Gene Expression Omnibus (GEO) Overview Version：2013-04-06Japanese page

An overview of the GEO entries broken down by the measurement platforms and the features of the measured samples.

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Human (2,851)   Primates (0)   Rodents (2,590)   Mammals (0)   Vertebrates (0)   Invertebrates (0)   Plants (464)   Bacteria (0)   Viruses (0)   Phages (0)   Unclassified (0)   All (6,302)

SAGE NlaIII (0)   SAGE RsaI (0)   SAGE Sau3A (5)   MPSS (0)   GeneChip (2,621)   Tiling Array (0)   cDNA Array (1,964)   Oligo Array (1,212)   Bead Array (0)   Protein Array (0)   Antibody (0)   RT-PCR (0)   HT-Seq (0)   Other (0)   All (6,302)     brain (446)   blood (514)   connective (80)   reproductive (0)   muscular (0)   digestive (0)   liver (76)   lung (0)   urinary (0)   endo/exo-crine (355)   embryo (0)   adult aerial structure (0)   young aerial structure (0)   root (0)   meristem/growing tissue (0)   flower/sexual organ (0)   seed/fruit/grain (0)   pooled (23)   unclassified (259)   all (2,621)   1   |   2   |   3   |   4   |   5      »      [132] Sample ID Title Number of Data Institute Submission date Platform Sample type Species Organ class Reasoning of the classification Keywords used for the classification are shown with bold font. 1 GSM38128 Zn4 22,277 Duke University Medical Center 2004-12-26 [GeneChip] [HG-U133A] Affymetrix Human Genome U133A Array (GPL96) RNA Homo sapiens lung Primary human Bronchial epithelial cells 2 GSM38127 Zn3 22,277 Duke University Medical Center 2004-12-26 [GeneChip] [HG-U133A] Affymetrix Human Genome U133A Array (GPL96) RNA Homo sapiens lung Primary human Bronchial epithelial cells 3 GSM38126 Zn2 22,277 Duke University Medical Center 2004-12-26 [GeneChip] [HG-U133A] Affymetrix Human Genome U133A Array (GPL96) RNA Homo sapiens lung Primary human Bronchial epithelial cells 4 GSM38125 Zn1 22,277 Duke University Medical Center 2004-12-26 [GeneChip] [HG-U133A] Affymetrix Human Genome U133A Array (GPL96) RNA Homo sapiens lung Primary human Bronchial epithelial cells 5 GSM34701 YSS89, T=60, c 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=60, c description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 6 GSM34696 YSS89, T=60, b 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=60, b description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 7 GSM34691 YSS89, T=60 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=60 description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 8 GSM34700 YSS89, T=40, c 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=40, c description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 9 GSM34695 YSS89, T=40, b 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=40, b description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 10 GSM34690 YSS89, T=40 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=40 description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 11 GSM34699 YSS89, T=30, c 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=30, c description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 12 GSM34694 YSS89, T=30, b 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=30, b description:Experiment Design: Keywords = IFH1 Keywords = Transcriptional control of RP genes 13 GSM34689 YSS89, T=30 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=30 description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 14 GSM34698 YSS89, T=20, c 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=20, c description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 15 GSM34693 YSS89, T=20, b 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=20, b description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 16 GSM34688 YSS89, T=20 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=20 description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 17 GSM34697 YSS89, T=0, c 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=0, c description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 18 GSM34692 YSS89, T=0, b 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=0, b description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 19 GSM34687 YSS89, T=0 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS89, T=0 description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 20 GSM34686 YSS37, T=60, c 9,335 University of Geneva 2004-11-05 [GeneChip] [YG_S98] Affymetrix Yeast Genome S98 Array (GPL90) RNA Saccharomyces cerevisiae unclassified source_name:Yeast title:YSS37, T=60, c description:Experiment Design: •Type of experiment: time course after GAL (galactose) induction •Experimental factor: time, genotype •Number of hybridizations performed in the experiment: 24 (eight conditions with three biological replicates each) Samples used, extract preparation and labeling: •The origin of the biological sample: Species: S. cerevisiae Cell type: wild-type (YSS37, IFH1-13myc-TRP1, MATa) UASIFH1::HIS3-UASGAL1 (YSS89, UASGAL1-IFH1-13myc-TRP1, MATa) •Growth conditions: log phase (2x107/mL) at 30°C in YPLG medium, then addition of Galactose to 2% •Treatments: all cells were harvested by rapid centrifugation at 4°C then flash frozen in liquid nitrogen. •RNA extraction: RNeasy Protect mini kit (Quiagen) •Labeling protocol(s): cDNA synthesis using Invitrogen reagents according to Affymetrix protocol (5 µg of total RNA) GeneChip IVT labeling kit (Affymetrix) •External controls (spikes): according to the Affymetrix protocols Hybridization controls Poly-A spike controls Keywords = IFH1 Keywords = Transcriptional control of RP genes 1   |   2   |   3   |   4   |   5      »      [132]