The embryo makes red blood cell progenitors in every tissue simultaneously with blood vessel morphogenesis

doi:10.1152/ajpregu.00543.2002

The embryo makes red blood cell progenitors in every tissue simultaneously with blood vessel morphogenesis

Maria Luisa S. Sequeira Lopez¹, Daniel R. Cherñavvsky¹, Takayo Nomasa¹, Lee Wall², Masashi Yanagisawa³, and R. Ariel Gomez¹

¹ Department of Pediatrics, University of Virginia, Charlottesville, Virginia 22908; ² Department of Medicine, Université de Montréal, Quebec H2L 4M1, Canada; and ³ Howard Hughes Medical Institute, Department of Molecular Genetics, University of Texas Southwestern Medical Center, Dallas, Texas 75390-9050

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS AND DISCUSSION
REFERENCES

During embryonic life, hematopoiesis occurs first in the yolk sac, followed by the aorto-gonado-mesonephric region, the fetalliver, and the bone marrow. The possibility of hematopoiesis inother embryonic sites has been suspected for a long time. Withthe use of different methodologies (transgenic mice, electronmicroscopy, laser capture microdissection, organ culture, andcross-transplant experiments), we show that multiple regions withinthe embryo are capable of forming blood before and during organogenesis.This widespread phenomenon occurs by hemo-vasculogenesis, theformation of blood vessels accompanied by the simultaneous generationof red blood cells. Erythroblasts develop within aggregates ofendothelial cell precursors. When the lumen forms, the erythroblasts"bud" from endothelial cells into the forming vessel. The extensivehematopoietic capacity found in the embryo helps explain why,under pathological circumstances such as severe anemia, extramedullaryhematopoiesis can occur in any adult tissue. Understanding theintrinsic ability of tissues to manufacture their own blood cellsand vessels has the potential to advance the fields of organogenesis,regeneration, and tissueengineering.

development; hematopoiesis; homeostasis; kidney

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS AND DISCUSSION REFERENCES

IN THE VERTEBRATE embryo, hematopoietic and vascular endothelial cells are the first cells to differentiate in response toinduction of the mesoderm (2). In mice, endothelial cells andhematopoietic cells are first observed (when primitive hematopoiesisbegins) in the yolk sac at 7.5 days post coitum (9). Primitivehematopoiesis is restricted to the formation of nucleated erythrocytesthat express embryonic hemoglobin (43) and macrophages (7).

Definitive hematopoiesis is the process whereby all types of blood cells are formed followed by their differentiation, includingthe enucleation of erythrocytes. The initial site of definitivehematopoiesis is controversial. It has been proposed that thefirst site is in the splanchnopleural/aorto-gonado-mesonephric(AGM) area (10, 14, 24) and that early in development endothelialcells from the AGM region may themselves give rise to hematopoieticcells (6, 20, 37). As embryonic development continues,the site for hematopoiesis changes to the fetal liver and as theanimal matures to the bone marrow, where hematopoiesis persistsin the adult. The possibility of hematopoiesis occurring in otherembryonic sites has not been explored. During development of theyolk sac, hematopoiesis is intimately linked to the developmentof blood vessels. In fact, the ontogenic relationship betweenhematopoietic cells and the endothelial cells of the blood islandsof the yolk sac has been observed almost 100 years ago (34).A similar observation has also been made in the aorta and postumbilical and vitelline arteries where hematopoietic clustersseem to originate from hemogenic endothelium (6, 18, 20,37). The existence of a common precursor for endothelial cellsand hematopoietic cells, the hemangioblast, has been suspectedfor a long time (25, 30, 31, 34). Taken altogether, theseobservations suggest that vasculogenesis and hematopoiesis arepart of the same process, in which formation of a blood vesselis accompanied by the simultaneous in situ production of bloodcells within that vessel (hemo-vasculogenesis).

Our experiments show that 1) hematopoiesis is widespread in the embryo: in addition to the AGM area, fetal liver, and bonemarrow, the embryo makes erythroblasts in every tissue examinedbefore and during organogenesis and 2) hematopoiesis is tied toand integrated with the differentiation and morphogenesis of bloodvessels: formation of a vessel is accompanied by the generationof red cell precursors, suggesting that hematopoietic and vascularcells share a commonprecursor.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS AND DISCUSSION REFERENCES

