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Defining Reprogramming Checkpoints from Single-Cell Analyses of Induced Pluripotency

About This Webinar

Elucidating the mechanism of reprogramming is confounded by heterogeneity due to the low efficiency and differential kinetics of obtaining induced pluripotent stem cells (iPSCs) from somatic cells. Therefore, we increased the efficiency with a combination of epigenomic modifiers and signaling molecules and profiled the transcriptomes of individual reprogramming cells. Contrary to the established temporal order, somatic gene inactivation and upregulation of cell cycle, epithelial, and early pluripotency genes can be triggered independently such that any combination of these events can occur in single cells. Sustained co-expression of Epcam, Nanog, and Sox2 with other genes is required to progress toward iPSCs. Ehf, Phlda2, and translation initiation factor Eif4a1 play functional roles in robust iPSC generation. Using regulatory network analysis, we identify a critical role for signaling inhibition by 2i in repressing somatic expression and synergy between the epigenomic modifiers ascorbic acid and a Dot1L inhibitor for pluripotency gene activation.

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Dr. Sridharan obtained her undergraduate and Masters degrees in India. She worked on transcriptional control of developmental transitions during thymocyte maturation for her Phd from University of California, Los Angeles. During her postdoctoral work she uncovered functional contributions of each Yamanaka factor in the reprogramming of somatic cells to induced pluripotent stem cells. Her lab at the University of Wisconsin, Madison has discovered mechanisms of epigenetic regulation of cell fate in the maintenance of pluripotency using ensemble and single cell genomic techniques. She is a recipient of the Basil O' Connor, Kimmel Scholar and the Greater Milwaukee Foundation-Shaw Scientist award
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