Ethics statement

This study was reviewed and approved by the Ethical Committee of Tarbiat Modares University. All samples were collected according to the institutional policies. We used archival FFPE samples that were collected 10–20 years ago, and most patients deceased so no written consent could be obtained. Also, as the Guidelines for Record and Specimen Retention suggest a retention period for paraffin blocks and slides of 10 years [32], the archived FFPE samples from this study could be studied without any ethical concern. However, all patients from this study provided verbal informed consent at the time of admission to the hospital and the verbal consent procedure was reviewed and approved by the Ethical Committee of Tarbiat Modares University.

RNA extraction from esophageal FFPE specimens

First, samples were deparaffinized with xylol and digested with Proteinase K solution (Fermentas, Lithuania). Several factors, including the proteinase K/buffer composition, temperature and digestion time, were altered to optimize the protein digestion procedure. The following protocol was then used: incubation in PK buffer (1 mM EDTA, 1 mM NaCl, 5 mM Tris-HCl, pH 7.4) supplemented with 15 μg/ml of proteinase K for 3 hours at 54°C. RNA was then extracted from deparaffinized tissue with TRIzol reagent (Invitrogen, USA) according to the manufacturer's instructions.

MiR-21 quantification in FFPE samples by quantitative RT-PCR

After treatment with DNase I (Fermentas, Lithuania; manufacturer' s recommendations), 100 ng of total RNA was subjected to qRT-PCR, using a two-step protocol of universal cDNA synthesis and SYBR green master mix kits, along with specific locked nucleic acid (LNA) PCR primer sets (Exiqon, Denmark) on an ABI 7500 real-time PCR machine. To evaluate the possibility of contamination by any RT-PCR inhibitors, an RNA spike-in (UniSp6; Exiqon, Denmark) was added to the samples prior to cDNA synthesis (10⁸ copies per 20 ng RNA) and qRT-PCR was performed with spike-in PCR primer sets (Exiqon, Denmark) as well.

For each sample a no-reverse transcription (no-RT) control was used to detect any potential non-specific amplification of genomic DNA. 5S rRNA and U6 snRNA were used as internal controls for data normalization in FFPE and cell culture samples, respectively.

In situ hybridization on FFPE samples of esophageal SCC

Deparaffinization by xylol and Proteinase K digestion (Fermentas, Lithuania) were performed as described in a previous section of the Experimental Procedures. Slides were then incubated with 5′ digoxigenin (DIG)-labeled miRCURY LNA microRNA detection probes (Exiqon, Denmark), which were diluted to 50 nM in hybridization buffer (50% Formamide, 5X SSC, 0.1% Tween-20, 9.2 mM citric acid, 50 μg/mL heparin, 500 μg/mL yeast RNA) for 1h in a ThermoBrite hybridizer (Fisher Scientific, USA). LNA antisense oligonucleotides were used to increase the oligo-miRNA binding affinity. The probe sequences were the following:

hsa-miR-21 probe: 5′-TCAACATCAGTCTGATAAGCTA-3′hsa/mmu/rno-U6 snRNA probe: 5′-CACGAATTTGCGTGTCATCCTT-3′.

A stringency wash was performed in descending serial dilutions of standard sodium citrate (SSC) buffer. After blocking unspecific binding of the antibody with sheep serum (Sigma, USA), immunological detection with alkaline phosphatase (AP)-conjugated sheep anti-DIG antibody (Roche, Germany) was carried out overnight at 4°C. A light-sensitive color reaction with 4-nitroblue tetrazolium and 5-bromo-4-chloro-3-indolyl phosphate (NBT/BCIP) ready-to-use tablets (Roche, Germany) was performed for 3 hours at 30°C in a humidified chamber.

