Background
Nasopharyngeal carcinoma (NPC) is a rare disease in most parts of the world but is one of the most prevalent malignasnt tumors and the leading cause of death among all head and neck cancers in Southern China[
1]. Although the major etiological factors, including genetic susceptibility, environmental carcinogens and Epstein-Barr virus infection, are well established, the complicated molecular basis of NPC development and progression remains unclear[
1]. In addition to genetic alterations, epigenetic inactivation of tumor suppressor genes (TSGs) by promoter hypermethylation has been increasingly recognized as a key event for nasopharyngeal carcinogenesis[
1‐
4]. Compared with the incidence of DNA mutation and deletion, that of aberrant DNA methylation of TSGs is high in NPC, which suggests a deep involvement of aberrant DNA methylation in this rare cancer[
1].
Besides having a role as a diagnostic or prognostic bio-marker, hypermethylated DNA can also be used to reveal novel TSGs[
5]. Identifying aberrant methylated genes may provide better understanding of the pathogenesis of NPC, thereby paving the way for the development of novel tumor markers and therapeutic targets. To discover novel TSGs in NPC, we conducted a genome-wide screening for genes downregulated by promoter hypermethylation. Analysis of an expression microarray with RNA from 2 NPC cell lines before and after treatment with a demethylating agent 5-aza-2'-deoxycytidine (5-aza-dC) revealed the transcriptional levels of
TFPI-2 in both cell lines significantly upregulated after demethylation(unpublished data). Thus,
TFPI-2 might be a target gene with expression suppressed by promoter hypermethylation in NPC.
The human
TFPI-2 gene is located on chromosome 7q22 and encodes a 32-kDa Kunitz-type serine protease inhibitor that negatively regulates the enzymatic activity of trypsin, plasmin, and VIIa-tissue factor complex[
6‐
8].
TFPI-2 was found to be abundantly expressed in various normal human tissues, including seminal vesicles, colon, stomach, brain, pancreas, oesophagus and liver[
9‐
13]. Several studies have provided suggestive evidence that
TFPI-2 is inactivated or absent during tumor progression. In addition, expression of
TFPI-2 decreases with an increasing degree of malignancy[
10]. Besides gene locus deletion and aberrant splicing, the mechanism responsible for
TFPI-2 down-regulation in tumor cells has been majorly attributed to promoter hypermethylation[
14‐
16]. The promoter region of
TFPI-2 contains a CpG island spanning exon 1 and the 3 transcription initiation sites[
17]. This region harbors sites for several transcription factors, including SP1, activiting enhancer-binding protein-1 (AP-1), NF-kB and NF-kB-like site, and lymphoid transcription factor-1 (Lyf-1)[
18]. Transcriptional silencing by promoter hypermethylation of
TFPI-2 was observed in some human cancers[
9,
19,
20]. Recent studies also suggest
TFPI-2 may function in the maintenance of the stability of the tumor environment and inhibit the growth of neoplasms, thus act as a candidate TSG with important roles in carcinogenesis and metastasis in human cancers[
9,
12].
In this study, we evaluated the transcriptional levels and methylation status of TFPI-2 in NPC cell lines and analyzed the methylation status of TFPI-2 in a set of NPC primary tumor biopsies. We further addressed the TSG properties of TFPI-2 in NPC by a series of functional experiments. Several lines of evidence support our hypothesis that TFPI-2 is epigenetically inactivated in NPC by promoter hypermethylation and plays a role as a TSG in NPC tumorigenesis.
Methods
NPC cell lines, primary tumor biopsies and normal nasopharyngeal epithelia (NNE)
Six NPC cell lines (CNE1, CNE2, TW03, C666-1, HNE1, and HONE1) were maintained at 37°C in the appropriate medium. The study was approved by the ethics committee of Guangxi Medical University. In total, 70 NPC primary tumor biopsies were collected from Department of Otolaryngology Head and Neck Surgery, First Affiliated Hospital of Guangxi Medical University (Nanning, China), with informed consent from donors, as previously described[
2,
3]. Diagnoses were established by experienced pathologists according to the World Health Organization (WHO) classification. We included 12 normal nasopharyngeal epithelial tissues obtained by tonsillectomy as normal controls. Biopsy samples were stored in liquid nitrogen before DNA or RNA extraction.
