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EPHB4 and Survival of Colorectal Cancer Patients

¹ Molecular Oncology Program and ² Functional Genomics Program, Molecular Oncology and Aging Group, Molecular Biology and Biochemistry Research Center, Vall d'Hebron Hospital Research Institute and ³ Translational Research Laboratory, Institut Catala d'Oncologia, Barcelona, Spain; ⁴ Montefiore Medical Center, Albert Einstein Cancer Center, Bronx, New York; and ⁵ Department of Medical Genetics, Biomedicum Helsinki, University of Helsinki, Helsinki, Finland

Requests for reprints: Diego Arango, Functional Genomics Program, Molecular Oncology and Aging Group, Molecular Biology and Biochemistry Research Center, Vall d'Hebron Hospital Research Institute, Passeig Vall d'Hebron 119-129, Barcelona 08035, Spain. Phone: 34-93-274-6739; Fax: 34-93-489-4040; E-mail: darango{at}ir.vhebron.net.

	Abstract

Top Abstract Introduction Materials and Methods Results and Discussion References

 
The family of receptor tyrosine kinases EPH and their Ephrin ligands regulate cell proliferation, migration, and attachment. An important role in colorectal carcinogenesis is emerging for some of its members. In this study, we evaluate the role of EPHB4 in colorectal cancer and its value as a prognostic marker. EPHB4 levels were assessed by immunohistochemical staining of tissue microarrays of 137 colorectal tumors and aberrant hypermethylation of the EPHB4 promoter was investigated using methylation-specific PCR. We found that EPHB4 expression is frequently reduced or lost in colorectal tumors. Patients with low EPHB4 tumor levels had significantly shorter survival than patients in the high EPHB4 group (median survival, 1.8 and >9 years, respectively; P < 0.01, log-rank test), and this finding was validated using an independent set of 125 tumor samples. In addition, we show that EPHB4 promoter hypermethylation is a common mechanism of EPHB4 inactivation. Moreover, reintroduction of EPHB4 resulted in a significant reduction in the clonogenic potential of EPHB4-deficient cells, whereas abrogation of EPHB4 in cells with high levels of this receptor lead to a significant increase in clonogenicity. In summary, we identified EPHB4 as a useful prognostic marker for colorectal cancer. In addition, we provide mechanistic evidence showing that promoter methylation regulates EPHB4 transcription and functional evidence that EPHB4 can regulate the long-term clonogenic potential of colorectal tumor cells, revealing EPHB4 as a potential new tumor suppressor gene in colorectal cancer. (Cancer Res 2006; 66(18): 8943-8)

	Introduction

Top Abstract Introduction Materials and Methods Results and Discussion References

 
EPHB4, a member of the largest family of receptor tyrosine kinases (RTK), is overexpressed in several tumor types, including prostate, breast, and bladder tumors and down-regulation of EPHB4 in tumor cell lines of these origins results in reduced cell viability, migration, and invasion (1–3). EPH receptors and their Ephrin (EFN) ligands regulate numerous developmental processes, particularly in the vasculature and nervous system (4, 5). The EPH family also has an important physiologic role in the intestinal epithelium. EPHB2 and EPHB3, together with their ligand Ephrin-B1, regulate proliferation and cell positioning within the intestinal crypts (6, 7). Mutations in key genes, such as adenomatous polyposis coli, which result in increased transcriptional activity of TCF/ß-catenin, are the initiating event in most colorectal sporadic tumors. However, although EPHB4 is a direct transcriptional target of the TCF/ß-catenin complex, the expression of EPHB4 is frequently lost in colorectal tumors (8), suggesting that inhibition of EPHB4 signaling may contribute to tumor progression; therefore, EPHB4 levels may be of prognostic significance in colorectal cancer patients. Colorectal cancer is the second most common type of cancer in the western world. Over 50% of the patients with locally advanced colorectal cancer are cured by the standard treatment options, which may include surgery and chemotherapy. However, a significant proportion of these patients will relapse and die of their disease. Currently, it is not possible to accurately differentiate between good and poor prognosis patients following surgical removal of the primary tumor; therefore, there is an acute need for markers capable of distinguishing these two groups.

