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Sustained Expression of Early Growth Response Protein-1 Blocks Angiogenesis and Tumor Growth

Departments of ¹ Vascular Biology and Thrombosis Research and ² Dermatology, ³ Clinical Department of Medical and Chemical Laboratory Diagnostics, ⁴ Ludwig Boltzmann Institute for Clinical and Experimental Oncology, Medical University of Vienna, Vienna, Austria and ⁵ Department of Cellular and Integrative Physiology, Indiana Center of Vascular Biology and Medicine, Indianapolis

Requests for reprints: Erhard Hofer, Department of Vascular Biology and Thrombosis Research, Center of Biomolecular Medicine and Pharmacology, Medical University of Vienna, Vienna Competence Center, Lazarettgasse 19, A-1235 Vienna, Austria. Phone: 43-1-40160-33111; Fax: 43-1-40160-933100; E-mail: erhard.hofer{at}meduniwien.ac.at.

	Abstract

Top Abstract Introduction Materials and Methods Results and Discussion References

 
Transient induction of the transcription factor early growth response protein-1 (EGR-1) plays a pivotal role in the transcriptional response of endothelial cells to the angiogenic growth factors vascular endothelial growth factor (VEGF) and basic fibroblast growth factor (bFGF), which are produced by most tumors and are involved in the angiogenic switch. We report here that sustained expression of EGR-1 by recombinant adenoviruses in endothelial cells, however, leads to the specific induction of potent feedback inhibitory mechanisms, including strong up-regulation of transcriptional repressors, negative cell cycle check point effectors, proteins with established antiangiogenic activity, and several proapoptotic genes. Sustained EGR-1 expression consistently leads to an antiangiogenic state characterized by an altered responsiveness to VEGF and bFGF and a striking inhibition of sprouting and tubule formation in vitro. Furthermore, EGR-1–expressing viruses potently inhibit cell invasion and vessel formation in the murine Matrigel model and repress tumor growth in a murine fibrosarcoma model. We propose that gene therapy involving sustained EGR-1 expression may constitute a novel therapeutic principle in the treatment of cancer due to the simultaneous induction of multiple pathways of antiangiogenesis, growth arrest, and apoptosis induction in proliferating cells leading to preferential inhibition of angiogenesis and tumor growth. (Cancer Res 2006; 66(13): 6708-13)

	Introduction

Top Abstract Introduction Materials and Methods Results and Discussion References

 
Angiogenesis, the formation of new capillaries from existing vessels, is essential for tumor growth and metastasis (1, 2). Antiangiogenesis therapies, which interfere with activation of growth factor receptors, such as vascular endothelial growth factor (VEGF) receptor (VEGFR)-2 (Flk-1/KDR) or basic fibroblast growth factor (bFGF) receptor, are functional in animal tumor models and as combination therapies in clinical studies (3). However, due to the multitude of factors produced by tumors and the genetic instability observed during cancer progression, current clinical results are lagging behind expectations. Strategies based on gene therapy interfering with pathways commonly used by different angiogenic inducers could therefore be of advantage.

One factor involved in responses to many different growth factors and environmental stresses, such as hypoxia, is early growth response protein-1 (EGR-1). It is a broadly expressed member of the Cys2-His2 zinc finger family of transcription factors and was first discovered as an immediate early gene induced in growth-quiescent fibroblasts exposed to serum (4). EGR-1 binds to GC-rich, cis-acting promoter elements and controls the expression of a wide variety of pathogenesis-relevant genes, including growth factors, cytokines, receptors, and proteases, many of which are involved in angiogenesis and tumorigenesis (5, 6), the response to ischemia (7) and the progress of several vascular diseases (8). EGR-1 activity is negatively controlled by the corepressor NAB2 (9), and the importance of a transient activation of EGR-1 for VEGF- and bFGF-mediated gene regulation and angiogenesis has been shown using DNAzyme for EGR-1 suppression (5) or NAB2 overexpression by our group (6).

