Cell Lines

The human radial growth melanoma cell line WM1552c and the human vertical growth melanoma cell line WM793b were provided by Dr. M. Herlyn (Wistar Institute, Philadelphia, PA) and cultured as previously described [22]. The human metastatic melanoma cell line MEL 39 was a gift from Soldano Ferrone (Harvard Medical School, Boston, MA) and cultured as previously described [23]. The A375 human metastatic melanoma cell line was obtained from American Type Cell Culture Collection (ATCC, Manassas, VA).

Oligonucleotide Transfections

Cells were plated on 60 mm² plates at a density of 1 × 10⁶ cells per plate. When the cells were 70–80% confluent, they were transfected with pre-miR-21 or control pre-miR (Ambion, Austin, TX) using TransIT TKO transfection reagent (Mirus Bio, Madison, WI). Twenty-four hours post-transfection, cells were collected for use in all assays. Tissue inhibitor of metalloproteinase 3 (TIMP3)-specific small-interfering RNA (siRNA) and negative control constructs were purchased from Santa Cruz Biotechnology, Inc (Santa Cruz, CA). The sequences for each oligo are as follows:

• Ambion Control miR: AGUACUGCUUACGAUACGGTT

• Ambion Pre-miR miRNA Precursor: hsa-miR-21–5p: (UAGCUUAUCAGACUGA UGUUGA)

• Ambion Anti-miR miRNA Inhibitor: hsa-miR-21–5p (UAGCUUAUCAGACUGAU GUUGA)

• Santa Cruz Control siRNA (UUCUCCGAACGUGUCACGU)

• Santa Cruz TIMP3 siRNA (h2) sc-44331 consists of a pool of three siRNAs with sequences:

  1. GGUAUCACCUGGGUUGUAAtt

  2. GAACCUGUAUUCCUCUUCUtt

  3. GAGAGUAGGUGAUAAUGUAtt

Transfection Efficiency

Transfection efficiency was assessed using a FAM labeled miR construct (Ambion, Austin, TX) with the same transfection method above. Following harvest, 5×10⁴ cells were plated on cover slips overnight before staining with DAPI. Confocal images were captured using an Olympus FV1000-Spectral microscope equipped with a PLANFLN 40x oil-immersion objective lens (N.A. 1.3) (S1 Fig.). All imaging for each fluorescence signal was performed under identical detector settings.

RNA extraction and Real-Time PCR

Total RNA from cells was isolated using TRIzol reagent (Invitrogen) as per the manufacturer’s recommendations for both mRNA and miR analyses. For analysis of miR expression, Fast Real-Time PCR analyses were carried out using TaqMan miR assays (Applied Biosystems) according to the manufacturer’s protocol. Relative expression was normalized to RNU6B, a small ubiquitous RNA. Relative levels of TIMP3 mRNA were examined using Fast Real-Time PCR and normalized to levels of Beta Actin. All reagents, primers and probes were obtained from Applied Biosystems (Foster City, CA). Gene and miR expression levels were quantified using the ABI Prism 7900HT Sequence Detection System (Applied Biosystems). Comparative Real-Time PCR, using the Ct method, was performed in triplicate, including no-template controls [24]. Expression was calculated as fold change (2^-ΔΔCt) compared with the control pre-miR-transfected cells or siRNA negative control-transfected cells.

Proliferation Assay

Cell proliferation was measured as absorbance at 570 nm using the 3-(4,5-Dimethylthiazol-2-yl)-2,5-Diphenyltetrazolium Bromide (MTT) Cell Proliferation Assay kit according to the manufacturer’s instructions (ATCC, Manassas, VA). All assays were performed in triplicate.