Here, we show that low levels of expression of EPHB4 can identify a subset of colorectal cancer patients that are at high risk of recurrence. Moreover, we provide evidence that EPHB4 is frequently down-regulated in colorectal tumors through the aberrant hypermethylation of its promoter. In addition, we found that blocking EPHB4 signaling with a dominant-negative form in cells expressing high EPHB4 levels results in increased clonogenicity, whereas reintroduction of EPHB4 into cells expressing low levels of this receptor results in a significant reduction in their long-term clonogenic potential, indicating that EPHB4 has tumor suppressor activity in colorectal cancer cells.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results and Discussion References

 
Cell Lines and Clinical Samples
The cell lines used in this study were obtained and maintained as described previously (9, 10). Primary colorectal tumor samples were collected at collaborating medical institutions in Spain and Finland. Informed consent for genetic analysis of the tumor sample was obtained from each patient according to research proposals approved by the Human Investigations and Ethical Committee in the corresponding institution. Three different series of samples were used in this study. (a) Tissue microarray (TMA)-1: 137 formalin-fixed, paraffin-embedded tumor samples from Finnish patients (11) that were used for immunohistochemical assessment of EPHB4 (mean follow-up, 8.7 years; range, 6.8-11.2 years). (b) TMA-2: 125 formalin-fixed, paraffin-embedded tumor samples from Spanish patients that were independently used for immunohistochemical assessment of EPHB4 (mean follow-up, 5.8 years; range, 5.4-6.3 years). Disease recurrence information was not available for these patients. (c) Fresh frozen colorectal tumors samples from 112 patients from Spain and Finland. The patients in the sample series (a) and (c) partially overlapped (30 patients). The clinicopathologic features of the patients in these three sample sets are shown in Supplementary Table S1 to S3.

Assessment of EPHB4 Protein Levels
Immunohistochemistry. A monoclonal antibody raised against the COOH terminus of the human EPHB4 receptor was used (clone 3D7G8; Zymed Laboratories, San Francisco, CA). The specificity of this antibody has been tested previously in formalin-fixed, paraffin-embedded samples (12). For immunohistochemical analysis, the commercial PowerVision Poly-HRP IHC detection kit was used (ImmunoVision Technologies, Brisbane, CA) as reported previously (11, 13). EPHB4 expression was evaluated blinded from the clinical data. A semiquantitative scale from 0 (no staining) to 4 (highest staining) was used to assess the intensity of the staining. EPHB4-immunostained sections of the TMA-1 and TMA-2 were independently stained and scored in different institutions. Kaplan-Meier plots were used to compare survival differences and statistical significance was assessed with the log-rank test (Prism 4.0, GraphPad Software, San Diego, CA). The optimal EPHB4 intensity threshold to allocate patients to the high or low EPHB4 groups was determined as described in Supplementary Materials. In addition, the Cox regression model was used to assess associations between survival and EPHB4 levels when considered as a continuous variable as well as the simultaneous contribution of the following covariates: EPHB4 tumor levels, histologic grade, sex, age, and tumor location (colon/rectum).

Western blot analysis. One hundred microgram aliquots of protein extracts from the indicated cell lines were fractionated in a 7% SDS-polyacrylamide gel. Proteins were transferred to a nitrocellulose membrane and probed with an anti-EPHB4 antibody as described previously (1:200 dilution; clone 3D7G8; ref. 10). The blot was then stripped and probed with an anti-ß-actin antibody (clone AC74; 1:1,000; Sigma, St. Louis, MO; ref. 10). The signal from the ß-actin probe was used as a loading control.

