The “Ets” Factor: Vessel Formation in Zebrafish—The Missing Link
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Lucy J. Patterson and Roger Patient are in the Weatherall Institute of Molecular Medicine, John Radcliffe Hospital, Oxford University, Headington, Oxford, United Kingdom.
As the major conduit of oxygen and nutrients to cells and tissues, blood vessels are the body's ultimate lifeline (Figure 1). From conception, embryos must perform all the necessary functions of life before they have developed the organs to do so. The raw materials and waste products of metabolism are initially exchanged through simple diffusion, but as the embryo grows larger and more complicated, this is no longer sufficient. Consequently, the cardiovascular system is the first functional organ to form in the developing embryo.
The accessibility and optical clarity of zebrafish embryos lend a particular advantage to the study of vascular development. Fluorescent microspheres can be injected into the blood stream, penetrating the entire patent vascular system, allowing imaging of the vasculature using confocal microscopy. (Photo: B. Weinstein)
New blood vessels are, in general, formed by two different processes. During vasculogenesis, new vessels arise from endothelial precursors (angioblasts) in the previously avascular early embryo. During angiogenesis, existing vessels undergo remodelling, and new vessels sprout from pre-existing ones. This latter process occurs both during development and in postnatal life. Although vasculogenesis and angiogenesis occur in different contexts, they are similar processes in molecular terms. During angiogenesis, mature endothelial cells must revert to an earlier, more plastic state in order to participate in the formation of new vessels. Therefore, many of the signals that initiate angiogenic remodelling, for example, vascular endothelial growth factor (VEGF), are also associated with vasculogenesis.
Deregulation of angiogenesis can contribute to the pathogenesis of a wide range of diseases, including cancer. Because tumours induce and depend on the growth of new blood vessels, factors that promote tumour angiogenesis are important targets for anticancer therapy. Given the molecular overlap between angiogenesis and vasculogenesis, a fuller understanding of vascular development in the early embryo is likely to provide valuable insight into potential therapeutic targets for treating vascular disease.
Blood and the vessels that transport it around the body emerge almost simultaneously, and in many cases, it is widely believed, from a common precursor. In this way, these two cell types, whose fates are so closely entwined, are specified at the same time and in the same place. This concept was first proposed by Florence Sabin early in the last century [1]. Studying the initial formation of blood and endothelial cells in the chick blastoderm, she observed how the two lineages arose from the same mesodermal tissue in the blood islands (an extraembryonic tissue surrounding the embryo on the surface of the yolk). The hypothesis was further advanced by P. D. F. Murray, who first coined the term “haemangioblast” (Figure 2) to describe the putative common precursor of the two lineages [2]. Ultrastructural studies of the mouse extraembryonic yolk sac revealed a similar close association between haematopoietic and endothelial development, and the concept of the haemangioblast was extended to mammalian development [3]. Since these early beginnings, many lines of evidence have accumulated to support the existence of the haemangioblast. Early haematopoietic and endothelial cells express many of the same genes, several of which are essential for the development of both lineages (reviewed in [4]). Similarly, a specific, although as yet uncharacterised, mutation in zebrafish, known as cloche, produces embryos with profound defects in both haematopoietic and endothelial lineages [5].
Many lines of evidence support the notion that blood and endothelium share a common precursor, the haemangioblast. EC, endothelial cell; Hmgb, haemangioblast; HSC, haematopoietic stem cell.
The most direct evidence for the existence of the haemangioblast comes from studies using a model system based on the in vitro differentiation of pluripotent mouse embryonic stem cells. In appropriate culture conditions, these cells spontaneously differentiate, forming colonies of cells, known as embryoid bodies, comprising a wide mix of cell types. The distribution and timing of the appearance of specific cell types, including haematopoietic and endothelial cells, in these colonies essentially recapitulates that of the developing embryo. Using this system, individual cells derived from embryoid bodies cultured in the presence of VEGF were identified that produced colonies of haematopoietic and endothelial cells [6]. These cells are termed blast-colony forming cells, and represent a transient population that develops prior to the emergence of identifiable haematopoietic cells during embryoid body differentiation. For these reasons, the blast-colony forming cell is thought of as the in vitro equivalent of the haemangioblast.
