in the dark.
Add:
35 microliters 100 mM NaOAc pH 5.2;
500 microliters PB buffer.
Apply to Qiaquick column.
Centrifuge for 1 minute at 15,000g.
Wash with 750 microliters PE buffer (Qiagen).
Centrifuge for 1 minute at 15,000g.
Repeat wash.
Empty collection tube and centrifuge for 1 minute at 15,000g.
Transfer column to fresh tube.
Add 30 microliters EB buffer (Qiagen).
Incubate for 1 minute.
Centrifuge for 1 minute at 15,000g.
Repeat elution for a final volume of 60 microliters.
Check quality of probes spectrophotometrically from 200nm to 700nm.
Store at -80 degrees C.
 
Channel 2
Source name wild type WH8102 MO8r-WH8102-w5
Organism Parasynechococcus marenigrum WH 8102
Characteristics strain: wild type
Biomaterial provider Martin Ostrowski
Growth protocol Cells were grown in 1 liter of artificial seawater (SOW) containing 4.5 millimolar NaNO3, 90 micromolar Na2PO4, 100 micromolar NH4Cl, 13.4 micromolar Na2EDTA, 10 micromolar Na2CO3, and 10 micromolar phosphate to just after onset of phosphatase activity in wild-type WH8102 (~125-150 hours after inoculation).
Extracted molecule total RNA
Extraction protocol RNA was extracted from one litre of harvested exponential phase cells using Trizol (Invitrogen) according to the manufacturer's recommendation. RNA was resuspended in 100 microliters DEPC-treated water. RNA was digested twice with DNase I (Qiagen) using an RNeasy Mini Kit (Qiagen) according to the manufacturer's instructions. RNA yield and purity were determined by measuring optical density spectrophotometrically at 260 and 280 nm. RNA was stored at -80 degrees C.
Label Cy5
Label protocol Make spike-in control pools from RNA amplified from cloned Arabidopsis thaliana genes (cab, ltp4, rca, rbcL, ltp6, rcp1, nac, xcp2, prk, and tim) using the MegaScript Kit (Ambion) by combining for Cy5 pool:
5.2 microliters 20.3 ng/microliter cab RNA;
12.5 microliters 16.839 ng/microliter ltp4 RNA;
18.6 microliters 22.634 ng/microliter rca RNA;
41.8 microliters 15.068 ng/microliter rbcL RNA;
4.7 microliters 13.279 ng/microliter ltp6 RNA;
11.8 microliters 21.313 ng/microliter rcp1 RNA;
40.7 microliters 23.23 ng/microliter nac RNA;
4.6 microliters 18.177 ng/microliter xcp2 RNA;
14.7 microliters 11.436 ng/microliter prk RNA;
18.9 microliters 11.084 ng/microliter tim RNA;
826.5 microliters water.
And for Cy3 pool:
5.2 microliters 20.3 ng/microliter cab RNA;
12.5 microliters 16.839 ng/microliter ltp4 RNA;
18.6 microliters 22.634 ng/microliter rca RNA;
41.8 microliters 15.068 ng/microliter rbcL RNA;
1.6 microliters 13.279 ng/microliter ltp6 RNA;
3.9 microliters 21.313 ng/microliter rcp1 RNA;
13.6 microliters 23.23 ng/microliter nac RNA;
13.9 microliters 18.177 ng/microliter xcp2 RNA;
44.1 microliters 11.436 ng/microliter prk RNA;
56.8 microliters 11.084 ng/microliter tim RNA;
788.1 microliters water.
To label RNA sample combine:
4 micrograms RNA;
2 microliters 3 mg/mL random hexamers (Invitrogen);
2 microliters arabidopsis spike-in control RNA;
DEPC water to a final volume to 17.5 microliters.
Mix and incubated at 70 degrees C for 10 minutes.
Snap-freeze in dry ice/ethanol for 30 seconds and centrifuged for 1 minute at approximately 16,000g.
Add:
6 microliters 5X Superscript II buffer (Invitrogen);
3 microliters 0.1 M dithiothreitol;
1.2 microliters aminoallyl-dNTP mix containing 12.5 mM dATP, 12.5 mM dCTP, 12.5 mM dGTP, 4.16 mM dTTP, and 8.33 mM aadUTP;
2 microliters SuperScript II (Invitrogen).
Mix and incubated overnight at 42 degrees C.
Add:
10 microliters 1 M NaOH;
10 microliters 0.5 M EDTA.
Incubate for 15 minutes at 65 degrees C.
Add:
25 microliters 1 M Tris pH 7.4;
400 microliters PB buffer (Qiagen).
Apply sample to QIAquick column (Qiagen).
Centrifuge for 1 minute at 15,000g.
Wash with 750 microliters phosphate wash buffer (84.25 mL 95% EtOH + 15.25 mL water + 0.5 mL 1 M KPO4 pH 8.5 solution made by combining 0.5 mL 1M KH2PO4 with 9.5 mL 1M K2HPO4).
Centrifuge for 1 minute at 15,000g.
Repeat wash.
Empty collection tube and centrifuge for 1 minute at 15,000g.
Transfer column to fresh tube.
Add 30 microliters phosphate elution buffer (4 mM KPO4 solution made by diluting 1 M KPO4 pH 8.5 solution).
Incubate for 1 minute.
Centrifuge for 1 minute at 15,000g.
Repeat elution for a final volume of 60 microliters.
Dry sample using a speed vac.
Resuspend cDNA in 4.5 microliters 0.1 M carbonate buffer (1 M Na2CO3 buffer pH 9.0 diluted 1:10 with water).
Allow the sample to resuspend for 15 minutes at room temperature.
Add 4.5 microliters NHS-Cy (Amersham) resuspended in 73 microliters DMSO.
Incubate for 1 hour at room temperature in the dark.
Add 4.5 microliters 4 M hydroxylamine.
Incubate for 15 minutes at room temperature in the dark.
Add:
35 microliters 100 mM NaOAc pH 5.2;
500 microliters PB buffer.
Apply to Qiaquick column.
Centrifuge for 1 minute at 15,000g.
Wash with 750 microliters PE buffer (Qiagen).
Centrifuge for 1 minute at 15,000g.
Repeat wash.
Empty collection tube and centrifuge for 1 minute at 15,000g.
Transfer column to fresh tube.
Add 30 microliters EB buffer (Qiagen).
Incubate for 1 minute.
Centrifuge for 1 minute at 15,000g.
Repeat elution for a final volume of 60 microliters.
Check quality of probes spectrophotometrically from 200nm to 700nm.
Store at -80 degrees C.
 
