1 UMR 5535, Institut de Génétique Moléculaire, IFR122, 1919 Route de Mende
2 INSERM U475, 99 rue Puech Villa, F 34000-Montpellier, France
3 UMR 5124, Institut de Génétique Moléculaire, IFR122, 1919 Route de Mende
* Author for correspondence (e-mail: mathieu{at}igm.cnrs-mop.fr)
Accepted 31 October 2003
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Summary |
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Key words: TAL-1/SCL, bHLH, Angiogenesis, Endothelial cells
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Introduction |
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Angiogenesis is required for a number of physiological situations in adult life such as pregnancy, menstrual cycle, and tissue repair. Neoangiogenesis is also observed under pathological conditions such as tumors, inflammatory disorders, atherosclerosis and diabetes. In adults, endothelial cells normally remain quiescent, show a low turnover rate and rarely proliferate. However, following an appropriate stimulus, endothelial cells are activated and participate in angiogenesis. Members of the vascular endothelial growth factor (VEGF) and angiopoietin families are considered to be key angiogenic mediators contributing to both physiological and pathological angiogenesis (for a review, see Gale and Yancopoulos, 1999).
Despite recent progress in the identification of signaling molecules and cell surface receptors that regulate blood vessel formation, little is currently known about the precise nuclear transcriptional events that govern endothelial fate. Gene knockout in mice has allowed the identification of several transcription factors such as ETS-1 (Lelievre et al., 2001), TEL (Wang et al., 1997
), FLI (Hart et al., 2000
) and the Lim-only protein LMO-2 (Yamada et al., 2000
), as potential mediators of angiogenesis.
Several basic helix-loop-helix factors, or bHLHs, (Henderson et al., 2001; Visvader et al., 1998
; Yamagishi et al., 2000
) and their inhibitors, the Id protein family (Lyden et al., 1999
; Lyden et al., 2001
) have been shown to participate in the formation and/or maturation of the vascular system. Initially identified by us and others as an oncogene in human T cell leukemia (Aplan et al., 1990
; Baer, 1993
; Begley et al., 1989
; Bernard et al., 1990
), the bHLH gene tal-1, also named scl, was found to be essential for normal embryonic and definitive hematopoiesis (Porcher et al., 1996
; Robb et al., 1995
; Shivdasani et al., 1995
) as well as for proper vascular development (Visvader et al., 1998
); tal-1/ embryos, rescued for tal-1 expression in primitive hematopoietic cells, exhibit defective yolk sac angiogenesis, presumably due to an intrinsic defect in tal-1/ endothelial cells (Visvader et al., 1998
). It also appears that tal-1 activity may be important for the commitment of the common precursor of both hematopoietic and endothelial lineages, the hemangioblast. During embryogenesis, tal-1 is one of the first markers detected in isolated mesodermal cells that give rise to angioblasts while its expression is down-regulated in the endothelium of mature vessels (Drake et al., 1997
; Drake and Fleming, 2000
). Overexpression of tal-1 in zebrafish embryos leads to an increase in both hematopoietic and endothelial markers (Gering et al., 1998
). Furthermore, tal-1/ ES cells are unable to generate hemangioblast-derived blast colonies, but do give rise to colonies that appear to represent a novel stage in the transition from mesoderm to hematopoietic and endothelial lineage commitment (Robertson et al., 2000
). In adults, tal-1 expression in non-hematopoietic cells is restricted to endothelial cells lining new blood vessels (Kallianpur et al., 1994
; Pulford et al., 1995
). Furthermore, TAL-1 has been proposed to modulate, in combination with GATA and ETS transcription factors, the Flk-1 gene that is known to play a pivotal role in both vasculogenesis and angiogenesis (Kappel et al., 2000
). Finally, TAL-1 protein is expressed at high levels in the vasculature of human tumors but not in mature quiescent vasculature (Chetty et al., 1997
). Based on these observations, tal-1 has been proposed to regulate molecular and cellular events involved in both vasculogenesis and angiogenesis.
In the present study, we have investigated the role of TAL-1 in the different processes of adult angiogenesis. TAL-1 expression was modulated in primary human endothelial cells using adenoviral vectors transducing wild-type or dominant-negative mutant TAL-1 protein, or knocked down by RNA interference, and the effects on migration, proliferation, and in vitro and in vivo angiogenesis were assessed.