Semi-quantitative RT-PCR
Total RNA of NPC cell lines and normal NNE was isolated with TRIzol reagent (Invitrogen, USA). First-strand cDNA was synthesized with M-MLV reverse transcriptase (Promega, USA) according to the manufacturer's instructions. Two micrograms of total RNA was used for each reaction. Primer sequences for
TFPI-2 cDNA were designed according to Norihiro
et al, generating a 209-bp PCR product: TFPI-2-RT-forward: CCAGATGAAGCTACTTGTATG and TFPI-2-RT-reverse: GCACATGCACGTTTGCAATC [
21]. PCR was carried out in a total volume of 20 μl. The PCR mixture contained 250 pmol of each primer, 250 pmol deoxynucleoside triphosphate, 1 × PCR buffer, one unit of ExTaq HS polymerase (Takara, Tokyo), and 2 μl cDNA. Glyceraldehyde-3-phosphate dehydrogenase (
GAPDH) was amplified from the same cDNA sample as the internal control. The primer sequences for
GAPDH cDNA were: GAPDH-RT-forward: AAGCTCACTGGCATGGCCTT, and GAPDH-RT-reverse: CTCTCTTCCTCTTGTGCTCTTG, generating a 375-bp PCR product. PCR conditions were 94°C for 30 s, 58°C for 30 s (
TFPI-2) or 60°C for 30 s (
GAPDH), and 72°C for 30 s, 33 cycles for the
TFPI-2 gene and 24 cycles for the
GAPDH gene. These cycle numbers fell into the exponential range of PCR amplification. The amplified PCR products were then identified on 2% agarose gels. Images of ethidium bromide-stained agarose gels were acquired with a CCD camera (Bio-Rad, USA), and semi-quantitative analysis involved use of the Quantity-one software, v4.4.0 (Bio-Rad, USA).
Sodium bisulphite modification of genomic DNA
High-molecular-weight genomic DNA was extracted from cell lines and biopsies by a conventional phenol/chloroform method. The sodium bisulphite modification procedure was as described [
22] with slight modification. In brief, 600 ng of genomic DNA was denatured in 3 M NaOH for 15 min at 37°C, then mixed with 2 volumes of 2% low-melting-point agarose. Agarose/DNA mixtures were then pipetted into chilled mineral oil to form agarose beads. Aliquots of 200 μl of 5 M bisulphite solution (2.5 M sodium metabisulphite, 100 mM hydroquinone, both Sigma, USA) were added into each tube containing a single bead. The bisulphite reaction was then carried out by incubating the reaction mixture for 4 h at 50°C in the dark. Treatments were stopped by equilibration against 1 ml of TE buffer, followed by desulphonation in 500 μl of 0.2 M NaOH. Finally, the beads were washed with 1 ml of TE buffer and directly used for PCR.
Methylation-specific PCR
The methylation status of the
TFPI-2 promoter region was determined by methylation-specific PCR. Primers distinguishing unmethylated (U) and methylated (M) alleles were designed to amplify the sequence of
TFPI-2 from - 44 to + 60 bp relative to the transcription start point[
21]: TFPI-2-M-forward: TTTCGTATAAAGCGGGTATTC; TFPI-2-M-reverse: ACGACCCGCTAAACAAAACG; TFPI-2-U-forward: GGATGTTTGTTTTGTATAAAGTG; TFPI-2-U-reverse: AAACATCCAAAAAAACACCTAAC. Each PCR reaction contained 20 ng of sodium bisulphite-modified DNA, 250 pmol of each primer, 250 pmol deoxynucleoside triphosphate, 1 × PCR buffer, and one unit of ExTaq HS polymerase (Takara, Tokyo) in a final reaction volume of 20 μl. Cycling conditions were initial denaturation at 95°C for 3 min, 40 cycles of 94°C for 30 s, 54°C (M) or 60°C (U) for 30 s, and 72°C for 30 s. For each set of methylation-specific PCR reactions,
in vitro-methylated genomic DNA treated with sodium bisulphite served as a positive methylation control. A water blank control was also included. PCR products were separated on 2% agarose gels, stained with ethidium bromide and visualized under UV illumination. For cases with borderline results, PCR analyses were repeated.
Bisulphite genomic sequencing
Sodium bisulphite-modified DNA was subjected to PCR with primers designed to amplify nucleotides from - 178 to + 166 bp relative to the transcription start point of the
TFPI-2 gene. Primers sequences were designed according to previous publication by Norihiro
et al. [
21] TFPI-2-BISQ-forward: AGGTAGGTTTAATTTTTTAATTTG and TFPI-2-BISQ-reverse: TACCTATTAACTCCTAAACAAC. PCR was carried out in a total volume of 20 μl, containing 20 ng of sodium bisulphite-modified DNA as template, 250 pmol of each primer, 250 pmol of deoxynucleoside triphosphate, 1× PCR buffer, and one unit of ExTaq HS polymerase (Takara, Tokyo). Cycling conditions were as follows: initial denaturation at 95°C for 3 min, 40 cycles of 94°C for 30 s, 58°C for 30 s, and 72°C for 30 s, and a final extension at 72°C for 5 min. PCR products were then gel-purified and cloned with use of the pMD18-T Vector (Takara, Tokyo) and JM109-competent
E. coli cells. Colonies were grown on agar plates, and 5 colonies of each sample were randomly selected. Plasmids were then isolated and purified. Sequencing were carried out using the BigDye terminator cycle sequencing kit 3.0 (Applied Biosystems, USA) on an ABI 3100 sequencer according to the manufacturer's guidelines.