Methylation-Specific PCR
DNA methylation status of an EPHB4 promoter-associated CpG island (from –793 to –34) was determined in 112 primary colorectal tumors (Supplementary Table S3) and 8 cell lines. DNA was extracted from fresh frozen tumor samples by phenol/chloroform extraction (14). EPHB4 promoter hypermethylation was studied by bisulfite conversion of unmethylated, but not methylated, cytosines to uracil as described previously (15, 16). PCRs using primers specific for either the methylated or the modified unmethylated DNA [methylation-specific PCR (MSP)] were carried out to determine the methylation profile of each sample. Primers were designed using MethPrimer 1.1 software (17). EPHB4 primers sequences for the methylated sequence were 5'-GTTTATTAGAGGGTGGTGGGC-3' (sense) and 5'-TATCCAAAACCGAACATATCGA-3' (antisense) and 5'-TTTATTAGAGGGTGGTGGGTGT-3' (sense) and 5'-CTATCCAAAACCAAACATATCAAA-3' (antisense) for the unmethylated sequence. PCR amplification was done using EcoStar DNA polymerase (Ecogen, Barcelona, Spain) under the following conditions: 95°C for 10 minutes, 35 cycles of 30 seconds at 95°C, 30 seconds at 61°C, and 30 seconds at 72°C, and 4 minutes of final extension at 72°C. In vitro–methylated DNA (CpG Genome Universal Methylated DNA, Chemicon International, Temecula, CA) was used as a positive control for methylated alleles, whereas DNA from normal lymphocytes was used as a negative control.

Quantitative Real-time Reverse Transcription-PCR
SW620 cultures were treated with the DNA methyltransferase inhibitor 5-aza-2'-deoxycytidine (5-Aza-dC; Sigma) for 72 hours (0, 5, or 10 µmol/L). RNA was isolated using Totally RNA (Ambion, Austin, TX) according to the manufacturer's recommendations. RNA aliquots were reverse transcribed and EPHB4 mRNA levels were quantified using real-time reverse transcription-PCR with the Taqman Gene Expression Assay Hs00174752_m1 (Applied Biosystems, Branchburg, NJ). 18S rRNA was used as endogenous control. Relative levels of EPHB4 were quantified using the C_T method as described previously (10).

Clonogenic Assays
Two colon cancer cell lines expressing high levels of EPHB4 (HT29 and LIM2405; see Fig. 3) were transfected (Lipofectamine 2000, Invitrogen, Carlsbad, CA) with a vector expressing the extracellular and transmembrane domains of EPHB4 (amino acids 1-584) and enhanced green fluorescent protein (EGFP) in place of the cytoplasmic domain (pEPHB4-C-EGFP) or with the corresponding control empty vector (pEGFP-N2; Clontech, Mountain View, CA). The resulting chimeric kinase-deficient protein has been shown previously to function as a dominant-negative form of EPHB4 (18, 19). After 24 hours, cells were trypsinized and plated at a 1:15 dilution in 100-mm plates. Two additional cell lines showing low levels of EPHB4 expression (SW837 and KM12; see Fig. 3) were transfected with a vector conferring neomycin resistance and expressing full-length EPHB4 (pcDNA-EPHB4) or the corresponding empty vector (pcDNA3.1, Invitrogen). After 24 hours, cells were trypsinized and plated at a 1:10 dilution in six-well plates. All cells were cultured for 14 days in the presence of 500 µg/mL neomycin (Invitrogen). All macroscopically visible colonies were scored after fixation with 4% paraformaldehyde and crystal violet staining. These experiments were done thrice in triplicate, and equal transfection efficiency of pEPHB4-C-EGFP or pcDNA-EPHB4 compared with the corresponding empty control vectors was confirmed (P > 0.3, ² test) through direct fluorescence-activated cell sorting analysis of the number of EGFP-positive cells or in parallel cotransfection experiments with pEGFP-C3 (Clontech), respectively.

View larger version (12K): [in this window] [in a new window]   Figure 3. EPHB4 expression in colorectal cancer cell lines. Western blotting with a monoclonal EPHB4 antibody revealed substantial variability in EPHB4 expression in colorectal cancer cell lines. ß-Actin was used as a loading control.

