Background
Colorectal cancer (CRC) is highly prevalent globally with new cases reportedly exceeding 100,000 annually [
1]. Although surgical and adjuvant treatment approaches have improved, malignancy-associated long-term survival remains unsatisfactory because of the recurrence and metastasis of the original tumor [
2,
3]. A clinically important objective is the identification of functionally important genes in CRC development and progression, and their utility in prognostic prediction.
Meprin is a member of the astacin family and a zinc metalloendopeptidase that was initially discovered as a protease that was highly expressed at kidney brush border membranes [
4] and intestinal epithelial cells [
5]. Meprin is comprised of two homologous subunit domains that include the meprin-α (MEP1A) domain and the meprin-β (MEP1B) domain that share 42 % identity in their amino acid sequence.
The broad proteolytic activity of meprin in health and disease displays many functions. Thus, meprin is linked to both cancer and inflammatory conditions [
6‐
8]. MEP1A expression is differentially associated with colorectal, breast, osteosarcoma, among other cancer types, and pancreatic cell-lines [
9,
10]. Furthermore, MEP1A is aberrantly secreted to the stroma in the setting of CRC [
6]. Additionally, human prostate cancer cell models, also expressed MEP1A where it promoted cellular replication and invasiveness [
11]. However, in cancer, the precise substrates and pathogenic role of meprins remains unresolved.
In the current report, we aimed to study the expression and clinical significance of MEP1A in CRC. This was achieved by determining MEP1A expression in CRC specimens, and paired comparative analysis to adjacent normal mucosal tissues. Next, by knocking down MEP1A expression with small hairpin RNA (shRNA), we studied functional relevance of MEP1A expression on in vitro and in vivo cellular proliferation and invasion in CRC. Moreover, we studied associations between MEP1A expression, the clinico-pathological features of CRC, and patient survival outcomes by immunohistochemical analysis of a CRC tissue microarray.
Methods
Patients and specimens
Collections of tissue specimens from 36 CRC patients (i.e., 24 male and 12 female; median age, 61.3 years, range 25–86 years) that had undergone tumor resection without chemotherapy or radiotherapy before surgery were conducted between October 2014 and April 2015 at the General Department of Surgery at Shanghai Jiao Tong University Affiliated Shanghai First People’s Hospital (China). Two pathologists confirmed the diagnoses and performed tumor staging according to the guidelines of the American Joint Committee on Cancer (AJCC). All CRC and paired adjacent normal mucosal specimens were collected in the General Surgery Department by protocols that were approved by the Institutional Review Boards of Shanghai Jiao Tong University Affiliated Shanghai First People’s Hospital Medical Center. Written and informed consent was provided by all patients for study participation. The freshly obtained cancer tissues and adjacent normal mucosa located 10 cm from the original tumor site were then immediately cryopreserved in liquid nitrogen and archived at −80 °C prior to RNA and protein extraction.
Cell-lines and reagents
LoVo, Caco2, RKO and HT29 cells are established CRC cell-lines, and were obtained from the Type Culture Collection of the Chinese Academy of Sciences (Shanghai, China). The healthy human colonic mucosal cell-line, NCM460, was obtained from INCELL (San Antonio, TX, USA). All cell-lines were cultured in a fully humidified atmosphere of 5 % CO2 in air at 37 °C. Cell-lines were cultured in DMEM/F12 culture media that was supplemented with 10 % FBS (Gibco, USA), 100 U/mL penicillin and 100 mg/L streptomycin.
Establishing MEP1A-KD cell-lines
Commercially available MEP1A shRNA constructs (Genechem Co. Ltd., Shanghai, China) were used to silence MEP1A. The MEP1A shRNA duplex sequences were as follows:
KD forward: CCGGCCGGGATGATTATGTGAACATCTCGAGATGTTCACATAATCATCCCGGTTTTTG,
KD reverse: AATTCAAAAACCGGGATGATTATGTGAACATCTCGAGATGTTCACATAATCATCCGG.
LoVo and Caco2 cells were transduced with 5 × 105 transducing units/mL of lentiviral particles. Antibiotic selection (1 μg/mL puromycin) was initiated for 7 days at 24 h immediately after transduction. Consequently, LoVo-sh-MEP1A and Caco2-sh-MEP1A were generated. Cells that were transduced with sh-control (LoVo-sh-control and Caco2-sh-control) were used as controls.
Total RNA was prepared from cell cultures, fresh primary tumors and normal mucosa of 36 CRC patients by the TRIzol reagent procedure (TaKaRa, Japan) in accordance with the manufacturer’s instructions. Using total RNA at 2 μg, first strand cDNA was synthesized by using the RevertAid™ First Strand cDNA Synthesis Kit, and following the procedures according to the manufacturer’s instructions (Fermentas, USA). To enable reverse transcription PCR, the following PCR conditions were employed: 30 cycles of 94 °C for 1 min, 55 °C for 1 min, 72 °C for 1 min, and a final extension step at 72 °C for 10 min. Next, 10 μl of the PCR-derived amplicon was resolved by 1 % agarose gel electrophoresis and counter-staining by ethidium bromide (EtBr), with resolved bands quantified by Quantity One software (Bio-Rad, USA).