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Materials and Methods |
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CD34 + cell separation and expansion of UCB-endothelial cells
Mononucleated cells (MNCs) were isolated from umbilical cord blood using the Histoplaque-density centrifugation method. CD34-positive cells were separated from 1-2x108 MNCs by positive selection using CD34 monoclonal antibody coupled to magnetic beads (MACS, Miltenyi Biotech). 1-2x106 CD34+ cells were plated on gelatin-coated tissue culture flasks in endothelial-specific medium supplemented with 10% FBS and appropriate cytokines (ECGF, bFGF and EGF). Non-adherent cells were eliminated by regularly changing the medium during the first 6 days of culture. By 3-4 weeks, the cells formed a monolayer with a typical endothelial spindle-shaped morphology; FACS analysis indicated that the majority of the cells expressed the specific endothelial markers, VE-cadherin and CD31 (85% and 95%, respectively).
Adenovirus construction and production
Recombinant adenoviruses were generated using the Adeno-XTM Tet-OffTM expression system (Clontech, USA) following the instructions of the manufacturer. Ad-TRE-wtTAL-1 contains a 1.35 kilobase fragment which is the entire human TAL-1 wild-type coding sequence (Leroy et al., 1995). Ad-TRE-
bas contains a 1.1 kilobase EcoRI fragment derived from pCSCL
B (Aplan et al., 1990
) in which the sequences encoding the basic region of human TAL-1 protein have been deleted (amino acids 188-199).
Recombinant defective adenoviruses were produced by transfection of human embryonic kidney (HEK) 293 cells. After serial amplifications in 293 cells, adenoviral particles were purified by two successive ultracentrifugations through a CsCl gradient. Virus stocks were resuspended in 3% sucrose in phosphate-buffered saline (PBS), aliquoted and stored at -80°C prior to infection. Independent productions were carried out in the laboratory and by `The Vector Core of the Hospital of Nantes' supported by the Association Française contre les Myopathies (AFM).
Transduction of endothelial cells
Exponentially growing ECs were seeded onto collagen I-coated dishes. After 4 hours at 37°C, ECs were co-infected with Ad-Tet-Off and either Ad-TRE-wtTAL-1, Ad-TRE-bas or control Ad-TRE-LacZ (ratio 2:1) at a multiplicity of infection of 100 for HUVECs and of 200 for UCB-ECs in endothelial-specific complete medium. Biological tests (in vitro angiogenesis, cell migration and proliferation) and preparation of whole cell lysates were carried out between 20 and 24 hours after adenoviral infection.
Matrigel-based in vitro angiogenesis
Wells of a 24-well plate were coated with Matrigel (BD Biosciences) and incubated at 37°C for 30 minutes. 1x105 cells (HUVECs), 8x104 cells (UCB-ECs) or 2x105 cells (HMEC-1) in complete EC medium were added to Matrigel-coated wells and incubated at 37°C with 5% CO2 for 24 hours. When required, cells were recovered from Matrigel and treated with Matrisperse (BD Biosciences) in the presence of a 5-fold concentrated cocktail of protease inhibitors (Boehringer Mannheim). After treatment, cells were centrifuged and washed with PBS for preparation of cell extracts.
Western blot analysis
Western blots were performed as described previously (Leroy et al., 1995). Membranes were probed with the monoclonal anti-TAL-1 antibody 3 BTL 73 (Pulford et al., 1995
) using a goat anti-mouse IgG/horseradish peroxidase conjugate (Amersham) as the secondary antibody. Bands were developed using a chemiluminescent substrate (ECL Plus, Amersham). As a control for loading and normalization, membranes were reprobed with an anti-GAPDH rabbit antiserum (kindly provided by Jean-Marie Blanchard, France). Bands were scanned with Snaps Scan 1236 (AGFA) and quantified using the program Scion.
Total RNA preparation and real-time PCR analysis
Total RNA was extracted using the High Pure RNA Isolation kit (Roche Diagnostics) following the manufacturer's instructions. Reverse transcription using 1.0 µg total RNA was performed with SuperScript II reverse transcriptase (Gibco-BRL) and oligo(dT) priming. The primer sequences of the oligonucleotides used for PCR were as follows:
tal-1 forward: 5'-CTCGGCAGCGGGTTCTTTGG-3'
tal-1 reverse: 5'-GCCTGCTTCACCACCTTCTTG-3'
GAPDH forward: 5'-ACAGTCCATGCCATCACTGCC-3'
GAPDH reverse: 5'-GCCTGCTTCACCACCTTCTTG-3'
PCR amplification reactions were performed in a DNA thermal cycler (Light cycler ROCHE). DNA was denatured at 95°C, followed by 45 PCR cycles; each cycle included denaturation at 95°C, primer annealing for 10 seconds at 65°C (for tal-1) or 5 seconds at 70°C (for GAPDH) and a final elongation step of 15 seconds at 72°C. PCR products were analyzed using the Light Cycler ROCHE program.
