Optimization of direct fibroblast reprogramming to cardiomyocytes using calcium activity as a functional measure of success

Addis, Russell C.; Ifkovits, Jamie L.; Pinto, Filipa; Kellam, Lori D.; Esteso, Paul; Rentschler, Stacey; Christoforou, Nicolas; Epstein, Jonathan A.; Gearhart, John D.

doi:10.1016/j.yjmcc.2013.04.004

Cited by 209 publications

(202 citation statements)

References 44 publications

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“…Later studies revealed that MyoD induces myogenin through cooperation with the Pbx factor, which is constitutively bound to MyoD target sites in fibroblasts prior to MyoD expression (Berkes et al 2004). There are many other examples of direct cell conversion within the same germ layer: the combination of PU.1 and C/EBPa into macrophage-like cells from fibroblasts (Feng et al 2008) and GATA4, MEF2C, TBX5, Hand2, and NKX2.5 for cardiomyocytelike cells from fibroblasts (Ieda et al 2010;Addis et al 2013). …”

Section: Espinosa and Emerson 2001mentioning

confidence: 99%

Pioneer transcription factors in cell reprogramming

2014

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A subset of eukaryotic transcription factors possesses the remarkable ability to reprogram one type of cell into another. The transcription factors that reprogram cell fate are invariably those that are crucial for the initial cell programming in embryonic development. To elicit cell programming or reprogramming, transcription factors must be able to engage genes that are developmentally silenced and inappropriate for expression in the original cell. Developmentally silenced genes are typically embedded in ''closed'' chromatin that is covered by nucleosomes and not hypersensitive to nuclease probes such as DNase I. Biochemical and genomic studies have shown that transcription factors with the highest reprogramming activity often have the special ability to engage their target sites on nucleosomal DNA, thus behaving as ''pioneer factors'' to initiate events in closed chromatin. Other reprogramming factors appear dependent on pioneer factors for engaging nucleosomes and closed chromatin. However, certain genomic domains in which nucleosomes are occluded by higher-order chromatin structures, such as in heterochromatin, are resistant to pioneer factor binding. Understanding the means by which pioneer factors can engage closed chromatin and how heterochromatin can prevent such binding promises to advance our ability to reprogram cell fates at will and is the topic of this review.Cell fate control represents the most extreme form of gene regulation. Genes specific to the function of a particular type of cell may be antagonistic to the function of another type of cell, so nature has evolved diverse regulatory mechanisms to ensure stable patterns of gene activation and repression. In prokaryotes, self-sustaining regulatory networks of transcription factors bound to DNA can be sufficient to regulate gene activation and repression (Ptashne 2011). In eukaryotes, ;200-base-pair (bp) segments of the genome are wound nearly twice around an octamer of the four core histones to form nucleosomes, providing steric constraints on how transcription factors can bind DNA (Kornberg and Lorch 1999). As described below, pioneer transcription factors have the special property of being able to overcome such constraints, enabling the factors to engage closed chromatin that is not accessible by other types of transcription factors (Fig. 1). However, further higher-order packaging of nucleosomes into heterochromatin can occlude access to DNA altogether, presenting an additional barrier to cell fate conversion (Fig. 1). This review focuses on the most recent studies of pioneer factors in cell programming and reprogramming, how pioneer factors have special chromatinbinding properties, and facilitators and impediments to chromatin binding. We project that such knowledge will greatly aid future efforts to change the fates of cells at will for research, diagnostic, and therapeutic purposes.

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Section: Espinosa and Emerson 2001mentioning

confidence: 99%

Pioneer transcription factors in cell reprogramming

2014

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“…This wave-like pattern is typical of cardiomyocytes created by direct reprogramming, whereas cardiomyocytes prepared from embryonic heart show a simultaneous increase of the fluorescence intensity in the entire cytoplasm. 4 The wave-like pattern appears to represent partially reprogrammed cardiomyocytelike cells. Indeed, only 30% of the cells expressed cTnT, a marker for terminally differentiated cardiomyocytes (see Supplementary material online, Figure S4A) on the same day that the wave-like pattern was observed.…”

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confidence: 99%

“…Ca 2+ oscillations in the cells were monitored using a transgene encoding the Ca 2+ indicator protein GCaMP5, which emits stronger green fluorescence in the presence of a higher intracellular Ca 2+ concentration. 4 When GSK126 was used from Day 1 to 4, numerous cells exhibited asynchronous oscillation of the fluorescence intensity, and thus the intracellular Ca 2+ concentration, on Day 14 (see Supplementary material online, Figure S1C and Videos 1A and 2A). Some cells were spontaneously beating (Phase and Hoechst panels in Supplementary material online, Figure S1C and Videos 1B and 2B).…”

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confidence: 99%

Inhibitors of suppressive histone modification promote direct reprogramming of fibroblasts to cardiomyocyte-like cells

Hirai

Kikyo

2014

Cardiovascular Research

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“…Since then, other labs around the world have reported success in reprogramming mouse fibroblasts into iCMs with similar cocktails of reprogramming factors [6][7][8][9][10]. We and others have also directly converted human cardiac and dermal fibroblasts into cardiac cells [11][12][13].…”

Section: Introductionmentioning

confidence: 95%

Reprogramming Approaches to Cardiovascular Disease: From Developmental Biology to Regenerative Medicine

Srivastava

2016

Etiology and Morphogenesis of Congenital Heart Disease

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Heart disease is a leading cause of death in adults and children. We, and others, have described complex signaling, transcriptional, and translational networks that guide early differentiation of cardiac progenitors and later morphogenetic events during cardiogenesis. We found that networks of transcription factors and miRNAs function through intersecting positive and negative feedback loops to reinforce differentiation and proliferation decisions. We have utilized a combination of major cardiac regulatory factors to induce direct reprogramming of cardiac fibroblasts into cardiomyocyte-like cells with global gene expression and electrical activity similar to cardiomyocytes. The in vivo efficiency of reprogramming into cells that are more fully reprogrammed was greater than in vitro and resulted in improved cardiac function after injury. We have also identified a unique cocktail of transcription factors and small molecules that reprogram human fibroblasts into cardiomyocyte-like cells and are testing these in large animals. Knowledge regarding the early steps of cardiac differentiation in vivo has led to effective strategies to generate necessary cardiac cell types for regenerative approaches and may lead to new strategies for human heart disease.

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Optimization of direct fibroblast reprogramming to cardiomyocytes using calcium activity as a functional measure of success

Cited by 209 publications

References 44 publications

Pioneer transcription factors in cell reprogramming

Pioneer transcription factors in cell reprogramming

Inhibitors of suppressive histone modification promote direct reprogramming of fibroblasts to cardiomyocyte-like cells

Reprogramming Approaches to Cardiovascular Disease: From Developmental Biology to Regenerative Medicine

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