Based on the observation that, during the latter phases of transient growth factor-mediated induction, EGR-1 expression can lead to strong up-regulation of the corepressor NAB2 (Table 1 ; ref. 6) and other molecules with the potential to limit proangiogenic responses in a negative feedback loop, we have now investigated to what extent this phenomenon could be exploited to induce an antiangiogenic state in endothelial cells. We have therefore analyzed the influence of sustained adenoviral overexpression of EGR-1 on gene expression in endothelial cells, angiogenesis, and tumor growth.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results and Discussion References

Recombinant adenoviral constructs and infection. The coding region of the human EGR-1 gene, including the single intron, was amplified from the PAC clone E13873Q3 (library no. 704, Deutsches Ressourcenzentrum für Genomforschung GmbH, Berlin-Charlottenburg, Germany) by PCR and subcloned into the pACCMVplpASR+ vector (6). EGR-1-expressing viruses (Ad.EGR-1) were obtained by homologous recombination as described (6). NAB2- and NAB2.as-expressing viruses (Ad.NAB2 and Ad.NAB2.as), an empty control virus (Ad.con), and a control virus expressing green fluorescent protein (GFP; Ad.GFP) have been reported previously (6). Adenovirus preparations were done, and plaque-forming units (pfu) were determined in 293 cells as described (6). For infection, HUVEC were incubated in PBS for 30 minutes at multiplicities of infection of 100. Thereafter, cells were washed and cultured in normal HUVEC medium. Under these conditions, 100% of the HUVEC were infected as determined by GFP expression.

Real-time reverse transcription-PCR. RNA was extracted from cultured endothelial cells with Trizol (Invitrogen, Carlsbad, CA). Total RNA (2 µg) was reverse transcribed into cDNA (SuperScript II RT, Invitrogen) using oligo(dT) primers, and real-time PCR was used to monitor gene expression using a LightCycler instrument (Hoffman-LaRoche, Basel, Switzerland) according to established procedures (11, 12). A list of the oligonucleotide primers used for gene amplification (Supplementary Table S1) can be obtained from the authors on request.

Western blots. Western blots were done as described by us previously (6). Total cell lysates in Laemmli buffer were separated by SDS-PAGE and transferred to Immobilon-P membranes (Millipore, Bedford, MA). The membranes were incubated with polyclonal anti-EGR-1, anti-VEGFR-1, or anti-Sp1 antibodies (Santa Cruz Biotechnology, Santa Cruz, CA) followed by horseradish peroxidase–labeled secondary antibodies (Amersham Life Sciences, Amersham Place, England). After washing, the membranes were incubated with enhanced chemiluminescence reagent (Amersham, Life Sciences).

Affymetrix microarray analysis. Preparation of cRNA, hybridization to the human U133 GeneChip set (Affymetrix, Santa Clara, CA), and scanning of the arrays were carried out according to the manufacturer's protocols¹ as described in more detail previously (13). Images were analyzed with GeneChip software (MAS 5.0, Affymetrix), and normalization was done by global scaling, with the arrays scaled to an average intensity of 500. Gene expression changes were calculated as the ratio of EGR-1- or control virus-infected cells to noninfected control cells. Genes were scored based on the putative biological functions of the encoded proteins, as determined by database searches using the NetAffx Gene Ontology Mining Tool¹ and a previously published classification scheme ("OntoExpress") for cellular functions (14). A full set of the Affymetrix data is available in the Gene Expression Omnibus (GEO) database (ID GSE2299), and a list of the 67 most highly up-regulated genes can be provided by the authors as Supplementary Table S2 on request.