Electrophoretic mobility shift assay (EMSA)
Nuclear extracts were prepared as described previously (Courtes et al., 2000). Each 10 µl reaction mixture contained, 3 or 10 µg of nuclear extract, 10 mM Hepes (pH 7.8), 50 mM KCl, 2 mM MgCl2, 1 mM EDTA, 1 mM dithiothreitol, 0.5 µg of poly(dIdC) and 100,000 cpm of a 32P-labeled double-stranded oligonucleotide probe containing the TAL-1 E-box sequence (5'-ACCTGAACAGATG-GTCGGCT-3'). For supershift, the following antibodies were used: mAb anti-TAL-1 (3BTL 73), mAb anti-E47 (BD Pharmingen) or the irrelevant 12CA5 mAb (anti-HA).
In vivo assessment of angiogenesis
500 µl ice-cold Matrigel (9-10 mg/ml; BD Biosciences) mixed with heparin (10 U/ml; Sigma), and bFGF (250 ng/ml; Peprotech, Inc. USA) were injected subcutaneously into 8- to 16-week-old male SCID mice at sites near the abdominal midline, with three injections per mouse. Injection sites were chosen such that each animal received the three different recombinant Ad-TRE: LacZ, wtTAL-1, bas along with the Ad-Tet-Off (3x108 total infectious particles; ratio Ad-Tet-Off/Ad-TRE-: 2:1). The mixture of adenoviral vectors was either incorporated in the Matrigel prior to subcutaneous implantation in the abdomen of SCID mice or injected within the plug 1 day after implantation. Animals were sacrificed 5 or 7 days after injection; implants together with associated skin were recovered and immediately photographed.
For histological analysis, implants were fixed in 3.7% buffered formaldehyde in PBS, embedded in paraffin wax, sectioned, deparaffined and stained with Hematoxylin and Eosin. For immunohistochemical analysis, Matrigel plugs were embedded in Cryomatrix compound (Thermo Shandon, USA) and snap frozen in liquid nitrogen. Frozen implants were then sectioned in 5 µM sections, fixed with 3.7% buffered formaldehyde in PBS and stained with anti-CD31 rat mAb (clone MEC13.3, Pharmingen). Bound rabbit anti-rat secondary biotinylated Ab was visualized using Extravidin horseradish peroxydase (Sigma Chemical Co).
Migration assays
Migration assays were performed as described previously (Levy et al., 2002). The cells that had migrated through the inserts were fixed in 3.7% formalin, stained with propidium iodide and analyzed under a fluorescence microscope. The cells that had spread on the lower side of the inserts were counted on photographs of six random fields per well (original magnification, x10).
SiRNA preparation and transfection
SiRNAs targeting two sites in the tal-1 mRNA, chosen on the basis of the criteria outlined in Elbashir et al. (Elbashir et al., 2001), were prepared by in vitro transcription using the Silencer siRNA construction kit (Ambion, Austin Texas, USA). Preliminary results (not shown) demonstrated that gene silencing was more efficient with one of the two targets (nt 879-897) (Bernard et al., 1991
). This sequence was targeted in further experiments with a chemically synthesized siRNA (Eurogentec, Belgium).
tal-1 sense strand: 5'-GAAGCUCAGCAAGAAUGAGTT-3'
tal-1 antisense strand: 5'-CUCAUUCUUGCUGAGCUUCTT-3'
A chemically synthesized siRNA targeting an irrelevant sequence was used as a control:
Control sense strand:5'-GUGUUGGGUCGCGAAAGGCTT-3'
Control antisense strand: 5'-GCCUUUCGCGACCCAACACTT-3'
(The 3' TT in all strands was DNA.)
The day before transfection, HUVECs were plated onto 60 mm dishes coated with gelatin, at 30-35% confluency in complete EC medium. Two successive transfections of siRNA (1.0 µg per 60 mm dish) at 24-hour interval were carried out with Lipofectamine Plus (Invitrogen). Cells were analyzed 24-48 hours after the second transfection.