5-aza-dC treatment
Three NPC cell lines (CNE1, CNE2 and C666-1) were treated with the methyltransferase inhibitor 5-aza-dC. An amount of 2 × 105 cells were seeded on 6-well plates and incubated for 96 h with 10 μM 5-aza-dC. The medium containing the drug was replaced every 24 h. RNA was isolated, and subsequent semi-quantitative RT-PCR was performed as described previously.
Vector construction and transfection
The full-length cDNA sequence of TFPI-2 was from Origene (USA) and subcloned into the pCMV-Tag3A mammalian expression vector (Stratagene, USA). Lipofectamine 2000 (Invitrogen, USA) was used to transfect the TFPI-2-containing plasmids and empty vectors into CNE2 cells, which lack TFPI-2 expression. Stable clones of TFPI-2 (CNE2-TFPI-2) or empty vector (CNE2 empty vector) were obtained by G418 selection (400 μg/ml) for 2 weeks. The expression of exogenous TFPI-2 was confirmed by RT-PCR.
An amount of 105 CNE2 cells was plated in 24-well plates 24 h before transfection. Lipofectamine 2000 was used for transfection according to the manufacturer's protocol. Cells were transfected with 2 μg pCMV-Tag3A-TFPI-2 plasmid or empty vector. Transfected cells were stripped and plated on 60-mm cell culture dishes 48 h after transfection. After selection by 400 μg/ml G418 for 2 weeks, Giemsa-stained colonies were photographed and counted by use of Quantitione software, v4.4.0 (Bio-Rad, USA).
Cell proliferation assay
The growth curves of CNE2 cells stably transfected with TFPI-2 gene (CNE2-TFPI-2) or empty vector (CNE2-empty vector) were monitored by cell counting. An amount of 104 cells of parent CNE2 cells, CNE2-TFPI-2 and CNE2-empty vector were seeded into 6-well plates. Cells were trypsinized and stained with a 0.4% trypan blue solution every 24 h. Dye-exclusive cells were counted by use of a hemocytometer.
Migration study
Cell migration was assessed by in vitro wound-healing assay. Stable transfectants of CNE2, CNE2-TFPI-2 and CNE2-empty vector were cultured on 35-mm dishes for 24-48 h until they reached confluence. A linear wound track was made by use of a sterile tip. Wounds were marked and scored in each dish. Plates were then washed twice with culture medium. Cells migrating into the wound were photographed under a phase-contrast microscope after 24 h incubation after wounding.
Annexin V-FITC/PI double-labeled flow cytometry
To determine apoptosis, the expression of Annexin V-FITC and exclusion of propidium iodide (PI) was detected by double-labeled flow cytometry. Cells transfected with empty vector and TFPI-2 were collected and washed with PBS 24 h after transfection, then resuspended in 100 μL binding buffer. Samples were incubated with 5 μL Annexin V-FITC in the dark for 10 min at 4°C, then the volume was adjusted to 500 μL with binding buffer. PI (5 μL) was added, and samples were incubated for another 10 min at 4°C. Fluorescence was measured with a flow cytometer (BD FACSCalibur, USA).
Statistical analysis
SPSS v11.5 (SPSS Inc., Chicago, IL) was used for statistical analysis. Association between methylated sample data and clinical pathological features of NPC patients were analyzed by Pearson chi-square test or Fisher's exact test. A p < 0.05 was considered statistically significant.
Discussion
Previously, we analyzed expression microarray data before and after treatment with demethylating agent in 2 NPC cell lines and speculated that the
TFPI-2 gene may be downregulated by promoter hypermethylation in NPC cells. TFPI-2, also known as placental protein 5 and matrix-associated serine protease inhibitor [
7,
23], is a novel serine protease inhibitor[
7,
24]. It was reported to be involved in tumorigenesis and metastasis in several types of cancers[
24]. Suppression of
TFPI-2 gene expression is frequently found in melanoma, liver and pancreatic cancer[
9,
25,
26]. Downregulation of
TFPI-2 mRNA and protein by promoter hypermethylation has been confirmed by RT-PCR, immunostaining, methylation specific PCR and bisulfate genomic sequencing [
9,
27]. In this study, hypermethylation of the
TFPI-2 promoter was detected in 4 of 6 (66.7%) NPC cell lines. We also showed a high frequency (88.6%) of
TFPI-2 promoter hypermethylation in NPC primary tumor biopsies but not in the NNE tissues, which implied that transcriptional silencing of the TFPI-2 pathway might be involved in NPC tumorigenesis. As well, we found a high frequency of promoter hypermethylation of
TFPI-2 in early stage (I and II) NPC, which indicates that this might be an early event in NPC carcinogenesis. In contrast to the high frequency of methylation of
TFPI-2 in NPC cell lines and primary tumors, the absence of promoter hypermethylation in 12 histological NNE tissues showed that hypermethylation of
TFPI-2 promoter is not necessary to maintain the normal phenotype in the nasopharyngeal epithelium. Thus, hypermethylation of
TFPI-2 is a frequent and highly tumor-specific event in NPC. Such characteristics may suggest
TFPI-2 methylation as a molecular marker for NPC.