Recently, comparable progenitor cells have been isolated from early mouse embryos, which form bilineage colonies under similar culture conditions [7]. These cells are the closest yet to a genuine in vivo haemangioblast, but their haematopoietic and endothelial potential has only been demonstrated in vitro. We cannot be sure that these cells would perform the same way if left in the embryonic environment. Thus, although there is considerable evidence for the haemangioblast's existence, definitive proof ultimately awaits an in vivo lineage labelling experiment showing that a single precursor cell can give rise to both haematopoietic and endothelial progeny.
Making a Choice—Determining Endothelial Cell Fate
Once formed, the putative haemangioblast must make the choice between haematopoietic and endothelial cell fate. While the hierarchy of transcription factors that programme haematopoietic development, spearheaded by Scl, is relatively well characterised, those governing endothelial cell specification remain more elusive. However, some of the signalling pathways involved in the differentiation and proliferation of endothelial precursors and in their subsequent migration and patterning have been identified. Most notably, VEGF is one of the most critical and specific drivers of vascular development, known to be intimately involved in endothelial precursor specification and patterning. Onset of expression of the VEGF receptor flk1, along with scl, marks the earliest precursors of the developing endothelial lineage, both in the yolk sac and in the embryo proper [8]. In the yolk sac blood islands, these cells give rise to both blood and endothelium, and thus appear to be haemangioblasts. Cells coexpressing flk1 and scl generated in vitro in embryoid bodies also give rise to both lineages [9]. Despite its early associations, flk1 expression is later restricted to endothelial cells [8,10]. Recently VEGF signalling via Flk1 has been shown to be crucial for the allocation of early mesoderm to the endothelial lineage [11].
Insight into the role of VEGF signalling during vascular development has also been provided by gene-targeting experiments in the mouse. Mice generated with mutations in three different proteins—Flk1/, VEGF+/, or plcg1/ (a downstream effector of VEGF signalling)—die at midgestation (E8.5–E9.5) due to a complete lack of endothelial or haematopoietic development [12–15]. Further studies in both murine and amphibian embryos suggested that VEGF signalling is required for the correct migration of haemangioblast/angioblast precursors to their sites of differentiation [16,17]. However, the defects of the flk1/ mouse cannot be ascribed to impaired migration alone, since development of angioblasts was completely blocked and the embryos failed to form even a primitive vascular plexus [12]. VEGF signalling is therefore essential for initial specification, proliferation, and migration of early vascular progenitors in mouse embryos.
In contrast to experiments in the mouse, disruption of the VEGF signalling pathway in zebrafish by way of mutation, antisense knockdown, or inhibition of ligand or receptors [18–21] does not produce the same severe early defects in vasculogenesis. Later defects in dorsal aorta specification and sprouting of intersomitic vessels are seen, but endothelial cells are specified and vessels are otherwise formed as normal. The most probable explanation for this stems from a fundamental difference in the regulation of flk1 expression in the zebrafish. In mouse embryos, flk1 is the first gene to be expressed in emerging haemangioblasts and endothelial precursors, initiating prior to and driving expression of scl. However, in zebrafish, flk1 expression commences later, when haemangioblasts have already been specified, and is partially dependent on Scl. Although the existence of an unidentified earlier-acting VEGF receptor cannot yet be completely ruled out, it seems unlikely that VEGF plays such a critical role in endothelial specification in zebrafish.
So what might be driving endothelial specification in the zebrafish embryo Ets factors are likely candidates. Gene expression is regulated by the binding of transcription factors to regulatory elements in the DNA, called enhancers, which promote transcription of the gene by RNA polymerase. One gene can have several different enhancers that serve to drive expression in different tissues and at different times during development. Ets factor binding sites in a flk1 regulatory enhancer sequence have been shown, through mutagenesis, to be essential for f k1 expression in endothelial cells in transgenic mice, and can be activated by coexpression with Ets1 and Ets2 [22]. Characterisation of a downstream enhancer that drives expression of scl in haematopoietic stem cells, endothelial cells, and haemangioblasts revealed critical GATA and Ets factor binding sites [23]. The same Ets-Ets-GATA motif was subsequently found to be present in candidate enhancers in the first introns of the Ets factor, fli1, and hhex—a transcription factor also expressed in haemangioblasts, in endothelial cells, and in the haematopoietic stem cell [24]. Expression of Lmo2, the partner of Scl, in endothelial cells has also recently been shown to be driven by its proximal promoter, which binds the Ets factors Elf1, Fli1, and Ets1 in vivo [25].
