Plasmid transfection

Cells were transfected with pGCMV/EGFP plasmids containing hsa-miR-21 inhibitor or hsa-miR-21 mimic, or empty vector (negative control [NC]), or with pGPU6 plasmids containing Sec23A shRNA (sh-Sec23A), or control shRNA (sh-NC). The group which cells without treatment defined MOCK. All constructs were synthesized by GenePharma (Shanghai, China). SW-480 and DLD-1 cells were grown to 80–90 % confluence and then transfected. Transfection was carried out with Lipofectamine 2000 (Invitrogen, Shanghai, China; DNA/Lipofectamine 2000 ratio=1/2.5) according to the manufacturer’s instructions. Six hours after transfection, the culture medium was replaced with fresh RPMI-1640 containing 10 % FBS. Stable transfectants were established by incubating cells in complete RPMI-1640 medium with Blasticidin (12 mg/mL; Sigma, Shanghai, China) for pGCMV/EGFP plasmids or G418 (500 mg/mL; Sigma) for pGPU6 plasmids for 15 days. Clones were verified by western blot and real-time quantitative polymerase chain reaction (RT-PCR), and the successful clones were pooled for the subsequent investigations.

Cell proliferation assay

For the cell proliferation assays, SW-480 cells stably expressing miR-21 inhibitor, sh-Sec23A, or empty vector or control shRNA were seeded at a density of 2×10³ cells in 96-well plates and incubated for various periods of time (0 to 5 days). DLD-1 cells stably expressing miR-21 mimic, sh-Sec23A, or empty vector or control shRNA were seeded at a density of 1×10³ cells per well in 96-well plates and incubated for the same periods of time. Following incubation, Cell Counter Kit-8 (CCK-8; 10 μL) reagent was added to each well and cells were incubated at 37 °C for 1.5 h. Absorbance was measured at 450 nm using an electroluminescence immunosorbent assay reader as we described previously [23].

Cell migration assay

SW-480 and DLD-1 cells were washed twice with serum-free RPMI-1640 medium and re-suspended in the same medium. Cells were seeded (SW-480, 1×10⁵; DLD-1, 1.5×10⁵) into the upper chambers of transwell culture plates, each with an 8-μm pore membrane insert (Corning, Shanghai, China). RPMI-1640 medium supplemented with 20 % FBS was placed in the lower chambers as a chemoattractant. After incubation for 48 h, cells that had penetrated through to the lower surface of the membrane were fixed with 4 % paraformaldehyde for 20 min, stained with crystal violet for 20 min at ambient temperature, photographed, and counted under a microscope (Nikon, Tokyo, Japan) at×100 magnification in five randomly chosen fields.

Cell invasion assay

The cell invasion assay was similar to the migration assay except that the transwell chambers were coated with matrigel solution (40 μL per chamber; matrigel:serum-free medium ratio 1:10). SW-480, (2×10⁵); or DLD-1, (1.5×10⁵) cells were seeded into the upper chambers of the transwells and RPMI-1640 medium with 20 % FBS (600 μL) was added to the lower chambers. After 48 h incubation, the cells that had penetrated the matrigel and moved to the lower surface of the membrane were fixed with 4 % paraformaldehyde and stained with crystal violet. Cells adhering to the upper surface of the membrane were removed with a cotton swab. The cells attached to the lower surface were counted and photographed under a microscope (Nikon) at×100 magnification in five randomly chosen fields.

Isolation of RNA and quantitative polymerase chain reaction analysis

Forty-eight hours after transfection or after tumor dissection, total RNA was extracted from cultured cells or ground tumor tissue using TRIzol (Invitrogen) according to the manufacturer’s protocols. Total miR-21 or Sec23A RNA (500 ng) was reverse transcribed to cDNA with miRNA-specific RT primers (RiboBio, Guangzhou, China) or random primers (TaKaRa, Dalian, China), respectively. Gene expression was measured by PCR using an Applied Biosystems 7500 Fast Sequence Detection System and SYBR Green PCR Kit (QIAGEN, Shanghai, China) under the following conditions: denaturation at 95 °C for 5 min, followed by 40 cycles of denaturation at 95 °C for 10 s and annealing and extension at 60 °C for 30 s. The relative miRNA and mRNA expression levels were normalized to U6 and β-actin expression, respectively.