Animals. Several mouse strains were studied: expressing Lac-Z driven by the Tie2 promoter (marks endothelial cells) (35) or underthe control of the $beta$ -globin LCR-promoter combination (marks erythroidcells) (16), expressing cre recombinase driven by the Tie2 promoter(22), ubiquitously expressing Lac-Z (ROSA 26), the ROSA26 LoxP reporter mice (38), and wild-type C57B6. Embryos at 11.5 daysof gestation (E11.5) were the source of fetal kidneys used forin vitro culture and for grafting under the kidney capsule. Time-datedpregnant mice were mated overnight and the females were checkedfor vaginal plugs the following morning. The day of detectionof a vaginal plug was regarded as day 0.5 of gestation. Graftingof embryonic kidneys under the kidney capsule was performed aspreviously described (36). All procedures were performed inaccordance with the Guiding Principles for Research InvolvingAnimals and Human Beings by the American Physiological Society(1) and were approved by the University of Virginia AnimalCareCommittee.

Immunohistochemistry and X-gal reaction. Embryonic tissues from mice were subjected to the X-gal reaction, paraffin embedded, sectioned (5 µm), and immunostained aspreviously described (36). The antibodies used were anti- $alpha$ -smoothmuscle actin ( $alpha$ -SMA) (Sigma) and anti-hemoglobin(DAKO).

Electron microscopy studies. E9.5 and E11.5 mouse embryos were dissected and fixed with 4% PFA and 2.5% glutaraldehyde at 4°C overnight, then postfixedin OsO₄, embedded in epoxy resin by conventional methods, cutinto 70- to 80-nm sections, and examined using a JEOL 100 CX transmissionelectronmicroscope.

Metanephric kidney culture. E11.5 kidneys from $beta$ -globin/LacZ + embryos (n = 24) were cultured for 72 h at 37°C as previously described (29). The definedserum-free medium (DMEM-F12) was supplemented with 10 mM HEPES,1.1 mg/ml NaHCO₃, 5 µg/ml insulin and transferrin, 2.8 nM selenite(Sigma), 25 ng/ml PGE₁ (Sigma), 32 pg/ml triiodothyronine (Sigma),50 U/ml penicillin G, and 50 U/ml mycostatin. The medium withadditives was changeddaily.

Metanephric kidney culture on top of embryonic stem cells. Embryonic stem (ES) cells from 129 SvEv mice were grown on top of irradiated feeder layers of primary murine embryonic fibroblastsplaced on top of cell culture inserts with 3-µm pore size (Falcon)on a six-well dish. Forty-eight hours later, E12 kidneys (n =17) from ROSA26 mice were dissected as previously described (36)and placed on top of the ES cell colonies for 5 days. Medium containingDMEM-H's (GIBCO) supplemented with 15% FBS (GIBCO), 1% sodiumpyruvate (GIBCO), 0.0008% $beta$ -mercaptoethanol (Sigma), 5 µg/ml insulinand transferrin, 2.8 nM selenite (Sigma), 25 ng/ml PGE₁ (Sigma),32 pg/ml triiodothyronine (Sigma), and 15 mU/ml erythropoietin(Sigma) was changed daily. Embryonic kidneys were fixed and subjectedto the X-Gal reaction as previously described (36).

Peripheral blood extraction. Mouse embryos at E12.5 and E14.5 were dissected from the uterus, membranes were opened, and the umbilical cord was cut tolet blood flow out from the cord. Blood samples were then collectedusing a P10 pipette. From anesthetized adult animals, blood wascollected from the abdominal aorta using a 1-ml syringe and a23-gaugeneedle.

Laser capture microdissection. Mouse embryos (E11.5) were harvested and fixed in 70% ethanol overnight. After dehydration with different alcohol gradientsand xylenes, tissues were embedded in paraffin and cut into 5-µmconsecutive sections. Sections were deparaffinized and stainedwith hematoxylin and eosin as follows: 70% ethanol for 30 s, hematoxylinfor 30 s, deionized H₂O for 30 s, bluing reagent (Richard-AllanScientific, Kalamazoo, MI) for 30 s, 70% ethanol for 1 min, 95%ethanol for 1 min, eosin for 30 s, 95% ethanol for 1 min two times,100% ethanol for 1 min, xylenes for 5 min two times, and thenair-drying for 20 min. Subsequently, the tissues were microdissectedusing a Pix Cell II laser capture microscope with an infrareddiode laser (Arcturus engineering, Santa Clara, CA) as described(3, 11). Briefly, the dehydrated section was overlaid witha cap that contains a thermoplastic membrane, and then focal meltingof the membrane through laser activation captured the cells. Aftervisual control of the completeness of dissection, the cap wasremoved and the captured cells were immersed in 50 µl of extractionbuffer (PicoPure RNA isolation Kit, Arcturus, Mountain View,CA).