Migration Assays

Cells were plated on 60 mm² plates at a density of 1 × 10⁶ cells per well. When the cells were 70–80% confluent, they were transfected with pre-miR-21 or control miR-21. Twenty-four hours post-transfection, cells were collected and counted. Radius 24-well Cell Migration Assays (Catalog # CBA-125-ECM, Cell Biolabs, Inc., San Diego, CA) were used, following the manufacturer’s instructions. Each well contains a circular 680 μm-diameter gel spot to which cells do not attach. Each plate has a row of 6 wells coated in Collagen I, a row coated in Fibronectin, a row coated in Laminin I, and an uncoated row. A375 cells were seeded at a density of 0.5 × 10⁶ cells per milliliter (mL), and WM1552c, WM793b, and MEL 39 cells were seeded at a density of 0.75 × 10⁶ cells per mL. The plated cells were incubated at 37°C for 16 hours to 80% confluence. The cells were treated with 10 µg/mL Mitomycin C (Sigma Aldrich, St. Louis, MO) for 3 hours to inhibit cell proliferation [25]. The Radius gel spot was removed according to the manufacturer’s protocol and media was changed to 10% serum. Wounds were monitored, and digital images of gap closure were taken using an Olympus IX50 inverted microscope at 10X magnification (1280 × 1024 pixels) (Olympus Imaging America, Inc., Center Valley, PA). Areas of gap closure were measured using ImageJ processing software (National Institutes of Health, Bethesda, MD). Data is shown as percentage of the original wound area.

Invasion Assays

Matrigel invasion assays were conducted according to manufacturer’s instructions (BD Biosciences, San Jose, CA). Briefly, 5 × 10⁴ transfected cells in media containing 2% FBS were plated in duplicate on Transwell filters coated with or without Matrigel. The lower compartments of the invasion chambers contained media with 10% FBS as chemoattractant. After an 18-hour incubation at 37°C, cells remaining on the upper surface of the filter were removed, and the cells that migrated through the filter were fixed, stained, and counterstained with Dip Quick Stain Kit (Jorgensen Laboratories, Inc., Loveland, CO). Photographs were taken of five 20X fields for each filter on an EVOS XL digital inverted microscope and cell numbers were enumerated from the images (2048 × 1536 pixels) (Advanced Microscopy Group, Bothell, WA). Data is expressed as the percent invasion through the Matrigel matrix by calculating the ratio of the mean number of cells that invaded through the Matrigel matrix to the mean number of cells that migrated through the control insert.

Immunoblot Analysis

Twenty-four hours post-transfection, cells were collected and lysed by standard procedure in radioimmunoprecipitation assay buffer (Sigma Aldrich, St. Louis, MO) containing protease inhibitor and phosphatase inhibitor cocktails (Thermo Fisher Scientific, Inc., Waltham, MA). Proteins were separated by SDS-PAGE, transferred to nitrocellulose or polyvinylidene difluoride filters and probed with antibodies specific for TIMP3, programmed cell death protein 4 (PDCD4), tropomyosin-1 (TM1), (Santa Cruz Biotechnology, Santa Cruz, CA), phosphatase and tensin homolog (PTEN) (Cell Signaling Technology, Danvers, MA), or β-actin (Sigma-Aldrich, St. Louis, MO). Following incubation with the appropriate horseradish peroxidase-conjugated secondary antibodies, immune complexes were detected using the Pierce ECL Western Blotting Substrate (Thermo Fisher Scientific, Inc., Waltham, MA). β-actin was used to confirm equal loading.

Flow Cytometry

TIMP3 protein expression was analyzed in Mel39 cells following overnight transfection with a pre-miR 21 or a control miR (25 uM) oligonucleotide prior to harvest. Cells were then incubated with PE-anti-TIMP3 or isotype control Ab, washed and fixed in 1% formalin. A total of 10,000 cells were analyzed on a LSRII flow cytometer.