In vitro tube formation and endothelial sprouting assays. The formation of capillary tube-like structures by HUVEC was analyzed on basement membrane matrix (Matrigel, Becton Dickinson, Franklin Lakes, NJ) as described (6). Cells were starved for 4 hours in M199 medium containing 1% SCS, seeded on Matrigel (3 x 10⁴ cells per well), and further incubated for 16 hours. Images of the network were taken on a phase-contrast microscope (Nikon Diaphot TMD, Kawasaki, Japan) using a cooled charge-coupled device camera (Kappa DX30, Kappa GmbH, Gleichen, Germany). The length of the tube-like structures formed was determined with the AnalySiS software (Softimaging System, Munster, Germany). Endothelial sprouting was assessed by a modification of the method used by Nehls et al. (15) as described previously (6). Briefly, microcarrier beads (Cytodex 3, Sigma Chemical Co., St. Louis, MO) were seeded with HSMEC and embedded into fibrin gels with or without 50 ng/mL VEGF, 50 ng/mL bFGF, or both factors. After formation of the fibrin gels, cultures were incubated with additional M199 medium containing 20% FCS with or without growth factors. After 2 days, the number of tube-like sprouts formed/microcarrier bead was counted. Only sprouts of 150 µm were scored. To visualize cell nuclei, cells were fixed with 3.7% formaldehyde and 2% sucrose in PBS and permeabilized with 0.5% Triton X-100 in PBS. Hoechst 333258 (500 ng/mL) was then added for 30 minutes, and the cytoskeleton stained with rhodamine-phalloidin (Invitrogen) for 1 hour in the dark.

Murine Matrigel assay. Matrigel basement solution (Becton Dickinson) was supplemented with 1.5 x 10⁸ pfu/mL recombinant adenoviruses and 300 ng/mL VEGF and injected s.c. into the flank region of female C57BL/6J mice (16). On day 6 after infection, the mice were sacrificed, and the Matrigel plug was removed and embedded in paraffin. Cryosections of the plug were prepared and stained with H&E (Merck, Darmstadt, Germany). Immunofluorescence was then done using rat anti-CD31 antibody, and nuclei were counterstained with 4',6-diamidino-2-phenylindole (DAPI; Vector Laboratories, Burlingame, CA) as described (16). Pictures were taken on an Olympus AX-70 microscope (Olympus Optical Co., Tokyo, Japan) using an F-View camera. The number of cells in the Matrigel plug was quantified on pictures displaying complete sections of the plug. The circular section images were divided into 10-degree segments, and the number of cells within six segments was counted for each section.

Murine fibrosarcoma model. MethA fibrosarcoma (10) cultures were harvested in exponential growth phase, and 1.5 x 10⁶ cells in 50 µL PBS were injected s.c. into the dorsal skin of C57Bl/6J female mice (10). Following tumor formation (4 days after inoculation), tumors were given 5 x 10⁸ pfu recombinant adenoviruses (Ad.GFP and Ad.EGR-1) diluted in 20 µL PBS, which was repeated after 2 days. Mice were sacrificed 3 days later, and tumor weights were determined. Frozen tumor sections (10 µm) were prepared for immunohistochemical analysis. Sections were then stained with either hematoxylin or immunofluorescence staining using rat anti-mouse VEGFR-2 (17), rat anti-mouse CD31, or rabbit anti-human EGR-1 antibodies (Santa Cruz) followed by incubation with Alexa Fluor 555–labeled anti-rabbit IgG, biotinylated goat anti-rat IgG, and Alexa Fluor 555– or Alexa Fluor 488–labeled streptavidin (Invitrogen). Nuclei were counterstained with DAPI. VEGFR-2, CD31, and EGR-1 staining was analyzed with an Olympus AX70 microscope. For quantification, six random microscopic fields representative of individual tumor sections were recorded with an F-View camera, and the fluorescent signals of VEGFR-2- or CD31-positive cells were quantified using AnalySiS Pro software.

	Results and Discussion

Top Abstract Introduction Materials and Methods Results and Discussion References

 
In endothelial cells transduced with EGR-1-expressing adenoviruses, high EGR-1 mRNA and protein levels accumulated over the first 24 to 48 hours after infection and then remained constant for several days (Fig. 1A and B ).

