From the Departments of Cardiovascular Research and
Molecular Oncology, Genentech, Inc.,
South San Francisco, California 94080
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ABSTRACT |
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We examined the role of vascular endothelial growth factor (VEGF) in preventing apoptosis in primary human umbilical vein endothelial (HUVE) cells. VEGF was capable of preventing serum starvation-induced apoptosis at concentrations between 10 and 100 ng/ml. The addition of VEGF to serum-starved HUVE cells led to a 5.2-fold induction of Bcl-2 after 36 h and to a transient, 2.4-fold induction of A1 after a 7-h incubation, as quantitated by real time reverse transcriptase-polymerase chain reaction analysis. Western blot analysis demonstrated a 2-3-fold induction of Bcl-2 protein after 18-36 h of exposure to VEGF and a transient induction of A1 after 7 h of VEGF stimulation. Moreover, overexpression of Bcl-2 by means of transient biolistic transfection experiments of HUVE cells was sufficient to prevent endothelial cells from apoptotic cell death in the absence of VEGF. These findings indicate that Bcl-2 plays an important role in mediating the survival activity of VEGF on endothelial cells.
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INTRODUCTION |
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Bcl-2 belongs to a growing family of apoptosis regulatory gene
products, which may either be death antagonists (Bcl-2, Bcl-XL, Bcl-w,
Bfl-1, Brag-1, Mcl-1, and A1) or death agonists (Bax, Bak, Bcl-Xs, Bad,
Bid, Bik, and Hrk; for review, see Ref. 1). Bcl-2 is an intracellular
protein that localizes to mitochondria, endoplasmic reticulum, and the
nuclear envelope (2, 3) and has been shown to block apoptosis without
inducing cellular proliferation (4, 5). In vitro, many
growth factors and cytokines have been shown to promote survival in
different cell lines tested by activation of the
Ras-Raf-mitogen-activated protein kinase module (for review, see
Refs. 6 and 7). However, the mechanisms by which growth factors control
proliferation and regression of endothelial cells remain poorly
understood. In human umbilical vein endothelial (HUVE)
cells,1 increased levels of
apoptosis and necrosis were observed when cells were incubated with
lipopolysaccharide. Vitamins C and E reduced the levels of apoptosis,
which was paralleled by an increase in Bcl-2 expression and a decrease
in Bax protein levels (8). Upon incubation of HUVE cells with
transforming growth factor-, decreased levels of Bcl-2 correlated
with increased levels of apoptotic cell death (9). 2-Methoxyestradiol
was found to induce apoptosis of cultured bovine pulmonary endothelial
cells (10). A1, a homolog of the Bcl-2 family of antiapoptotic proteins
originally cloned from phorbol ester-stimulated endothelial cells, was
shown to be induced by the inflammatory cytokines tumor necrosis factor and interleukin-1 (11). Infection of microvascular endothelial cells
with retroviral constructs encoding A1 led to inhibition of tumor
necrosis factor-
-induced cell death in the presence of actinomycin D
(11). Similar findings were reported when Bcl-2 was overexpressed by
means of retroviral infection of murine aortic endothelial cells.
Enforced expression of Bcl-2 prevented apoptosis of these cells when
cultured in fibroblast growth factor-depleted medium (12).
The endothelial cell-specific mitogen vascular endothelial growth factor (VEGF) has been shown to be a key positive regulator of normal and pathological angiogenesis (13). A growing body of evidence indicates that VEGF may also act as a survival factor for newly formed blood vessels. In the developing retina, vascular regression in response to hyperoxia has been correlated with inhibition of VEGF release by glial cells (14). Furthermore, administration of anti-VEGF monoclonal antibodies results in regression of established tumor-associated vasculature in xenograft models (15). More recently, using a tetracycline-regulated VEGF expression system in xenografted C6 glioma cells, it has been shown that decreased levels of VEGF production lead to detachment of endothelial cells from the walls of preformed vessels in the tumor (16).
We have found recently that VEGF can counteract endothelial cell apoptosis induced upon serum starvation of HUVE cells in culture (see Fig. 3).2 This survival activity was critically dependent on the phosphatidylinositol 3-kinase/Akt pathway.
In this report, we found increased expression of the antiapoptotic proteins A1 and Bcl-2 but not Bax or Bcl-XL upon challenging primary HUVE cells with VEGF. Thus Bcl-2 and A1 are two novel VEGF target genes.
