Negative regulation of primitive hematopoiesis by the FGF signaling pathway

doi:10.1182/blood-2006-05-021386

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Blood, 15 November 2006, Vol. 108, No. 10, pp. 3335-3343.
Prepublished online as a Blood First Edition Paper on August 3, 2006; DOI 10.1182/blood-2006-05-021386.

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HEMATOPOIESIS
Negative regulation of primitive hematopoiesis by the FGF signaling pathway
Fumie Nakazawa, Hiroki Nagai, Masahiro Shin, and Guojun Sheng
From the Laboratory for Early Embryogenesis, RIKEN Center for Developmental Biology, Kobe, Hyogo, Japan.

   Abstract

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Hematopoiesis is controlled by multiple signaling moleculesduring embryonic and postnatal development. The function ofthe fibroblast growth factor (FGF) pathway in this process isunclear. Here we show that FGF plays a key role in the regulationof primitive hematopoiesis in chicks. Using hemoglobin mRNAexpression as a sensitive marker, we demonstrate that timingof blood differentiation can be separated from that of initialmesoderm patterning and subsequent migration. High FGF activityinhibits primitive blood differentiation and promotes endothelialcell fate. Conversely, inhibition of FGFR activity leads toectopic blood formation and down-regulation of endothelial markers.Expression and functional analyses indicate that FGFR2 is thekey receptor mediating these effects. The FGF pathway regulatesprimitive hematopoiesis by modulating Gata1 expression leveland activity. We propose that the FGF pathway mediates repressionof globin gene expression and that its removal is essentialbefore terminal differentiation can occur.

   Introduction

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

During the early development of amniotes, blood cells are generatedexclusively from the extraembryonic yolk sac mesoderm.^1-3 Intraembryonichematopoietic niches such as aorta-gonad-mesonephros and livermature later and initiate the second wave of hematopoiesis.^4-6Located in the extreme lateral regions of the developing embryo,primitive blood cells are derived from ventral mesoderm precursorsingressing through the posterior part of the primitive streakduring gastrulation. In birds, postingression precursor cellsundergo extensive migration before the establishment of thecirculation to populate the entire hemogenic region called areavasculosa.^3,7-9 Endothelial cells have a similar origin andgastrulate through the posterior streak. Molecular, genetic,and cell biologic analyses have demonstrated that precursorcells in the streak and during early migration still have thepotential to differentiate into either the blood or the endotheliallineage.^10-15 Extraembryonic mesoderm (EEM) contains at least2 additional tissue types, somatic and splanchnic EEM, whichdifferentiate into smooth muscle and connective tissue and constitutedorsal and ventral linings of the extraembryonic coelom.^16,17Blood and endothelial cells separate early from the splanchnicmesoderm as aggregates on its ventral side, variously calledblood islands, angioblasts, or hemangioblasts.^18-20 These aggregatesare referred to as blood islands in this work. In lateral EEM,blood islands (BIs) give rise to both blood and endothelialcells, whereas in medial EEM and the lateral plate, only endothelialcells are generated.^18,21,22 It is not well understood why someBIs give rise to both, whereas others give rise to only endothelialcells.
Chicken hemoglobins were used for initial descriptive and biochemicalstudies on primitive hematopoiesis^21,23 and for later investigationson transcriptional control.^24-26 More recent studies using differentmodel organisms revealed a complex genetic network controllingprimitive hematopoiesis.^{3,10,13,15,27-29} Analyses focusing onsignaling molecules indicated the involvement of the BMP,^30-32VEGF,^33-36 WNT,^37,38 and Notch^39,40 pathways in various aspectsof primitive hematopoiesis. The role of the fibroblast growthfactor (FGF) pathway in this process is unclear. It is knownto be important for mesoderm induction during gastrulation,^41-43for dorsoventral patterning of the mesoderm,^44,45 and for mesodermcell movement during and after gastrulation.^46,47 In addition,FGF can act as a potent inducer of neovascularization and neoangiogenesis^48,49and plays a role in promoting proliferation and maintenanceof hematopoietic progenitors and stem cells.⁵⁰ Its precise functionin primitive hematopoiesis has been debated, with some evidencesuggesting a positive regulatory role^51-53 and other evidenceindicating a negative one.^54,55
In this study, we investigate the function of the FGF pathwayin chick primitive hematopoiesis. Globin mRNA expression isused as a sensitive readout for terminal differentiation. Wefocus our study on the differentiation step only, separatingit from potential roles of the FGF pathway in earlier (induction,patterning, and migration) or later (proliferation and maturation)steps. We demonstrate that FGF signals can elicit strong inhibitionof hemoglobin expression and up-regulate endothelial markers.Inhibition of the FGF signaling pathway results in ectopic bloodformation and completely inhibits endothelial marker expression.Among 4 known FGFRs, we show that FGFR2 is the key receptorfunctioning in this process. These effects are achieved throughcrosstalk with the VEGF pathway yet can be attributed primarilyto the FGF pathway. We also show that it acts in primitive hematopoiesisthrough Gata1 by modulating Gata1 expression level and activity.

