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Links from GEO DataSets

Items: 20

1.

cRNA amplification methods enhance microarray identification of transcripts expressed in the nervous system

(Submitter supplied) Background: DNA microarrays provide a powerful method for global analysis of gene expression. The application of this technology to specific cell types and tissues, however, is typically limited by small amounts of available mRNA, thereby necessitating amplification. Here we compare microarray results obtained with two different methods of RNA amplification to profile gene expression in the C. elegans larval nervous system. more...
Organism:
Caenorhabditis elegans
Type:
Expression profiling by array
Platform:
GPL200
8 Samples
Download data: CEL, CHP
Series
Accession:
GSE9485
ID:
200009485
2.

Cell-specific microarray profiling of the C. elegans nervous system.

(Submitter supplied) Background: With its fully sequenced genome and simple, well-defined nervous system, the nematode C. elegans offers a unique opportunity to correlate gene expression with neuronal differentiation. The lineal origin, cellular morphology and synaptic connectivity of each of the 302 neurons are known. In many instances, specific behaviors can be attributed to particular neurons or circuits. Here we describe microarray-based methods that monitor gene expression in C. more...
Organism:
Caenorhabditis elegans
Type:
Expression profiling by array
Platform:
GPL200
24 Samples
Download data: CEL, CHP, EXP
Series
Accession:
GSE8004
ID:
200008004
3.

A gene expression fingerprint of C. elegans embryonic motor neurons.

(Submitter supplied) Background: Differential gene expression specifies the highly diverse cell types that constitute the nervous system. With its sequenced genome and simple, well-defined neuroanatomy, the nematode C. elegans is a useful model system in which to correlate gene expression with neuron identity. The UNC-4 transcription factor is expressed in thirteen embryonic motor neurons where it specifies axonal morphology and synaptic function. more...
Organism:
Caenorhabditis elegans
Type:
Expression profiling by array
Dataset:
GDS2786
Platform:
GPL200
7 Samples
Download data: CEL, EXP
Series
Accession:
GSE8159
ID:
200008159
4.
Full record GDS2786

Embryonic motor neurons

Analysis of embryonic motor neurons marked with an unc-4::GFP reporter transgene. UNC-4 is a homoedomain transcription factor expressed in 13 embryonic motor neurons. Results contribute to a comprehensive picture of gene expression in a subset of motor neurons.
Organism:
Caenorhabditis elegans
Type:
Expression profiling by array, count, 2 cell type sets
Platform:
GPL200
Series:
GSE8159
7 Samples
Download data: CEL, EXP
5.

Use of an Isothermal Linear Amplification Method with Small Samples on DNA Microarrays

(Submitter supplied) Experiment 1: U133A arrays (2) hybridized to duplicate sscDNA samples prepared from 20 ng Clontech UHR RNA Experiment 2: Mu6500A arrays (6) hybridized to triplicate sscDNA samples prepared from 3 x 5 ng mouse liver RNA and 3 x 100 ng mouse liver RNA Experiment 3: U95Av2 arrays (6) hybridized to triplicate sscDNA samples prepared from 3 x 10 ng K562 RNA and 3 x 10 ng Stratagene UHR RNA Experiment 4: U95Av2 array (1) hybridized to sscDNA sample prepared from template minus reaction (negative control) Keywords: parallel sample
Organism:
Mus musculus; unidentified; Homo sapiens
Type:
Expression profiling by array
Platforms:
GPL8300 GPL96 GPL1857
15 Samples
Download data: CEL, EXP
Series
Accession:
GSE2252
ID:
200002252
6.

Evaluation of methods for amplification of picogram amounts of total RNA for whole genome expression profiling

(Submitter supplied) For more than a decade, microarrays have been a powerful and widely used tool to explore the transcriptome of biological systems. However, the amount of biological material from cell sorting or laser capture microdissection is much too small to perform microarray studies. To address this issue, RNA amplification methods have been developed to generate sufficient targets from picogram amounts of total RNA to perform microarray hybridisation. more...
Organism:
Homo sapiens
Type:
Expression profiling by array
Platform:
GPL570
27 Samples
Download data: CEL, CHP
Series
Accession:
GSE15398
ID:
200015398
7.

T7-based linear amplification of low concentration mRNA samples using beads and microfluidics

(Submitter supplied) We have demonstrated in vitro transcription (IVT) of cDNA sequences from purified Jurkat T-cell mRNA immobilization on microfluidic packed beads down to single-cell quantities. The microfluidic amplified aRNA was nearly identical in length and quantity compared with benchtop reactions using the same starting sample quantities. Microarrays were used to characterize the number and population of genes in each sample, allowing comparison of the microfluidic and benchtop processes. more...
Organism:
Homo sapiens
Type:
Expression profiling by array
Platform:
GPL6098
36 Samples
Download data
Series
Accession:
GSE13595
ID:
200013595
8.