The Ets factors comprise a large multigene family of transcription factors. Previous attempts to identify Ets factors with important roles in zebrafish endothelial development have proven unsuccessful. Although the Ets factor fli1 is one of the earliest genes to be expressed in haemangioblasts in the lateral plate mesoderm in zebrafish embryos, its loss-of-function phenotype, both in zebrafish and in mice, is relatively mild (A. Rodaway, N. Lawson, personal communication; [26]). In a recent study, knockdown of several zebrafish Ets factors, including ets1, fli1, fli1b, or mef/elf4, either alone or combined, failed to reveal any requirement for haematopoietic or endothelial development [27].
Therefore, it is of great interest that in this edition of PLoS Biology, Sumanas and colleagues [28] report the expression and functional characterisation of a novel Ets factor, Ets1-related protein (Etsrp), which is essential for endothelial development in zebrafish embryos. Crucially, this is the earliest identified gene in the hierarchy of transcription factors governing endothelial development that does not also affect haematopoietic development, unlike cloche, for example, and may therefore be involved in specification of endothelial cell fate from the haemangioblast. While cloche acts to specify the haemangioblast, Etsrp may be required in the subsequent decision—whether to become a blood cell or an endothelial cell (Figure 3).
Cloche acts to specify the haemangioblast and is required for the expression of both scl and etsrp [5,29]. Scl is essential for the initiation of GATA1 expression and for all subsequent haematopoietic development [30]. Although endothelial cells are formed in the absence of Scl, flk1 expression is reduced from the outset, culminating in the failure of dorsal aorta specification [30]. Conversely, Etsrp is essential for flk1 expression and for elaboration of the endothelial programme.
The Emphasis on Different Signals and Factors at Different Stages of Vascular Development May Vary between Species
Previous experiments in avian and amphibian embryos have suggested that fibroblast growth factor (FGF) signalling can induce angioblast formation in mesodermal tissues [31–33]. Although FGF signalling is known to be involved in angiogenesis [34], how the FGF pathway influences endothelial commitment is still unclear. Interestingly, many Ets factors have been shown to be targeted by the mitogen-activated protein kinase (MAPK) signalling pathway. Phosphorylation of different Ets factors by MAPK can affect DNA binding, transcriptional activity, protein stability, and subcellular localisation [35]. The MAPK signalling cascade is one of the major pathways that transmit FGF signals [36]. It is therefore possible that in the absence of VEGF signalling, FGF/MAPK signalling to Etsrp drives endothelial specification in zebrafish. Conceivably, different signalling pathways play more or less dominant roles during early development in different species. In this way, the players and set pieces are essentially the same, but the order of play can vary. For example, whereas VEGF signalling is important early in vasculogenesis in the mouse, it is only required at later stages in the zebrafish. The precise roles of individual Ets factors in the mouse may differ from those in the zebrafish, but an understanding of their functions in zebrafish will also likely inform our overall understanding of their roles in mammalian vascular development.
References
Sabin FR (1920) Studies on the origins of blood-vessels and of red blood-corpuscles as seen in the living blastoderm of chicks during the second day of development. Contrib Embryol 36:213–262.
Murray PDF (1932) The development in vitro of the blood of the early chick embryo. Proc R Soc Lond B Biol Sci 11:497–521.
Haar J, Ackermann GA (1971) Ultrastructural changes in mouse yolk sac associated with the initiation of vitelline circulation. Anat Rec 170:437–456.
Keller G (2001) The hemangioblast. In: Marshak DR, Gardner RL, Gottlieb D, editors. Stem cell biology New York: Cold Spring Harbor Laboratory Press. pp 329–348.
Stainier DYR, Weinstein BM, Detrich HW, Zon LI, Fishman MC (1995) Cloche, an early acting zebrafish gene, is required by both the endothelial and hematopoietic lineages. Development 121:3141–3150.
Choi K, Kennedy M, Kazarov A, Papadimitriou JC, Keller G (1998) A common precursor for hematopoietic and endothelial cells. Development 125:725–732.
