Endothelio-hematopoietic relationship: getting closer to the beginnings

The close association between hematopoietic and endothelial cells during embryonic development led to the proposal that they may originate from a common ancestor - the hemangioblast. Due to a lack of unique specific markers for in vivo cell fate tracking studies, evidence supporting this theory derives mainly from in vitro differentiation studies. Teixeira and colleagues describe a novel enhancer that drives specific eGFP expression in blood islands of the electroporated chick embryo, thereby presenting a tool potentially suitable for analysis of hemangioblast differentiation and development of blood islands. See research article: http://www.biomedcentral.com/1471-213X/11/76

For over a century researchers have observed an intricate relationship between hematopoietic and vascular endo thelial cells. These cell types are closely linked and together they constitute a system that penetrates tissues and organs, thereby providing nutrients, oxygen and immune defense, as well as participating in other impor tant functions. As early as the late 19th century researchers noticed that primitive erythroid and endo the lial cells develop in close juxtaposition within structures in the embryonic yolk sac known as blood islands. These subsequently cavitate and remodel to form vascular networks filled with hemato poietic cells (reviewed in [1]). This observation led researchers to postulate the existence of the hemangio blast, a bipotent embryonic precursor cell that can generate both blood and vascular endothelial cells. Other evidence has suggested that hematopoietic cells originate from already specialized endothelial cells, known as hematogenic (hemogenic) endothelium [2]. During mid gestation, hematopoietic clusters associated with the endothelial lining of major vessels were found to co express endothelial and hematopoietic markers, further suggesting a developmental relationship between these two lineages [3]. The current view presents hemangio blasts and hematogenic endothelial cells as two consecu tive developmental stages leading to formation of blood [4] ( Figure 1A).
Despite a long history of studies in several model organisms, the hemangioblast has remained somewhat elusive. Histological observations and immunostaining have not allowed direct identification of the hemangio blast in the early embryo due to the rarity of these cells and the lack of known uniquely specific markers; and experimental evidence for the hemangioblast in vivo has been obtained only relatively recently using in vitro assays [47]. How exactly does the hemangioblast behave in vivo? In the paper by Teixeira et al. [8], the authors describe a green fluorescent protein (GFP) reporter driven by a cisregulatory region of the Cerberus gene that labels the earliest cells of blood islands in the chicken yolk sac. Using live fluorescent imaging, the authors ob served ingression of the GFP+ cells through the primitive streak the site of mesoderm and endoderm formation in mammalian, avian and reptilian embryos during gastru la tion, resulting in the formation of yolk sac blood islands. Most hematopoietic cells in yolk sac blood islands and some endothelial cells express the reporter, which led the authors to propose that the initial labeling occurred in the hemangioblast, though further experiments are required to confirm this.

Studying the hemangioblast: in vitro and in vivo
What experimental confirmation is there of the existence of the hemangioblast? Due to the relative simplicity of manipulations and the ability to track cell populations of interest, pluripotent embryonic stem (ES) cells became broadly used to model hematopoietic development in vitro. The first evidence pointing to the existence of the bipotent hemangioblast was obtained when mouse ES cellderived progenitors were shown to be capable of