Quantitative real-time PCR (qRTPCR) assays were performed using 4 μl of cDNA (at a dilution of 1:10) and SYBR green (TaKaRa) in a final volume of 20 μl using the ABI 7900 Real-time PCR System (ABI, USA). The amplification protocol used the following conditions: 95 °C for 2 min, and then 95 °C for 10 s, 60 °C for 30 s, and 72 °C for 30 s, with a final extension at 72 °C for 30 s. Relative quantities of the PCR amplicons were determined by normalizing to GAPDH using the Δ cycle threshold (Ct) values. Each assay reaction was performed in triplicate using the following specific primers:
GAPDH, sense 5’-GGAGCGAGATCCCTCCAAAAT-3’ and anti-sense 5’-GGCTGTTGTCATACTTCTCATGG-3’;
MEP1A, sense 5’- AAAGGCCAAGGAAGTGACCT-3’ and anti-sense 5’-ATGTGGGGCAGAGAGATGAC-3’;
PCNA, sense 5’- CTTCCCGCCGTCCTGTAGC -3’ and anti-sense 5’-CTCCTTCTGCACACATTTGAA-3’;
Ki67, sense 5’-TTCGCAAGCGCATAACCCA-3’ and anti-sense 5’-GCCGGCGCATTTTAGTATTTTG-3’.
Western blot assays
A RIPA lysis buffer (Beyotime Biotechnology, China) was used to isolate total protein from tissue samples or cultured cells and the BCA protein assay kit (Beyotime Biotechnology) determined total protein concentrations. Equal concentrations of isolated protein (i.e., at 30 μg) were resolved through 10 % sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and electro-transferred to a PVDF membrane, which was then blocked for 1 h at room temperature in a 5 % fat-free milk proteins solution that was supplemented with 0.1 % Tween-20. Membranes were reacted with a primary detection antibody (1:500 dilution for MEP1A, R&D Systems, USA and 1:1,000 dilution for GAPDH, Abgent, USA) at 4 °C overnight followed by cross-reaction for 2 h at room temperature with a secondary detection antibody (1:5,000, Abgent) that was directed against goat/rabbit IgG-HRP. To detect cross-reacted proteins, we used an enhanced chemiluminescence (ECL) reagent (Pierce Biotechnology, USA). Quantification by grayscale analysis was performed by employing Quantity One software program analysis (Bio-Rad, USA).
The plate colony-forming assay measures cell proliferation, and follows the recommendations set out in the manufacturer’s instructions. Briefly, 800 log-phase cells were seeded into six-well tissue culture plates then subsequently incubated at 37 °C under a fully humidified atmosphere of 5 % CO2 in air for two weeks. Cells were then fixed for 15 min in methanol and stained with Giemsa solution for 20 min. Colonies were then counted and images recorded by standard photography. Independent assays were performed in triplicate. For Cell Counting Kit-8 (CCK-8), cells were seeded in triplicate into 96-well microtiter plates at a density of 2 × 103 cells/well. At appropriate time-points (i.e., 12, 24, 36, 48 h), cells were incubated with CCK-8 reagent (10 μl) for 2 h at 37 °C. Absorbance values were determined at a wavelength of 450 nm using a Gen5 microplate reader (BioTek, USA).
Scratch assays
Cells were plated in six-well dishes and the scratch assay was conducted. In this assay, LoVo cells were incubated in endothelial cell culture medium that was supplemented with 5 % FBS. When cells had achieved 80 % confluence, a scratch was made across the adherent cultured cells using a sterile plastic micropipette tip that provoked a single homogeneous wound along each well, following which, displaced cells were removed by two PBS washes. Cells were cultured for 36 h and microscopic images were recorded using an ocular grid. Three wounds were samples for each treatment. The relative wound area was calculated as previously described [
12].
Matrigel invasion assays
For this procedure, 24-well Transwell plates with pore diameters of 8 μm (Corning, New York, NY, USA) were pre-coated with a Matrigel matrix (BD Biosciences, San Diego, CA, USA), following which 1 × 105 transfected LoVo cells were suspended in 200 μL of 1 % FBS supplemented RMPI 1640 media, and then seeded to the upper compartment of each inserted well.