Statistical analysis
All results were expressed as the mean±s.d. Significance of differences was determined with the Student's t-test with significance at P<0.05.
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Results |
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tal-1 expression is reduced in non-proliferating ECs in the absence of endothelial-specific growth factors
Several studies have reported that quiescent human and murine endothelia do not express tal-1 (Chetty et al., 1997; Kallianpur et al., 1994
). Therefore, we analyzed tal-1 expression in non-proliferating ECs. Exponentially growing HUVECs were brought to confluence in complete endothelial-specific medium. Thereafter, the medium was replaced by M199 medium containing 5% serum without EC-specific growth factors. Total cell lysates and total RNA were prepared at different time points and tal-1 expression was analyzed. The kinetics of TAL-1 protein expression in HUVEC maintained in the absence of endothelial-specific growth factors demonstrated a 60% and 80% decrease after 3 and 8 hours of starvation respectively (Fig. 1B, left). The decrease in TAL-1 expression was not specific to the confluent nature of the cells as maintenance of these cells in complete endothelial-specific medium for an additional 24 hours resulted in a slight increase in TAL-1 protein content (about 1.5- to 2-fold as compared to exponentially growing ECs; data not shown).
To investigate whether TAL-1 down-regulation was associated with decreased mRNA levels, real-time PCR analysis was performed using the Light Cycler System (Roche) and GAPDH expression was used for normalization. As shown in Fig. 1B (right), tal-1 mRNA levels were decreased by 80% following a 3-hour culture without endothelial-specific growth factors as compared to exponentially growing cells. Thus, this phenomenon is associated with diminished tal-1 mRNA and protein levels.
Modulation of TAL-1 protein during in vitro angiogenesis
In vitro angiogenesis operates on the principle that ECs form capillary-like structures when cultured on a supportive matrix derived from a murine tumor (Matrigel). This assay reproduces the angiogenic processes of migration, alignment and cell differentiation, and has proved to be an important tool for studying the mechanisms of angiogenesis (Cid et al., 1993; Nicosia and Ottinetti, 1990
).
A typical in vitro angiogenesis experiment is shown in Fig. 2A. ECs plated on Matrigel underwent alignment and elongation within 1-3 hours after seeding, establishing the pattern for further capillary networking. By 6 hours, formation of cords had begun and by 12 hours virtually all cells had fused into continuous cords. Stabilization and refinement of the cords progressed until 24 hours. We studied the kinetics of endogenous TAL-1 expression during in vitro angiogenesis of human ECs. Fig. 2B illustrates an immunoblot analysis from one typical experiment with HUVECs. Whereas a small decrease in TAL-1 was detected within the first hours (5 hours), a significant increase in TAL-1 protein levels was repeatedly observed during the step of the cord-maturation process (12-24 hours), 3- to 5-fold higher than that detected in exponentially growing cells (Fig. 2B). Similar experiments were carried out with UBC-ECs (Fig. 2C) and immortalized HDMECs (HMEC-1 cells; fig. 2D) and in a similar manner to HUVECs, TAL-1 protein decreased by 3 or 5 hours (60% and 80% reduction respectively), followed by a progressive increase, which reached a maximum at 24 hours when the capillary-like network was formed.
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Altogether, our data show that TAL-1 expression is modulated during in vitro angiogenesis: down regulated within the early steps of migration and upregulated during tubule-like morphogenesis process.
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Effects of overexpression of wild-type or mutant TAL-1 protein on in vitro angiogenesis |
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Recombinant adenoviral vectors were used to mediate gene transfer; the transgenes encoding TAL-1 proteins were placed under the control of tetracycline responsive elements (Ad-TRE-) and a minimal cytomegalovirus promoter (Adeno-X Tet-Off; Clontech). In this system, transgene expression is activated by co-infection of an adenovirus constitutively expressing the tetracycline repressor (Ad-Tet-Off). Using these recombinant adenoviruses, we routinely observed high efficiency of infection of human ECs (essentially 100% at a m.o.i. of 100 for HUVECs and of 200 for UCB-ECs) as assessed by co-infection with the control adenovirus transducing the ß-galactosidase gene (Ad-TRE-LacZ).