In vivo Studies

LNA oligonucleotides against miR-21 and a negative control oligonucleotide were obtained from Exiqon, Inc. (Woburn, MA). For the experiments of the in vitro transfected A375 cells, knockdown oligonucleotides were transfected using TransIT TKO transfection reagent (Mirus Bio, Madison, WI) into A375 cells at a final concentration of 50 nM each. After 24 hours from transfection, cells were collected, and miR-21 expression was analyzed by Real-Time PCR to verify effective miR knockdown. At the same time point, 2 × 10⁶ cells were resuspended in PBS and subcutaneously injected into the right flank of 6 week old female 01B74 Athymic NCr-nu/nu mice (n = 4 for the control LNA group and n = 6 for the anti-miR-21 LNA group) (Frederick National Library—NCI, Frederick, MD). Tumor growth was monitored by caliper measurement three times a week for 3 weeks.

For the in vivo antagomir treatments, 6 week old female 01B74 Athymic NCr-nu/nu mice (Frederick National Library—NCI, Frederick, MD) were subcutaneously injected in the right flank with 2 × 10⁶ cells A375 cells. After the tumors had reached an average volume of 100 mm³, the tumors were directly injected with 50 μL of PBS alone, or 50 μL of PBS and diluted TransIT TKO transfection reagent containing 500 nM control LNA or 500 nM anti-miR-21 LNA (n = 5 per group). Tumors were treated intra-tumorally at days 0, 4, 7, and 11, for a total of 4 injections per tumor. Tumor growth was monitored by caliper measurement three times a week for 4 weeks.

Tumor volume was calculated as follows: V = L × l² × 0.5, where L and l represent the larger and the smaller tumor diameter, respectively. At the end of each study, animals were sacrificed, and tumors were collected with a portion fixed in formalin for immunohistochemistry. Animals were housed by the University Laboratory Animal Resources according to institutional guidelines, and all experiments were approved by the Institutional Animal Care and Use Committee (The Ohio State University, Columbus, OH).

Immunohistochemistry

The tumors were excised, fixed in a 10% formaldehyde solution, embedded in paraffin, and cut into slices for staining. A set of slides was stained with haematoxylin eosin for the morphological study and for the count of mitosis. To evaluate the mitotic index, three fields at 400X magnification were randomly selected, and the number of mitoses was counted. Another set of slides was stained with the goat IgG polyclonal antibody to TIMP3 (Santa Cruz Biotechnology, Santa Cruz, CA) or with normal goat IgG as a control (Sigma-Aldrich, St. Louis, MO). Brown, granular intracellular staining was considered to be positive for TIMP3. Immunostaining was scored on tumor tissue sections from each mouse by an independent pathologist who was blinded to group identity.

Increased miR-21 activity leads to increased invasion but not migration in vitro

For metastasis to occur, primary melanoma cells must degrade the basement membrane and extracellular matrix and migrate through the stroma. In order to assess the effects of elevated miR-21 expression on melanoma cell movement, each of the four cell lines was transfected with pre-miR-21 or the control and plated onto Radius Migration Assay ECM-coated plates that have uniform wounds in the cell monolayers. Changes in lesion area were monitored over 0 to 20 hours (Fig. 2A, S2 Fig.). The difference in wound closure between control pre-miR-transfected and pre-miR-21-transfected monolayers was unremarkable in each of the collagen-coated wells (Fig. 2B), fibronectin-coated wells (S2 Fig.), and on the uncoated wells (S2 Fig.).

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Figure 2

Migration assay wound closure following transfection with pre-miR-21 is consistent with control results.

Following transfection with control pre-miR or pre-miR-21, cells were plated on Radius Migration Assay ECM-coated plates that have uniform wounds. Photographs were taken of the wound immediately following migration initiation and 14 hours later. Photographs of representative experiments for each cell line on the collagen-coated wells are shown (A). Migration was measured as the percent of the original wound area on the collagen-coated wells (n = 4) (B). Boyden chamber assays were used to evaluate invasive activity of melanoma cells transfected with control pre-miR or pre-miR-21. Photographs of representative experiments for each cell line are shown (C). Data are represented as the ratio of the average number of cells migrating through control inserts to the average number of cells invading through inserts coated with matrigel (n = 4) (D). Following transfection with control pre-miR or pre-miR-21 at 3.125, 6.25, or 12.5 nM, cells were plated on Boyden chamber assays to evaluate invasive activity of A375 melanoma cells at lower doseage of oligonucleotide. Data are represented as the ratio of the average number of cells migrating through control inserts to the average number of cells invading through inserts coated with matrigel (E). Error bars represent standard error. * p < 0.05.