Normal growth medium that was supplemented with 10 % FBS, was then added to the lower wells. Cells were allowed to migrate for 48 h at 37 °C, following which, those that had migrated were fixed for 5 min in 10 % methanol and then air dried at room temperature. The invaded cells that were present on the lower surface of the membrane were stained with 2 % crystal violet for 5 min, and then scored by visual inspection and standard light microscopy. To minimize bias, at least five independent fields of view at × 100 magnification were scored following which, the aggregated counts were averaged.
Nude mouse xenograft models
Xenografts of CRC were established in male BALB/C nude mice (aged 4-weeks) that were provided by the Institute of Zoology, Chinese Academy of Sciences of Shanghai. Briefly, Luciferase tagged sh-MEP1A and sh-control LoVo cells were suspended in 100 μL of PBS at a density of 3 × 106 and adoptively transferred to the above described recipient mice. Half of the mice were subcutaneously adoptively transferred and the remainder were adoptively transferred through the lateral tail vein. Following anesthesia, mice were treated at weekly intervals with D-luciferin (150 mg/kg) by i.p. injection, and imaged 10 min later by an IVIS Illumina System (Caliper Life Sciences). Ten weeks after the tail vein injection, mice were euthanized and examined for the presence of both subcutaneous tumors and lung metastases. All animal procedures strictly followed the Shanghai Jiao Tong University Affiliated Shanghai First People’s Hospital Animal Care and Use Guidelines. All humane efforts were made to minimize animal suffering.
Immunohistochemistry on tissue microarrays
Since the 36 paired tissue specimens were collected only one year ago and their follow-up data was lacked, we chose to use a tissue microarray (TMA) with an over 5 years’ follow-up data and a detailed clinico-pathological data to determine whether MEP1A expression correlated with CRC clinico-pathological factors and survival. The TMA containing 88 paired CRC specimens was obtained from the Xin Chao Company (Shanghai, China). Tumors were resected between July 2006 and May 2007, with a final follow-up of August 2012. In surviving patients, the median follow-up time was 46.62 months, and a range of 3–73 months. Samples were obtained from 46 male and 42 female patients with a mean age of 68.72 years; range, 24–90 years. Tumor staging was completed by following the AJCC staging criteria [
13]. Detailed information on the demographics of the recruited patients was collected (Table
1). Dewaxing of sections by xylene treatment was followed by rehydrating specimens in a graded series of ethanol concentrations followed by antigen retrieval with 0.01 M sodium citrate buffer (pH 6.0).
Table 1
Relationship between clinicopathologic parameters and MEP1A or E-cadherin protein expression (n = 88)
Age | | | | | | | |
<65 | 31 | 13 | 18 | | 16 | 15 | |
≥65 | 57 | 24 | 33 | 0.988a
| 39 | 18 | 0.120a
|
Gender | | | | | | | |
Male | 46 | 18 | 28 | | 29 | 17 | |
Female | 42 | 19 | 23 | 0.562a
| 26 | 16 | 0.912a
|
Location | | | | | | | |
Right | 37 | 15 | 22 | | 21 | 16 | |
Others | 51 | 22 | 29 | 0.808a
| 34 | 17 | 0.343a
|
Tumor size (cm) | | | | | | | |
<5 | 47 | 25 | 22 | | 31 | 16 | |
≥5 | 41 | 12 | 29 | 0.023*a
| 24 | 17 | 0.473a
|
AJCC stage | | | | | | | |
I + II | 52 | 27 | 25 | | 26 | 26 | |
III + IV | 36 | 10 | 26 | 0.024*a
| 29 | 7 | 0.004*a
|
T stage | | | | | | | |
T1 + T2 | 9 | 7 | 2 | | 6 | 3 | |
T3 + T4 | 79 | 30 | 49 | 0.032*b
| 49 | 30 | 1.000b
|
N stage | | | | | | | |
N0 | 54 | 30 | 24 | | 29 | 25 | |
N1 + N2 | 34 | 7 | 27 | 0.001*a
| 26 | 8 | 0.032*a
|
M stage | | | | | | | |
M0 | 86 | 37 | 49 | | 53 | 33 | |
M1 | 2 | 0 | 2 | 0.507b
| 2 | 0 | 0.526b
|
Differentiation | | | | | | | |
Well + Moderate | 78 | 35 | 43 | | 51 | 27 | |
Poor | 10 | 2 | 8 | 0.182b
| 4 | 6 | 0.167b
|
Vascular invasion | | | | | | | |
No | 84 | 37 | 47 | | 51 | 33 | |
Yes | 4 | 0 | 4 | 0.135b
| 4 | 0 | 0.292b
|
A MEP1A-specific primary antibody (at a dilution of 1:200; R&D Systems Inc, USA) or an E-cadherin specific primary antibody (1:100; Santa Cruz, USA) was used for immuno-histochemical staining assays. Primary antibody staining was immediately followed by detection with an HRP-conjugated secondary antibody (Dako Cytomation, Glostrup, Denmark). Two specialists blinded to patient outcome provided independent evaluation of the staining. For both MEP1A and E-cadherin, scoring of the staining intensity followed a system of semi-quantitative criteria as described here: 0 (negative), 1 (weak), 2 (moderate), and 3 (strong). The extent of staining was scored as 0 (0 %), 1 (1–25 %), 2 (26–50 %), 3 (51–75 %), and 4 (76–100 %) according to the percent frequency of positively stained cells. Additionally, multiplying the scores of the staining intensity with that of the extent of staining gave “the final staining score.” According to the final scores, two groups were derived; i.e., 1) a low scoring group (0–6), and 2) a group that scored high (7–12).
