
We report that the efficiency of reprogramming human somatic cells to induced pluripotent stem cells (hiPSCs) can be dramatically improved in a microfluidic environment. Microliter-volume confinement resulted in a 50-fold increase in efficiency over traditional reprogramming by delivery of synthetic mRNAs encoding transcription factors. In these small volumes, extracellular components of the TGF-β and other signaling pathways exhibited temporal regulation that appears critical to acquisition of pluripotency. The high quality and purity of the resulting hiPSCs (μ-hiPSCs) allowed direct differentiation into functional hepatocyte- and cardiomyocyte-like cells in the same platform without additional expansion.
reprogramming, pluripotency, pluripotent stem cell, microfluidic, hepatic, cardiac, Induced Pluripotent Stem Cells, Microfluidics, Humans, Cellular Reprogramming Techniques, RNA, Messenger, Fibroblasts, Cellular Reprogramming, Cells, Cultured, Biotechnology; Molecular Biology; Biochemistry; Cell Biology
reprogramming, pluripotency, pluripotent stem cell, microfluidic, hepatic, cardiac, Induced Pluripotent Stem Cells, Microfluidics, Humans, Cellular Reprogramming Techniques, RNA, Messenger, Fibroblasts, Cellular Reprogramming, Cells, Cultured, Biotechnology; Molecular Biology; Biochemistry; Cell Biology
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