View larger version (12K): [in this window] [in a new window]   Figure 1. Effects of sustained EGR-1 expression in endothelial cells. HUVEC were infected with EGR-1 adenoviruses or control viruses for 24 hours or as indicated, and mRNA was isolated from uninduced samples or cultures induced with VEGF and bFGF for 1 to 3 hours and analyzed using real-time RT-PCR. EGR-1 and VEGFR-1 protein levels were determined by Western blotting in (B) and (D), respectively. A, EGR-1 mRNA and (B) EGR-1 protein produced from the EGR-1 adenovirus. C, up-regulation of VEGFR-1 mRNA by EGR-1 virus. D, up-regulation of VEGFR-1 protein by EGR-1 and inhibition by Ad.NAB2. ns, unspecific band. E, loss of VEGF/bFGF inducibility of uPA mRNA through EGR-1 expression.

We first confirmed the effects of sustained EGR-1 expression on described EGR-1 target genes, which have potential influence on angiogenesis. These experiments revealed that sustained EGR-1 expression induced VEGFR-1 (Flt-1) expression on the mRNA and protein level (Fig. 1C and D). Coinfections using NAB2 and NAB2.as adenoviruses revealed the specificity of EGR-1–mediated up-regulation (Fig. 1D). Whereas NAB2 inhibited EGR-1–mediated up-regulation (Fig. 1D, lane 6), a truncated nonrepressive variant NAB2.as (9) failed to show a similar effect (Fig. 1D, lane 7). In this context, it is important that several reports have shown that transmembrane and soluble forms of VEGFR-1 can counteract proangiogenic VEGFR-2 activity and function as decoy receptors (18, 19), although recent data also support a synergistic role of VEGFR-1 and VEGFR-2 in tumor angiogenesis (20). We also evaluated the influence of sustained EGR-1 expression on the induction of the proangiogenic urokinase-type plasminogen activator (uPA) gene (21), which is up-regulated by VEGF and bFGF (6). In contrast to VEGFR-1, uPA mRNA was reduced two-fold in EGR-1 virus compared with control virus-infected cells and was not induced by combined VEGF and bFGF stimulation (Fig. 1E).

In the microarray data (Table 1), we detected up-regulated genes with repressive functions on transcription, including not only NAB1 and NAB2, two specific corepressors of EGR-1 (9), but also JunB and JunD. JunB has been proposed to counteract the induction of cell cycle–promoting genes by activator protein 1 complexes by replacing c-Jun in the complex (22), and JunD has been shown to reduce tumor angiogenesis (23). Regulated genes with antiproliferative activity also include two cell cycle check point effectors, p57/KIP2 (24) and GADD45B (25), as well as transforming growth factor-ß (TGF-ß; ref. 26).

Importantly, we also detect several changes, which could interfere with specific processes essential for angiogenesis. The chemokine ligand BRAK/CXCL14, known to block endothelial chemotaxis and angiogenesis, was up-regulated by EGR-1 (27). In addition, both tissue inhibitor of metalloproteinase (TIMP)-1 and TIMP-3, which can inhibit the invasive potential of cells (28), were strongly induced. TIMP-3 also inhibits angiogenesis directly by blocking the binding of VEGF to VEGFR-2 (29). Potential antiangiogenic effects triggered by sustained EGR-1 expression include a reduction of VEGFR-2 (KDR) message (Table 1).

A third group of regulated transcripts likely contributing to the antiangiogenic and antitumoral effects described below comprises several genes linked to the induction of apoptosis, such as SIVA (30), DEDD2 (31), and DUSP2 (32).

These data were in accordance with the hypothesis that sustained EGR-1 expression would shift the balance from activation to repressive feedback mechanisms in endothelial cells. We therefore investigated whether these effects on gene expression are reflected in angiogenesis assays. Indeed, when the ability of EGR-1 virus-infected HUVEC to migrate and form a tubular network on Matrigel was tested, we observed an almost complete inhibition of migration and tubule formation, whereas GFP control virus-infected cells formed normal tubular structures within 12 to 24 hours (Fig. 2A ). When seeded on Matrigel, EGR-1 virus-infected cells undergo rapid apoptosis within 16 hours. This could be facilitated by the lack of survival signals in cells on Matrigel when stabilizing cell-cell contacts cannot be formed under conditions inhibitory for migration and tube formation. In accordance with this assumption, EGR-1 virus-infected cells seemed not affected after 24 hours when seeded on gelatin (Fig. 2A, bottom). However, apoptosis also became apparent in cells seeded on gelatin after 3 to 4 days (Fig. 2C), likely caused by the increased expression of proapoptotic genes as displayed in Table 1. Apoptotic cell death was confirmed by the presence of apoptotic bodies and DNA laddering assays (Fig. 2C).