Statistical analysis
The Student’s two-tailed T-test determined the statistical significance of in vitro and in vivo data. In addition, the two-tailed χ2 test and Fisher’s exact test determined the statistical significance of covariate differences. The Kaplan–Meier method determined patient survival rates, and comparisons of survival curves was done using the log-rank test. For experimental variables, the Cox proportional hazards model was used to determine multivariate Hazard Ratios (HRs). An alpha value of P <0.05 was considered a statistically significant difference. All statistical analyses were determined by the SPSS version 19.0 statistical software package (SPSS Inc., Chicago, IL, USA).
Discussion
The involvement of the metalloprotease MEP1A in multiple cancers was previously shown [
14]. However, studies on MEP1A expression during tumorigenesis and progression of CRC are rare and the molecular mechanisms that implicate involvement of MEP1A in CRC remain unclear.
For the first time, the current study showed that mRNA and protein expression of MEP1A were increased in primary CRC tissues. Immunohistochemistry showed that high MEP1A expression in CRC tissues was significantly aligned to other features of the malignant tumor. These characteristics included tumor size, AJCC stage, tumor depth, and lymph node metastasis, which suggested that expression of MEP1A might serve as a CRC biomarker.
E-cadherin is a transmembrane glycoprotein and the major structural component of adherent junctions of the epithelium that mediate homotypic interactions between adjacent cells that are calcium-dependent. In cancer, decreased E-cadherin expression is functionally important in the progression of well-differentiated adenoma to invasive carcinoma [
15], Moreover, E-cadherin might thus serve as a tumor suppressor [
16].
In this immunohistochemical study, we found that high MEP1A expression correlated negatively with E-cadherin expression, suggesting that MEP1A is involved in tumor migration and invasion. To confirm this hypothesis, scratch and matrigel invasion assays revealed decreased migration and invasion of LoVo cells in the sh-MEP1A group as compared their control group counterparts.
Studying the effects of MEP1A on CRC cell proliferation in CCK-8 assays revealed that MEP1A knock-down in Caco2 and LoVo cells inhibited their proliferation. Moreover, we noted significantly reduced colony formation in MEP1A knock-down cells. These data collectively suggested that suppressed MEP1A expression blocked cell proliferation and further implied specific therapeutic targeting of MEP1A in the setting of CRC.
Based on these in vitro findings, we proceeded to investigate the tumorigenicity of sh-MEP1A and sh-control cells. As anticipated, down-regulation of MEP1A suppressed both subcutaneous and metastatic tumor formation in nude mice. These in vivo data were consistent with observation made in vitro, and confirmed that MEP1A knock-down inhibited CRC growth and invasion.
The potential utility of MEP1A expression as a prognostic marker in CRC has not been previously reported. In this report, Kaplan-Meier survival analysis demonstrated that high MEP1A expression was significantly related to poor prognosis that is commonly seen in CRC patients following surgical resection (P < 0.001). In our study, patients with elevated MEP1A expression were significantly linked to a poorer OS outcome. Furthermore, MEP1A expression was suggested as an independent prognostic factor by Cox regression analysis. These observations suggested that MEP1A might uniquely offer prognostic prediction in the setting of CRC.
It should be noted that there are some limitations of our study. First, there might be a potential selection bias for only patients who had undergone tumor resection without chemotherapy or radiotherapy were included in the mRNA and protein expression study. Second, MEP1A overexpressing cell lines were not investigated in our study in the present day. Third, further studies are required to confirm MEP1A/E-cadherin association and our hypothesis that MEP1A is a potential therapeutic target for CRC.
Abbreviations
AJCC, American Joint Committee on Cancer; CCK-8, Cell Counting Kit-8; CRC, colorectal cancer; Ct, cycle threshold; ECL, enhanced chemiluminescence; EtBr, ethidium bromide; MEP1A, meprin-ɑ; MEP1B, meprin-β; qRTPCR, quantitative real-time PCR; SDS-PAGE, sodium dodecyl sulfate-polyacrylamide gel electrophoresis; TMA, tissue microarray
Acknowledgements
We thank Yang Han and Chenwei Yuan for critical reading of the manuscript and Feifei Cui for helpful suggestions.