Western blot analysis

Seventy-two hours after transfection or tumor dissection, cells were harvested and subjected to lysis in the presence of a protease inhibitor cocktail and then to centrifugation at 14,000g for 15 min at 4 °C. The supernatant fraction was collected and the protein concentration was measured by using a bicinchoninic acid protein assay kit (Beyotime, Hangzhou, China). An aliquot of 40 μg of denatured protein from each sample was treated with sodium dodecyl sulfate and applied to a 10 % polyacrylamide gel for electrophoretic separation, then transferred onto a nitrocellulose membrane. After blocking with 5 % nonfat milk for 2 h at ambient temperature, membranes were incubated with primary antibody (1:1000 dilution; Abcam, Shanghai, China) at 4 °C overnight and horseradish peroxidase-conjugated secondary antibody (1:1000 dilution, Abcam) for 1 h at ambient temperature. The blots were then incubated with enhanced chemiluminescence solution for 1 min. The signals were detected and quantified by densitometry using Quantity One software. GAPDH was used as an endogenous control.

Tumor xenografts in mice

Fifteen male athymic BALB/c nude mice (4-week-old) were obtained from the Shanghai Medical Experimental Animal Care Commission (Shanghai, China). All animal procedures and experimental protocols were approved by Laboratory Animal Ethics Committee of Wenzhou Medical University. Based on in vitro findings, mice were randomized into 3 groups. The experiment was performed only once.

To establish xenograft tumors, DLD-1 cells (8×10⁶ in 200 μL of medium) stably expressing miR-21mimic were injected subcutaneously into the dorsal flank of each mouse. Other mice were injected with cells transfected with empty vector as NC as negative control or cells without treatment as MOCK. Each mouse’s tumor was measured weekly, beginning on day 7 after the injection, by a Vernier caliper along two perpendicular axes. The volume of the tumor was calculated with the formula: volume=(length×width²)/2. Twenty-one days after the injection, the mice were killed and the tumors were dissected for analyses.

Immunohistochemical analysis

Tumor tissues were subjected to immunohistochemical analysis for Sec23A with a kit (Boster, Wuhan, China) used according to manufacturer’s instructions. Briefly, each tissue section was deparaffinized, rehydrated, and rinsed with phosphate-buffered saline solution (PBS). High- pressure antigen retrieval was carried out in citrate buffer, which was then removed by rinsing with PBS. The sections were incubated with 3 % H₂O₂ for 8 min and then with 5 % normal goat serum for 30 min. The sections were then sequentially incubated with specific primary antibody (anti-Sec23A, Abcam), biotinylated goat anti-rabbit IgG, and avidin-biotin-peroxidase complex and rinsed with PBS. The slides were stained with 3,3-diaminobenzidine, counterstained with hematoxylin, and photographed under a light microscope (×200 magnification).

MiR-21 overexpression stimulates proliferation, migration, and invasion of CRC cells

Inhibition of miR-21 expression in SW-480 cells resulted in decreased proliferation, migration, and invasion compared with controls (all panels, p<0.01; Fig. 2a-​-c).c). In contrast, cell proliferation, migration, and invasion were markedly increased in miR-21 over-expressing DLD-1 cells compared with the controls (all panels, p<0.01; Fig. 2d-​-ff).