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EXPERIMENTAL PROCEDURES |
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Cell Culture-- HUVE cells, human microvascular endothelial cells, and CS-C medium were purchased from Cell System (Kirkland, WA). HUVE cells are pooled primary isolates from 300 individual donor umbilical veins. Cells were maintained in CS-C complete medium containing 10% fetal bovine serum and mitogens, according to the recommendations of the supplier. 24 h before initiation of serum starvation, cells were treated with trypsin and plated to a density of 20-25 × 103 cells/cm2 on six-well dishes (reverse transcriptase-polymerase chain reaction (RT-PCR) analysis) or 6-cm dishes (biolistic transfection experiments). Immediately before the experiment, cells were washed twice with phosphate-buffered saline. For serum starvation, CS-C medium without serum and mitogen, complemented with 0.1% bovine serum albumin, was added for the indicated amount of time.
After biolistic transfection, cells were allowed to recover for 24 h in medium containing 10% serum. After washing the cells twice with Tris-buffered saline, minimal medium (without mitogen and serum) complemented with 0.1% bovine serum albumin was added, and the levels of apoptosis were analyzed 24 h after induction of serum starvation.Real Time RT-PCR Analysis-- HUVE cells were initially expanded for 8-10 days in the presence of completed medium. Routinely, cells between passages 4 and 10 were used in the different experimental procedures. 24 h before serum starvation, cells were split and seeded in complete medium at a density of 200,000 cells/well in six-well plates, following the procedures recommended by the manufacturer. Cells were washed for 5 min before adding Cell System basic medium complemented with 0.1% bovine serum albumin. After incubations of various duration, cells were harvested by the STAT 60 method (TEL-TEST "B", Inc., Friendswood, TX), and total RNA was prepared according to the manufacturer's recommendations. The RNA was dissolved in 50 µl of H2O, and the concentration was determined by spectrophotometer (A260/280 nm).
To monitor gene expression we used real time RT-PCR analysis. This novel approach has been described previously (18). Briefly, 100 ng of total RNA was added to a 50-µl RT-PCR (PCR-Access, Promega). The reaction master mix was prepared according to the manufacturer's protocol to give final concentrations of 1 × avian myeloblastosis virus/Tfl reaction buffer, 0.2 mM dNTPs, 1.5 mM MgSO4, 0.1 unit/ml avian myeloblastosis virus reverse transcriptase, 0.1 unit/µl Tfl DNA polymerase, a 250 nM concentration of the primers, and a 200 nM concentration of the corresponding probe. Primers and probes for real time PCR analysis Bcl-2, A1, Bax, and Bad genes were designed by the Primer Express Program according to Heid et al. (19). For sequence information of all oligonucleotides, see Table I. The primers for the human Bcl-2 gene were HUMBCL-2 555.F and HUMBCL-2 639.R, and the probe was HUMBCL-2 598.FP. For A1 analysis, the following primers were used: HUMA1 14.F and HUMA1 131.R; the probe was HUMA1 59.FP. For Bcl-XL analysis we used HSBCLXL 408.F and HSBCLXL 851.R primers, the probe was HSBCLXL 585.FP. For Bax-A analysis, we used HUMBAXA 155.F and HUMBAXA 301.R as primers and HUMBAXA 235.FP as probe. Primers and probes were synthesized at Genentech using conventional nucleic acid synthesis chemistry. The
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Western Blotting-- Cells cultured in 10-cm dishes were washed twice in Tris-buffered saline, and 0.6 ml of RIPA buffer (1 × phosphate-buffered saline, 1% Nonidet P-40, 0.5% sodium deoxycholate, 0.1% SDS, 100 µg/ml phenylmethylsulfonyl fluoride, 30 µl/ml aprotinin, and 1 µM sodium orthovanadate) containing freshly added protease inhibitors was added. Mouse monoclonal antibody directed against human Bcl-2 (Bcl-2(100)) was purchased from Santa Cruz Biotechnology (Santa Cruz, CA). Affinity-purified goat polyclonal antibody against human A1 (A1(N-20)) was from the same manufacturer. The secondary antibody to Bcl-2(100) was goat anti-mouse Ig (biotin-labeled) from Southern Biotechnologies (Birmingham, AL). The secondary antibody to A1(N-20) was biotinylated anti-goat IgG from Vector Laboratories (Burlingame, CA). Total endothelial cell extract, polyacrylamide gel electrophoresis, blotting, and immunodetection were performed according to the Santa Cruz Biotechnology protocol. 60 µg of whole cell extract was loaded on each lane of a 4-16% polyacrylamide gel. The ECL reaction kit was purchased from Amersham Pharmacia Biotech, and horseradish peroxidase streptavidin from Vector Laboratories was used.