RNA extraction, DNase treatment, and reverse transcription. With the use of laser capture microdissection (LCM), three different kinds of samples were extracted: 1) immature blood cells(vessel contents), 2) endothelial cells (vessel walls), and 3)"budding" cells (cells that were clearly budding from the vesselsinto the lumen). Samples of whole blood (E12.5, E14.5, and adultmouse) were also collected. RNA from these cells was obtained(PicoPure RNA isolation kit, Arcturus) following the manufacturer'sprotocol (5). The RNA pellets were dissolved in water and thentreated with RNase-free DNase (Ambion, Austin, TX). RNA reversetranscription was done using 5 µl of RNA, 1 µg oligo(dt) primer,25 µmol/l dNTPs, and 200 U M-MLV reverse transcriptase (Promega,Madison, WI) in 14 µl total volume. A mock reaction without additionof reverse transcriptase was also performed for each sample. Erythroid,endothelial, and smooth muscle markers were detected by PCR. $alpha$ -SMAmRNA was tested in peripheral blood samples from E12.5, E14.5,and adult mice and in LCM samples of the three groups of cells(immature blood cells, endothelial cells, and "budding" cells). $beta$ -Globin mRNA was tested in LCM samples of the three groups ofcells mentioned above. Tie2 mRNA was tested in peripheral bloodsamples from E12.5, E14.5, and in LCM samples of blood cells.Primers and PCR conditions for mouse $alpha$ -SMA were 5'-TAT GTA GCTCTG GAC TTT GAA-3' and 5'-CAG AGC AGG GGG GAC TTA GAA-3'. Annealingtemperature was 55°C, and the number of cycles was 40 (EppendorfMastercycler, Westbury, NY). Expected product of the cDNA amplificationwas 492bp.

$beta$ -Globin primers were 5'-CAC AAC CCC AGA AAC AGA CA-3' and 5'-CTG ACA GAT GCT CTC TTG GG-3'. Conditions were annealing temperature55°C, and the number of cycles was 40. The expected product sizewas 525 bp. For Tie2, we performed nested RT-PCR. Outer primerswere 5'-TGT CAA TCA GGC CTG GAA ATA C-3' and 5'-GAG GAG GGA GAATGT CAC TAA GG-3'. Conditions were annealing temperature 56.6°C,and the number of cycles was 40. The expected product size was464 bp. Inner primers were 5'-TAC TTG GAG CCG CGG ACT GAC-3' and5'-CGC CTT GGT GTT GAC TCT AGC-3'. Conditions were annealing temperature56.8°C, and the number of cycles was 40. The expected productsize was 351 bp. The amplification was performed using Taq DNApolymerase 0.75 U (Promega), 2 µl for the RT, and 25 µl totalvolume reaction. Negative controls included reaction without reversetranscriptase and without RNA. The PCR product was separated on1% agarose gel stained with ethidiumbromide.

	RESULTS AND DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS AND DISCUSSION REFERENCES

Erythropoiesis throughout the embryo. To study the lineage relationship between endothelial and erythroid cells and to define whether the latter cells and bloodvessels develop simultaneously from a common precursor as a widespreadphenomenon occurring throughout the embryo, we examined mouseembryos expressing LacZ under the control of the Tie2 promoter(marks endothelial cells) (35) or under the control of the $beta$ -globinLCR-promoter combination (marks erythroid cells) (16). In addition,to define whether endothelial cell precursors give origin to bloodcells, we examined embryos derived from the cross of Tie2-Cre(22) with the ROSA26 Lox P reporter mice (38). In mice derivedfrom this cross, endothelial cells and their progeny express LacZbecause once Cre-mediated recombination occurs, it activates LacZexpression and the recombined LacZ transgene is inherited throughthe cellular lineage. Thus, any cell that expresses the Tie2-Cretransgene and its descendants, whether they are still expressingthe transgene or not, will be blue with the X-galreaction.

