Clinical tissue samples were collected from 4 male and 4 female patients (mean age, 35±8 years) who underwent total thyroidectomy (cancerous samples were collected from unilateral glandular lobe, and non-cancerous samples were collected from unilateral glandular lobe on the other side) and who were histopathologically diagnosed with TC between January 2016 and January 2017 at Guangzhou First People's Hospital (Guangzhou, China). The samples were immediately cryopreserved in liquid nitrogen and stored at −80°C until further use. In order to investigate the expression of miR-3690 in association with TC, the miR-3690 expression data of 59 patients were downloaded from The Cancer Genome Atlas (TCGA; http://cancergenome.nih.gov/) database and subsequently analyzed.

The human thyroid follicular cell line Nthy-ori 3–1, and various human TC cell lines, including TPC-1, SW1736, FRO, K1 and 8505C, were purchased from the National Rodent Laboratory Animal Resource. The TC cell lines were authenticated by STR profiling, and were cultured in RPMI-1640 medium (Invitrogen; Thermo Fisher Scientific, Inc.) containing 10% FBS (Thermo Fisher Scientific, Inc.), 100 U/ml penicillin and 0.1 mg/ml streptomycin. Nthy-ori 3-1 cells were cultured in F-12K medium (Genom Biotech Pvt., Ltd.) containing 10% FBS, 100 U/ml penicillin and 0.1 mg/ml streptomycin, and all cells were cultured in a humidified atmosphere at 37°C (5% Co₂).

Synthetic miR-3690 (cat. no. miR10018119-1-5), miR-3690-inhibitor (cat. no. miR20018119-1-5), miR-3690-mutant (mut, 5′-GCUUGGACCCAGCGUAGACAAAG-3′) and relative negative control miRNAs (vector: Cat. no. miR1N0000001-1-5, NC: Cat. no. miR2N0000001-1-5) were synthesized by Guangzhou RiboBio Co., Ltd. Cells transfections with 50 nM miRNAs were performed using Lipofectamine^® 2000 (Thermo Fisher Scientific, Inc.), according to the manufacturer's instructions.

Silencing DKK3 siRNAs (cat. no. HSH007526) were synthesized and purified by GeneCopoeia, Inc., and transfections were performed using Lipofectamine^® 2000 transfection reagent (Thermo Fisher Scientific, Inc.) according to the manufacturer's protocol. All cells were harvested for subsequent experimentation 48 h post-transfection.

Total RNA from the human clinical tissues and cultured cells was extracted using TRIzol^® reagent according to the manufacturer's recommendations (Thermo Fisher Scientific, Inc.). Reverse transcription and detection of mRNA (Cyclin E and c-myc) was performed using BlazeTaq™ SYBR^® Green qPCR mix 2.0 (GeneCopoeia, Inc.). RT-qPCR was performed to detect miR-3690 expression using the All-in-One™ miRNA qRT-PCR Detection kit 2.0 (GeneCopoeia, Inc, Guangzhou). Thermocycling conditions were as follows: At 95°C for 30 sec, followed by 40 cycles of amplification at 95°C for 5 sec, at 59°C for 30 sec and at 72°C for 30 sec. The following PCR primers were synthesized by GeneCopoeia, Inc.: miR-3690 (cat. no. HmiRQP1976), cyclin E (cat. no. HQP021819) and MYC (cat. no. HQP011597). U6 small nuclear RNA (cat. no. HmiRQP9001) and GAPDH (cat. no. HQP006940) were used as endogenous controls, and mRNA quantification was performed using the 2^−ΔΔCq method (17).

In order to determine the cell proliferation rate, an MTT assay (Sigma-Aldrich; Merck KGaA) was used according to the manufacturer's protocol. The reaction was stopped by 200 µl DMSO; the relative optical density was determined at a wavelength of 490 nm, and the results are expressed as the mean ± standard deviation.

For the anchorage-independent growth assays, transfected K1 cells (1×10³ cell per well) were seeded into 2 ml complete medium with 0.3% soft agar (Invitrogen; Thermo Fisher Scientific, Inc.) and overlaid onto 2 ml preset 1.5% agar in the same medium. The cells were cultured at 37°C with 5% CO₂ for 2 weeks, the colonies were then stained with 0.05% crystal violet for 10 min at room temperature, and colonies sized >0.1 mm were counted under a microscope (Motic AE30 inverted fluorescence microscope; Microscope Systems Limited; magnification, ×40).

The potential target genes of miR-3690 were predicted using Target Scan Human (version 7.1; http://www.targetscan.org/vert_71). Luciferase reporter assays. Based on the binding sites of DDK-3 and miR-3690, which were predicted using TargetScan, wild-type DDK-3 sequences were designed and cloned into the pGL3 luciferase reporter vector (Promega Corporation). Cells were then co-transfected with the vectors and miR-3690, miR-3690-in or miR-3690-mut, using Lipofectamine^® 2000 transfection reagent. Following a 48-h incubation, luciferase signals were measured using the Dual luciferase reporter gene assay kit (BioVision, Inc.) according to the manufacturer's protocol. Firefly luciferase activity was normalized to that of Renilla luciferase.