	Results and Discussion

Top Abstract Introduction Materials and Methods Results and Discussion References

In this study, we evaluate the potential value of EPHB4 as a prognostic marker in colorectal cancer by immunohistochemically assessing the level of EPHB4 tumor expression. In good agreement with EPHB4 being a direct transcriptional target of Wnt signaling (8), levels of EPHB4 expression were maximal in the lower crypt, where TCF/ß-catenin transcriptional activity is highest, and a gradient of expression was observed with lower EPHB4 levels in the colonic flat mucosa (Fig. 1A, 1 and 2 ). The majority of tumors studied showed a membrane-associated pattern of expression (Fig. 1A, 3). The level of expression of EPHB4 was evaluated in sections of a TMA containing triplicate tumor samples from 137 Dukes C colorectal cancer patients from Finland (TMA-1). EPHB4 expression showed great variability in this tumor series from complete lack of immunoreactivity (Fig. 1A, 4) to very high levels of expression (Fig. 1A, 8). The level of expression of EPHB4 was assessed blinded from the clinical data using a semiquantitative scale from 0 (no staining) to 4 (strong staining). A significant association was observed between low EPHB4 levels and poor prognosis (Fig. 1B). The median disease-free survival (time to disease recurrence in 50% of the patients) in the low EPHB4 group was 1.8 years, whereas patients in the high EPHB4 group had a median survival >9 years (Fig. 1B).

View larger version (58K): [in this window] [in a new window]   Figure 1. EPHB4 as a prognostic marker in colorectal cancer. A, 1 and 2, immunohistochemical staining revealed a gradient of EPHB4 expression in the normal colonic epithelium, with maximal levels in the lower crypt; 3, EPHB4 expression was localized to the cellular membrane in the majority of the colorectal tumors investigated; 4 to 8, there was great variability in EPHB4 expression in the 137 tumors in this study. B, Kaplan-Meier plots of overall and disease-free survival in 137 colorectal cancer patients as a function of EPHB4 tumor levels. Patients with low EPHB4 tumor levels (immunostaining <2.2) had significantly shorter survival than patients with high EPHB4 tumor expression (P < 0.01, log-rank test).

To further validate our results, we used an independent set of 125 colorectal tumors from Spanish patients (TMA-2). Sections of this TMA were independently stained and scored for EPHB4 levels at a different institution blinded from the clinical data. Patients with low EPHB4 tumor levels had significantly shorter survival than patients with high EPHB4 tumor levels (P = 0.02, log-rank test; Supplementary Fig. S1). No associations were found between EPHB4 levels and other clinicopathologic variables (Supplementary Table S2). This independent validation further shows that low EPHB4 tumor levels can identify a subset of colorectal cancer patients with poor prognosis.

The clinical management of patients with locally advanced colorectal cancer is currently limited by the impossibility to accurately predict the probability of recurrence following surgical resection of the primary tumor. Patients with tumors that are indistinguishable at the histopathologic level frequently show great difference in the course of their disease. Approximately 50% of these patients are cured by the standard treatment, whereas the remaining 50% have disease recurrence and die of their disease within 5 years of initial treatment. We show here that low EPHB4 tumor levels can identify a subset of patients that have higher risk of disease recurrence and these patients could therefore benefit from a more aggressive treatment of their disease.

Frequent hypermethylation of the EPHB4 promoter in colorectal tumors. Loss of EPHB4 expression is a common event in colorectal tumors, but the mechanisms of EPHB4 inactivation have not been investigated. Hypermethylation of CpG islands within the promoter sequences of genes with tumor suppressor activity is emerging as an important mechanism capable of silencing these genes, and we have reported recently the presence of aberrant methylation of the promoter of EPHB2, a related EPHB subfamily member, in >50% of the 101 colorectal tumors studied (15). The proximal promoter of EPHB4 contains a CpG island spanning 759 bp starting 34 bp upstream of the transcription start site, which could be methylated and thus regulate the expression of this gene. We used MSP with primers complementary to the methylated or unmethylated bisulfite-treated sequence to investigate the presence of promoter hypermethylation in 112 primary tumors.