Abstract
The close association between hematopoietic and endothelial cells during embryonic development led to the proposal that they may originate from a common ancestor -the hemangioblast. Due to a lack of unique specific markers for in vivo cell fate tracking studies, evidence supporting this theory derives mainly from in vitro differentiation studies. Teixeira and colleagues describe a novel enhancer that drives specific eGFP expression in blood islands of the electroporated chick embryo, thereby presenting a tool potentially suitable for analysis of hemangioblast differentiation and development of blood islands.  [6,7]. ES cell differentiation has been extensively used to model the stepwise transi tion of the bipotent hemangioblast to the blood and endothelial lineages, shedding light on surface markers expressed at each stage as well as genetic regulation of this process [4,5,8] ( Figure 1A). During hematopoietic differentiation, mouse ES cells first generate the primitive streak mesoderm marked by brachyury expression, followed by quick upregulation of Flk1, which marks the formation of extraembryonic mesoderm and the onset of endothelial specification. A fraction of hematogenic endo thelial cells subsequently generates CD41+ and CD45+ hematopoietic cells, which critically depends on the transcription factor Runx1. It is broadly accepted that ES cell hematopoietic differentiation replicates yolk sac hemato poiesis; however, both yolk sac and intra embry onic hematopoietic compartments are believed to origi nate through an endothelialhematopoietic transition.
Due to limitations in embryonic material and technical approaches, including lack of unique markers, in vivo studies of the endothelialhematopoietic relationship in the early embryo are less abundant. Paradoxically, yolk sac blood islands, which prompted the concept of the hemangioblast in the first place, were for a long time a source of controversy. Initial attempts to identify bipotent cells capable of generating both endothelial and hemato poietic cells failed in both chicken and mouse embryos. Only later was evidence presented that hemangioblasts are transient cells localized to the posterior primitive streak and that by the time of migration to the yolk sac, hematopoietic and endothelial lineages are already segre gated [6] ( Figure 1B). Interestingly, while in the mouse the blood island appears as a single beltlike structure encompassing the yolk sac [1], blood islands in the chick represent multiple more distinct clusters of cells. One of the most interesting observations made by Teixeira et al. using live imaging is that blood island formation in the chick yolk sac involves very dynamic aggregation and recruitment of GFP+ cells during migration from the primitive streak. Thus, despite the morphological appear ance of blood islands as individual clones in the chick, their clonal origin seems to be unlikely, as was proposed for the mouse [9]. However, distinct multiple blood islands and availability of genetic markers such as that described by Teixeira et al. make the chick embryo a highly attractive model for studying hemangioblast biology and mechanisms underlying the segregation of endothelial and blood lineages.

Hematogenic endothelium: role in blood production
Although in vitro hematopoietic cells can be generated from the hemangioblast through a hematogenic endo the lium intermediate, exact details of this process in vivo remain obscure. For example, how and where exactly in the embryo do hematopoietic cells transit through an endothelial stage? Do all hematopoietic cells pass through an endothelial stage during embryonic development? In addition, some data indicate that hemangioblasts can generate smooth muscle cells, whereas other reports argue against this [610]. The full potency of these cells awaits further elucidation.
The relationship between hematopoietic cells and the endothelium is not limited to yolk sac blood islands. It is broadly thought that the best morphological demon stra tion of blood cell production by the endothelium is displayed in the midgestational dorsal aorta, umbilical cord and vitelline vessels connecting the embryo proper with the placenta and the yolk sac [11] (Figure 1C). Hematopoietic cells emerging in intraaortic clusters show distinct morphological features and express markers common to both endothelial and hematopoietic cells, suggesting they are in transition from the underlying endothelium toward a blood cell fate. Individual cells with early hematopoietic markers such as ckit, CD41 and CD45 can be detected prior to cluster formation in the endothelial layer of the dorsal aorta. Analysis of cultured thick sections of the mouse aortagonad mesonephros region, an area containing intraaortic hematopietic clusters, have shown that individual cells within the endothelial layer of the dorsal aorta can leave it and migrate inside the aortic lumen [12]. Interestingly, live imaging of zebrafish embryos showed that during an endothelialhematopoietic transition, cells leave the endothelial lining of the dorsal aorta in the opposite direction to that observed in mouse, and move away from the lumen before entering circulation through the cardinal vein below [13,14].

Prospective
The importance of finding novel specific markers for hemangioblasts and hematogenic endothelium in higher vertebrates cannot be overestimated. Such specific markers can significantly enhance in vitro clonal analysis of endothelialhematopoietic differentiation and facilitate our understanding of hematopoietic development in vivo. Now that a methodology for generating transgenic chickens has become available [15], it is likely that the availability of useful markers and the accessibility of chick embryos for live imaging will significantly increase the use of avian models and will boost research in this area.