Huber TL, Kouskoff V, Fehling HJ, Palis J, Keller G (2004) Haemangioblast commitment is initiated in the primitive streak of the mouse embryo. Nature 432:625–630.
Drake CJ, Fleming PA (2000) Vasculogenesis in the day 6.5 to 9.5 mouse embryo. Blood 95:1671–1679.
Faloon P, Arentson E, Kazarov A, Deng CX, Porcher C, et al. (2000) Basic fibroblast growth factor positively regulates hematopoietic development. Development 127:1931–1941.
Yamashita J, Itoh H, Hirashima M, Ogawa M, Nishikawa S, et al. (2000) Flk1-positive cells derived from embryonic stem cells serve as vascular progenitors. Nature 408:92–96.
Giles PB, Candy CL, Fleming PA, Owens RW, Argraves WS, et al. (2005) VEGF directs newly gastrulated mesoderm to the endothelial lineage. Dev Biol 279:169–178.
Shalaby F, Rossant J, Yamaguchi TP, Gertenstein M, Wu XF, et al. (1995) Failure of blood-island formation and vasculogenesis in Flk-1 deficient mice. Nature 376:62–66.
Carmeliet P, Ferreira V, Breier G, Pollefeyt S, Kieckens L, et al. (1996) Abnormal blood vessel development and lethality in embryos lacking a single VEGF allele. Nature 380:435–439.
Ferrara N, Carver-Moore K, Chen H, Dowd M, Lu L, et al. (1996) Heterozygous embryonic lethality induced by targeted inactivation of the VEGF gene. Nature 380:439–442.
Liao HJ, Kume T, McKay C, Xu MJ, Ihle JN, et al. (2002) Absence of erythrogenesis and vasculogenesis in Plcg1-deficient mice. J Biol Chem 277:9335–9341.
Shalaby F, Ho J, Stanford WL, Fischer KD, Schuh AC, et al. (1997) A requirement for Flk1 in primitive and definitive hematopoiesis and vasculogenesis. Cell 89:981–990.
Cleaver O, Krieg PA (1998) VEGF mediates angioblast migration during development of the dorsal aorta in Xenopus. Development 125:3905–3914.
Habeck H, Odenthal J, Walderich B, Maischein H, Schulte-Merker S (2002) Analysis of a zebrafish VEGF receptor mutant reveals specific disruption of angiogenesis. Dev Biol 12:1405–1412.
Lawson ND, Vogel AM, Weinstein BM (2002) Sonic hedgehog and vascular endothelial growth factor act upstream of the Notch pathway during arterial endothelial differentiation. Dev Cell 3:127–136.
Lawson ND, Mugford JW, Diamond BA, Weinstein BM (2003) phospholipase C gamma-1 is required downstream of vascular endothelial growth factor during arterial development. Genes Dev 17:1346–1351.
Gering M, Patient R (2005) Hedgehog signaling is required for adult blood stem cell formation in zebrafish embryos. Dev Cell 8:389–400.
Kappel A, Schlaeger TM, Flamme I, Orkin SH, Risau W, et al. (2000) Role of SCL/Tal-1, GATA, and ets transcription factor binding sites for the regulation of flk-1 expression during murine vascular development. Blood 96:3078–3085.
Gottgens B, Nastos A, Kinston S, Piltz S, Delabesse EC, et al. (2002) Establishing the transcriptional programme for blood: The SCL stem cell enhancer is regulated by a multiprotein complex containing Ets and GATA factors. EMBO J 21:3039–3050.
Donaldson IJ, Chapman M, Kinston S, Landry JR, Knezevic K, et al. (2005) Genome-wide identification of cis-regulatory sequences controlling blood and endothelial development. Hum Mol Genet 14:595–601.
Landry JR, Kinston S, Knezevic K, Donaldson IJ, Green AR, et al. (2005) Fli1, Elf1, and Ets1 regulate the proximal promoter of the LMO2 gene in endothelial cells. Blood 106:2680–2687.
Spyropoulos DD, Pharr PN, Lavenburg KR, Jackers P, Papas TS, et al. (2000) Hemorrhage, impaired hematopoiesis, and lethality in mouse embryos carrying a targeted disruption of the Fli1 transcription factor. Mol Cell Biol 20:5643–5652.