Gene Transfer of HUVE Cells by Microprojectile
Bombardment--
Experiments were done using the Bio-Rad 500 optimization kit in the Biolistic PDS-1000/He* Particle Delivery System
(Bio-Rad). In a series of pilot experiments using luciferase reporter
gene DNA, conditions were established which yield the highest levels of
luciferase activity in HUVE cells (data not shown). The settings used
are as follows: particle size, 1.0 µm; rupture disc, 1,100 p.s.i.;
bombardment chamber vacuum, 25 mmHg; and target shelf position 3 (from
the top). Gold particles were prepared according to the manufacturer's
recommendations and stored as 50-µl aliquots for several months at
20 °C. Aliquots were coated with DNA immediately before gene
transfer following the manufacturer's recommendations. Briefly, for
five samples, a 50-µl aliquot of gold particles was Vortex mixed for
3 min, and plasmid DNA (1 mg/ml) was added to a total of 10 µg.
Vortexing was continued for 2 min. Thereafter, 100 µl of a 2.5 M CaCl2 solution was added to the mix. After 2 min of additional vortexing, 20 µl of a freshly prepared 0.1 M spermidine solution was added followed by 2 min of
constant vortexing. The mixture was allowed to settle for 1 min before
tubes were centrifuged for 5 s in a tabletop microcentrifuge. The
supernatant was removed, and the gold pellet was washed first with 140 µl of 70% EtOH followed by 140 µl of 100% EtOH. After removing
the supernatant, the gold particles were taken up in 55 µl of 100% EtOH, and 10 µl was used per biolistic transfection. Immediately after bombardment, 5 ml of complemented medium was added.
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RESULTS |
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VEGF Induces Expression of Bcl-2 and A1 When Added to Serum-starved Endothelial Cells-- To find putative VEGF target genes mediating the VEGF survival activity, we analyzed total RNA of HUVE cells treated with VEGF by quantitative RT-PCR (TaqMan). We designed primer probe sets for quantitative RT-PCR analysis of genes known to be involved in mediating antiapoptotic activities such as Bcl-2, A1, Bcl-XL, or apoptosis-inducing genes such as Bax (for sequence information, see Table I). In the primary human endothelial cell types tested, umbilical vein and lung microvascular endothelial cells, we have observed induction of Bcl-2 as early as 7 h after the addition of VEGF (Fig. 1 and data not shown). The levels of Bcl-2 in HUVE cells increased over time and reached 5.2-fold after 33 h of incubation with VEGF. No significant induction of A1 or Bcl-2 message in response to VEGF stimulation was observed when endothelial cells were grown in the presence of 10% fetal calf serum (data not shown).
Interestingly, the A1 message was transiently increased 2.4-fold after 7 h of VEGF addition and decreased after prolonged incubation time. In a previous report, Northern blots of HUVE cells did not reveal an increase in the A1 message after incubation with a mixture of VEGF and basic fibroblast growth factor for 3 h (20). The failure to observe increased levels for A1 message in response to VEGF may be caused by the decreased sensitivity of the Northern blot analysis, or because the cells were exposed to a mixture of basic fibroblast growth factor (4 ng/ml) and VEGF (10 ng/ml), or because of the different incubation length with VEGF (3 h versus 7 h). When we analyzed total RNA from HUVE cells for Bcl-XL and Bax expression, we could not detect any significant change in their expression levels in response to VEGF under serum starvation conditions (data not shown). To verify if increased expression of A1 and Bcl-2 in response to VEGF stimulation is also reflected in increased protein levels, we performed Western blot experiments with whole cell extracts of HUVE cells cultured under the same conditions as those employed for the RT-PCR analysis. We found a direct correlation between the mRNA and the protein levels (Fig. 2) of Bcl-2 and A1 in human endothelial cells in response to VEGF stimulation. These findings suggest that VEGF exerts its up-regulatory activity on the Bcl-2 and A1 genes primarily at the transcriptional level.
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Bcl-2 Is Sufficient to Mediate Survival of Serum-starved
Endothelial Cells--
We found decreased levels of Bcl-2 and A1
proteins in endothelial cells cultured in the absence of VEGF,
suggesting that these genes may be involved in mediating survival
activity of VEGF on endothelial cells (Fig.