   Materials and methods

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Chick embryology
Fertilized hens' eggs were purchased from Shiroyama Farm (Kanagawa,Japan) and incubated at 38.5°C to the desired stages. Fortissue graft, bead graft, chemical treatment, and electroporationexperiments, we used the modified New culture method.⁶⁸ Differentiationof isolated streak tissue pieces was performed on vitellinemembrane as in New culture but without a host embryo. For insitu hybridization and immunohistochemistry, standard publishedprotocols were followed.⁵⁶ All in situ analyses were carriedout with either digoxigenin- or fluorescein-labeled RNA probesand developed with alkaline phosphatase staining. All tissuesections shown were 10-µm paraffin sections. Electroporationwas performed with Intracel electroporator (Intracel, Hertfordshire,United Kingdom) at the following setting: 5 volts, 3 pulses(50 ms with 250-ms interval). All image-acquisition equipmentwas purchased from Olympus (Tokyo, Japan). Whole-mount embryoswere visualized in PBS solution with an Olympus SZX12 microscopeusing a DF PLAPO 1.2x/0.133 PF2 objective lens. Embryo sectionswere mounted with canada balsam and visualized with an OlympusBX51 microscope using Olympus UPlanSApo objective lenses (20x/0.75;40x/0.9; 100x/1.40 oil-immersion). For both whole-mount embryosand embryo sections, an Olympus DP70 camera was used to captureimages, and DP Controller 2.1 image software was used to acquirethem. Final images were assembled with Photoshop 8.0 (AdobeSystems, San Jose, CA).
Chemicals
Proteins and chemical inhibitors were purchased from commercialsources. The following concentrations were used for bead soakingprior to graft: BMP2 (20 µg/mL, 355-BEC); BMP4 (20 µg/mL,314-BP); Chordin (100 µg/mL, 758-CN); Noggin (12 µg/mL,1967-NG); FGF4 (50 µg/mL, 235-F4); Nodal (12 µg/mL,1315-ND); Dkk1 (25 µg/mL, 1096-DK); VEGF165 (10 µg/mL,93-VE); Wnt3a (10 µg/mL, 1324-WN); Epo (25 µg/mL,959-ME) (all from R&D Systems, Minneapolis, MN); FGF8 (50µg/mL; Sigma, St Louis, MO; no. F6926); SU5402 (42 mM;Calbiochem, San Diego, CA; no. 572630). For chemical treatment,embryos were cultured with SU5402 (85 µM, 6 x 50% inhibitoryconcentration [IC₅₀]) or SU5416 (10 µM, 10 x IC₅₀, Calbiochem;no. 676487) dissolved in albumen, with less than 0.2% of finalDMSO presence.
Molecular biology
DNA fragments for gene-specific in situ probes were generatedby polymerase chain reaction (PCR), cloned in pGEM-T vectors,and confirmed by sequencing ( ${rho}$ : nucleotides [nt's] 31-465 ofCHEST324a16; ${epsilon}$ nt's 55-475 of CHEST26i6; ${alpha}$ : nt's 39-488 of CHEST23l23; ${alpha}$ ^A nt's 40-485 of CHEST973g24; gata1: nt's 577-1061 of NM_205464 [GenBank] with full-length cDNA kindly given by T. Evans (Albert EinsteinCollege of Medicine, New York, NY); ets1: nt's 41-782 of 052594.1;lmo2: nt's 7-962 of NM204271; vegfr2: nt's 3477-5149 of AY382882 [GenBank] ;Vecad: nt's 642-2368 of AF522067 [GenBank] ; fgfr1-4: Shin et al⁵⁷). Constitutivelyactive FGFR2 (CA-FGFR2) was constructed based on studies byWebster and Donoghue.⁵⁸ A chick FGFR2 fragment lacking the extracellularand transmembrane domains was created by PCR (forward: 5'-ATCGATATGGGGAGCAGCAAGCCCAAGGACCCCAGCCAGCGCCCTGACTTCAGCAGCCAGCCCGCTGTC-3',and reverse: 5'-ACTAGTTCATGTTTTAACGCTCCCATTC-3', with myristoylationsequence from c-Src: MGSSKSKPKDPSQR tagged to the 5' end ofthe forward primer). An additional Lys661Glu mutation was introducedto create ligand-independent kinase activity. Final CA-FGFR2was cloned into pCAGGS vector for efficient expression in vivo.⁵⁹The activity was confirmed by double-phosphorylated ERK (dp-ERK)antibody staining. FGFR2-specific fluorescein-tagged morpholino(5'-CTAGAATGATTTACCTTCGGGTTCC-3') was designed against exon1-intron1boundary and purchased from Gene Tools (Philomath, OR) togetherwith standard control morpholino. Chick FGFR2 contains a 14.3-kbfirst intron, and blocking the splicing of first exon led tosevere reduction of the mature transcript as revealed by insitu analysis with c-terminal–specific probe (Figure 5R-S).Morpholinos were electroporated at 3 mM and DNA constructs at1 µg/µL.

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Figure 1.. Hemoglobin expression during early development. (A-H) Expression at HH10 of ${alpha}$ (A), ${alpha}$ ^A (B), ${rho}$ (C), and ${epsilon}$ (D) globin transcripts and sections through indicated level of ${alpha}$ (E), ${alpha}$ ^A (F), ${rho}$ (G), and ${epsilon}$ (H). (I-W) Expression of ${rho}$ at HH5 (I), 7 (J), 8 (K), 10 (L), and 12 (M). Sections of HH7 (N-P) and HH8 (Q-S) embryos are shown as indicated. Arrows point to cells initiating expression within a BI. Representative BI morphology is shown for HH9 (T), 10 (U), 11 (V), and 12 (W).