Zhu H, Traver D, Davidson AJ, Dibiase A, Thisse C, et al. (2005) Regulation of the lmo2 promoter during hematopoietic and vascular development in zebrafish. Dev Biol 281:256–269.
Sumanas S, Lin S (2006) Ets1-related protein is a key regulator of vasculogenesis in zebrafish. PLoS Biol 4:e10 DOI: 10.1371/journal.pbio.0040010.
Sumanas S, Jorniak T, Lin S (2005) Identification of novel vascular endothelial-specific genes by the microarray analysis of the zebrafish cloche mutants. Blood 106:534–541.
Patterson LJ, Gering M, Patient R (2005) Scl is required for dorsal aorta as well as blood formation in zebrafish embryos. Blood 105:3502–3511.
Cox CM, Poole TJ (2000) Angioblast differentiation is influenced by the local environment: FGF-2 induces angioblasts and patterns vessel formation in the quail embryo. Dev Dyn 218:371–382.
Vokes SA, Krieg PA (2002) Endoderm is required for vascular endothelial tube formation, but not for angioblast specification. Development 129:775–785.
Pardanaud L, Dieterlen-Lievre F (1999) Manipulation of the angiopoietic/ hemangiopoietic commitment in the avian embryo. Development 126:617–627.
Presta M, Dell'Era P, Mitola S, Moroni E, Ronca R, et al. (2005) Fibroblast growth factor/fibroblast growth factor receptor system in angiogenesis. Cytokine Growth Factor Rev 16:159–178.
Sharrocks AD (2001) The ETS-domain transcription factor family. Nat Rev Mol Cell Biol 2:827–837.
Eswarakumar VP, Lax I, Schlessinger J (2005) Cellular signaling by fibroblast growth factor receptors. Cytokine Growth Factor Rev 16:139–149.(Lucy J. Patterson, Roger )
As the major conduit of oxygen and nutrients to cells and tissues, blood vessels are the body's ultimate lifeline (Figure 1). From conception, embryos must perform all the necessary functions of life before they have developed the organs to do so. The raw materials and waste products of metabolism are initially exchanged through simple diffusion, but as the embryo grows larger and more complicated, this is no longer sufficient. Consequently, the cardiovascular system is the first functional organ to form in the developing embryo.
The accessibility and optical clarity of zebrafish embryos lend a particular advantage to the study of vascular development. Fluorescent microspheres can be injected into the blood stream, penetrating the entire patent vascular system, allowing imaging of the vasculature using confocal microscopy. (Photo: B. Weinstein)
New blood vessels are, in general, formed by two different processes. During vasculogenesis, new vessels arise from endothelial precursors (angioblasts) in the previously avascular early embryo. During angiogenesis, existing vessels undergo remodelling, and new vessels sprout from pre-existing ones. This latter process occurs both during development and in postnatal life. Although vasculogenesis and angiogenesis occur in different contexts, they are similar processes in molecular terms. During angiogenesis, mature endothelial cells must revert to an earlier, more plastic state in order to participate in the formation of new vessels. Therefore, many of the signals that initiate angiogenic remodelling, for example, vascular endothelial growth factor (VEGF), are also associated with vasculogenesis.
Deregulation of angiogenesis can contribute to the pathogenesis of a wide range of diseases, including cancer. Because tumours induce and depend on the growth of new blood vessels, factors that promote tumour angiogenesis are important targets for anticancer therapy. Given the molecular overlap between angiogenesis and vasculogenesis, a fuller understanding of vascular development in the early embryo is likely to provide valuable insight into potential therapeutic targets for treating vascular disease.
Blood and the vessels that transport it around the body emerge almost simultaneously, and in many cases, it is widely believed, from a common precursor. In this way, these two cell types, whose fates are so closely entwined, are specified at the same time and in the same place. This concept was first proposed by Florence Sabin early in the last century [1]. Studying the initial formation of blood and endothelial cells in the chick blastoderm, she observed how the two lineages arose from the same mesodermal tissue in the blood islands (an extraembryonic tissue surrounding the embryo on the surface of the yolk). The hypothesis was further advanced by P. D. F. Murray, who first coined the term “haemangioblast” (Figure 2) to describe the putative common precursor of the two lineages [2]. Ultrastructural studies of the mouse extraembryonic yolk sac revealed a similar close association between haematopoietic and endothelial development, and the concept of the haemangioblast was extended to mammalian development [3]. Since these early beginnings, many lines of evidence have accumulated to support the existence of the haemangioblast. Early haematopoietic and endothelial cells express many of the same genes, several of which are essential for the development of both lineages (reviewed in [4]). Similarly, a specific, although as yet uncharacterised, mutation in zebrafish, known as cloche, produces embryos with profound defects in both haematopoietic and endothelial lineages [5].