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Fig. 2

MiR-21 overexpression stimulates proliferation, migration, and invasion of CRC cells. a-c Inhibition of miR-21 in SW-480 by miR-21 inhibitor reduced cell proliferation, migration, and invasion relative to negative control (NC) and mock-treated cells (MOCK). d-f Up-regulation of miR-21 in DLD-1 by miR-21 mimic increased proliferation, migration, and invasion relative to negative control and mock-treated cells. In panels b, c, e, and f, photos on the left are representative images of migrated (b, e) and invaded cells on matrigel membranes (c, f), while the graphs on the right indicate quantification of cells. ** p<0.01

MiR-21 inhibits expression of Sec23A in CRC cell lines

Inhibition of miR-21 expression significantly increased the expression of Sec23A protein in SW-480 cells compared with controls (p<0.01; Fig. 3a). There was no significant difference in expression of Sec23A mRNA between the SW-480 cells transfected with miR-21 inhibitor and controls (Fig. 3b). In contrast, miR-21 over-expression significantly suppressed the expression of Sec23A protein and mRNA in DLD-1 cells compared with controls (p<0.01, p<0.05, respectively; Fig. 3c-​-dd).

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Fig. 3

MiR-21 inhibits expression of Sec23A in CRC cell lines. a Inhibition of miR-21 expression promoted the expression of Sec23A protein in SW-480 cells relative to negative control (NC) and mock-treated cells (MOCK). b There was no significant difference in expression of Sec23A mRNA in SW-480 cells relative to negative control and mock-treated cells. c-d Over-expression of miR-21 by miR-21 mimic decreased the expression of Sec23A protein and mRNA in DLD-1 cells relative to negative control and mock-treated cells. Protein expression in these cells was determined by densitometric analysis. * p<0.05, ** p<0.01

Expression of Sec23A and miR-21 in CRC cells

Sec23A mRNA levels were lower in untreated HT-29 and SW-480 cells than in untreated DLD-1 cells (all p<0.01; Fig. 4a). Sec23A mRNA levels did not differ significantly between HT-29 and SW-480 cells. The expression of Sec23A protein and mRNA levels in SW-480 or DLD-1 cells was significantly suppressed by transfection with sh-Sec23A compared with cells tranfected with sh-NC (all panels, p<0.01; Fig. 4b-​-e).e). On the other hand, transfection with sh-Sec23A significantly increased the expression of miR-21 in SW-480 or DLD-1 cells compared with cells transfected with sh-NC (all p<0.01; Fig. 4f-​-gg).

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Fig. 4

Sec23A knockdown increases expression of miR-21 in CRC cell lines. a Expression of Sec23A mRNA in untreated HT-29, SW-480, and DLD-1 cell lines. b-c Sec23A mRNA and protein expression was suppressed in Sec23A knockdown SW-480 cells. d-e Sec23A mRNA and protein expression was suppressed in Sec23A knockdown DLD-1 cells. Protein expression in these cells was quantified by densitometric analysis. f-g MiR-21 expression was increased in Sec23A knockdown SW-480 and DLD-1 cells. ** p<0.01

Downregulation of Sec23A promotes the proliferation, migration, and invasion of CRC cells

Although downregulation of Sec23A had no significant effect on SW-480 cell proliferation, it did promote the migration and invasion of these cells compared with sh-NC transfectants (all p<0.01; Fig. 5a-​-c).c). DLD-1 cells in which Sec23A expression was inhibited exhibited significantly greater proliferation, migration, and invasion (all p<0.05–0.01) than cells transfected with sh-NC (Fig. 5d-​-ff).

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Fig. 5

Downregulation of Sec23A promotes the proliferation, migration, and invasion of CRC cells. a-c Sec23A knockdown increased migration, and invasion of SW-480 cells relative to negative controls (sh-NC). d-f Sec23A knockdown increased proliferation, migration, and invasion of DLD-1 cells relative to negative controls. In panels b, c, e, and f, photos on the left are representative images of migrated (b, e) and invaded cells on Matrigel membranes (c, f) while the graphs on the right indicate quantification of cells. * p<0.05, ** p<0.01

The authors would like to thank Dr. Haihua Gu and Dr. Wei Li for their technical support and scientific inputs during this study.