Cell culture conditions and cell lines

The KYSE-30 esophageal SCC cell line was obtained from the National Cell Bank of Iran, and cultured in RPMI 1640 (Gibco, USA) and Ham' s F12 (Invitrogen, USA) (11) supplemented with 10% fetal bovine serum (FBS) (Sigma, USA). The esophageal adenocarcinoma cell lines OE-33 and FLO-1 originated from the American Type Culture Collection (ATCC) and were kindly provided by Dr. Dipen Maru (Department of Pathology, The University of Texas MD Anderson Cancer Center, Houston, TX, USA). OE-33 and FLO-1 were cultured in RPMI 1640 and DMEM Dulbecco' s Modified Eagle Media (Gibco, USA) supplemented with 10% FBS, respectively. Human normal fibroblasts of gingiva (HGF-1) were obtained from the American Type Culture Collection (ATCC) and cultured in DMEM supplemented with 10% FBS.

The conditioned media from HGF-1 fibroblasts and the esophageal cancer cell lines, containing secreted growth factors, were collected at different time points, centrifuged for 5 min at 1500 rpm, equally mixed with fresh media and used for further experiments.

MiR-21 quantification in cell lines

For microRNA quantification in cell lines, a miR-21 and U6 snRNA specific reverse transcription reaction with MultiScribe Reverse Transcriptase and microRNA specific primers (Applied Biosystems, USA) was performed on 50 ng of total RNA. Quantitative RT-PCR was carried out with a Taqman assay (primers and probes) (Applied Biosystems, USA) and SsoFast Probe Supermix (BioRad, USA) according to manufacturer's protocol.

Co-culture of esophageal cancer cell lines with normal human gingival fibroblasts (HGF-1)

To evaluate the effect of normal fibroblasts on miR-21 expression levels, we separately juxtaposed all 3 esophageal SCC and adenocarcinoma cell lines with HGF-1 fibroblast cells in a Transwell system. In this system, HGF-1 cells were seeded in the wells of a 12-well plate, while esophageal cancer cells were seeded in the 0.4 μm pore-sized inserts (BD Biosciences, USA) that were placed in each well to avoid physical contact between the two cell types. Both fibroblasts and cancer cells were harvested after 1, 2 and 3 days of incubation. The time point day 1 after co-culture was considered as a reference for comparison.

To overcome the effects of the use of different media on cell stress in the co-culture experiments, OE-33 and KYSE-30 cells, normally cultured in RPMI 1640 supplemented with 10% FBS and in RPMI 1640/Ham' s F12 (11) supplemented with 10% FBS, respectively, were adapted to DMEM medium supplemented with 10% FBS. In three consecutive passages, cells were grown in mixtures of RPMI 1640 and DMEM supplemented with 10% FBS in a 31, 11 and 13 ratio, respectively. From the fourth passage onwards, cells were cultured in DMEM supplemented with 10% FBS.

Evaluating fibroblastic markers and CAF markers in HGF-1 cells

PCR primers for the fibroblast markers TGFβ1 (MIM: 190180), FGF1 (MIM: 131220), STAT3 (MIM: 102582), STAG2 (MIM: 300826), TIMP3 (MIM: 188826), COL4A1 (MIM: 120130) and for the CAF markers ACTA2 (MIM: 102620), FAP (MIM: 600403), S100A4 (MIM: 114210) and CSPG4 (MIM: 601172) were designed over exon boundaries in order to amplify the most common splicing variants of each gene without amplifying the genomic DNA. Primer sequences for the fibroblast markers can be found in Table S1, CAF marker primer sequences are available upon request. Each primer pair was validated and all PCR products were confirmed by Sanger sequencing (Figure S1; data not shown).

Gene expression quantification was performed with SuperScript III reverse transcriptase (Invitrogen, USA) for the reverse transcription reaction and iQ™ SYBR Green Supermix (Biorad, USA) for qRT-PCR. β2M was, among 8 common normalizers (PGK1, HPRT1, GUSB, PPIA, RPLPO, TBP, β2M and β Actin) and based on Cq values (Figure S2), selected as the best internal control for these experiments. Primer sequences of the normalizers are available upon request.