Invasive potential was examined using the Boyden chamber assay (Fig. 2C). Two of the four melanoma cell lines tested exhibited increased invasion upon transfection with pre-miR-21 as compared to control pre-miR-transfected cells (WM1552c: 25.3% ± 0.9 v. 5.6% ± 0.7; WM793b: 19.5% ± 2.9 v. 6.2% ± 0.5; A375: 7.1% ± 3.2 v. 8.0% ± 4.2; MEL 39: 23.0% ± 8.4 v. 12.8% ± 8.2) (Fig. 2D). This increase was significant in WM1552c and WM793b (p < 0.05) and approached significance in MEL 39. Notably, there appeared to be an effect of miR-21 at lower doses of oligonucleotide in A375 cells (Fig. 2E).

Changes in TIMP3 protein expression are associated with miR-21 expression

Several mRNA targets for miR-21 have been recently verified, including phosphatase and tensin homolog (PTEN), tropomyosin-1 (TM1), and programmed cell death protein 4 (PCDC4) [20, 26–29]. Additionally, tissue inhibitor of metalloproteinases-3 (TIMP3) has been identified as a putative target and has been shown to be decreased in response to miR-21 [19, 20]. Immunoblots of cell lysates obtained 24 hours post-transfection revealed a decrease in the TIMP3 protein in all four melanoma cell lines transfected with pre-miR-21 (Fig. 3A and S3 Fig.). There were no reproducible trends in the expression of TM1 and PCDC4. Interestingly, an increase in PTEN protein was observed in the WM1552c and A375 cell lines in response to pre-miR-21 transfection. Because miRs can achieve a decrease in protein expression by causing the degradation of target mRNAs and by inhibiting translation of mRNA, Real-Time PCR was performed to evaluate changes in TIMP3 mRNA expression in response to increased miR-21. TIMP3 mRNA expression was variable between transfection experiments and could not be associated with the consistently observed decrease in TIMP3 protein (Fig. 3B). Additionally, flow cytometric analysis of TIMP3 protein expression in the Mel 39 cell line following transfection with a pre-miR-21 construct showed a decrease in TIMP3 expression from 63.45% to 30.75% (Fig. 3C).

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Figure 3

Changes in TIMP3 protein expression relate to miR-21 expression.

Cells were collected 24 hours post-transfection for lysis, total RNA isolation, and flow cytometry. Twenty micrograms of protein were loaded and subjected to immunoblotting for the miR-21 putative target proteins TM1, TIMP3, PDCD4, and PTEN (A). Immunobloting for β-actin was used as the loading control. The RNA was converted to cDNA and Real-Time PCR for TIMP3 was performed (B). Induction of expression was calculated relative to β-actin and compared to control-transfected cells. Cells were incubated with PE-anti-TIMP3 or isotype control Ab, washed and fixed in 1% formalin. A total of 10,000 cells were analyzed on a LSRII flow cytometer (C). Error bars represent standard error.

Decreased TIMP3 expression increases melanoma invasiveness

The finding that TIMP3 expression was decreased in melanoma cells with elevated miR-21 and increased invasiveness prompted an exploration into the influence of TIMP3 on invasion. Invasive potential was examined using the Boyden chamber assay (Fig. 4A). Three of the four melanoma cell lines tested exhibited increased invasion when TIMP3 expression was down-regulated by siRNA as compared to the negative control-transfected cells (WM1552c: 44.6% ± 11.8 v. 6.4% ± 4.3; WM793b: 18.2% ± 4.5 v. 4.2% ± 2.5; A375: 10.3% ± 3.5 v. 9.7% ± 4.3; MEL 39: 19.1% ± 4.1 v. 7.9% ± 5.7) (Fig. 4B). This increase was significant in WM1552c and WM793b (p < 0.05) and approached significance in MEL 39, mimicking the effects of miR-21 over-expression in cell lines. Reduction of TIMP3 transcript following siRNA transfection was confirmed by immunoblot (Fig. 4C) and Real-Time PCR (Fig. 4D).