3).2 It has been shown
previously that A1 levels are induced upon incubation of human
endothelial cells to inflammatory mediators such as tumor necrosis
factor- and interleukin-1
, and a possible role for the
A1 gene in inflammation was suggested.
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DISCUSSION |
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VEGF exerts its biological effects by binding to its respective transmembrane receptors Flt-1 and Flk-1/KDR, which are expressed mainly on endothelial cells. Stimulation of endothelial cells with VEGF and subsequent immunoblot analysis demonstrated that VEGF induces phosphorylation of phosphatidylinositol 3-kinase, Ras GTPase-activating protein, p190-rhoGAP, p62, PLC-y, the oncogenic adaptor protein NcK, p125 focal adhesion kinase (p125 FAK), paxilin, and several others (22-30; for review see Ref. 31). The signal transduction pathways involved in mediating the various biologic functions of VEGF on endothelial cells such as migration, proliferation, or survival remain to be characterized. Both VEGF receptors, Flk-1/KDR and Flt-1, were found previously to be expressed on HUVE cells by cell binding and cross-linking studies with VEGF or the Flt-1-specific ligand PlGF (32) or by RT-PCR analysis (18). The HUVE cells used in our experiments were pooled primary isolates from 300 individual donor umbilical veins and thus are likely to represent an average population of endothelial cells. Upon incubation of primary human endothelial cells with VEGF, we found increased expression of two antiapoptotic proteins, Bcl-2 and A1. The increase in Bcl-2 message in response to VEGF can reflect the sum of an increase in the transcriptional level as well as an increase in RNA stability. The overall increase of the Bcl-2 protein observed in these cells may represent higher levels of Bcl-2 mRNA as well as the result of an increase in the protein stability.
Recently, several reports identified altered Bcl-2 levels in endothelial cells engaged in physiologic as well as pathologic angiogenesis. In human corpora lutea, Bcl-2 was found to be expressed in the vascular endothelium of some luteal arterioles and venules (33). During normal luteal phase or after treatment with chorionic gonadotrophin, the corpus luteum undergoes a rapid and massive increase in size and vasculature. This process was completely inhibited by administration of a truncated soluble Flt-1 receptor in a rat model of hormonally induced ovulation (34). These findings indirectly suggested a correlation between the levels of VEGF and Bcl-2 in endothelial cells. However, the numbers of blood vessels exhibiting Bcl-2 staining showed little variation throughout the luteal phase implying that other mechanisms are involved in luteal maintenance (33). An increase in the levels of Bcl-2 expression within the vascular endothelial spindle-shaped cells in Kaposi sarcoma lesions in humans was observed, indicating that up-regulation of Bcl-2 may be important in the pathogenesis of both classical and AIDS-associated Kaposi sarcoma (35). In vitro, overexpression of Bcl-2 in a bovine endothelial cell line blocked the effects of oxidative stress such as lipid peroxidation. In these cells, Bcl-2 also blocked hyperglycemia-induced formation of advanced glycation end products, which are thought to cause tissue damage observed in diabetes-associated hyperglycemia (36).
The identification of two novel VEGF target genes, Bcl-2 and A1, appears timely, given the emerging concepts that VEGF is a survival factor for endothelial cells2 and that VEGF withdrawal may result in regression of the vasculature in several cases (14-16). The role of Bcl-2 in endothelial cells during pathologic and physiologic neoangiogenesis or during vessel regression remains to be analyzed.
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ACKNOWLEDGEMENTS |
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We thank the FACS laboratory at Genentech for excellent support; and M. Vasser, P. Ng, and P. Jhurani for oligonucleotide synthesis. We thank David Wood and Charles Hoffman for excellent graphic artwork.
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FOOTNOTES |
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* The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
§ To whom correspondence should be addressed: Dept. of Cardiovascular Research, Genentech, Inc., 1 DNA Way, South San Francisco, CA 94080. Tel.: 650-225-2968; Fax: 650-225-6327.
1 The abbreviations used are: HUVE cells, human umbilical vein endothelial cells; VEGF, vascular endothelial growth factor; RT-PCR, reverse transcriptase-polymerase chain reaction; GFP, green fluorescent protein.
2 H. P. Gerber, A. McMurtrey, H. Nguyen, Y. Minhong, V. Dixit, and N. Ferrara, submitted for publication.
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REFERENCES |
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