At E8.5, there is already widespread expression of $beta$ -globin in erythroblasts and endothelial cells: it is not limited to theaorta and major vessels. In fact, $beta$ -globin expression is encounteredin multiple tissues throughout the embryo (Fig. 1, A-E) including,but not limited to, the areas surrounding the optic pit of thedeveloping head (Fig. 1B), the neural tube (Fig. 1, C and E),and in between the developing somites (Fig. 1D). Figure 1E shows $beta$ -globin/LacZ-positive erythroid cells "budding" from endothelialcells, a phenomenon that still persists at E11.5 while the vesselsare still forming (Fig. 1, F-H). Endothelial cells of "budding"areas share $beta$ -globin expression with erythroblasts. Confirmingthose findings, similar results are obtained in mice harboringa different promoter-reporter transgene. In Tie2/LacZ mouse embryos,as shown at E10.5 (Fig. 2, A-F and H-J), expression of LacZ isobserved both in endothelial cells and hematopoietic cells andin their mesenchymal precursors throughout the embryo. Figure2, B, C, and F, shows that mesenchymal derivatives surroundingthe developing brain contain LacZ-expressing cells in endotheliumand blood precursors. This tight relationship between endothelialcells and blood precursors is also evident during organogenesisin multiple organs of the developing embryo. For example, Fig.2G shows this relationship in the developing kidney at E16.5.

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Fig. 1. Distribution of $beta$ -globin expression as assessed by the X-Gal reaction in $beta$ -globin/LacZ embryos at embryonic day 8.5 (E8.5; A to E) and at E11.5 (F to H). LacZ expression in the whole embryo (A), surrounding the optic pit (op; B), surrounding the neural tube (nt; C), in between developing somites (s) (arrows) (D), and lining the dorsal aorta (arrowheads). E: LacZ expression is evident in both erythroid cells ("budding" from) and in endothelial cells (arrowhead), adjacent to the neuroepithelium (n). F: LacZ expression in "budding" cells (arrows) and endothelial cells (arrowheads) in the cephalic mesenchyme, in the developing plexus coroideus (G), and in a marginal vein in the left hindlimb bud (H). Scale bars: 200 µm (A); 100 µm (C); 50 µm (B, D, and G); 25 µm (E, F, and H).

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Fig. 2. Tie2 distribution, as assessed by the X-Gal reaction in Tie2/LacZ embryos at E10.5 (A-F and H-J) and in the developing kidney at E16.5 (G). H-J: smooth muscle cell identification by specific immunostaining with antibody against $alpha$ -smooth muscle actin (SMA) (36). LacZ staining in the whole embryo (A), higher magnification of (A) showing abundant Tie2 expression in cephalic mesenchyme (B), cephalic mesenchyme adjacent to the neuroepithelium (n) (C), dorsal mesenteric vessel showing cells budding from the endothelium (arrows) (D), concomitant expression of Tie2 by endothelial and circulating blood cells in a primary head vein (E), Tie2-expressing cells budding from endothelial cells in the cephalic mesenchyme (arrows) (F). G: developing capillaries adjacent to developing glomeruli show blood cells "budding" from endothelial cells (arrows). Insets, top, middle, and bottom: higher-magnification areas depicted by the arrows. H: coexistence of $alpha$ -SMA expression and Tie2 (LacZ) in circulating blood cells of a peripheral blood vessel. I: circulating blood cells expressing $alpha$ -SMA in the lumen of the aorta (a) and in a developing intersegmental artery adjacent to the dermomyotome (d) component of somites. J: higher magnification of I at the level of the intersegmental artery; the arrow indicates a blood cell expressing $alpha$ -SMA. Scale bars: 200 µm (A); 100 µm (B and I); 50 µm (C-H and J).

To define the lineage relationship between endothelial and erythroid cells, we took advantage of the Cre-Lox system. Tie2-Cretransgenic mice crossed to ROSA26 LoxP reporter mice generatedembryos expressing LacZ, after Cre-mediated recombination, inendothelial cells and their descendants. As shown in Fig. 3, theexpression pattern was similar to that seen in the Tie2/LacZ and $beta$ -globin/LacZ transgenic mice, supporting the concept that erythroidcells share a common precursor(s) with endothelial cells. Becauseoccasionally some mammalian cells exhibit endogenous $beta$ -galactosidaseactivity during development or apoptosis, we performed the X-galreaction in all littermates (Tie2-Cre alone, ROSA26 LoxP alone,and wild type) resulting from the aforementioned cross (Tie2-Cre× ROSA26 LoxP) at different embryonic and postnatal ages (E8.5,E9.5, E10.5, E11.5, E13.5, E16.5, newborns 2 and 5 days old) andnone of them showed $beta$ -galactosidase staining, demonstrating thatthe staining was specific and due to Cre-mediated recombinationin the appropriate cell types.

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Fig. 3. LacZ distribution in Tie2-Cre/R26R double transgenic embryos at E9.5 (A-C) and E10.5 (D). A: LacZ expression is observed in the endothelial cells of the forming vessels, in the cells that are budding (arrows) from them, and in the blood cells within the vessels. B-D: cells at different stages of budding from the endothelium. Scale bars: 100 µm (A); 50 µm (B-D).