The ectopic expression of both wt and bas TAL-1 proteins was systematically confirmed by western blot analysis. As illustrated in Fig. 3A, HUVECs transduced with either TRE-wtTAL-1 or TRE-
bas overexpressed the ectopic protein about 100-fold over endogenous TAL-1 levels. In hematopoietic cells, TAL-1 proteins have been shown to bind a specific E-box DNA motif (AACAGATGGT) as heterodimers with ubiquitous bHLH (E proteins), preferentially with the E47 isoform encoded by the E2A gene (Hsu et al., 1994a
; Hsu et al., 1994b
). Therefore, we assessed the DNA-binding activity of endogenous TAL-1 in ECs by electrophoretic mobility shift assays (EMSA). Nuclear extracts (10 µg) from non-infected HUVECs were incubated with a DNA probe containing the specific E-box sequences. In addition to the major complexes, which contain homo- and heterodimers of E proteins, EMSA revealed a slower migrating specific complex which contained TAL-1/E47 heterodimers as demonstrated by an anti-TAL-1 mAb-induced supershift and reduced complex in the presence of the anti-E47 antibody (Fig. 3B, left). Thus, in endothelial cells, TAL-1 interacts with E47 to bind the TAL-1 E-box motif.
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The DNA-binding properties of the exogenous TAL-1 were controlled by EMSA experiments. Ad-wtTAL-1-infected HUVECs overexpressed active TAL-1 as demonstrated by a significant increase in TAL-1/E-DNA complex formation in nuclear extracts (Fig. 3B, right). As expected, no TAL-1/E DNA complex was detected in Ad-bas-infected HUVECs. Complexes formed by endogenous TAL-1 were not detected in control Ad-LacZ-infected HUVECs, because of the experimental conditions (only 3 µg of nuclear extracts were used in these assays).
Twenty hours post-infection, transduced ECs were plated onto Matrigel and incubated for an additional 24 hours; a typical experiment with HUVECs is shown in Fig. 3C. At 90 minutes after seeding, most of the Ad-LacZ- and Ad-wtTAL-1-infected ECs had lost their cobblestone morphology and had formed chains of cells. Repeatedly, the cytoplasmic extensions that precede cord formation occurred earlier and were more numerous in wtTAL-1-transduced ECs as compared to LacZ-control ECs (Fig. 3C, 90 minutes). In contrast, bas-transduced cells displayed a very poor alignment and developed very few cytoplasmic extensions. At 20 hours, transduction of wtTAL-1 did not result in gross modifications in tubule-like network as compared to control infected cells. In striking contrast, Ad
bas transduction provoked a complete disorganization of capillary-like structures. Similar observations were made with UCB-ECs (not shown).
These in vitro experiments showed that wt TAL-1 ectopic expression accelerates the process of tubule-like morphogenesis, while bas overexpression completely inhibits this process. Therefore, TAL-1 activity appears to function as a signal to stimulate endothelial cell morphogenesis as measured in this in vitro assay.
Effects of wild-type and bas TAL-1 overexpression on EC proliferation and migration
Both proliferation and migration of ECs are essential early events of angiogenesis. Therefore, we investigated whether TAL-1 ectopic overexpression affected either or both of these processes.
To assess the effect of TAL-1 on cell proliferation, the same number of HUVECs were infected with Ad-Tet-Off and with one of the following, TRE-LacZ, TRE-wtTAL-1 or TRE-bas and cultured in complete medium. Cell numbers were counted at 72 hours post-infection. As shown in Fig. 4A, no major differences were observed between the different populations, except for a slight increase in cell numbers (15%) associated with wtTAL-1 overexpression. This indicates that neither wt nor
bas TAL-1 overexpression markedly modifies EC proliferation.
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Cell migration was assessed with HUVECs and UCB-ECs transduced with the different adenoviruses using Boyden chamber assays. As presented in Fig. 4B, similar results were obtained with HUVECs and UCB-ECs. Migration was stimulated by the chemoattractant medium in control LacZ-infected cells (about 2-fold over background). In contrast, when ECs were transduced with either TRE-wtTAL-1 or TRE-bas, there was no increase in the number of cells transmigrating towards chemoattractant medium as compared with control medium (background). These experiments demonstrate that ectopic overexpression of either wt or
bas TAL-1 in ECs inhibits their chemotactic activities towards angiogenic factors as measured in this in vitro assay.