View larger version (27K): [in this window] [in a new window]   Figure 2. Inhibition of tubule and sprout formation in angiogenesis models in vitro and induction of apoptosis. A, in vitro Matrigel model: HUVEC were infected with EGR-1 and control GFP adenoviruses and seeded in parallel on either Matrigel- or gelatin-coated tissue culture plates 24 hours after infection. Sixteen hours thereafter, cultures were assessed by phase-contrast microscopy (top, Matrigel-coated plates; bottom, gelatin-coated plates). Right, the total length of tubules formed was measured. B, in vitro sprout formation assay in fibrin gels: HUMEC infected for 24 hours were seeded onto Cytodex beads, incubated overnight, and then incorporated into fibrin gels in the presence or absence of VEGF or a mixture of VEGF and bFGF. Left, after 48 hours, the cytoskeleton and nuclei were stained with rhodamine-phalloidin (red) and Hoechst dye 333258 (blue), respectively, and evaluated by phase-contrast microscopy; right, the numbers of sprouts were scored to quantitate percentage inhibition. Three independent experiments with duplicate samples were done for both assays. Columns, mean; bars, SD. C, apoptosis induction in EGR-1 virus-infected cells 72 hours after infection: HUVEC seeded on gelatin-coated plates were infected with the viruses. Left, 48 hours after infection, cells started to show increasing signs of apoptosis, such as formation of apoptotic bodies, which led to a reduction in cell number of >50% at 72 hours. Inset, arrow, the formation of apoptotic bodies was displayed by staining with Hoechst dye. Right, apoptotic cell death was confirmed by DNA laddering assays 72 hours after infection. Survival was partially restored by coinfection with Ad.NAB2.

We next evaluated the effects of EGR-1 overexpression in the murine Matrigel plug model, a widely used model of angiogenesis in vivo (6, 16). When Matrigel plugs containing the control viruses and VEGF were injected s.c. into C57Bl/6J mice, a massive migration and invasion of cells and the formation of vessel-like structures were observed in the plug within 6 days (Fig. 3A and B ). In contrast, when Ad.EGR-1 was mixed into the VEGF-supplemented Matrigel, no increased cell invasion was observed (Fig. 3B). Vessels were found solely in the cell layer formed regularly on the outside of the Matrigel plug. These results show that EGR-1 possesses a strong inhibitory capacity on the angiogenic activity of VEGF in vivo.

View larger version (42K): [in this window] [in a new window]   Figure 3. Inhibition of angiogenesis and tumor growth in vivo. A, murine Matrigel model: Ad.EGR-1 and Ad.GFP (1.5 x 108 pfu/mL) were added to Matrigel solution with or without addition of VEGF (300 ng/mL) and injected s.c. into mice. After 6 days, sections were prepared from the plugs and stained with H&E (HE; top) or with anti-CD31 antibodies and DAPI (bottom). Left to right, the images display first the rim of cells regularly formed around the Matrigel plug followed by a section through the plug. Arrows, the border between the rim and the Matrigel. B, total cells in sections of the Matrigel plug were quantified as described in Materials and Methods. Columns, mean of two experiments in duplicates; bars, SD. C, murine fibrosarcoma model: MethA fibrosarcoma cells were injected s.c. into the back of C57Bl/6J mice. On day 4 and, again, on day 6, fibrosarcomas were inoculated with EGR-1 adenoviruses or control GFP viruses. On day 9, tumors were resected, tumor masses were determined, and sections were prepared for histochemical analysis. Cryosections were either stained with hematoxylin (top), rat anti-mouse VEGFR-2 (middle), or rabbit anti-human EGR-1 antibodies and DAPI (bottom). D, reductions in fibrosarcoma tumor weight (top) and VEGFR-2 staining (bottom). Columns, mean of three experiments with three animals per group; bars, SD. Flourescence intensities of VEGR-2 staining of individual sections of the tumors were measured as described in Materials and Methods.