In separate experiments, to corroborate whether LacZ expression corresponded to mRNA expression, we obtained endothelial cells,budding cells, and blood cells within vessels by the LCM technique(3, 11) and determined the expression of erythroid and endothelialmarkers by PCR. Endothelial cells from LCM samples were positivefor $beta$ -globin, and blood cells from both LCM and E12.5 and E14.5peripheral blood samples were positive for Tie2 (Fig. 4). Theseresults are in agreement with those obtained using the transgenicanimals described above.

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Fig. 4. RT-PCR gene expression analysis from laser capture microdissection (LCM) (E11.5) and embryonic peripheral blood samples (E12.5 and E14.5). LCM samples were obtained from developing vessels, from which 3 different cells were picked: blood cells present in the lumen (BC), endothelial cells (EC), and budding cells (Bd). $alpha$ -SMA, $beta$ -globin, and Tie2 transcripts were detected in LCM and blood samples. Peripheral blood was obtained from blood freely flowing from the umbilical cord. Reactions were performed in the presence (+) or absence ( $-$ ) of reverse transcriptase.

The overlap of erythroid and endothelial marker expression suggests a common origin between endothelial and erythroid cells.Altogether, the experiments suggest that vasculogenesis and hematopoiesisare intimately linked and occur concomitantly during vessel formation:as a new vessel is formed, erythroblasts also form. Kisanuki etal. (22) also observed circulating LacZ-positive cells in embryosderived from crossing Tie2-Cre mice with reporter mice as describedabove. Although it was hypothesized that these cells could becirculating endothelial progenitors, the present results suggestthat they are more likely to be red cell precursors. To clarifythis issue, we immunostained Tie2/LacZ embryos for hemoglobinand observed that the blue staining cells within the forming vesselswere also positive for hemoglobin (Fig. 5). We, therefore, concludethat those circulating cells (derived from a common precursortogether with endothelial cells) belong to the erythroid lineage.It also seemed possible that all cell types from a forming vessel,including smooth muscle cells of arterioles, as well as endothelialand erythroid cells, derive from the same precursor(s). To addressthis issue, we performed immunostaining for $alpha$ -SMA, a marker forsmooth muscle cells of the vessel wall (4, 40). Figure 2,H-J, shows expression of $alpha$ -SMA protein in blood cells within developingvessels throughout the Tie2/LacZ embryos at E10.5. Confirmingthese results, $alpha$ -SMA mRNA expression was detected by PCR in bloodfrom E12.5, E14.5 embryos, and adult mice (Fig. 4). $alpha$ -SMA mRNAexpression was also present in samples of blood, endothelium,and "budding" cells obtained by LCM (Fig. 4). Recently, Yamashitaet al. (45) demonstrated in vitro that cells expressing $alpha$ -SMA,as well as hematopoietic and endothelial cells, could arise froma population of cells originally derived from ES cells that expressthe vascular endothelial growth factor receptor 2, Flk1. Our resultssuggest that this phenomenon also occurs in vivo in the embryo,and together with the results of Yamashita et al. (45) the findingsindicate that all three cell types, vascular smooth muscle, endothelialand erythroid cells, may arise from a common precursor. Theseresults support the notion for a common ancestor for these celltypes. Whether this progenitor is the suspected hemangioblast(25, 30, 31, 34) remains to be determined.

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Fig. 5. Hemoglobin expression in Tie2/LacZ embryo at E10.5 (A and B) and in Tie2-Cre/R26R double transgenic embryo at E16.5 (C). A and B: arrows show that blood cells and budding cell immunostained for hemoglobin (dark brown) also express Tie2/LacZ (blue). C: concomitant expression of LacZ and hemoglobin is observed in blood and endothelial cells in embryonic tissue of skeletal muscle. Bars: 25 µm.

A summary of evidence supporting the relationship between endothelial cells and erythroid cells is depicted in Table 1.

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Table 1. Summary of findings: evidence for relationship between endothelial cells and erythroblasts during embryonic development

Hematopoiesis by budding. Clusters of hematopoietic cells have previously been observed within the aorta, vitelline, and umbilical arteries (13, 20,27, 32, 44). Budding cells from endothelial cells in thefloor of the aorta have been described (13, 20, 32) andthe concept of a hemogenic endothelium has been proposed basedon in vivo and in vitro studies that demonstrate that hematopoieticcells can be generated from endothelial cells (6, 18, 20,26, 37).