   Results

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Expression of hemoglobin genes during chick primitive hematopoiesis
Based on pseudoperoxidase activity of the heme group, chemicalssuch as benzidine and diaminofluorene have traditionally beenused for staining differentiated red blood cells.^8,60,61 Asan alternative and more sensitive and specific method, we investigatedmRNA expression patterns of hemoglobin genes during early chickdevelopment. Chick hemoglobin loci contain 4 beta-type ( $beta$ ^H, $beta$ ^A, ${rho}$ , and ${epsilon}$ ) and 3 alpha-type ( ${alpha}$ , ${alpha}$ ^A, and ${alpha}$ ^D) globin genes. Five ofthem ( ${alpha}$ , ${alpha}$ ^A, ${alpha}$ ^D, ${rho}$ , and ${epsilon}$ ) are expressed in primitive blood cells.^21,23We generated probes for ${alpha}$ ^A, ${alpha}$ , ${rho}$ , and ${epsilon}$ and performed in situ analysiswith precirculation chick embryos (before Hamburger and HamiltonStage 13 [HH13]). All 4 genes were strongly expressed in areavasculosa. Figure 1 shows the expression patterns at HH10 of ${alpha}$ (A), ${alpha}$ ^A (B), ${rho}$ (C), and ${epsilon}$ (D), respectively. As revealed in sections(Figure 1E-H), each gene was expressed in all differentiatedblood cells. Since all 4 genes were detected at the early somitestage, we performed detailed analysis on hemoglobin ${rho}$ ( ${rho}$ ) expression(Figure 1I-M). The earliest expression was seen at HH6-7. AtHH7, ${rho}$ can be readily detected in differentiating BIs (Figure 1J,N-P).Within individual BIs, a few inner cells were observed to initiate ${rho}$ expression (Figure 1O), followed by more cells within a cluster(Figure 1P-S). Mature and laterally located BIs from HH8 onwardcontained all inner cells positive for ${rho}$ ( ${rho}$ ⁺) surrounded by negativecells (Figure 1S-W). Morphologically distinct blood cells werevisible from HH10 (Figure 1L-M,U-W). At the onset of circulation(HH12-13; Figure 1M,W), the majority of blood cells had lostcontact with each other and with the endothelial wall, whichwas a prominent feature for ${rho}$ ⁺ cells up to HH10-11 (Figure 1U-V).The detection sensitivity with globin mRNA probes (presomitestage) is greater than with heme group–reacting compounds(4-5 somite stage), in agreement with biochemical studies onchicken globin proteins^23,62,63 and mouse globin genes.⁶⁴ Using ${rho}$ as a sensitive marker, we performed further experiments toinvestigate the regulation of primitive hematopoiesis.
Posterior streak mesoderm can differentiate into ${rho}$ -expressing blood cells in the absence of cell migration
Explant culture showed streak tissue, and dissociated streakcells are able to differentiate into blood cells in mice.¹⁴In chicks, dissociated posterior streak and early migratorymesoderm cells can form blood colonies in culture.³⁵ This wasconfirmed by streak tissue graft using ${rho}$ as a marker (Figure 2A-D).We separated HH4 streak into 3 pieces (anterior, middle, andposterior; Figure 2A), transplanted each piece to the extremelateral region of the area opaca of same-stage host embryos,and cultured to HH10. The posterior streak piece can differentiateinto ${rho}$ ⁺ cells with developmental timing similar to that of thehost embryo (Figure 2D). Both the intensity of ${rho}$ expression andthe spatial distribution of BIs were comparable to the host(Figure 2D). The middle piece can also differentiate, but toa lesser degree as predicted from fate map studies, into ${rho}$ ⁺ cells(Figure 2C). The anterior piece failed to generate any ${rho}$ ⁺ cell(Figure 2B) and instead differentiated into more axial structureswith notochord and somites (data not shown). These data suggestedthat posterior streak mesoderm precursors contain intrinsicability to undergo proper migration and differentiation. Sincethe host area opaca can provide a substrate for migration andpossible inducing signals from the extraembryonic ectoderm andendoderm, we cultured posterior pieces directly onto the vitellinemembrane (Figure 2E). The posterior half of the HH4 streak wasfurther divided into anterior (third quarter) and posterior(fourth quarter) pieces. Explants were cultured until controlembryo reached HH10 (Figure 2F). The ${rho}$ ⁺ cells can be seen inboth the third and the fourth quarters (Figure 2G-H), with more ${rho}$ ⁺ cells and stronger expression in the fourth quarter (Figure 2G).In vitelline membrane culture, the cells failed to migrate andas a consequence the characteristic spatial distribution ofBIs was lost.

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Figure 2.. Differentiation potential of posterior streak mesoderm. (A-D) HH4 streak pieces are grafted to the lateral area opaca of host HH4 embryo and cultured to HH10 (A). Differentiation is assayed by ${rho}$ expression for anterior (B), middle (C), and posterior (D) pieces. Red dotted lines indicate the limit of host ${rho}$ expression. (E-H) HH4 streak pieces are cultured on vitelline membrane (E). Differentiation is assayed by ${rho}$ when control reaches HH10 (F) for posterior (G) and third (H) quarters.