All of the fibroblastic markers were predicted by databases (TargetScan and/or DIANA-microT) to be potentially targeted by miR-21, and some of them have already been validated as miR-21 targets.

RNA extraction and miR-21 quantification from conditioned medium

The conditioned media from KYSE-30 and HGF-1 cells was harvested after 1, 2 and 3 days, centrifuged for 5 minutes at 1500 rpm and kept at −20°C for further experiments. RNA was extracted from 300 μl of conditioned medium with the Total RNA Purification Kit (Norgen, Canada). A mixture of 25 fmol of the synthetic C. elegans microRNAs cel-miR-39 and cel-miR-54 (Ambion, USA) were spiked in all samples immediately after adding lysis buffer. 10 ng of each sample was used for qRT-PCR analysis in which the synthetic miRNAs (Applied Biosystems, USA) were used as internal controls. Data were normalized to the expression in the 6 hour old media from each cell line.

Migration assay

To determine the effects of normal fibroblasts on KYSE-30 migration, 7.5×10⁴ fibroblasts were seeded in 24-well plates. The next day, 7.5×10⁴ KYSE-30 cells were seeded in the upper chamber of Transwells with 8 μm pore size, which were uniformly coated with 0.1% gelatin (BD Biosciences, USA) and placed in the wells in which the fibroblasts were growing. KYSE-30 cells that were not co-cultured with fibroblasts were used as controls. After 16 hours of incubation, the membranes were fixed and stained using the Hema3 manual staining system (Fisher Scientific, USA). With a cotton swap, the cells in the upper surface of each membrane were removed and the cells on the bottom surface were counted under the microscope.

Invasion assay

In this assay, the 8 μm pore-sized Transwell membranes (BD Biosciences, USA) were coated evenly with a matrix containing type IV collagen, human laminin and gelatin (Sigma, USA). 6.25×10⁴ cells were seeded in the upper chamber and co-cultured with previously seeded HGF-1 cells. The cells were fixed and stained after 20 hours of incubation with the aforementioned protocol for migration.

MiR-21 is mainly localized in the cancer associated fibroblasts

Using specific LNA-oligo probes against miR-21, we analyzed endogenous miR-21 expression in the FFPE sections prepared from either tumor or non-tumoral esophageal samples. In situ hybridization (ISH) demonstrated a primarily cytoplasmic signal of miR-21 in tumor regions; however, the signal was mainly found in cancer associated fibroblasts (CAFs) of the tumor stroma, with much weaker signals in the tumor cells ( Figure 2A ). The stroma of apparent normal squamous tissue showed no detectable signal ( Figure 2B ), suggesting a preferential upregulation of miR-21 in stromal fibroblasts adjacent to the tumor cells. This was observed in all analyzed samples (N=6, Figure S3). The nuclear localization of U6 snRNA was used as an internal control ( Figure 2C ), and slides without probe treatment were used as negative controls ( Figure 2D ).

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Figure 2

MiR-21 expression is mainly confined to the tumor stroma.

A) In situ hybridization in FFPE samples of esophageal cancer localized miR-21 expression (blue signals) in cancer associated fibroblasts of the tumor stroma, but not in the tumor cells. Slides were counterstained with nuclear fast red. B) The adjacent normal squamous part on the same slide did not show miR-21 expression neither in the stroma nor in the squamous cells; C) Nuclear staining of U6 snRNA was used as an internal control; D) Negative control without probe. Bottom-left inserts show a 2 times bigger magnification of each image; E) Samples with high stromal component showed significantly higher levels of miR-21 expression than samples with a low stromal content. (P value =0.04 with unpaired T-test with Welch' s correction).

MiR-21 expression levels are correlated with the stromal proportion of the tumors

Next, we re-examined miR-21 expression in the esophageal FFPE samples with different stromal ratios. Based on the stromal contents, determined by an expert pathologist for each sample, we categorized the samples into two groups: high stroma (more than 50%) vs. low stroma. The obtained qRT-PCR data demonstrate that miR-21 levels are significantly higher in tumors with high stroma (P=0.04), as compared to those with low levels of stroma ( Figure 2E ).