We found evidence of EPHB4 promoter hypermethylation in 54 of the 112 tumors tested (48.2%; Fig. 2A ). There was a trend for rectal cases to have higher incidence of promoter hypermethylation compared with tumors in the colon (P = 0.06, ² test), and a higher proportion of tumors from older patients showed EPHB4 promoter methylation (P = 0.014, Mann-Whitney test; Supplementary Table S3). Information about both EPHB4 protein levels and promoter hypermethylation was available from our immunostainings for 30 of these cases. The mean level of EPHB4 in the 14 tumors with promoter hypermethylation was 2-fold lower than in the 16 cases with no evidence of promoter methylation (mean EPHB4 IHC intensity, 0.8 and 1.6, respectively; P = 0.01, t test; Supplementary Table S3), suggesting that methylation of the EPHB4 promoter in the region studied could regulate EPHB4 transcriptional activity. To further investigate this possibility, we identified a colon cancer cell line displaying EPHB4 promoter methylation (SW620) and exposed it to increasing concentrations of the DNA methyltransferase inhibitor 5-Aza-dC for 72 hours. This treatment resulted in demethylation of the EPHB4 promoter and a significant up-regulation of EPHB4 mRNA levels in SW620 cells (5-fold; Fig. 2B). Collectively, these results show that aberrant methylation of the EPHB4 promoter occurs frequently in colorectal tumors and that this mechanisms can regulate EPHB4 expression. Increased TCF/ß-catenin signaling is one of the hallmarks of colorectal cancer, and EPHB4 is a direct transcriptional target of this transcriptional complex (8). The finding that EPHB4 is frequently lost or reduced in colorectal tumors compared with normal colonic epithelium and premalignant lesions suggests that inactivation of EPHB4 is necessary for the oncogenic potential of the elevated TCF/ß-catenin signaling to be fully realized. Here, we provide mechanistic evidence showing that hypermethylation of the regulatory sequences of EPHB4 is a common event that can result in reduced EPHB4 levels in colorectal tumors.

View larger version (19K): [in this window] [in a new window]   Figure 2. EPHB4 promoter hypermethylation in colorectal tumors. A, primers specific for the methylated or unmethylated bisulfite-treated sequence were used to PCR amplify DNA samples from a series of 112 colorectal tumors. Representative results of tumor samples with and without EPHB4 promoter hypermethylation. U, unmethylated; M, methylated; NL, DNA from normal lymphocytes; IVD, in vitro–methylated DNA; arrows, tumors with EPHB4 promoter methylation. B, bottom, treatment of SW620 cells showing EPHB4 promoter hypermethylation with the DNA methyltransferase inhibitor 5-Aza-dC for 72 hours resulted in a substantial reduction in the level of EPHB4 promoter methylation as revealed by PCR amplification with primers specific for the methylated bisulfite-treated sequence (see Materials and Methods); top, measurement of relative EPHB4 mRNA levels by real-time RT-PCR showed that demethylation of the EPHB4 promoter was associated with a significant increase in EPHB4 levels in 5-Aza-dC-treated cells.

We then wanted to investigate the functional effects of reintroducing EPHB4 in colorectal cancer cells that have low levels of this tyrosine receptor kinase on tumor cell survival. For this purpose, we transfected two colon cancer lines expressing low EPHB4 levels (SW837 and KM12) with an EPHB4 expression vector. The number of colonies observed following 14 days of selection with neomycin was scored in three independent experiments in triplicate. Forced expression of EPHB4 in SW837 and KM12 cells resulted in a significant reduction in the number of colonies observed (3-fold reduction; P < 0.0008, t test; Fig. 4A and B ), showing that restoring EPHB4 expression can reduce the clonogenic potential of colorectal cancer cells. In addition, we transfected two cell lines expressing high EPHB4 levels (HT29 and LIM2405) with a vector expressing a chimeric EPHB4-C-EGFP protein, which has been shown to act as a dominant-negative form of EPHB4 (18, 19). Transfection of these two lines with the dominant-negative EPHB4 vector resulted in 2-fold increase in the number of neomycin-resistant colonies compared with cultures transfected with the control empty vector (P < 0.001, t test; Fig. 4C and D).