Our results show that budding of hematopoietic cells from endothelial cells is not restricted to a few areas and is observedthroughout the mouse embryo (Figs. 3 and 6). Also, the resultssupport the hypothesis of a common origin for both cell types.Hematopoietic cells are formed within and concomitantly with thedevelopment of new blood vessels. As a new blood vessel is formed,erythroid cells are seen "budding" from primitive endothelialcells lining the developing endothelial tubes. Mice expressingLacZ under the control of $beta$ -globin regulatory sequences showedthat endothelial cells and erythroid cells shared expression of $beta$ -globin. Moreover, expression of $beta$ -globin is limited to the areaswhere erythroid cells are actively developing from endothelialcells and is not seen in adult or developed vessels. Figure 3,B and C, describes different stages of the budding process foundthroughout the embryo, and Fig. 6, A-C, shows, at high magnification,the tight relationship between an endothelial cell and an erythroblastduring the budding process, indicating that it is not nonspecificsticking of erythroid cells or circulating endothelial cells.Clearly, the presence of "budding" hematopoietic cells is a commonoccurrence throughout the embryo and is encountered in a varietyof tissue types, including kidney, brain, skin, and others (seeFigs. 1-3 and 6). The "budding" process seen here in small developingvessels mimics the budding of blood cells from endothelial cellsthat occurs in the aorta as seen in Fig. 6, H and I. Furthermore,electron microscopy studies of developing vessels within the headof mice embryos (E9.5 and E11.5) allowed us to show the intimaterelationship between erythroblasts and endothelial cells duringvessel formation and to reconstruct the main stages of hemo-vasculogenesis(Fig. 7).

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Fig. 6. Budding of hematopoietic cells from endothelial cells is observed in multiple sites throughout the embryo in mice expressing LacZ under $beta$ -globin or Tie2 control. A-C: consecutive sections of E11.5 $beta$ -globin/LacZ embryo showing the close relationship between endothelial and erythroid cells adjacent to the facio-acoustic preganglion complex. A blue erythroid cell (arrow) is budding from an endothelial cell (arrowhead). The budding process in cells expressing $beta$ -globin is seen in the cephalic mesenchyme adjacent to the neuroepithelium (D) and also adjacent to the neuroepithelium at E8.5 (E). Mice expressing LacZ under Tie2 control show the budding process in dorsal posterior root ganglion (F) in the lower part of the embryo (G) adjacent to the neuroepithelium and in the aorta (H and I).

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Fig. 7. Stages of hemo-vasculogenesis. Electron microscopy of cephalic mesenchyme adjacent to the neuroepithelium (ne) of E9.5 mouse embryos. A: erythroblast (e) surrounded by mesenchymal cells (endothelial precursors). B: lumen starts to form but the e is still attached to the endothelial precursor. C: EC are lining the forming capillary; * indicates the area where the e and EC show communication. D: higher magnification of the area denoted by * in C showing "pore-like" communications (arrowheads). E: e detaching from EC; ** indicates the detaching region. F: higher magnification of the area denoted by ** in E showing the detaching region in more detail. Original magnification: A, ×27,000; B, ×17,820; C and E, ×8,910; D and F, ×54,000.

Hemo-vasculogenesis starts as an aggregate of cells (Fig. 7A). Eventually, the cells undergo further differentiation intoerythroblasts and vascular cells (Fig. 7B). Then, a cavity(s)is formed followed by formation of a lumen and the separationof erythroblasts from endothelial cells (Fig. 7, B-F). The factthat the process starts as a cell aggregate containing both celltypes (erythroblasts and endothelial cells) before lumen formationhas occurred suggests that both cell types develop in situ, aprocess that we described as hemo-vasculogenesis. The mechanismsgoverning hemo-vasculogenesis are unclear. The Cbfa2 gene (alsoknown as AML1, Runx1, and PEBPA2A) is required for the formationof intra-aortic hematopoietic clusters and cystic detachment ofcells into the lumen during embryonic life (27, 28). Thosefindings resemble the results presented here for hemo-vasculogenesisin the developing head. It remains to be determined whether thisgene or related ones are involved in the process of hemo-vasculogenesisin other tissues besides theaorta.