Effects of wild-type and bas TAL-1 overexpression on vascularisation in mice
Based on our in vitro studies, we used the mouse model of subcutaneously implanted Matrigel to evaluate the in vivo effects of TAL-1 (SCID mice). Each animal received three implants containing Ad-Tet-Off together with either Ad-TRE-LacZ, used here as the control, Ad-TRE-wtTAL-1 or Ad-TRE-bas. In this assay, host ECs that infiltrate the plug become transduced and express the transgene. On day 5 or 7, animals were sacrificed and implants were photographed and processed for histological analysis. The experiment was repeated three times with five or six animals, such that a total of 16 implants for each Ad-TRE vector was analyzed.
Macroscopic analysis showed no consistent differences between each of the three experiments. Fig. 5A shows representative experiments derived from two animals. In control Ad-LacZ formulated plugs, there was a significant angiogenic response as indicated by the pink/orange hue throughout the plug. In 50% of the Ad-wtTAL-1 formulated plugs (8/16) angiogenesis was markedly enhanced as judged by the much redder color of the implants; in the other 50%, the angiogenic response appeared similar to that of control Ad-LacZ plugs, and this occurred essentially when vascularization of the control implants was already high. In contrast, a large majority of Ad--bas formulated implants (15/16) were almost white, indicating a strong reduction of angiogenesis as compared to control plugs.
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Histological analysis of the plugs after Hematoxylin and Eosin staining were consistent with the macroscopic observations (Fig. 5B). Importantly, EC infiltration of the plugs, as assessed by CD31 immunostaining, were detected in all plugs (see Fig. 5C). However, the densities and the organization of ECs were quite different between the three types of formulated implants. In control LacZ implants, histological analysis showed the presence of numerous endothelial cells well organized into tube-like structures; red blood cells appeared in some of these capillaries indicating their functionality (see Fig. 5B). In wtTAL-1 transduced implants, although EC density seemed similar to that of the control, blood vessel morphology was strikingly different: vascular structures with a lumen were more numerous and there was a significant increase in cross-sectional diameter (Fig. 5B,C); indeed, many ECs were already organized either into capillaries or into large vascular cavities engorged with blood cells. A typical vascular lacuna associated with wtTAL-1-transduced implants is shown in Fig. 5B. In contrast, the implants transduced with Ad-bas had only occasional small-caliber capillary-like structures and no red blood cells were present, consistent with the white color of the implant. The large majority of the infiltrated ECs were organized as chains of cells at the host tissue/Matrigel boundary but no lumen formation was visible (Fig. 5B,C).
Altogether, these experiments indicate that wtTAL-1 transduction in ECs enhances in vivo angiogenesis, whereas that of bas mutant markedly blocks this process.
tal-1 silencing in ECs and its effects on in vitro angiogenesis
We next wanted to investigate whether TAL-1 protein was absolutely required for angiogenesis. Small interfering double-stranded RNAs (siRNAs) have become a powerful tool to knockdown specific gene expression in mammalian cells (Gitlin et al., 2002; Yu et al., 2002
). Transfections of HUVECs were carried out with siRNA targeting tal-1 coding sequences; siRNAs targeting irrelevant sequences, not transcribed in ECs, were used as a control. 24 hours after transfection, whole cell lysates were assayed for TAL-1 expression by immunoblotting. Endogenous TAL-1 expression was repeatedly abolished with the tal-1 siRNA while TAL-1 levels were constant for control siRNA- and mock-treated samples. These experiments, as illustrated in Fig. 6A, demonstrated that endogenous TAL-1 expression was efficiently blocked by transfection of tal-1 siRNA. We then investigated the effects of tal-1 knockdown on in vitro endothelial differentiation on Matrigel. Several experiments were carried out with HUVECs. We noticed a significant lag in the appearance of cords in both tal-1 and control siRNA-transfected ECs (two different control siRNAs were tested) as compared to mock-transfected cells (Fig. 6B), indicating that the entry of siRNAs into primary ECs provokes non-specific adverse biological effects. At 24 hours, we found no obvious differences between the resulting tubule-like networks formed by tal-1 and control siRNA-transfected ECs (not shown). However, an additional delay in the formation of the cord-like structures was repeatedly observed with tal-1 siRNA-transfected ECs as compared to control siRNA-transfected ECs (Fig. 6B). Thus, the knockdown of TAL-1 protein, even if it slightly delays it, does not prevent in vitro endothelial cell morphogenesis.