Transcfeted TC cells were lysed in protein RIPA buffer (cat. no. P0013; Beyotime Institute of Biotechnology) according to the manufacturer's protocol. The protein concentration was determined using a bicinchoninic acid protein assay. Proteins (40 µg) were separated via 10% SDS-PAGE and subsequently transferred onto PVDF membranes (EMD Millipore). Membranes were blocked with 5% bovine serum albumin (BSA) for 1 h at room temperature, and incubated with primary antibodies against: DKK3 (1:1,000; cat. no. SAB2701251; Sigma-Aldrich; Merck KGaA), cyclin E (1:1,000; cat. no. 20808; Cell Signaling Technology, Inc.) and c-myc (1:1,000; cat. no. 18583; Cell Signaling Technology, Inc.) overnight at 4°C, as previously described (17). To control sample loading, the membranes were stripped and re-probed with an anti-α-tubulin antibody (1:500; cat. no. SAB5600206; Sigma-Aldrich; Merck KGaA). The membranes were then probed with a peroxidase-conjugated secondary antibody goat-anti-rabbit IgG (1:5,000; ZDR5306 or ZDR5307; Zhongshan Golden Bridge Biotechnology, Inc.), and the protein bands were quantified using Quantity One software version 4.6 (Bio-Rad Laboratories, Inc.).

To assess cell proliferation, cells were cultured for 24 h following transfection. The medium was then supplemented with 10 h BrdU and the cells were incubated for a further 6 h. The labeled cells were thoroughly rinsed with PBS and incubated with an anti-BrdU antibody (1:500; cat no. 61273; Upstate Biotechnology, Inc.) for 1 h at 37°C, according to the manufacturer's protocol. Images were captured using a laser scanning microscope (magnification, ×100; Axioskop 2 plus; Carl Zeiss AG).

Following miRNA-transfection for 48 h, the cells were harvested, washed in ice-cold PBS, and fixed with pre-chilled 75% ethanol at 4°C overnight. The cells were stained using a propidium iodide/RNase staining buffer (BD Biosciences) at room temperature for 30 min in the dark, and the cell cycle distribution was analyzed using a FACSCalibur™ flow cytometer (BD Biosciences) according to the manufacturer's instructions.

Statistical analysis was performed using SPSS 17.0 (SPSS, Inc.). The data were analyzed using a paired Student's t-test for pair-wise comparisons or one-way analysis of variance followed by a post hoc Tukey test for multiple comparisons. P<0.05 was considered to indicate a statistically significant difference.

Based on the expression data downloaded from TCGA, the expression level of miR-3690 was found to be higher in TC tissues compared with that in adjacent non-tumor tissues (Fig. 1A). Consistently, miR-3690 expression was also significantly increased in TC cell lines (TPC-1, SW1736, FRO, K1 and 8505C) compared with that in human thyroid follicular cells (Nthy-ori 3-1; Fig. 1B). Furthermore, RT-qPCR analysis of samples from 8 patients with TC revealed significantly increased levels of miR-3690 in TC tissues (T) compared with tumor-adjacent normal tissues (TAT; Fig. 1C).

To determine the effects of miR-3690 on cellular proliferation, TC cells were transfected with miR-3690 and assessed using RT-qPCR, MTT and anchorage-independent growth assays, in addition to BrdU labeling, immunofluorescence and cell cycle analysis. Following transfection of K1 cells, the expression level of miR-3690 was found to be significantly upregulated (Fig. 2A), and miR-3690 overexpression facilitated cellular proliferation (Fig. 2B-D). Furthermore, miR-3690 overexpression significantly decreased the number of cells in the G₁/G₀ phase, but increased the proportion of S phase cells, compared with the control at 48 h post-transfection (Fig. 2E). In turn, miR-3690 expression was successfully inhibited by miR-3690-in transfection in K1 cells (Fig. 3A), which significantly suppressed proliferation and cell cycle progression compared with the control-transfected cells (Fig. 3B-E). Further to the effects of miR-3690 on TC cell proliferation, the results of the MTT and anchorage-independent growth assays revealed that the SW1736 cell line exhibited a lower miR-3690 expression level compared with the K1 line, and thus was selected for further experimentation. As presented in Fig. S1, the results reflected those obtained from K1 cells.

In order to identify the potential targets of miR-3690, a bioinformatics analysis was conducted using TargetScan, and revealed that DKK3 contains a putative binding site for miR-3690 (Fig. 4A). The effect of miR-3690-mut on TC cells was detected via RT-PCR analysis, the result showed that no effects were observed following transfection with miR-3690-mut compared with that in NC (Fig. 4B). To investigate the potential regulatory effect of miR-3690 on DKK3, protein expression levels were examined by western blot analysis in the present study. miR-3690 overexpression significantly decreased the expression levels of the DKK3 protein in K1 cells, while the levels were found to be upregulated following miR-3690-in transfection (Fig. 4C). Furthermore, luciferase reported assays indicated that miR-3690 significantly decreased the luciferase activity of the wild-type 3′-UTR of DKK3, whereas miR-3690-in transfection resulted in increased activity; no suppressive effects were observed following transfection with miR-3690-mut (Fig. 4D). These findings indicate that DKK3 is a direct target of miR-3690.

As miR-3690 promoted cell proliferation and cell cycle progression, regulatory genes associated with these processes were detected. RT-qPCR and western blot analysis revealed elevated mRNA and protein expression levels, respectively, of cyclin E and c-myc in miR-3690-transfected cells, which was consistent with the increased proportion of S phase and decreased proportion of G₁/G₀ phase cells (Fig. 4E and F). By contrast, decreased expression of cyclin E and c-myc was detected following transfection with miR-3690-in, which was reflected by cell cycle arrest in the G₁/G₀ phase (Fig. 4D and E).

As DKK3 was confirmed to be a direct target of miR-3690, the effects of DKK3 downregulation on miR-3690-in-induced proliferative arrest were investigated. Following treatment with miR-3690-in, DKK3 was knocked down in K1 cells using specific siRNAs; knockdown efficiency was confirmed by western blotting (Fig. 5A). The growth-suppressive effect of miR-3690-in was partially abrogated by DKK3-knockdown, as demonstrated by anchorage-independent growth (Fig. 5B), BrdU labeling and immunofluorescence assays (Fig. 5C). These findings indicate that DKK3 was involved in the miR-3690-in-induced suppression of cellular proliferation.