Differentiation of primitive blood cells is inhibited by FGF signaling
The previous experiment suggested that signals regulating precursorcell migration can be separated from those regulating differentiation.In chicks, these 2 processes can also be separated temporally.Differentiation of primitive blood as marked by ${rho}$ expressionis initiated at about HH7 (Figure 1J). Migration of EEM cellsstarts before HH4 and the majority of them reach their destinationsby HH7. We focused on the step of hemoglobin gene transcriptionas a marker for the initiation of terminal differentiation.We first looked at the ability of molecules involved in varioussignaling pathways to affect the endogenous ${rho}$ expression. Beadssoaked with secreted molecules were grafted either within oroutside the future ${rho}$ domain (Figure 3A). HH6-7 embryos were usedto minimize possible secondary effects due to their influenceon cell migration. Results are summarized in Table 1. We foundno single factor capable of inducing ${rho}$ ectopically, whereas onlyFGF beads (FGF4, 40/53, 75%; FGF8, 15/29, 52%) showed remarkableinhibition of endogenous ${rho}$ expression. As shown in Figure 3B and D,control beads had no effect on ${rho}$ expression, whereas FGF4 beadsexerted strong inhibition (Figure 3C,E). A similar effect wasseen with FGF8 beads (Figure 3G). The inhibitory effect of FGFswas not due to their ability to repel mesoderm cells, as sectionsrevealed large numbers of ${rho}$ ^– mesoderm cells near beads(Figure 3F). As summarized in Table 1 and shown in Figure 3H(BMP7) and Figure 3I (Noggin), we did not observe a similarprominent effect with other factors tested. We then asked whetherthe cells that failed to adopt blood fate can differentiateinto endothelial cells. The effect of FGF bead graft was analyzedwith 2 endothelial markers, Vegfr2 and Ets1. Both have beendescribed to specifically mark endothelial cells at HH10.^65,66We generated RNA probes for Vegfr2 and Ets1 and extended theexpression study by focusing on EEM differentiation (Figure 3J-L,Vegfr2; Figure 3O-Q, Ets1). When FGF4 beads were grafted fromHH6-7 and analyzed at HH10, strong up-regulation of both transcriptswas observed in cells adjacent to grafted beads (Figure 3M-N,R-S).

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Table 1.. Effect of signal molecules on ${rho}$ expression

Inhibition of the FGF signaling pathway leads to ectopic blood cell differentiation
Our graft analysis suggested that FGF mediates the choice betweenblood and endothelial fates. Activation of FGF signaling inhibitsblood differentiation and promotes endothelial formation. Wethen asked whether more blood cells can be generated when thispathway is inhibited. The ${rho}$ expression was analyzed in embryostreated with SU5402, a small molecule inhibitor specific forFGFR class RTK proteins.⁶⁷ We applied SU5402 starting from HH6-7,when the induction and extensive migration of mesoderm cellshas largely been accomplished. Beads soaked in control DMSOhad no effect (Figure 4A,C). Grafting of SU5402 beads resultedin large numbers of blood cells in their vicinity (Figure 4B,D-E).In particular, we saw blood cells being induced in medial regions(Figure 4F), which was not observed in normal embryos or ingraft experiments with secreted factors (Table 1). This promptedus to investigate the effect of SU5402 in more detail.

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Figure 3.. FGF inhibits ${rho}$ and enhances endothelial marker expression. (A) HH6-7 embryos are grafted with factor-soaked beads either within (black) or outside (yellow) the future ${rho}$ -expressing domain and cultured to HH10. (B-I) FGF4 beads inhibit ${rho}$ expression (C,E) and control beads have no effect (B,D). Boxed areas in panels B and C are magnified in panels D and E, respectively. Arrows point to grafted beads and arrowheads show the repression. F (section of E) shows presence of ${rho}$ ^– cells around the bead. A similar effect is seen with FGF8 (G) but not BMP7 (H) or Noggin (I). (J-N) Expression of Vegfr2 at HH4 (J), 6 (K), and 10 (L). FGF4 beads enhance its expression (M-N). Arrows point to grafted beads. (O-Q) Normal expression of Ets1 at HH4 (O), 6 (P), and 10 (Q). FGF4 beads enhance its expression (R-S).

To confirm this effect, we cultured whole embryos with SU5402dissolved in the albumen in the modified New culture setting.⁶⁸As mentioned earlier, we chose to test the effect with embryosfrom HH6-7 onward. Earlier treatment resulted in malformationsin the embryo proper as well as a greatly reduced area vasculosa,likely as a consequence of mesoderm induction and migrationdefects (data not shown). No obvious defect or delay in embryonicdevelopment was seen with the concentration used (DMSO: Figure 4G,I;SU5402: Figure 4H,J; Paraxis staining: I-J insets). Control-treatedembryos showed normal ${rho}$ expression (Figure 4G,K). SU5402 causeddramatic medial expansion of the ${rho}$ -expressing domain (Figure 4H,L).Sections of treated embryos revealed ${rho}$ ⁺ cell clusters below thesplanchnic mesoderm in the lateral plate (Figure 4Ni-v), farmore medial than in control embryos (Figure 4M). In the endogenoushemogenic domain, the intensity of ${rho}$ expression and the patternof BI distribution were not greatly affected (Figure 4G-H).In most cases, we saw ${rho}$ ⁺ clusters still surrounded by ${rho}$ ^–cells with endothelial cell morphology (Figure 4Ni-v).
Since endothelial-like cells were still observed in treatedembryos, we next investigated whether FGF activity is requiredfor endothelial marker expression. We compared the effect ofSU5402 with DMSO control using endothelial markers Ets1, Vegfr2,and Vecad. Expression of all 3 was potently inhibited by SU5402(compare Figure 4Oi, Pi, and Qi with Figure 4Oii, Pii, and Qii),indicating that endothelial development was greatly compromisedwith the inhibition of FGFR activity. This was further confirmedby analyzing the effect on Lmo2. Analysis of Lmo2 RNA expression(Figure 4Ri-iii) showed similar patterns as previously described.⁸At HH10, Lmo2 was expressed in both blood and endothelial cells(Figure 4S,Ui-ii,Wi-ii) in control embryos. With SU5402 treatment,Lmo2 expression in blood cells was not affected, whereas expressionin endothelial cells was completely abolished (Figure 4T,Vi-ii,Xi-ii).In agreement with these observations, no vascular network orblood flow was observed (data not shown) when treated embryoswere cultured until controls reached circulation stage (>HH13). These data indicated that inhibition of the FGF pathwayseverely blocked endothelial differentiation.
FGFR2 is a key negative regulator of primitive blood differentiation
SU5402 can inhibit tyrosine kinase activity of all FGF receptors.We performed further experiments to investigate which FGF receptor(s)may be mediating our observed effects. As in mammals, chickshave 4 FGFRs. The expression patterns of FGFR1, 2, and 3 havebeen described in chicks⁶⁹ but not in the context of EEM differentiation.We first carried out detailed in situ analyses for FGFR1-4 fromHH4 to HH12, with special attention to their possible involvementin blood and endothelial differentiation. Among them, we foundFGFR2 (Figure 5Bi-vi) to be the likely candidate in mediatingthese observed effects. FGFR2 was expressed in the endothelialcells in the extraembryonic region (Figure 5Bvi,F), whereasprimitive blood cells were devoid of its transcripts (Figure 5Finset). The splanchnic mesoderm in the lateral plate and medialEEM was also positive for FGFR2 (Figure 5F). FGFR1 transcriptswere not detected in EEM in either blood or endothelial cells(Figure 5Avi,E), although they were present in both somiticand lateral plate mesoderm (Figure 5E). FGFR3 (Figure 5Ci) wasexpressed at HH4 in all ectoderm cells except those adjacentto the streak. At HH10, nascent somites and neighboring intermediatemesoderm were strongly positive (Figure 5Ciii,G). In lateralplate and medial EEM, signals can be detected in somatic andsplanchnic mesoderm but not in endothelial cells or blood cellsat any axial level (Figure 5G). Expression patterns of FGFR1and 3 indicated they may also play a role in restricting primitiveblood differentiation to more lateral regions. For FGFR4 (Figure 5Di-iii),we did not observe obvious expression in the extraembryonicregion at any stage. FGFR4 signals were seen in the neural platefrom HH4 (Figure 5Di-iii).