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Figure 4

Invasion assays show that decreased TIMP3 expression increases melanoma invasiveness.

Boyden chamber assays were used to evaluate invasive activity of melanoma cells transfected with negative control or TIMP3-specific siRNA. Photographs of representative experiments for each cell line are shown (A). Data are represented as the ratio of the average number of cells migrating through control inserts to the average number of cells invading through inserts coated with matrigel (n = 4) (B). Cells were also collected 24 hours post-transfection for lysis and total RNA isolation. Immunoblot performed on lysates confirmed down-regulation of TIMP3 expression (C). Immunoblotting for β-actin was used as the loading control. The RNA was converted to cDNA and Real-Time PCR for TIMP3 further confirmed down-regulation of TIMP3 expression (D). Error bars represent standard error. * p < 0.05.

In vitro depletion of miR-21 in melanoma cells leads to decreased tumor size in vivo

The data obtained demonstrating that miR-21 over-expression enhances invasion indicates that miR-21 may represent a treatment target. To test this hypothesis, A375 cells were transfected with an LNA oligonucleotide targeting miR-21 or a control LNA oligonucleotide. Real-Time PCR was performed on the cells 24 hours post-transfection and demonstrated reduced miR-21 expression in the cells transfected with anti-miR-21 LNA (Fig. 5A). Notably, microRNA have been shown to resist degradation for up to three weeks through associations with target sequences, adenylation, and decreased uridylation [30]. Transfected cells were then injected subcutaneously into athymic nude mice, and tumor growth was followed. Mice injected with the anti-miR-21 LNA-transfected cells developed significantly smaller tumors than those that received the control LNA-transfected cells. This difference became apparent beginning 6 days after tumor cell injection (p < 0.05) (Fig. 5B). At the completion of the study, tumors were harvested, fixed in formalin, embedded in paraffin, and evaluated for TIMP3 protein expression by immunohistochemistry. All control LNA-transfected tumors demonstrated 1+ staining for TIMP3, while the anti-miR-21 LNA-transfected tumors stained diffusely darker and exhibited 2+ staining on immunohistochemistry (Fig. 5C). Areas of confluent necrosis were negligible in both groups, and the mean mitotic indices were comparable in both groups (data not shown).

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Figure 5

Decreased tumor size in vivo is achieved by depletion of miR-21 in vitro.

A375 cells were transfected in vitro with an LNA oligonucleotide targeting miR-21 or a control LNA oligonucleotide. Cells were collected 24 hours post-transfection for total RNA isolation. The RNA was converted to cDNA, and Real-Time PCR for miR-21 confirmed reduced miR-21 expression (A). Transfected cells were then injected subcutaneously into athymic nude mice, and tumor growth was followed. Tumor volume was calculated as V = L × l² × 0.5, where L and l represent the larger and the smaller tumor diameter, respectively. Mean tumor volumes are represented (B). At the completion of the study, tumors were harvested, fixed and embedded, and evaluated for TIMP3 protein by immunohistochemistry, where TIMP3 immunoreactivity is in brown (C). N = 4 for control LNA tumors and n = 6 for anti-miR-21 LNA tumors. Error bars represent standard error. * p < 0.05.

We thank the OSU CCC Nucleic Acid Shared Resource and the OSU CCC Comparative Pathology and Mouse Phenotyping Shared Resource. Confocal images were obtained from the Campus Microscopy and Imaging Facility at The Ohio State University.