By bisulfite genomic sequencing assay, we found methylation degrees ranging from 60% to 100% in most of the CpG dinucleotides in the TFPI-2-silenced NPC cell lines CNE2 and C666-1. A heavy degree of methylation was also observed in NPC primary tumors, despite the inevitable normal tissue contamination in the biopsy samples without micro-dissection. Moreover, TFPI-2 was completely restored by demethylation treatment in all 3 TFPI-2-silenced NPC cell lines. In this context, epigenetic inactivation of TFPI-2 by promoter hypermethylation is a major, if not the only, mechanism responsible for the loss of TFPI-2 expression in NPC.
Although promoter hypermethylation of
TFPI-2 is frequently found in NPC, it is not associated with sex, age, nodal metastasis or cancer stage in our series. This finding is inconsistent with observations in pancreatic and non-small-cell lung cancer; a high methylation rate of
TFPI-2 was reported in pancreatic cancer patients with liver metastasis[
25]. In non-small-cell lung cancer,
TFPI-2 promoter hypermethylation was frequently found in patients with late-stage cancer (stages III and IV) and with lymph node metastases[
27]. These findings suggest that the prognostic value of promoter hypermethylation of
TFPI-2 is tissue-specific.
The tumor-suppressive functions of
TFPI-2 have been demonstrated in several human malignancies such as lung cancer, prostate cancer, glioma, melanoma and esophageal carcinoma. Ectopic expression of TFPI-2 protein in these cancer cell lines negatively regulates colony formation and inhibits cell proliferation[
12,
27‐
30]. Additional studies have shown that TFPI-2 inhibits tumor-related angiogenesis and some members of the extracellular matrix (ECM) therefore implicates tumor invasion and progression[
8,
12,
17,
29]. Degradation of the ECM is an essential process for tumor invasion and metastasis and involves various matrix-degrading proteinases. The most important proteolytic ECM enzymes are matrix metalloproteinases (MMPs), and upregulated MMP expression has been demonstrated to be strongly associated with the progression of malignancy in several types of cancer, including NPC[
31,
32]. By inhibiting plasmin, TFPI-2 effectively decreases the activation of MMP-1, MMP-3 and MMP-9 and reduces the invasive potential of several cancer cell lines[
9,
12,
33,
34]. In accordance with previous studies, we demonstrated that ectopic expression of
TFPI-2 significantly inhibited cell proliferation, colony formation and migration in NPC cells. We also demonstrated that restoration of
TFPI-2 induces apoptosis in NPC cells. All these evidence strongly implies that
TFPI-2 is a putative TSG and plays a role in nasopharyngeal carcinogenesis.
Methylation-mediated inactivation is reversible, up-regulating
TFPI-2 by demethylating agent may reverse the malignant phenotype of tumor cells. Therefore TFPI-2 can serve as a novel target for gene therapy in NPC treatment. On the other hand, TFPI-2 functions extracellularly as a secreted protein. Treatment with recombinant TFPI-2 protein inhibited tumor growth and metastasis of esophageal cancer[
12]. Thus, TFPI-2 protein might be used directly as an anticancer drug. Further studies will be necessary to explore the great therapeutic potential of
TFPI-2 in NPC and other cancer.
Acknowledgements
This study was supported by grants from the National Natural Foundation of China (30660197, 30960416), Ministry of Education of China and Science & Technology Committee of Guangxi Province, China (0728052). Ministry of Education, Culture, Sports, Science, Japan(2240606).
Competing interests
The authors declare that they have no competing interests.
Authors' contributions
SW and XX carried out the molecular studies. CD was responsible for the sample collection and MSP. XZ, YM, JZ performed the sample collection and MSP experiment. LL and XZ was responsible for statistical data analysis. YN and TH carried out the functional studies. GH, NM and MM participated in the design of the study and manuscript review. ZZ conceived of the study, and participated in its design and draft the manuscript. All authors read and approved the final manuscript.