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Figure 4.. Inhibition of FGFR causes ectopic blood formation and down-regulation of endothelial markers. (A-F) Control DMSO bead has no effect (A,C) and SU5402 bead has excessive surrounding ${rho}$ ⁺ clusters (B,D). Panels E and F show additional examples of blood induction by SU5402 beads. Arrows point to grafted beads. (G-N) Whole embryo culture in the presence of DMSO (G,I) or SU5402 (H,J) does not affect general growth (I-J, insets: Paraxis in situ). SU5402 drastically expands medial limit of blood formation (H,L) compared with DMSO (G,K), as outlined by yellow dotted line. Sections of panels L (Ni-v) and K (M) show clear induction of ectopic ${rho}$ ⁺ clusters (arrowhead). Panels Nii-v show presence of endothelial-like cells (arrows) surrounding induced (Niii-v) and endogenous (Nii) clusters. (O-X) Down-regulation of Ets1 (Oii), Vegfr2 (Pii), and Vecad (Qii) by SU5402 compared with respective controls (Oi, Pi, and Qi). Lmo2 expression is shown for HH4 (Ri), 5 (Rii), and 8 (Riii). At HH10 (S), it is expressed in both endothelial and blood cells laterally (Ui and section in Uii) and only in endothelial cells medially (Wi-ii). SU5402 abolishes endothelial expression of Lmo2 while maintaining blood expression laterally (Vi-ii). Ectopic blood clusters in the medial region also express Lmo2 (Xi-ii) but only in inner cells like ${rho}$ globin (Niii-v). Arrows indicate blood expression; arrowheads, endothelial expression.

Since FGFR2 was expressed in endothelial cells and absent inprimitive blood cells, we next tested whether activation ofthe FGF pathway mediated through FGFR2 can influence cell fate.For this purpose, we constructed an expression vector for theconstitutive active form of FGFR2 (CA-FGFR2; see "Molecularbiology"). A DNA construct expressing CA-FGFR2 together witha reporter GFP gene was cointroduced into posterior streak mesodermat HH4 by electroporation. Control embryos were electroporatedwith the GFP construct alone. We scored the distribution ofCA-FGFR2–positive cells at HH10 in comparison with controlembryos. To exclude a possible secondary effect due to migratorydefect, only cells that had reached the endogenous ${rho}$ ⁺ domainwere scored. In control embryos (Figure 5H-I,L; electroporatedcells, brown; blood cells, blue), GFP-positive cells were distributedamong different lineages. For our analysis, we grouped the locationof positive cells into 3 categories: primitive blood ( ${rho}$ ⁺), endothelial(cells with flattened morphology surrounding ${rho}$ ⁺ cluster), andothers (all other positive cells). Among 1571 cells scored (Table 2),36.0% control GFP-positive cells (565) became blood cells, whereas29.9% (470) went to endothelial lineage. The remaining 34.1%(536) contributed to other cell types. Among the CA-FGFR2–positivecells, distribution ratios were greatly altered (Figure 5J-K,M).In 1703 total cells scored (Table 2), we found fewer than 50(2.8%) CA-FGFR2–positive cells differentiated into primitiveblood, whereas the vast majority (1366, 80.2%) became endothelialcells.

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Table 2.. Statistical distributions

To confirm these effects, we performed a knockdown experimentusing FGFR2-specific splice-block morpholino (see "Molecularbiology"). Antimorpholino staining did not yield sharp cellboundaries, making statistical analysis difficult. Nevertheless,the general distribution patterns of morpholino-positive cellswere easily recognizable. Cells with control morpholino weredistributed among different lineages (Figure 5N,P; morpholinocells, blue; blood cells, brown), similar to control GFP cells.FGFR2 morpholino cells showed a distribution pattern oppositeto that of CA-FGFR2 and contributed primarily to blood cells(Figure 5O,Q). The efficacy of FGFR2 morpholino was confirmedby down-regulation of the mature FGFR2 transcript in neuralectoderm at HH4 (Figure 5R-S). These observations demonstratedthat FGFR2 plays a critical role in preventing primitive blooddifferentiation and promoting endothelial formation, consistentwith phenotypical analysis of fgfr2 null mice.⁷⁰