Many lines of evidence support the notion that blood and endothelium share a common precursor, the haemangioblast. EC, endothelial cell; Hmgb, haemangioblast; HSC, haematopoietic stem cell.
The most direct evidence for the existence of the haemangioblast comes from studies using a model system based on the in vitro differentiation of pluripotent mouse embryonic stem cells. In appropriate culture conditions, these cells spontaneously differentiate, forming colonies of cells, known as embryoid bodies, comprising a wide mix of cell types. The distribution and timing of the appearance of specific cell types, including haematopoietic and endothelial cells, in these colonies essentially recapitulates that of the developing embryo. Using this system, individual cells derived from embryoid bodies cultured in the presence of VEGF were identified that produced colonies of haematopoietic and endothelial cells [6]. These cells are termed blast-colony forming cells, and represent a transient population that develops prior to the emergence of identifiable haematopoietic cells during embryoid body differentiation. For these reasons, the blast-colony forming cell is thought of as the in vitro equivalent of the haemangioblast.
Recently, comparable progenitor cells have been isolated from early mouse embryos, which form bilineage colonies under similar culture conditions [7]. These cells are the closest yet to a genuine in vivo haemangioblast, but their haematopoietic and endothelial potential has only been demonstrated in vitro. We cannot be sure that these cells would perform the same way if left in the embryonic environment. Thus, although there is considerable evidence for the haemangioblast's existence, definitive proof ultimately awaits an in vivo lineage labelling experiment showing that a single precursor cell can give rise to both haematopoietic and endothelial progeny.
Making a Choice—Determining Endothelial Cell Fate
Once formed, the putative haemangioblast must make the choice between haematopoietic and endothelial cell fate. While the hierarchy of transcription factors that programme haematopoietic development, spearheaded by Scl, is relatively well characterised, those governing endothelial cell specification remain more elusive. However, some of the signalling pathways involved in the differentiation and proliferation of endothelial precursors and in their subsequent migration and patterning have been identified. Most notably, VEGF is one of the most critical and specific drivers of vascular development, known to be intimately involved in endothelial precursor specification and patterning. Onset of expression of the VEGF receptor flk1, along with scl, marks the earliest precursors of the developing endothelial lineage, both in the yolk sac and in the embryo proper [8]. In the yolk sac blood islands, these cells give rise to both blood and endothelium, and thus appear to be haemangioblasts. Cells coexpressing flk1 and scl generated in vitro in embryoid bodies also give rise to both lineages [9]. Despite its early associations, flk1 expression is later restricted to endothelial cells [8,10]. Recently VEGF signalling via Flk1 has been shown to be crucial for the allocation of early mesoderm to the endothelial lineage [11].
Insight into the role of VEGF signalling during vascular development has also been provided by gene-targeting experiments in the mouse. Mice generated with mutations in three different proteins—Flk1/, VEGF+/, or plcg1/ (a downstream effector of VEGF signalling)—die at midgestation (E8.5–E9.5) due to a complete lack of endothelial or haematopoietic development [12–15]. Further studies in both murine and amphibian embryos suggested that VEGF signalling is required for the correct migration of haemangioblast/angioblast precursors to their sites of differentiation [16,17]. However, the defects of the flk1/ mouse cannot be ascribed to impaired migration alone, since development of angioblasts was completely blocked and the embryos failed to form even a primitive vascular plexus [12]. VEGF signalling is therefore essential for initial specification, proliferation, and migration of early vascular progenitors in mouse embryos.