 
Hybridization protocol Combine Cy3 and Cy5 samples and 1 microliter cy-labeled arabidopsis 70-mer positional controls (This is a pool of 4 70-mers labeled with Cy3 and Cy5 for a total of 8 70-mers at 2 ng/microliter each. The sequences are: At2g14610a_219_rev - AAAAAAATATATCAACAATGGCAAAGCTACCGATACGAAACAATATTAGGAAAAATGTGTGTAAGGACAA; At2g14610b_265_rev - AATTTAAACTGCGTATTAGTGTTTGGAAAAAAAAAACAAAGTGTATACAATGTCAATCGGTGATCTTTTT; At2g14610c_305_rev - TTAATAACATATAATATTGAATAGGATATCATAGGATATTATTACGTAATAATATCCTATGGTGTCATTT; At2g14610d_298_rev - CGACTTTTCTTGCTTAGAAGTCTTTGCATTGTTAATAGATTGTTGAAAAGGTTTATTCATTACTTTCATG).
Dry using a speed vac.
Make pre-hybridization buffer by combining:
0.5 g BSA;
37 mL DEPC water;
12.5 mL 20X SSC;
0.5 mL 10% SDS.
Incubate pre-hybridization buffer for 20 minutes at 42 degrees C.
Filter using a 0.45 micrometer cellulose acetate filter into a coplin jar.
Incubate for 20 minutes at 42 degrees C.
Make hybridization buffer by combining:
500 microliters fomamide;
250 microliters 20X SSC;
10 microliters 10% SDS;
240 microliters DEPC water.
Filter hybridization buffer through a 0.45 micrometer cellulose acetate filter.
Add 50 uL sheared salmon sperm DNA (Ambion) to hybridization buffer.
Add 60 microliters hybridization buffer to speed vac-dried probes.
Put slide into pre-hybridization buffer in coplin jar.
Incubate for 45 minutes at 42 degrees C.
Wash slide 4 times in water and 3 times in isopropanol for 2 minutes per wash with gentle shaking by hand.
Dry slide by spinning.
Clean 25 mm x 60 mm lifterslip (Erie Scientific Company) by dipping in MilliQ water for 5 minutes at room temperature.
Dip in 100% EtOH and dry with a Chem Wipe.
Heat probes for 15 minutes at 95 degrees C with occassional "flicking" to resuspend probes.
Remove probes from heat block and centrifuge for 2 minutes at 15,000g.
Place lifterslip onto slide and add probes by allowing capillary action to pull the probes under the lifterslip.
Hybridize overnight at 42 degrees C.
Wash slide 2 times in glass staining dish with 1X SSC, 0.2% SDS for 5 minutes at 42 degrees C.
Wash slide in 0.1X SSC, 0.1% SDS for 5 minutes at room temperature.
Wash slide 3 times in 0.1X SSC for 5 minutes at room temperature.
Dry slide by spinning.
Scan protocol Slide were scanned at 10 micrometer resolution using an Axon 4000B scanner with GenePix 4.0 software.
Description This slide measures gene expression of a ptrA mutant under phosphorus-deplete conditions as compared to gene expression of wild-type WH8102 under the same conditions.
Data processing Tiff images were processed using TIGR-Spotfinder (www.tigr.org/software) with Otsu thresholding, a minimum spot size of 10 and a maximum spot size of 15, and applying the default quality control filter options. The data were normalized ignoring controls with the LOWESS algorithm in block mode with a smooth parameter of 0.33 by using TIGR-MIDAS (www.tigr.org/software).
 