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Figure 5.. FGFR2 is the key mediator. (A) FGFR1 at HH4 (Ai), 5 (Aii), 6 (Aiii), 8 (Aiv), and 10 (Av). (B) FGFR2 at HH4 (Bi), 6 (Bii), 7 (Biii), 9 (Biv), and 10 (Bv). (C) FGFR3 at HH4 (Ci), 6 (Cii), and 10 (Ciii). (D) FGFR4 at HH4 (Di), 7 (Dii), and 10 (Diii). (E-G) Sections of FGFR1 (E), FGFR2 (F), and FGFR3 (G). Inset in panel F shows FGFR2 in endothelial but not blood cells. (H-M) Brown indicates electroporated cells; blue, blood cells stained with ${rho}$ ; arrowheads, endothelial distribution; arrows, blood distribution. CA-FGFR2 cells contribute mainly to endothelium (J,K,M), whereas control cells are seen among different lineages (H-I,L). See Table 2. (N-S) Blue indicates morpholino electroporated cells; brown, blood cells stained with ${rho}$ . Knockdown of FGFR2 with a splice block morpholino leads to blood localization (O,Q), and control morpholino cells are distributed among different lineages (N,P). Arrowheads indicate endothelial distribution; arrows, blood distribution. FGFR2 splice morpholino blocks FGFR2 mature transcript accumulation in neural ectoderm at HH4 (compare R with Bi). (S) Brown indicates morpholino-positive cells and blue FGFR2 expression (R shows embryo before morpholino staining).

Relationship with the VEGFR signaling pathway
Some of our observed effects may be explained by proposed rolesof VEGFR signaling during primitive hematopoiesis. VEGFR2 isinitially expressed in blood and endothelial precursors andvegfr2 null embryos die lacking both lineages.^34,35 In our analyses,FGF can induce the VEGFR2 expression and SU5402 resulted inits suppression, suggesting some effects were mediated via VEGFR.In bead graft with VEGF165 protein, however, we did not seeinhibition of ${rho}$ (Table 1). Since SU5402 can block kinase activityof both FGFRs and VEGFRs, we used a VEGFR-specific inhibitorSU5416⁷¹ to assess its contribution. As a control, we incubated15–hours after fertilization (hpf) zebrafish embryos withSU5416 until 30 hpf and observed enlarged pericardial cavityand failure of the establishment of circulation (data not shown),similar to what has been previously described.⁷² We then culturedchick embryos from HH6-7 in the presence of SU5416. Unlike intreatment with SU5402, no obvious effect on ${rho}$ expression wasobserved with SU5416 (Figure 6A,E), nor did we observe any remarkabledifference with Lmo2 (Figure 6D,H). Interestingly, we observeda slight up-regulation of endothelial marker Ets1 and Vegfr2with SU5416 treatment (Figure 6B-C, F-G), contrary to stronginhibition seen with SU5402. This evidence suggested that FGFRplays important roles during hematopoietic and endothelial differentiation,distinct from those mediated via VEGFR.
FGFR activity modulates expression level of hematopoietic marker Gata1
Primitive blood progenitors express earlier lineage markersGata2, Scl, and Gata1 before hemoglobin expression, indicatingthat events to separate the endothelial and hematopoietic lineagestake place prior to terminal differentiation. Gata1 has beensuggested as a definitive marker for the hematopoietic lineage,before the expression of terminal differentiation genes. Toinvestigate whether Gata1 plays a role in FGF-mediated inhibitionof terminal differentiation, we first analyzed Gata1 expressioncarefully during early development (Figure 6Ii-ii,Ji-ii,K-L,Mi-ii).The earliest expression of Gata1 in ventral mesoderm was detectedat HH5-6 (Figure 6Ji-ii), which covered the entire EEM area.Compared with globin genes, Gata1 was expressed both earlierand in a wider region. Up-regulation of Gata1 expression wasobserved from HH6-7 in future globin-positive cells (Figure 6Ji-ii,K).This suggested that the expression or activity level of Gata1is critical for its role as terminal activator. We then investigatedthe effect of FGF bead graft on Gata1 expression. Control beadsdid not affect Gata1 expression (0/40; Figure 6N-O), which atHH10 is up-regulated in blood cells and down-regulated in nonbloodcells. In cells adjacent to FGF4 beads, Gata1 can be detectedat low levels (Figure 6P-Q), which were weaker than in bloodcells (Figure 6R) but comparable to the level seen at HH5-6in the EEM (48/60). These Gata1-expressing cells adjacent tothe graft beads were completely devoid of globin expression(Figure 3E-F). This suggested that FGF activity can block theup-regulation of Gata1, which is critical in determining whetherto initiate the terminal differentiation program. Supportingthis hypothesis, we observed up-regulated Gata1 expression andexpanded Gata1-positive blood island clusters in medial EEMand lateral plate mesoderm in SU5402-treated embryos (compareFigure 6T,V with Figure 6S,U), similar to the effect on ${rho}$ expression(Figure 4L).

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Figure 6.. Contributions of VEGFR and hematopoietic marker Gata1 in FGFR-mediated effects. (A-H) Specific inhibition of VEGFR pathway by SU5416 does not affect ${rho}$ (E) or Lmo2 (H) expression and slightly up-regulates Vegfr2 (F) and Ets1 (G) compared with their respective controls (A,D,B,C). (I-M) Gata1 expression at HH4 (Ii-ii), 6 (Ji-ii), 7 (K), 8 (L), and 10 (Mi-ii). Arrowhead points to weak but broad expression in EEM. Sections of panels Ii, Ji, and Mi at indicated levels are shown in Iii, Jii, and Mii, respectively. (N-R) Control bead does not affect Gata1 expression (N-O), which at HH10 is up-regulated in blood and absent in nonblood cells (Mi-ii). FGF4 bead maintains low-level expression of Gata1 in adjacent cells (P-Q and section in R). These cells are completely negative for ${rho}$ (Figure 3F). Dotted line marks bead and arrow points to weak expression. (S-V) SU5402 treatment of whole embryo results in up-regulated and expanded Gata1 expression (T,V) compared with control (S,U), similar to the effect on ${rho}$ globin (Figure 4L).