In contrast to experiments in the mouse, disruption of the VEGF signalling pathway in zebrafish by way of mutation, antisense knockdown, or inhibition of ligand or receptors [18–21] does not produce the same severe early defects in vasculogenesis. Later defects in dorsal aorta specification and sprouting of intersomitic vessels are seen, but endothelial cells are specified and vessels are otherwise formed as normal. The most probable explanation for this stems from a fundamental difference in the regulation of flk1 expression in the zebrafish. In mouse embryos, flk1 is the first gene to be expressed in emerging haemangioblasts and endothelial precursors, initiating prior to and driving expression of scl. However, in zebrafish, flk1 expression commences later, when haemangioblasts have already been specified, and is partially dependent on Scl. Although the existence of an unidentified earlier-acting VEGF receptor cannot yet be completely ruled out, it seems unlikely that VEGF plays such a critical role in endothelial specification in zebrafish.
So what might be driving endothelial specification in the zebrafish embryo Ets factors are likely candidates. Gene expression is regulated by the binding of transcription factors to regulatory elements in the DNA, called enhancers, which promote transcription of the gene by RNA polymerase. One gene can have several different enhancers that serve to drive expression in different tissues and at different times during development. Ets factor binding sites in a flk1 regulatory enhancer sequence have been shown, through mutagenesis, to be essential for f k1 expression in endothelial cells in transgenic mice, and can be activated by coexpression with Ets1 and Ets2 [22]. Characterisation of a downstream enhancer that drives expression of scl in haematopoietic stem cells, endothelial cells, and haemangioblasts revealed critical GATA and Ets factor binding sites [23]. The same Ets-Ets-GATA motif was subsequently found to be present in candidate enhancers in the first introns of the Ets factor, fli1, and hhex—a transcription factor also expressed in haemangioblasts, in endothelial cells, and in the haematopoietic stem cell [24]. Expression of Lmo2, the partner of Scl, in endothelial cells has also recently been shown to be driven by its proximal promoter, which binds the Ets factors Elf1, Fli1, and Ets1 in vivo [25].
The Ets factors comprise a large multigene family of transcription factors. Previous attempts to identify Ets factors with important roles in zebrafish endothelial development have proven unsuccessful. Although the Ets factor fli1 is one of the earliest genes to be expressed in haemangioblasts in the lateral plate mesoderm in zebrafish embryos, its loss-of-function phenotype, both in zebrafish and in mice, is relatively mild (A. Rodaway, N. Lawson, personal communication; [26]). In a recent study, knockdown of several zebrafish Ets factors, including ets1, fli1, fli1b, or mef/elf4, either alone or combined, failed to reveal any requirement for haematopoietic or endothelial development [27].
Therefore, it is of great interest that in this edition of PLoS Biology, Sumanas and colleagues [28] report the expression and functional characterisation of a novel Ets factor, Ets1-related protein (Etsrp), which is essential for endothelial development in zebrafish embryos. Crucially, this is the earliest identified gene in the hierarchy of transcription factors governing endothelial development that does not also affect haematopoietic development, unlike cloche, for example, and may therefore be involved in specification of endothelial cell fate from the haemangioblast. While cloche acts to specify the haemangioblast, Etsrp may be required in the subsequent decision—whether to become a blood cell or an endothelial cell (Figure 3).
Cloche acts to specify the haemangioblast and is required for the expression of both scl and etsrp [5,29]. Scl is essential for the initiation of GATA1 expression and for all subsequent haematopoietic development [30]. Although endothelial cells are formed in the absence of Scl, flk1 expression is reduced from the outset, culminating in the failure of dorsal aorta specification [30]. Conversely, Etsrp is essential for flk1 expression and for elaboration of the endothelial programme.
The Emphasis on Different Signals and Factors at Different Stages of Vascular Development May Vary between Species
Previous experiments in avian and amphibian embryos have suggested that fibroblast growth factor (FGF) signalling can induce angioblast formation in mesodermal tissues [31–33]. Although FGF signalling is known to be involved in angiogenesis [34], how the FGF pathway influences endothelial commitment is still unclear. Interestingly, many Ets factors have been shown to be targeted by the mitogen-activated protein kinase (MAPK) signalling pathway. Phosphorylation of different Ets factors by MAPK can affect DNA binding, transcriptional activity, protein stability, and subcellular localisation [35]. The MAPK signalling cascade is one of the major pathways that transmit FGF signals [36]. It is therefore possible that in the absence of VEGF signalling, FGF/MAPK signalling to Etsrp drives endothelial specification in zebrafish. Conceivably, different signalling pathways play more or less dominant roles during early development in different species. In this way, the players and set pieces are essentially the same, but the order of play can vary. For example, whereas VEGF signalling is important early in vasculogenesis in the mouse, it is only required at later stages in the zebrafish. The precise roles of individual Ets factors in the mouse may differ from those in the zebrafish, but an understanding of their functions in zebrafish will also likely inform our overall understanding of their roles in mammalian vascular development.