View larger version (31K): [in this window] [in a new window]   Figure 4. EPHB4 regulates the clonogenic potential of colon cancer cells. A and B, transfection of SW837 and KM12, two colon cancer cell lines with low EPHB4 levels, with an EPHB4 expression vector resulted in a significant reduction in the number of neomycin-resistant colonies after 14 days of selection; C and D, transfection of two colon cancer cell lines with high EPHB4 expression levels (HT29 and LIM2405) and with a vector expressing a dominant-negative form of EPHB4 resulted in a significant increase in the number of neomycin-resistant colonies. Bottom, representative examples of crystal violet–stained colonies; top, results of quantifying the number of neomycin-resistant colonies in one of three independent experiments run in triplicate. Columns, mean; bars, SD; Ps are from Student's t test.

Epigenetic silencing of tumor suppressor genes through aberrant methylation of their promoter sequence is a common event in cancer cells and is of key importance in the initiation and progression of human tumors. Recently, there has been considerable interest in epigenetic therapeutic strategies with DNA methyltransferase inhibitors, such as 5-azacytidine and 5-Aza-dC, aimed at the targeted demethylation of methylated regulatory sequences of tumor suppressor genes in cancer cells (23). These nucleoside analogues are currently undergoing clinical testing and showing encouraging results in hematopoietic malignancies (24). Our finding showing that the promoter of EPHB4 (and EPHB2; ref. 15) is methylated in 50% of colorectal tumors, coupled with the observation that colorectal cancer patients with higher tumor levels of EPHB4 (and EPHB2; ref. 25) have significantly better prognosis than patients with lower EPHB receptor levels and that restoring EPHB4 expression in EPHB4-deficient cells severely compromises the clonogenic potentical of tumor cells, may provide the necessary rationale for testing the efficacy of these nucleoside analogues in colorectal cancer patients.

In conclusion, in this study, we show that EPHB4 expression is frequently reduced or lost in colorectal tumors and that reintroduction of EPHB4 into EPHB4-deficient tumor cells significantly reduces the long-term clonogenic potential of these cells, suggesting that EPHB4 has tumor suppressor activities in colorectal cancer cells. Moreover, we show that EPHB4 promoter hypermethylation is a common mechanism of EPHB4 inactivation. Collectively, these results significantly contribute to establish EPHB4 as a new putative tumor suppressor gene and strengthen the emerging view of an important role of the EPH/EFN family of RTKs in colorectal cancer. In addition, we show that low EPHB4 tumor levels identify a subset of colorectal cancer patients with high risk of recurrence. Therefore, assessment of EPHB4 levels in biopsy or resection tumor samples could be used to identify poor prognosis patients that could benefit from more aggressive treatment options.

	Acknowledgments

 
Grant support: Sigrid Juselius Foundation grant, the Spanish Fondo de Investigaciones Sanitarias grant PI051394, and Fundación de Investigación Médica Mutua Madrileña grant (D. Arango); grants from Academy of Finland (44870/Finnish Center of Excellence Program 2000-2005, 76227, 77547, 213183, and 214268), Sigrid Juselius Foundation, Cancer Society of Finland, and Helsinki University Central Hospital (L.A. Aaltonen); National Cancer Institute grant CA10082-01 (J.M. Mariadason); grant AGL2004-07579-04-04/ALI del Plan Nacional I+D (G. Capella); and Vall d'Hebron Research Institute Predoctoral Fellowship (V. Davalos).

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 Drs. Jens Glienke (Research Laboratories of Schering AG, Berlin, Germany) and Elena B. Pasquale (Burnham Institute, La Jolla, CA) for kindly providing the vector pcDNA-EPHB4 and pEPHB4-C-EGFP, respectively, and Laura García Latorre for her technical assistance.

	Footnotes

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

Received 12/27/05. Revised 7/11/06. Accepted 7/28/06.

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