   Discussion

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Abstract
Introduction
Materials and methods
Results
Discussion
References

The early phase of primitive hematopoiesis is dedicated to generatingerythrocytes, providing the sole source for circulating erythrocytesuntil embryonic day 12 (E12) in mice⁷³ and day 10 in chicks.⁷⁴Hemoglobin serves as a critical marker for its terminal differentiation.In this study, we report that 4 of the globin genes are expressedfrom early stages of primitive hematopoiesis. Each globin isexpressed in all blood cells, suggesting no allelic exclusionof embryonic globins within single blood cells. The initiationof ${rho}$ expression always takes place in a couple of cells followedby expression in surrounding cells, suggesting a stepwise terminaldifferentiation from precursor cells.
At HH7, ${rho}$ ⁺ cells are limited to the posterior and outer edgeof area vasculosa. The majority of EEM cells, having migratedextensively from their origin in the streak, are still ${rho}$ ^–at this stage. Our data suggest that migration and differentiationevents are distinctly regulated. Nevertheless, early steps ofdifferentiation marked by Gata2, Scl, and Gata1 for hematopoiesisand Vegfr2, Est1, and Vecad for vasculogenesis take place duringmigration, indicating differentiation itself is a multistepprocess. Aside from Gata1, however, these markers are initiallyexpressed in both lineages and only later resolve to a specificone. Other described terminal transcriptional regulators forhematopoiesis, such as EKLF, have their onset of expressionprior to the up-regulation of Gata1. The delayed expressionof hemoglobin indicates a tight regulation of the onset of terminaldifferentiation. Further investigation will be needed to understandthe precise mechanism of this delay.
We found that none of the factors tested can ectopically inducehemoglobin expression and only FGFs cause inhibition. Sincewe have not exhausted the list or tested combinations, we donot rule out the involvement of pathways that did not elicitan effect. The effects we observe with FGF are achieved throughcrosstalk with the VEGFR pathway, as Vegfr2 is up-regulatedby high FGFR activity and down-regulated by its inhibition.However, our data suggest the FGF pathway plays a distinct roleand is the primary mediator in this process, as specific inhibitionof VEGFR did not cause similar phenotypes. Crosstalk betweenthese 2 pathways as well as their distinct roles have been welldocumented in other systems.^48,75-77
Our evidence suggests FGF acts by modulating Gata1 expressionlevel or activity. Gata1 expression is considered the last stepbefore terminal differentiation. However, it is expressed bothearlier and more widely than globins, suggesting the requirementof intermediate steps. A recent study on the global gene regulationprofile of gata1 null erythroblasts demonstrated a significantdelay of globin gene transcription after reintroduction of Gata1,suggesting the involvement of additional signals.⁷⁸ Up-regulationof Gata1 expression, however, coincides with its purported roleas a terminal activator, suggesting the importance of Gata1level in terminal differentiation. A reduction of 4- to 5-foldin Gata1 expression was shown to markedly impair erythroid cellmaturation in mice.⁷⁹ In our analyses, FGF strongly inhibitsglobin gene expression, although the cells surrounding FGF beadsstill express weak but detectable levels of Gata1. The up-regulationof Gata1 expression, however, is inhibited by high FGF activity,and inhibition of FGFR activity prominently up-regulates Gata1expression in ectopically induced blood cells. Whether thisis achieved by a direct or indirect effect of the FGF signalingpathway will require further investigation.
In chicks, prestreak-stage marginal zone tissue can be inducedto form blood by bFGF.⁵¹ This is likely due to FGF's role inearly mesoderm induction and reflects different FGF functionsat different stages of early development. A similar report withdissociated quail prestreak-stage epiblast cells showed thatFGF can induce both blood and endothelial cells in culture.⁸⁰In Xenopus, midblastula animal cap cells can be induced by acombination of FGF and BMP to form Gata1-positive cells.⁵² AnotherXenopus study reported that FGF inhibits blood island formationand dominant-negative FGFR expands blood islands to the lateralplate mesoderm.⁵⁴ Although our analyses tend to agree with thelatter observation, and beads soaked with both BMP and FGF causedsimilar inhibition of ${rho}$ expression as with FGF alone (F.N. andG.S., unpublished data, 2006), these effects in Xenopus cannotbe easily compared with ours. The FGF pathway is well documentedto play pleiotropic roles in multiple early developmental processesand for this reason we have chosen to study only the terminaldifferentiation step within a defined developmental window.Our analyses, however, support studies on cultured progenitorcells. bFGF was reported to maintain the immature state of primitiveblood progenitors while blocking final differentiation.⁵⁵ Removalof FGF signaling effectively promoted final maturation.⁵⁵ Similarly,FGF activity was recently shown to block the final maturationof presomitic mesoderm (PSM) cells during somitogenesis.⁸¹ Inaddition, our study provides strong evidence that FGFR2 is themain mediator in this process. It is premature, however, tohypothesize which ligand/receptor pair may be involved, as thereare at least 22 FGF ligands and 2 FGFR2 isoforms.⁸² FGF4 and8 used in this study were described to be expressed mediallyin mesoderm precursor cells^83,84 and possibly create an FGFR2activity gradient along the medio-lateral axis to control thetiming of differentiation. Progressive decay of FGF8 mRNA canserve as a key mechanism for creating a morphogenetic gradientof FGF8 protein.⁸³ Both FGFs were shown to bind and activateFGFR2 effectively.⁷⁰ In addition to these 2 FGFs, other FGFtranscripts (3, 10, 12, 13, 14, and 19) were reported to beexpressed in ventral mesoderm precursors.^84,85 None has beenstudied in detail in the context of EEM differentiation. Throughgene array analysis, we have identified 5 additional FGFs expressedmedially and at least 3 FGFs expressed more laterally in differentiatingEEM cells (M.S., F.N., and G.S.; unpublished data, 2006). Additionalcomplexity was highlighted by specific roles played by differentisoforms.⁸⁶ Comprehensive analysis of dynamic expression patternsof different FGF molecules and their isoforms during EEM differentiationis currently being carried out.
Blood and endothelial differentiation are developmentally linked.The existence of bipotential precursor cells has been shownwith in vitro differentiation assays. Whether bipotential precursorcells exist at the single-cell level remains to be shown invivo. Within a population of undifferentiated blood island cells,the bias toward a particular lineage, the restriction of differentiationpotentials, and the terminal differentiation happen progressivelyand may require a delicate balance of inputs from transcriptionalregulators and signaling molecules. A surprising find in ourstudies is the tightness of this link. In our SU5402-treatedembryos, we found strong inhibition of all endothelial markerstested, yet endothelial-like cells still surround blood cells.However, they are not functional endothelial cells and failto establish a proper vascular network later in development.In medial regions where ectopic blood cells are induced, globin-negativecells with endothelial morphology are still observed withinthe same BI, no matter how few cells the BI contains. Theseobservations suggest that primitive hematopoiesis is tightlyregulated to occur in conjunction with endothelial differentiation,possibly controlled by yet unknown mechanisms to ensure thatall blood cells generated are properly connected to the circulatorysystem.

