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GSE16678

GSE GEO
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MicroRNA expression data from differentiation of human Cyt49 ESCs into definitive endoderm in feeder-free conditions

Organism: Homo sapiens
Platform: GPL8733
Samples: 8
Experiment Types:
Non-coding RNA profiling by array
Submitted: Jun 17 2009
Last Updated: Mar 21 2012
Status: Public on Jul 30 2010
Contact: Andrew,,Hinton (UC, San Diego)

Relations

SubSeries of: GSE16690 BioProject: https://www.ncbi.nlm.nih.gov/bioproject/PRJNA122715

Summary

Pluripotent hESCs can differentiate into the three primary embryonic lineages (endoderm, mesoderm, ectoderm) as well as extraembryonic tissues. Definitive endoderm is the first step into the pathway to endoderm dreived tissues (pancreas, liver, gut, lung). We used microarrays to detail the changes in microRNA expression during the transition from pluripotent hESCs into definitive endoderm.

Overall Design

hESCs (Cyt49) were differentiated in the presence of Activin A and Wnt3A under low serum conditions to induce DE formation. Samples were collected at day 0 (2 samples), day 2 (3 samples) and day 4 (3 samples).

Analysis (7 steps)

View Data Processing
Processing steps for GSE16678
  1. The signal processing implemented for the Ambion miRCHIP is a multi-step process involving probe specific signal detection calls, background estimate and correction, constant variance stabilization and either array scaling or global normalization.
  2. For each probe, an estimated background value is subtracted that is derived from the median signal of a set of G-C matched anti-genomic controls.
  3. Arrays within a specific analysis experiment were normalized together according to the variance stabilization methods described by Huber et al. (Huber et al., 2002).
  4. Detection calls were based on a Wilcoxon rank-sum test of the miRNA probe signal compared to the distribution of signals from GC-content matched anti-genomic probes.
  5. For statistical hypothesis testing, a two-sample t-Test, with assumption of equal variance, was applied.
  6. One-way ANOVA was used for experimental designs with more than two experimental groupings or levels of the same factor.
  7. These tests define which probes are considered to be significantly differentially expressed, or significant, based on a default p-value of 0.001 and log2 difference > 1.

Supplementary Files (1)

GSE16678_RAW.tar Download
GEO Samples (8)
GSM418003 GSM418004 GSM418005 GSM418006 GSM418007 GSM418008 GSM418009 GSM418010

Dataset Citations (1)

A distinct microRNA signature for definitive endoderm derived from human embryonic stem cells.
PMID 19807270 · 2010 · Stem cells and development
Andrew Hinton, Ivka Afrikanova, Mike Wilson, Charles C King, Brian Maurer, Gene W Yeo, Alberto Hayek, Amy E Pasquinelli

Linked Publications (1)

A distinct microRNA signature for definitive endoderm derived from human embryonic stem cells.
Stem cells and development · 2010