Based on the reduced VEGFR-2 staining and the very strong inhibition of in vitro and in vivo angiogenesis assays described in Fig. 2A and B and Fig. 3A and B, we assume that the reduction of tumor growth observed is at least in part due to inhibition of angiogenesis. It is possible that a direct inhibition of tumor cell proliferation, as suggested by the results of others (34), contributes to the effect. We have further preliminary evidence that different tumor cells infected with EGR-1 viruses up-regulate several of the genes identified in this study in endothelial cells, which could further contribute to inhibition of angiogenesis (e.g., by increased TIMP production) or be involved in direct inhibition of growth and induction of apoptosis in tumor cells.

The data obtained are in accordance with the possibility that the genes described are up-regulated in a negative feedback loop to limit biological effects triggered by EGR-1 activity. EGR-1 is normally induced only transiently and in a balanced way in response to growth factors because prolonged and excessive activation of some of the genes induced by EGR-1 might otherwise be harmful to normal cells leading to uncontrolled responses. EGR-1 seems to be able to do two opposing functions: a proangiogenic after transient expression and an antiangiogenic, antiproliferative after sustained expression. In line with this suggestion, it has been recently shown that EGR-1 can induce or repress transcription of certain genes depending on the stimulus. These pleiotropic effects of EGR-1 are regulated by post-translational modification of EGR-1 (35). Whereas serum induction of EGR-1 leads to up-regulation of p300/CBP, acetylation of EGR-1, and induction of survival and growth genes, UV irradiation induces phosphorylation of EGR-1, which then triggers growth-inhibitory and proapoptotic responses (35). UV induction of EGR-1 also leads to more sustained production of EGR-1 over several hours when compared with the transient induction by growth factors (35). Similar to UV induction, it is possible that sustained overexpression of EGR-1 by adenoviruses leads to preferential production of EGR-1 forms, which function in inhibitory responses.

Based on the results described, we propose that gene therapy using EGR-1–expressing adenoviruses or nonviral vectors might constitute a new therapeutic principle to inhibit tumor angiogenesis and tumor growth. When delivered by direct injection into tumors, it can exert effects not only by interfering with several growth-promoting and survival pathways in the infected cells but also by inducing the secretion of a series of antiangiogenic molecules affecting neighboring cells. Furthermore, it could possibly be of advantage to apply viruses targeted to the tumor vasculature via the bloodstream, which are currently in development (36). It is conceivable that disseminated metastases could be targeted in this way. We believe that the prominent effects displayed warrant further evaluation to establish the therapeutic potential of sustained EGR-1 expression.

	Acknowledgments

 
Grant support: Austrian Science Fund grant NFN-S94-3 and European Commission grant QLK3-2002-02059 (E. Hofer) and Marie Curie Intra-European Fellowships, MEIF-CT-2003-500034 (M. Lucerna).

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

We thank all the members of the Department for Vascular Biology, Medical University of Vienna (Vienna, Austria) for help and discussions throughout the work, Christa Rabeck for preparations of endothelial cells, and Drs. Trevor Lucas and Renate Hofer-Warbinek for corrections and suggestions on the article.

	Footnotes

 
Note: Supplementary data for this article are available at Cancer Research Online (http://cancerres.aacrjournals.org).

Current address for M. Lucerna: Division of Biopharmaceutics, Leiden/Amsterdam Center for Drug Research, Leiden University, Einsteinweg 55, NL-2333 Leiden, the Netherlands.

Current address for D. Mechtcheriakova and Y. Sobanov: Novartis Research Institute, Brunnerstrasse 59, A-1230 Vienna, Austria.

Current address for A. Kadl: Cardiovascular Research Center, University of Virginia, P.O. Box 801394, Charlottesville, VA 22908.

¹ http://www.affymetrix.com

Received 8/ 2/05. Revised 4/13/06. Accepted 4/24/06.

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