Submission date Oct 09, 2009
Last update date Apr 08, 2010
Contact name Ian Paulsen
E-mail(s) ipaulsen@cbms.mq.edu.au
Organization name Macquarie University
Department Department of Chemistry and Biomolecular Sciences
Street address Macquarie University
City Sydney
State/province NSW
ZIP/Postal code 2109
Country Australia
 
Platform ID GPL7449
Series (1)
GSE18511 PtrA is required for coordinate regulation of gene expression during phosphate depletion in a marine Synechococcus

Data table header descriptions
ID_REF
IA spot intensity in channel A (cy3) corrected for background
IB spot intensity in channel B (cy5) corrected for background
VALUE log2 ratio of (experimental channel)/(reference channel)

Data table
ID_REF IA IB VALUE
791 189469 778035 -2.037873236
4351 113820 413504 -1.861147201
7191 173458 572253 -1.722066741
10751 114851 358844 -1.64359338
13591 226517 705542 -1.639112639
17151 151002 552251 -1.870756468
2068 194409 200262 -0.042793685
5628 177034 184562 -0.060079081
8468 176684 186408 -0.077292377
12028 145287 156704 -0.109136387
14868 209960 215809 -0.039640529
18428 175284 181168 -0.04763384
344 566456 238599 1.247375901
4144 697027 342544 1.024925226
6744 879748 322777 1.446552548
10544 617926 311665 0.987437929
13144 648706 295922 1.132347827
16944 996433 429250 1.214954668
675 97401 98114 -0.010522427
4475 63302 76593 -0.274961465

Total number of rows: 15156

Table truncated, full table size 468 Kbytes.




Supplementary file Size Download File type/resource
GSM461232_TAV_README.txt.gz 1.2 Kb (ftp)(http) TXT
GSM461232_bsy89280d0054_13049789_532_nm.tif.gz 16.9 Mb (ftp)(http) TIFF
GSM461232_bsy89280d0054_13049789_635_nm.tif.gz 16.2 Mb (ftp)(http) TIFF
GSM461232_bsy89280d0054_NIF.tav.gz 571.8 Kb (ftp)(http) TAV
Processed data included within Sample table
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