Induction of miR-21 expression in a co-culture assay of esophageal cancer cells and normal fibroblasts

To examine whether the tumor microenvironment has a role on miR-21 intra-tumor distribution, we used a co-culture system in which the fibroblasts that were cultured in a 12-well plate shared the media with the KYSE-30 cells that were grown on an insert located within the same well ( Figure 3A ). We then compared miR-21 expression in this co-culture system with miR-21 expression in fibroblasts grown without KYSE-30 cells. The fibroblasts showed a significant upregulation of miR-21 when grown in a co-culture system with KYSE-30 (P=0.04; Figure 3B , black bars). Interestingly, we found a similar and significant effect of fibroblasts on the expression levels of miR-21 in KYSE-30 cells (P=0.02; Figure 3B , white bars). This upregulating effect on miR-21 expression was even more obvious for HGF-1 fibroblast cells co-cultured with FLO-1 cells ( Figure 3D ). However, these differences were not statistically significant.

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Figure 3

Effect of co-culturing normal fibroblasts with esophageal cancer cell lines on miR-21 expression levels.

A) A schematic view of the co-culture system; B) MiR-21 expression in KYSE-30 cells and normal fibroblasts (HGF-1) after juxtaposition in a co-culture system; C) MiR-21 expression levels in KYSE-30 and HGF-1 cells after treatment with CM of HGF-1 and KYSE-30 cells, respectively; D) MiR-21 expression levels in FLO-1 adenocarcinoma and HGF-1 fibroblast cells after juxtaposition in a co-culture system; E) MiR-21 expression levels in FLO-1 and HGF-1 cells after treatment with CM of HGF-1 and FLO-1 cells, respectively. Data were normalized to expression after 24 h of co-culture. Each experiment was performed at least 2 times in triplicates.

To understand the nature of this micro-environmental effect, we added conditioned media (CM) obtained from the normal fibroblasts to the esophageal SCC cell line KYSE-30 and to the adenocarcinoma cell line FLO-1. As shown in Figure 3C , the fibroblast conditioned media induces miR-21 expression in the KYSE-30 cells (white bars), with longer conditioning period leading to higher miR-21 expression. Moreover, treatment of HGF-1 cells with CM from FLO-1 induced higher expression levels of miR-21 in the HGF-1 fibroblasts ( Figure 3E , black bars). The basic miR-21 expression levels were not significantly different in all 4 cell lines used in these experiments (Figure S4). Altogether, these results indicate that the effect of neighboring fibroblasts on the cancer cells might be different in different histological subtypes.

Both cancer cells and normal fibroblasts can release miR-21 into the environment

Quantitative RT-PCR on RNA extracted from the conditioned media of fibroblast cultures showed an up to 8.4 fold overexpression of miR-21 after 3 days of incubation, relative to the media which was collected from the same cell passage after 6 hours of culturing (P=0.02). In addition, we observed a 9.3 fold increase in miR-21 expression in the 3 day old conditioned media from KYSE-30 cells, relative to the media collected from the same cell passage after 6 hours, but this increase was not significant (Figure S5).

Normal fibroblasts as well as conditioned media from normal fibroblasts can potentiate migration and invasion of neighboring cancer cells

While juxtaposed with normal fibroblasts, KYSE-30 cells show a significantly higher propensity to migrate and invade through the matrix, which simulates the ECM. KYSE-30 cells not juxtaposed with normal fibroblasts were used as negative controls ( Figure 4A ). Incubation of KYSE-30 cells with the conditioned media of HGF-1 fibroblast cells also results in significantly higher rates of migration (P<0.0001) and invasion (P<0.0001) of KYSE-30 cells through the matrix ( Figure 4B ). To investigate the role of induced miR-21 in the capacity of KYSE-30 cells to migrate and invade through the matrix, we inhibited miR-21 in HGF-1 prior to co-culturing with KYSE-30. We found that miR-21 was significantly downregulated at the end of the experiment (Figure S6A–B) and that KYSE-30 cell migration and invasion was reduced, although this reduction was not significant (Figure S6C–D). In addition, TIMP3 and COL4A1 seem to be increased in HGF-1 cells treated with miR-21 inhibitor and co-cultured with KYSE-30 (Figure S6E–F).