Kidney as a model for hematopoiesis during organogenesis. To address the question whether hematopoiesis occurs during organogenesis, we chose the kidney as a model to perform furtherexperiments. We demonstrate herein that the embryonic kidney iscapable of producing its own blood cells, particularly cells ofthe erythroid lineage. Although it has been suggested that theAGM area is a site for blood formation in the early mouse embryo(10, 14, 20, 24), the formation of blood by the definitive(metanephric) kidney during the period of active organogenesiswas previously unknown. The studies presented below clearly showthat blood precursors, presumably erythroblasts, are present inthe undifferentiated metanephric mesenchyma before nephrogenesishas ensued (Fig. 8, A and C). When these embryonic kidneys aregrown in vitro, nephrogenesis takes place. However, under theusual culture conditions, glomerular development is avascular.To study the capacity of the embryonic kidney to generate itsown blood and taking advantage of the mouse model that expressesLacZ under the control of the $beta$ -globin promoter (16), E11.5kidneys from $beta$ -globin/LacZ + embryos were cultured for 72 h. Asshown in Fig. 8, A and C, at E11.5, when the embryonic kidneyis still avascular, the metanephric blastema possesses only fewand scattered individual LacZ + cells, mostly surrounding thedeveloping ureteric bud. After 72 h in culture, there was an increasein the number of erythroid cells (Fig. 8, B and D) and the distributionof the LacZ + cells resembled the normal pattern encountered inthe E14.5 kidneys from animals that develop in utero (Fig. 8E).These results indicate that erythropoietic precursors within themetanephric mesenchyma continue to proliferate under culture conditions.

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Fig. 8. Hemo-vasculogenesis in embryonic kidneys grown in vitro (A-D), on top of embryonic stem (ES) cells (F-H), and under the kidney capsule (I and J). In vitro culture of E11.5 kidneys from $beta$ -globin/LacZ embryos. A: E11.5 whole kidney with scattered cells expressing $beta$ -globin. B: after 72 h in culture, there is an increase in the number of $beta$ -globin expressing cells. C: section of A with scattered blue cells surrounding the developing ureter (arrows); D: section from B shows an increase in the number of $beta$ -globin-positive cells. For comparison, E shows the normal in vivo increase in $beta$ -globin expressing cells at E14.5. Hemo-vasculogenesis in ROSA26 embryonic kidneys either grown (F-H) on top of ES cells or transplanted under the kidney capsule of an adult mouse (I and J). E11.5 ROSA26 embryonic kidneys were cultured for 5 days on top of wild-type ES cells. F: embryonic kidneys were invaded by ES cells (pink) that underwent branching morphogenesis and developed tubular structures. G and H: however, the metanephric mesenchyme derived from the embryonic kidney underwent hemo-vasculogenesis (arrows). H: enlarged view of a focus of hemo-vasculogenesis in the embryonic kidney. The budding process also observed here is indistinguishable from the one observed in vivo. X-gal reaction and counterstaining with nuclear fast red (36) show that the cells derived from the ROSA26 kidneys have blue cytoplasm and pink nuclei, whereas the ones derived from the wild-type ES cells have pink nuclei and cytoplasm. I and J: ROSA26 embryonic kidneys transplanted under the kidney capsule of a wild-type mouse differentiated, forming blue nephrons, blood vessels, and blood cells (arrows) demonstrating that these structures originated from the embryonic kidney. J: blood cell within the developing arteriole expresses $alpha$ -SMA (arrow), further suggesting a common origin of vascular and blood cells. Smooth muscle cells are identified by specific immunostaining (brown color) with antibody against $alpha$ -SMA (4). Bars: 100 µm (F); 50 µm (D, E, G, I, and J).

To strengthen the hypothesis that the kidney produces its own blood, we cultured embryonic kidneys from ROSA 26 mice (in whichall cells are blue with the X-gal reaction) on top of wild-typeES cells for 5 days. This in vitro system showed that whereasureteric branches developed from ES cells (Fig. 8F), $beta$ -gal + bloodislands originated from the ROSA 26 embryonic kidney (Fig. 8,G and H) demonstrating the embryonic kidney's intrinsic capacityto form its own blood. Furthermore, in these culture conditions,blood cells also originate by "budding" (Fig. 8H) as it occursin the intact embryo, suggesting that this is a built-in processprogrammed to occur even under in vitro conditions. Similarly,in vivo experiments, in which E11.5 Rosa 26 embryonic kidneys(all cells are blue) were transplanted under the kidney capsuleof adult wild-type mice kidneys for 7 days, revealed that allvascular elements, including blood cells, stained blue after theX-gal reaction (Fig. 8, I and J), suggesting the intrinsic metanephricorigin of blood and vascular cells. Although we cannot completelyexclude the possibility that errand cells coming from the AGMregion may have seeded the embryonic kidney, the possibility seemsremote considering that hemo-vasculogenesis occurs initially asan aggregate of cells that later differentiate in situ into erythroblastand endothelial cells. If the origin of the blood cells were extrarenal,it would not invalidate the fact that they undergo further differentiationplus cell division in situ. Our data suggest, however, that theprocess occurs in situ, not from migrating cells but very likelyfrom mesenchymal precursors residing in the embryonic organ. Thelineage relationship between "hemo-vasculogenic" cells and othercell types in the kidney remains to be studied. The ability ofthe kidney to make its own blood has also been observed in earlynonmammalian species, such as adult frogs, suggesting that thismechanism is phylogenetically conserved. The presumptive mesonephricanlagen in nonmammalian vertebrates generates hematopoietic precursorsand the promesonephros serves as a hematopoietic site (42).Interestingly, as we showed for the whole embryo, these cross-transplantationexperiments also revealed the expression of $alpha$ -SMA protein by bloodcells within the transplanted embryonic kidney (Fig. 8J) reflectingthe fact that blood and blood vessel development have a commonorigin and occurconcomitantly.

