Publication | Open Access
Identification of a Novel Gene Signature of ES Cells Self-Renewal Fluctuation through System-Wide Analysis
23
Citations
29
References
2014
Year
Gene Regulatory NetworkGene Expression ProfilingCellular PhysiologySupport Vector MachineNovel Gene SignatureSingle Cell SequencingStem CellsHealth SciencesSystem-wide AnalysisEscs BiologyGene ExpressionSingle-cell AnalysisEmbryonic Stem CellsCell BiologyFunctional GenomicsTumor MicroenvironmentInduced Pluripotent Stem CellSignal TransductionDevelopmental BiologySystems BiologyMedicineEmbryonic Stem Cell
Embryonic Stem cells (ESCs) can be differentiated into ectoderm, endoderm, and mesoderm derivatives, producing the majority of cell types. In regular culture conditions, ESCs' self-renewal is maintained through molecules that inhibit spontaneous differentiation enabling long-term cellular expansion. This undifferentiating condition is characterized by multiple metastable states that fluctuate between self-renewal and differentiation balance. Here, we aim to characterize the high-pluripotent ESC metastate marked by the expression of Zscan4 through a supervised machine learning framework based on an ensemble of support vector machine (SVM) classifiers. Our study revealed a leukaemia inhibitor factor (Lif) dependent not-canonical pluripotency signature (AF067063, BC061212, Dub1, Eif1a, Gm12794, Gm13871, Gm4340, Gm4850, Tcstv1/3, and Zfp352), that specifically marks Zscan4 ESCs' fluctuation. This novel ESC metastate is enhanced by high-pluripotency culture conditions obtained through Extracellular signal Regulated-Kinase (ERK) and Glycogen synthase kinase-3 (Gsk-3) signaling inhibition (2i). Significantly, we reported that the conditional ablation of the novel ESC metastate marked by the expression of Gm12794 is required for ESCs self-renewal maintenance. In conclusion, we extend the comprehension of ESCs biology through the identification of a novel molecular signature associated to pluripotency programming.
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