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Figure 4

Cell migration and invasion properties of KYSE-30 cells are increased upon co-culture with HGF-1.

A) KYSE-30 cells juxtaposed with HGF-1 fibroblasts showed a significantly higher potential to migrate (P<0.0001) or invade (P=0.0001) through the coated 8.0 μm pore-sized membrane as compared to the KYSE-30 cells not grown co-culture with normal fibroblasts. Images of representative microscopic pictures are shown on the left; B) 3 day old conditioned media from HGF-1 fibroblasts could significantly induce migration and invasion of KYSE-30 cells (P<0.0001 for both experiments). Images of representative microscopic pictures are shown on the left.

The fibroblastic markers TIMP3 and COL4A1 showed decreased expression levels in the co-culture system

We first selected 6 fibroblastic markers that were predicted by target prediction databases (Targetscan and/or DIANA-MicroT) to be potential targets for miR-21: TGFβ1, transforming growth factor beta1; FGF1, acidic fibroblast growth factor 1; STAT3, signal transducer and activator of transcription 3; STAG2, stromal antigen 2; TIMP3, tissue inhibitor metalloproteinase 3; and COL4A1, Collagen, type IV, alpha 1. We then analyzed the expression of these 6 fibroblastic markers in the normal fibroblast cell line HGF-1, as well as in HGF-1 cells co-cultured with KYSE-30, FLO-1 and OE-33, and found that HGF-1 normal fibroblasts expressed all 6 selected markers. Interestingly, TIMP3 and COL4A1 expression was reduced on the second and third day of incubation compared to the expression levels at the first day of co-culture ( Figure 5 ). In addition, this reduction was negatively correlated with the expression of miR-21 in HGF-1 fibroblast cells co-cultured with any cell lines (KYSE-30, FLO-1 and OE-33) ( Figure 3 ; data not shown). We then analyzed TIMP3 and COL4A1 protein expression in the HGF-1 – KYSE-30 and HGF-1 – FLO-1 co-culture systems and could not detect any TIMP3 protein, while COL4A1 was expressed, but the expression was not altered due to co-culture (Figure S7). The four other fibroblastic markers had similar and stable expression levels during the co-culture experiment, suggesting that their expression levels were not affected by the presence of cancer cells.

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Figure 5

Expression analysis of 6 fibroblastic markers in normal fibroblasts co-cultured with esophageal cancer cell lines KYSE-30 (A), FLO-1 (B) and OE-33 (C).

COL4A1 expression in fibroblasts was significantly decreased after 2 days of incubation with KYSE-30 (P=0.03) and OE-33 (P=0.04) cells and after 3 days of incubation with FLO-1 cells (P=0.01). TIMP3 expression was significantly decreased after 2 and 3 days of incubation with KYSE-30 (P=0.0002 and P>0.0001, respectively), after 2 and 3 days of incubation with FLO-1 cells (P=0.0013 and P=0.0006, respectively) and after 2 and 3 days of incubation with OE-33 cells (P=0.0017 and P=0.0004, respectively) when compared to the measurement 24 h after the start of the co-culture.

We thank Dr. Ehsan Farashahi Yazd (Yazd University of Medical Sciences, Iran) for his technical assistance in tissue culture procedures. We are also thankful to Mrs Azimi from the pathology laboratory of the Shariati hospital and Mrs Karimian from the children medical center of the Imam Khomeini hospital for their technical assistance.