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Discussion |
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Endothelial cells from different sources are known to be heterogeneous; they differ in their expression of adhesion proteins, and responsiveness to cytokines (Garlanda and Dejana, 1997; Mason et al., 1997
; Salcedo et al., 2000
). Our study now shows that these distinct endothelial cells also differ with regard to TAL-1 expression. While TAL-1 proteins were detected in all types of proliferating ECs tested, their levels ranged from nearly undetectable in ECs derived from bone marrow to high in ECs derived from microvessels. When proliferating ECs were brought to quiescence and deprived of endothelial growth factors, a progressive disappearance of TAL-1 protein occurred and correlated with a rapid down-regulation of tal-1 mRNA levels. As the half-life of the TAL-1 protein is 4 hours (C.D., unpublished), its degradation was not significantly accelerated by starvation conditions. The lack of EC-activating factors was directly responsible for tal-1 down-regulation since quiescent ECs maintained in a medium containing these growth factors still expressed TAL-1. These findings are consistent with the tal-1 expression profile in vivo: TAL-1 protein is not detected in resting vasculature deprived of pro-angiogenic factors but is expressed in newly forming vessels in which ECs are under the influence of angiogenic stimuli (Chetty et al., 1997
; Hwang et al., 1993
; Kallianpur et al., 1994
).
Our studies show that TAL-1 protein expression is modulated during the process of in vitro angiogenesis and significantly, this was observed with ECs derived from three different tissues (large vessels, small vessels and blood circulating endothelial precursors). Proliferative and migratory activities of ECs constitute basal mechanisms of in vivo angiogenesis. Several observations indicate that TAL-1 does not directly modulate endothelial cell proliferation. First, quiescent ECs, when maintained in the presence of endothelial growth factors, expressed TAL-1 at even higher levels than proliferating cells (about 2-fold, data not shown). Second, our data show that ectopic overexpression of wt or bas TAL-1 did not modify endothelial cell growth. Finally, in tal-1-deficient embryos, no reduction in the number of endothelial cells was observed (Visvader et al., 1998
).
A significant reduction in TAL-1 protein level occurs during the first hours of in vitro angiogenesis at the time when the cells are forming chains. This TAL-1 decrease was high in microvascular HMEC-1 cells and in UCB-ECs (80% and 60% reduction, respectively) but rather modest in HUVECs (20% reduction). If we consider the 4-hour half-life of TAL-1 protein, TAL-1 degradation is accelerated in both HMEC-1 and UCB-ECs but not in HUVECs. These observations are consistent with a recent report demonstrating that hypoxia, a well-known angiogenic signal, induces accelerated turnover of TAL-1 in proliferating microvascular ECs but not in ECs from large vessels (HUVECs) (Tang et al., 2002). Hypoxia-induced acceleration of TAL-1 degradation was shown to be mediated by mitogen-associated protein kinase (MAP kinase) through phosphorylation of Ser122 that serves as a signal for ubiquitination and degradation by the proteasome (Tang et al., 2002
). The decrease in TAL-1 during the early steps of angiogenesis is likely to be also mediated through MAP kinase phosphorylation.
Our data show that TAL-1 activity modulates motility properties of endothelial cells. Cell migration is a complex dynamic process, which includes directed motion requiring cell polarization and random walk motion. As we discussed above, down-expression of endogenous TAL-1 happens during in vitro angiogenesis at the time when the cells are moving in all directions to form chains. In addition, our in vitro assays show that TAL-1 overexpression inhibits migration in the direction of chemoattractant signals. The assays used in this study (Boyden assays) do not provide information about the dynamics of cell migration or the mode of motility, adhesion-based or amoeboid (Sahai and Marshall, 2003). Thus, it is possible that the apparent inhibition of chemotactic migration associated with TAL-1 overexpression reflects a change in the mode of cell motility. Time-lapse analysis of cell movement as well as cell behavior in a 3D environment will be required to delineate how TAL-1 regulates endothelial cell motility.
Our findings clearly link TAL-1 activity to endothelial morphogenesis. This is consistent with the high levels of TAL-1 expression in forming vessels (Chetty et al., 1997; Kallianpur et al., 1994
). First, the highest expression of endogenous TAL-1 during in vitro angiogenesis corresponded to the window of capillary-like formation. Second, we found that ectopic wtTAL-1 accelerated the appearance of those cytoplasmic extensions that precede the formation of cords in vitro. In agreement with this, the marked increase in angiogenesis observed in Matrigel implants transduced with wild-type TAL-1 was associated with a general enlargement of capillary lumens, which in some cases led to the formation of large vascular cavities. Finally, the dominant-negative mutant
bas completely impaired all these processes.