   Acknowledgements

We thank Erike Sukowati for help in embryology; Masahiko Hibifor help with fish experiments; and Shinichi Nishikawa, LeonardZon, Claudio Stern, Fred Wilt, and Brendan McIntyre for criticalcomments. This work was initiated in Claudio Stern's laboratory,and we thank him for continuous support.

   Footnotes

Submitted May 5, 2006; accepted July 10, 2006.
Prepublished online as Blood First Edition Paper, August 3,2006; DOI 10.1182/blood-2006-05-021386.

The authors declare no competing financial interests.

G.S. designed the experiments; F.N., H.N., M.S., and G.S. performedthe experiments; G.S., F.N., H.N., and M.S. analyzed the data;and G.S. wrote the paper.

F.N. and H.N. contributed equally to this study.

The publication costs of this article were defrayed in partby page charge payment. Therefore, and solely to indicate thisfact, this article is hereby marked "advertisement" in accordancewith 18 USC section 1734.

Reprints: Guojun Sheng, Laboratory for Early Embryogenesis, RIKEN Center for Developmental Biology, Kobe, Hyogo 650-0047, Japan; e-mail: sheng{at}cdb.riken.jp.

   References

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Baron MH. Early patterning of the mouse embryo: implications for hematopoietic commitment and differentiation. Exp Hematol. 2005;33: 1015-1020.[CrossRef][Medline] [Order article via Infotrieve]
McGrath KE, Palis J. Hematopoiesis in the yolk sac: more than meets the eye. Exp Hematol. 2005;33: 1021-1028.[CrossRef][Medline] [Order article via Infotrieve]
Dieterlen-Lievre F, Le Douarin NM. From the hemangioblast to self-tolerance: a series of innovations gained from studies on the avian embryo. Mech Dev. 2004;121: 1117-1128.[CrossRef][Medline] [Order article via Infotrieve]
Orkin SH, Zon LI. Hematopoiesis and stem cells: plasticity versus developmental heterogeneity. Nat Immunol. 2002;3: 323-328.[CrossRef][Medline] [Order article via Infotrieve]
Kondo M, Wagers AJ, Manz MG, et al. Biology of hematopoietic stem cells and progenitors: implications for clinical application. Annu Rev Immunol. 2003;21: 759-806.[CrossRef][Medline] [Order article via Infotrieve]
Dzierzak E. The emergence of definitive hematopoietic stem cells in the mammal. Curr Opin Hematol. 2005;12: 197-202.[CrossRef][Medline] [Order article via Infotrieve]
Psychoyos D, Stern CD. Fates and migratory routes of primitive streak cells in the chick embryo. Development. 1996;122: 1523-1534.[Abstract]
Minko K, Bollerot K, Drevon C, Hallais MF, Jaffredo T. From mesoderm to blood islands: patterns of key molecules during yolk sac erythropoiesis. Gene Expr Patterns. 2003;3: 261-272.[CrossRef][Medline] [Order article via Infotrieve]
Garcia-Martinez V, Schoenwolf GC. Positional control of mesoderm movement and fate during avian gastrulation and neurulation. Dev Dyn. 1992;193: 249-256.[Medline] [Order article via Infotrieve]
Hsia N, Zon LI. Transcriptional regulation of hematopoietic stem cell development in zebrafish. Exp Hematol. 2005;33: 1007-1014.[CrossRef][Medline] [Order article via Infotrieve]
Park C, Ma YD, Choi K. Evidence for the hemangioblast. Exp Hematol. 2005;33: 965-970.[CrossRef][Medline] [Order article via Infotrieve]
Jaffredo T, Nottingham W, Liddiard K, Bollerot K, Pouget C, de