Molecular Landscape of Induced Reprogramming: A Dissertation

Yang, Chao-Shun

26 February 2014

Recent breakthroughs in creating induced pluripotent stem cells (iPS cells) provide alternative means to obtain embryonic stem (ES) cell-like cells without destroying embryos by introducing four reprogramming factors (Oct3/4, Sox2, and Klf4/c-Myc or Nanog/Lin28) into somatic cells. However, the molecular basis of reprogramming is largely unknown. To address this question, we employed microRNAs, small molecules, and conducted genome-wide RNAi screen, to investigate the regulatory mechanisms of reprogramming. First we showed that depleting miR-21 and miR-29a enhances reprogramming in mouse embryonic fibroblasts (MEFs). We also showed that p53 and ERK1/2 pathways are regulated by miR-21 and miR-29a and function in reprogramming. Second, we showed that computational chemical biology combined with genomic analysis can be used to identify small molecules regulating reprogramming. We discovered that the NSAID Nabumetone and the anti-cancer drug OHTM could replace Sox2 during reprogramming. Nabumetone could also replace c-Myc or Sox2 without compromising self-renewal and pluripotency of derived iPS cells. To identify the cell-fate determinants during reprogramming, we integrated a genome-wide RNAi screen with transcriptome analysis to dissect the molecular requirements in reprogramming. We found that extensive interactions of embryonic stem cell core circuitry regulators are established in mature iPS cells, including Utf1, Nr6a1, Tdgf1, Gsc, Fgf10, T, Chrd, Dppa3, Fgf17, Eomes, Foxa2. Remarkably, genes with non-differential change play the most critical roles in the transitions of reprogramming. Functional validation showed that some genes act as essential or barrier roles to reprogramming. We also identified several genes required for maintaining ES cell properties. Altogether, our results demonstrate the significance of miRNA function in regulating multiple signaling networks involved in reprogramming. And our work further advanced the reprogramming field by identifying several new key modulators.

Embryonic Stem Cells

Fibroblasts

Gene Expression Profiling

Induced Pluripotent Stem Cells

MicroRNAs

Nuclear Reprogramming

Octamer Transcription Factor-3

RNA Interference

SOXB1 Transcription Factors

Dissertations, UMMS

Biochemistry

Cell Biology

Molecular Biology

Molecular Genetics

Pluripotency Factors Determine Gene Expression Repertoire at Zygotic Genome Activation

Gao, Meijiang, Veil, Marina, Rosenblatt, Marcus, Riesle, Aileen J., Gebhard, Anna, Hass, Helge, Buryanova, Lenka, Yampolsky, Lev Y., Grüning, Björn, Ulianov, Sergey V., Timmer, Jens, Onichtchouk, Daria

10 February 2022

Awakening of zygotic transcription in animal embryos relies on maternal pioneer transcription factors. The interplay of global and specific functions of these proteins remains poorly understood. Here, we analyze chromatin accessibility and time-resolved transcription in single and double mutant zebrafish embryos lacking pluripotency factors Pou5f3 and Sox19b. We show that two factors modify chromatin in a largely independent manner. We distinguish four types of direct enhancers by differential requirements for Pou5f3 or Sox19b. We demonstrate that changes in chromatin accessibility of enhancers underlie the changes in zygotic expression repertoire in the double mutants. Pou5f3 or Sox19b promote chromatin accessibility of enhancers linked to the genes involved in gastrulation and ventral fate specification. The genes regulating mesendodermal and dorsal fates are primed for activation independently of Pou5f3 and Sox19b. Strikingly, simultaneous loss of Pou5f3 and Sox19b leads to premature expression of genes, involved in regulation of organogenesis and differentiation.

animals

cell differentiation

chromatin (metabolism)

female

gastrulation

gene expression regulation

developmental

genome

male

SOX transcription factors (genetics)

transcription factors (metabolism)

zebrafish (genetics

growth & development

metabolism)

zebrafish proteins (genetics

metabolism)

zygote (growth & development

metabolism)

Biological Sciences