tal-1 inactivation by RNA interference did not impede capillary-like network formation in vitro but only delayed the onset of tubule-like differentiation, indicating that TAL-1 is not absolutely required for EC morphogenesis, at least in vitro. This finding was not expected from the phenotype of tal-1/ embryos rescued for tal-1 expression in hematopoietic tissues; these embryos died by day 9.5 p.c. (E9.5) because of severe defects in yolk sac vascular remodeling (Visvader et al., 1998). Nevertheless, these latter observations are not inconsistent with those reported here, since our experiments involved angiogenesis of ECs derived from adult tissues rather than from early embryos. One possibility is that another factor expressed in mature ECs, but not in embryonic endothelial cell lineage at E9.5, may compensate the lack of TAL-1 activity in the process of cell morphogenesis. This possibility is supported by our findings that the dominant-negative
bas strongly inhibits angiogenesis. Indeed, the
bas mutant, although lacking a DNA-binding domain, is still able to mediate protein interactions through its HLH domain. Hence, one of the consequences of
bas overexpression could be not only the competition with TAL-1 for its partners, but also that of other HLH-interacting proteins; the function of some of these proteins might be redundant with TAL-1, at least for mediating endothelial morphogenesis.
To our knowledge, no partners of TAL-1 have been identified in endothelial cells. We show here that the bHLH E47 heterodimerizes with TAL-1 to bind specific E-box sequences in endothelial cells, similar to what has been described in hematopoietic cells (Hsu et al., 1994a; Hsu et al., 1994b
). In immature erythroid cells, TAL-1 is part of a large multifactorial nuclear complex, which includes E47, GATA-1, LMO-2 and its regulator Ldb1 (Wadman et al., 1997
) and transactivates the c-kit gene (Krosl et al., 1998
; Vitelli et al., 2000
). LMO-2 was found to be required for proper vascular network formation during developmental angiogenesis (Yamada et al., 2000
) and has recently been proposed to be a key regulator of tumor angiogenesis (Yamada et al., 2002
). Because LMO-2 and TAL-1 are able to directly interact, it is tempting to speculate that both proteins may be present in the same multiprotein complexes in endothelial cells to mediate specific cellular events during angiogenesis. Like myogenic and neural bHLH proteins (reviewed by Massari and Murre, 2000
), endothelial-specific bHLH factors may control the transcription of a set of genes according to a highly regulated hierarchy. We propose that the activity of multiprotein complexes including TAL-1 and LMO-2 is modulated by the presence or the absence of certain HLH proteins. In this model, distinct events during angiogenesis might be regulated by the expression of one specific HLH protein. Notably, the observation that
bas-overexpression produces the same inhibitory effects on chemotactic cell migration as does that of wtTAL-1 strongly suggests that endothelial migration might be mediated by an unknown HLH-containing or HLH-interacting protein.
Id proteins, which lack a basic domain, have been proposed to modulate the timing of bHLH activity during angiogenesis (Lyden et al., 1999). The absence of Id1/Id3 in mice embryos leads to severe defects in the secondary vascular network, and a partial reduction in Id results in angiogenic defects in adult mice (Lyden et al., 2001
; Lyden et al., 1999
). Significantly, the expression profile of Id1/Id3 parallels that of TAL-1 (Chetty et al., 1997
; Kallianpur et al., 1994
): both are detected at high levels in the vasculature of human tumors, in newly formed vessels but not in resting vasculature. Although Id proteins do not interact directly with TAL-1, they efficiently dimerize with the TAL-1 partner E47, and as a consequence, inhibit the formation of TAL-1/E47 heterodimers. Therefore, TAL-1 may be one of the bHLH factors that Id proteins regulate in endothelial cells.
While our experiments clearly identify TAL-1 as a regulator of endothelial cell morphogenesis, the mechanisms by which it does so remain to be determined. Certain clues, however, can be derived from our observations. Non confluent control ECs (i.e. infected with Ad-TRE-LacZ) plated in complete endothelial-specific medium displayed a classic elongated spindle-shaped morphology. In contrast, most TAL-1 overexpressing ECs displayed a more spread out and flattened morphology (data not shown). We propose that TAL-1 mediates morphological changes in endothelial cells, which allow their differentiation into cords and tubules. Further studies will aim to identify the signaling pathways downstream of TAL-1 that mediate cytoskeleton rearrangements required for proper endothelial morphogenic differentiation.
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