Gene Expression Profiling of Whole Blood: Comparison of target preparation methods

(Submitter supplied) Peripheral blood is an accessible and informative source of transcriptomal information for many human disease and pharmacogenomic studies. While there can be significant advantages to analyzing RNA isolated from whole blood, particularly in clinical studies, the preparation of samples for microarray analysis is complicated by the need to minimize artifacts associated with highly abundant globin RNA transcripts. more...
Organism:
Homo sapiens
Type:
Expression profiling by array
Platform:
GPL201
24 Samples
Download data: CEL, CHP
Series
Accession:
GSE13292
ID:
200013292
9.

Expression data from the PVD and OLL neurons in C. elegans

(Submitter supplied) Nociceptive neurons develop a complex dendritic arbor to sense noxious stimuli, which enables animals to react to environmental insults and perform self-protective behaviours. The genetic programs controlling neuronal dendritic morphogenesis are poorly understood. In C. elegans, the PVD sensory neuron generates a complex dendritic arbor that envelops the body of the animal. This nociceptive neuron enables study of dendrite formation in vivo. more...
Organism:
Caenorhabditis elegans
Type:
Expression profiling by array
Platform:
GPL200
6 Samples
Download data: CEL
Series
Accession:
GSE21162
ID:
200021162
10.

Comparison between NuGEN's WT-Ovation Pico and One-Direct Amplification Systems

(Submitter supplied) Differential gene expression between groups of homogenous cell types is a biological question whose time has come. RNA can be extracted from small numbers of cells, such as those isolated by laser capture microdissection, but the small amounts obtained often require amplification to enable whole genome transcriptome profiling by technologies such as microarray analysis and RNA-seq. Recently, advances in amplification procedures make amplification directly from whole cell lysates possible. more...
Organism:
Arabidopsis thaliana
Type:
Expression profiling by array
Platform:
GPL198
20 Samples
Download data: CEL
Series
Accession:
GSE21981
ID:
200021981
11.

Variability in Microarray Labeling Methods

(Submitter supplied) Considerable variation in gene expression data from different DNA microarray platforms has been demonstrated. However, no characterization of the source of variation arising from labeling protocols has been performed. To analyze the variation associated with T7-based RNA amplification/labeling methods, aliquots of the Stratagene Human Universal Reference RNA were labeled using 3 eukaryotic target preparation methods and hybridized to a single array type (Affymetrix U95Av2). more...
Organism:
Homo sapiens
Type:
Expression profiling by array
Dataset:
GDS1954
Platform:
GPL8300
20 Samples
Download data: CEL, EXP
Series
Accession:
GSE3254
ID:
200003254
12.
Full record GDS1954

Various T7 RNA polymerase-based RNA amplification/labeling methods

Comparison of expression profiles generated using various T7 RNA polymerase-based in vitro transcription (IVT) RNA labeling methods. The length of the IVT reactions ranged from 4 to 16 hours. Results provide evidence for amplification method-dependent biases in gene expression data.
Organism:
Homo sapiens
Type:
Expression profiling by array, count, 3 protocol, 3 time sets
Platform:
GPL8300
Series:
GSE3254
20 Samples
Download data: CEL, EXP
13.

Comparison of linear and exponential protocols using moderate amplifications

(Submitter supplied) Gene expression profiling has become a tool of choice to study pathological or developmental questions but in most cases the material is scarce and requires sample amplification. Two main procedures have been used: in vitro transcription (IVT) and polymerase chain reaction (PCR), the former known as linear and the latter as exponential. Previous reports identified enzymatic pitfalls in PCR and IVT protocols; however the possible differences between the sequences affected by these amplification defaults were only rarely explored. more...
Organism:
Bos taurus
Type:
Expression profiling by array
Platform:
GPL6284
96 Samples
Download data
Series
Accession:
GSE9929
ID:
200009929
14.

TAcKLE - Transcriptome Amplification and cDNA Labeling for Expression analysis

(Submitter supplied) To characterize the properties and evaluate the performance of the TAcKLE procedure, a novel method providing effective transcriptome amplification for expression analyses on oligonucleotide microarrays, we performed 20 two-color hybridizations using self-spotted Operon 27k arrays. A single source of universal human reference RNA (pooled from 10 cell lines) and RNA extracted from healthy breast tissue was used for all experiments to avoid differences in transcript abundance imposed by the RNA preparation. more...
Organism:
Homo sapiens
Type:
Expression profiling by array
Platform:
GPL1384
20 Samples
Download data: TIFF
Series
Accession:
GSE1645
ID:
200001645
15.