References
Sabin FR (1920) Studies on the origins of blood-vessels and of red blood-corpuscles as seen in the living blastoderm of chicks during the second day of development. Contrib Embryol 36:213–262.
Murray PDF (1932) The development in vitro of the blood of the early chick embryo. Proc R Soc Lond B Biol Sci 11:497–521.
Haar J, Ackermann GA (1971) Ultrastructural changes in mouse yolk sac associated with the initiation of vitelline circulation. Anat Rec 170:437–456.
Keller G (2001) The hemangioblast. In: Marshak DR, Gardner RL, Gottlieb D, editors. Stem cell biology New York: Cold Spring Harbor Laboratory Press. pp 329–348.
Stainier DYR, Weinstein BM, Detrich HW, Zon LI, Fishman MC (1995) Cloche, an early acting zebrafish gene, is required by both the endothelial and hematopoietic lineages. Development 121:3141–3150.
Choi K, Kennedy M, Kazarov A, Papadimitriou JC, Keller G (1998) A common precursor for hematopoietic and endothelial cells. Development 125:725–732.
Huber TL, Kouskoff V, Fehling HJ, Palis J, Keller G (2004) Haemangioblast commitment is initiated in the primitive streak of the mouse embryo. Nature 432:625–630.
Drake CJ, Fleming PA (2000) Vasculogenesis in the day 6.5 to 9.5 mouse embryo. Blood 95:1671–1679.
Faloon P, Arentson E, Kazarov A, Deng CX, Porcher C, et al. (2000) Basic fibroblast growth factor positively regulates hematopoietic development. Development 127:1931–1941.
Yamashita J, Itoh H, Hirashima M, Ogawa M, Nishikawa S, et al. (2000) Flk1-positive cells derived from embryonic stem cells serve as vascular progenitors. Nature 408:92–96.
Giles PB, Candy CL, Fleming PA, Owens RW, Argraves WS, et al. (2005) VEGF directs newly gastrulated mesoderm to the endothelial lineage. Dev Biol 279:169–178.
Shalaby F, Rossant J, Yamaguchi TP, Gertenstein M, Wu XF, et al. (1995) Failure of blood-island formation and vasculogenesis in Flk-1 deficient mice. Nature 376:62–66.
Carmeliet P, Ferreira V, Breier G, Pollefeyt S, Kieckens L, et al. (1996) Abnormal blood vessel development and lethality in embryos lacking a single VEGF allele. Nature 380:435–439.
Ferrara N, Carver-Moore K, Chen H, Dowd M, Lu L, et al. (1996) Heterozygous embryonic lethality induced by targeted inactivation of the VEGF gene. Nature 380:439–442.
Liao HJ, Kume T, McKay C, Xu MJ, Ihle JN, et al. (2002) Absence of erythrogenesis and vasculogenesis in Plcg1-deficient mice. J Biol Chem 277:9335–9341.
Shalaby F, Ho J, Stanford WL, Fischer KD, Schuh AC, et al. (1997) A requirement for Flk1 in primitive and definitive hematopoiesis and vasculogenesis. Cell 89:981–990.
Cleaver O, Krieg PA (1998) VEGF mediates angioblast migration during development of the dorsal aorta in Xenopus. Development 125:3905–3914.
Habeck H, Odenthal J, Walderich B, Maischein H, Schulte-Merker S (2002) Analysis of a zebrafish VEGF receptor mutant reveals specific disruption of angiogenesis. Dev Biol 12:1405–1412.
Lawson ND, Vogel AM, Weinstein BM (2002) Sonic hedgehog and vascular endothelial growth factor act upstream of the Notch pathway during arterial endothelial differentiation. Dev Cell 3:127–136.
Lawson ND, Mugford JW, Diamond BA, Weinstein BM (2003) phospholipase C gamma-1 is required downstream of vascular endothelial growth factor during arterial development. Genes Dev 17:1346–1351.
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