Stem Cells in Development and Disease -

Stem Cells in Development and Disease (eBook)

Michael Rendl (Herausgeber)

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2014 | 1. Auflage
472 Seiten
Elsevier Science (Verlag)
978-0-12-391435-4 (ISBN)
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This new volume of Current Topics in Developmental Biology covers Stem Cells in Development and Disease. The chapters provide a comprehensive set of reviews covering such topics as the mechanisms of pluripotency in vivo and in vitro, hematopoietic stem cell development, intestinal stem cells and their defining niche, epithelial stem cells in adult skin, the mammary stem cell hierarchy, satellite cells, neural stem cells of the hippocampus, lung stem and progenitor cells in tissue homeostasis and disease, spermatogonial stem cell functions in physiological and pathological conditions, the origin, biology, and therapeutic potential of facultative adult hepatic progenitor cells, nephron progenitor cells, adult stem cell niches, cancer stem cells, pluripotency and cellular heterogeneity, and cellular mechanisms of somatic stem cell aging - Covers the area of Stem Cells in Development and Disease - International board of authors - Provides a comprehensive set of reviews covering such topics as Intestinal Stem Cells, Nephron Stem Cells/Progenitors, Skin epithelial Stem Cells and Lung Stem Cells
This new volume of Current Topics in Developmental Biology covers Stem Cells in Development and Disease. The chapters provide a comprehensive set of reviews covering such topics as the mechanisms of pluripotency in vivo and in vitro, hematopoietic stem cell development, intestinal stem cells and their defining niche, epithelial stem cells in adult skin, the mammary stem cell hierarchy, satellite cells, neural stem cells of the hippocampus, lung stem and progenitor cells in tissue homeostasis and disease, spermatogonial stem cell functions in physiological and pathological conditions, the origin, biology, and therapeutic potential of facultative adult hepatic progenitor cells, nephron progenitor cells, adult stem cell niches, cancer stem cells, pluripotency and cellular heterogeneity, and cellular mechanisms of somatic stem cell aging- Covers the area of Stem Cells in Development and Disease- International board of authors- Provides a comprehensive set of reviews covering such topics as Intestinal Stem Cells, Nephron Stem Cells/Progenitors, Skin epithelial Stem Cells and Lung Stem Cells

Chapter One

Mechanisms of Pluripotency In Vivo and In Vitro


Eszter Posfai *; Oliver H. Tam *; Janet Rossant *,,1    
* Developmental and Stem Cell Biology, The Hospital for Sick Children Research Institute, Toronto, Ontario, Canada

† Department of Molecular Genetics, University of Toronto, Toronto, Ontario, Canada
1 Corresponding author: email address: janet.rossant@sickkids.ca

Abstract


During the course of preimplantation development, the mammalian embryo develops from a single totipotent cell into a blastocyst that is composed of three distinct cell types. Two waves of lineage specification events take place, setting aside a pluripotent cell population, the epiblast, from extraembryonic tissues. The epiblast that will form the somatic cells and germ line of the adult organism remains pluripotent until gastrulation, which commences shortly after the embryo implants. The epiblast’s remarkable property of pluripotency has been harnessed by researchers for decades through derivation of embryonic stem cells and epiblast stem cells. Both types of cells can self-renew indefinitely and still retain the ability of germ layer differentiation. However, a central conundrum to the field of stem cell biology is the extent to which these in vitro cultured cells represent their in vivo tissue of origin. In this review we discuss the development of in vivo pluripotency, and compare and contrast the role of signaling pathways and downstream transcription factors in embryo-derived stem cell types and their in vivo equivalent lineage counterparts.

Keywords

Mouse embryo

Embryonic stem cell

Epiblast stem cell

Pluripotency

Signaling pathway

Transcription factor

Lineage specification

Lineage maintenance

1 Introduction


At the onset of mouse development, fertilization of an oocyte by a sperm generates a 1-cell embryo, also known as a zygote. The zygote possesses totipotency, the ability to generate an entire organism, including its extraembryonic supporting tissues. As the zygote travels through the oviduct, it undergoes cleavage to form an 8-cell embryo around embryonic day 2.5 (E2.5) (Fig. 1.1). Individual 8-cell blastomeres are still totipotent (Kelly, 1977; Tarkowski, 1959; Tarkowski & Wróblewska, 1967). However, this period of totipotency does not persist, with the blastomeres gradually restricting their developmental fate. The first lineage restriction (and the subsequent loss of totipotency) begins with the compaction of the 8-cell embryo and ends in the formation of the inner cell mass (ICM) and the trophectoderm (TE) of the blastocyst at E3.5. The ICM will undergo another lineage segregation event prior to uterine implantation, whereby cells become restricted to either the primitive endoderm (PE) or epiblast (EPI) lineages (Arnold & Robertson, 2009; Schrode et al., 2013; Stephenson, Rossant, & Tam, 2012). These lineages become clearly distinguishable by the late blastocyst stage (~ E4.5), with the TE forming an outer layer of epithelium surrounding a fluid-filled cavity (blastocoel), the EPI forming a ball of cells on one side of the blastocyst, and the PE migrating to generate an epithelial layer of cells separating the EPI from the blastocoel cavity. From fertilization to the time of implantation, a period also known as preimplantation development, the single-cell totipotent zygote has segregated into three developmentally distinct lineages, each of which will contribute to discrete cell populations essential for embryonic growth and development.