DKFZ Operon 27k long oligonucleotide array

(Submitter supplied) Spotted long oligonucleotide array produced using the Operon Human Genome Oligo Set Version 2.1 (21,329 70mer oligonucleotides, based on build 147 of the Human UniGene database and the Human RefSeq Database, plus 24 controls) and the Operon Human Genome Oligo Set Version 2.1 Upgrade (5,462 70mer oligonucleotides, based on build 13.31 of the Human Ensembl Database). Spotting was performed in duplicates (replicate arrays) with 4x6 SMP3 pins (Telechem) at 18-20 °C and 40-50% RH on epoxysilane coated slides (Quantifoil) using 40 µM oligos in FBNC spotting buffer (G. more...
Organism:
Homo sapiens
2 Series
32 Samples
Download data
Platform
Accession:
GPL1384
ID:
100001384
16.

Microarray Based Comparison of three Amplification Methods For Nanogram Amounts of Total RNA

(Submitter supplied) Two T7 based methods One round of Amplification (Affymetrix) and Two round of Amplification were compared to two Ribo-SPIA based systems, RiboSPIA and pico Ribo SPIA systems. Data for Pico-RiboSPIA are listed here. All Hybridisation were performed using Affymetrix Mouse 430-2 gene chips. Data were all scaled to 500. For 12 chips performed with pico Ribo SPIA the scaling factor average was 2.0 +/- 0.3, background intensities 74.4 +/- 12.7 , noise 3.9 +/- 0.6, rawQ 2.5 +/- 0.3 Keywords: ordered
Organism:
Mus musculus
Type:
Expression profiling by array
Platform:
GPL1261
12 Samples
Download data: CEL
Series
Accession:
GSE2019
ID:
200002019
17.

Microarray Based Comparison of two Amplification Methods For Nanogram Amounts of Total RNA

(Submitter supplied) Two T7 based methods One round of Amplification (Affymetrix) and Two round of Amplification were compared to two Ribo-SPIA based systems, RiboSPIA and pico Ribo SPIA systems. Data for One Round of amplification , Two round of amplification and RiboSPIA are listed here. All Hybridisation were performed using Affymetrix Mouse 430-2 gene chips. Data were all scaled to 500 and scaling factor average was 3.6 +/- 0.9, background intensities 46 +/- 5 , noise 2.9 +/- 0.6, rawQ 1.5 +/- 0.2 Keywords: other
Organism:
Mus musculus
Type:
Expression profiling by array
Platform:
GPL1261
27 Samples
Download data: CEL, RPT, TXT
Series
Accession:
GSE1435
ID:
200001435
18.

Strand-specific transcriptome profiling with directly labeled RNA on genomic tiling microarrays

(Submitter supplied) Background: With lower manufacturing cost, high spot density, and flexible probe design, genomic tiling microarrays are ideal for comprehensive transcriptome studies. Typically, transcriptome profiling using microarrays involves reverse transcription, which converts RNA to cDNA. The cDNA is then labeled and hybridized to the probes on the arrays, thus the RNA signals are detected indirectly. Reverse transcription is known to generate artifactual cDNA, in particular the synthesis of second-strand cDNA, leading to false discovery of antisense RNA. more...
Organism:
Porphyromonas gingivalis; Porphyromonas gingivalis W83
Type:
Expression profiling by genome tiling array
Platform:
GPL11291
18 Samples
Download data: PAIR
Series
Accession:
GSE25876
ID:
200025876
19.

Whole transcription data for mouse spermatogonial cells

(Submitter supplied) Spermatogenesis is a multi-step yet tightly regulated developmental process to produce male gemetes for reproduction. In mouse spermatogenesis, a sub-group of type A spermatogonia (Spga) known as spermatogonial stem cells (SSCs) maintain their population by self-renewal, and differentiate through mitosis and meiosis to form tetraploid (4n) pacchytene spermatocytes (Spcy) and haploid (n) round spermatids (Sptd), which further differentiate into functional sperms. more...
Organism:
Mus musculus
Type:
Expression profiling by genome tiling array
14 related Platforms
126 Samples
Download data: BAR, CEL
Series
Accession:
GSE55381
ID:
200055381
20.

Flexible multiplatform RNA profiling at the single cell level applied to enriched cancer initiating cells

(Submitter supplied) This SuperSeries is composed of the SubSeries listed below.
Organism:
Homo sapiens
Type:
Expression profiling by array; Expression profiling by high throughput sequencing; Expression profiling by RT-PCR
Platforms:
GPL17989 GPL570 GPL16288
64 Samples
Download data: CEL
Series
Accession:
GSE52717
ID:
200052717
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