It has been well recognized that during embryonic life, hematopoiesis occurs first in the yolk sac followed by the AGM region,the fetal liver, and then the bone marrow. In the present study,we used different approaches and techniques and showed that multipleembryonic tissues have the capacity to produce blood cells. Thepresent findings provide strong evidence for hemo-vasculogenesis,the simultaneous, local generation of blood and vessels likelyderived from related precursor cell(s). The results do not invalidatethe possibility that cells originating from distant sites (i.e.,AGM region) could coexist in situ or in the circulation with bloodcells that developed locally simultaneously with vessel morphogenesis.However, it should be noted that in many organs, we observed erythroblastsbefore vascularization to that organ had occurred, implying thatdistant cells could not access the tissue via the circulation.It is still possible that seeding from distant sites may occurthrough other mechanisms such as cell migration. Future work willbe needed to ascertain thispossibility.

The fact that hemo-vasculogenesis is widespread throughout the whole embryo during development may explain why extramedullaryhematopoiesis occurs in adult life in almost any tissue and organ[i.e., skull (21), brain (12), liver, spleen, kidneys, adrenalglands, breast, paravertebral and presacral areas (41), skin,testicles (33), heart (17), lung (46), gastrointestinaltract (39), pancreas (8), prostate (19), and others] whenblood availability is affected. It would appear that hematopoiesiscan be reactivated as a compensatory mechanism in organs or regionswhere it previously occurred during embryonic and fetallife.

The above observations suggest that many adult tissues have the capacity to reactivate gene expression after a period of latencyunder circumstances of abnormal physiology or disease. This processcan occur in vivo under pathophysiological circumstances as away of compensating the lack or malfunction of a specific tissue.As discussed above, the ability of adult tissues to generate bloodcould be explained either by the reactivation of a gene programin differentiated cells that have retained the capacity to reacquirean embryonic phenotype, or likely, the differentiation of residentprecursor cells with hemo-vasculogenic potential when the physiologicalconditions demand it to maintain homeostasis. Examples for bothpossibilities seem to occur in nature for other systems (15,23, 31). Further work will be necessary to define which oneof these possibilities occurs during extramedullaryhematopoiesis.

A fundamental problem in experimental organogenesis is to obtain appropriate tissue circulation. A substantial amount of experimentalwork will be needed to understand the mechanisms underlying hemo-vasculogenesis.Nevertheless, because hemo-vasculogenesis can be reproduced invitro and in transplanted embryonic tissues, it offers new opportunitiesin tissue regeneration andorganogenesis.

	ACKNOWLEDGEMENTS

We are grateful to O. Smithies, A. N. Goldfarb, B. Gumbiner, and D. De Simone for discussions and suggestions. We thank E.S. Pentz for advice in primer design and ES cellculture.

	FOOTNOTES

This work was supported by National Institutes of Health Grants (Center of Excellence in Pediatric Nephrology, DK-52612; RO1,HL-66242; CHRC, HDO-1421-01). Dr. Sequeira Lopez is a Howard HughesMedical Institute Physician PostdoctoralFellow.

Address for reprint requests and other correspondence: R. Ariel Gomez, Robert J. Roberts Professor of Pediatrics and Biology,Vice President for Research and Public Service, MR4 Bldg., Rm.2001, Univ. of Virginia, 300 Lane Road, Charlottesville, VA 22908(E-mail: rg{at}virginia.edu).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

First published December 19, 2002;10.1152/ajpregu.00543.2002

Received 6 September 2002; accepted in final form 17 December 2002.

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