Figure 1.1Schematic overview of early mouse development and origins of pluripotent stem cell types. The totipotent zygote undergoes three rounds of cleavage, producing an 8-cell embryo, which then undergoes compaction and polarization. From the 8-cell stage onward, cell divisions produce two populations of cells: outside cells, which will become the trophectoderm (TE), and inside cells, which will form the inner cell mass (ICM). The ICM further segregates into the primitive endoderm (PE) and the pluripotent epiblast (EPI) by the blastocyst stage. The EPI matures after implantation and gradually loses pluripotency when gastrulation commences at E6.5 (E, embryonic day). During gastrulation, the three germ layers are formed: mesoderm and endoderm precursors migrate through the primitive streak, while nonmigrating EPI cells form ectodermal tissues. Two types of pluripotent stem cells can be derived from the EPI at indicated stages: embryonic stem (ES) cells and epiblast stem cells (EpiSCs).

Although there are clear molecular and morphological differences between the three cell populations (EPI, TE, PE) of the preimplantation embryo, their divergent developmental potential is more apparent after implantation (Nowotschin & Hadjantonakis, 2010). In mouse, the cluster of EPI cells in the blastocyst rapidly expands to form a cup-shaped single-layer epithelium known as the postimplantation EPI. These cells subsequently generate embryonic ectoderm, mesoderm, endoderm, and germ cells of the developing organism, and contribute extraembryonic mesoderm to structures such as the allantois, amnion, yolk sac, and chorion (Lawson, Meneses, & Pedersen, 1991). The ability of the EPI population to generate the three major embryonic germ layers and the germ line has led to its classification as the pluripotent population of the developing embryo. In contrast, the TE and PE populations contribute almost exclusively to the extraembryonic tissues, forming structures such as the placenta (Cross, 2005; Rossant & Cross, 2001) and the parietal yolk sacs (Arnold & Robertson, 2009; Rossant & Tam, 2009).

2 Phases of Lineage Restriction


A complex cellular process such as lineage restriction and determination is unlikely to be a single-step event. Molecular markers, some of which are lineage-determining transcription factors (TFs), allow us to separate lineage restriction into three phases: initiation, commitment, and maintenance. During the initiation phase, differences in cellular states arise, either “stochastically” or through subtle external cues, in the previously homogenous cell population (Johnston & Desplan, 2010). Despite these differences, these cells remain “plastic” and are able to interconvert between different cellular states depending on external stimuli. Early-response TFs are then expressed in cells that become biased toward a specific developmental fate and are often used to identify populations that progress toward lineage commitment. In the commitment phase, the cellular state is no longer “plastic,” and becomes refractory to the initial inducing signal. In turn, specific developmental programs are activated that become increasingly dependent on cell-intrinsic cues, as seen in germ cell differentiation (Magnúsdóttir, Gillich, Grabole, & Surani, 2012). This is typically achieved by the activity of the early-response TFs, which can act by (a) forming positive feedback loops to strengthen their expression and (b) activating downstream (late response) TFs that are hallmarks of the cellular state (Zernicka-Goetz, Morris, & Bruce, 2009). In the final maintenance phase, the cell faces the task of stably maintaining expression of its gene set and inhibiting reversion or conversion into inappropriate cell fates (Pietersen & van Lohuizen, 2008). In many cases (such as in stem or progenitor cells), a cell must also be responsive to cues that direct appropriate downstream differentiation. Therefore, many genes that are involved in the formation of differentiated cell types are likely to be poised for activation, awaiting the right signals to produce downstream lineages (Dillon, 2012).

Given the difficulties in studying lineage specification in vivo, there have been significant efforts to establish culture systems to study these events in vitro.

We are now able to derive and maintain several stem cell populations from the mouse embryo that recapitulate the three early developmental lineages in vitro. These include embryonic stem (ES) (Brook & Gardner, 1997; Evans & Kaufman, 1981; Martin, 1981) and epiblast stem cells (EpiSC) (Brons et al., 2007; Tesar et al., 2007), trophoblast stem (TS) cells (Tanaka, 1998), and extraembryonic endoderm cells (Kunath et al., 2005), which represent the EPI (ES and EpiSC), TE, and PE lineages, respectively. These cell lines serve as potentially useful models for studying the maintenance phase of their respective embryonic cell type as well as their downstream differentiation capabilities.

However, we must be cautious when interpreting observations of in vitro cellular states, as they have been artificially stabilized by culture conditions in the absence of various extracellular and positional cues that exist in an intact mouse embryo. Therefore, these cell lines, although invaluable, might be overly simplistic snapshots of in vivo states, and their adaptation to culture conditions might have resulted in de novo regulative properties.

In this review, we examine and...

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