The murine B16F10 melanoma cell line was obtained from the National Centre for Cell Sciences and was grown and maintained in Dulbecco's modified Eagle's medium (DMEM; Gibco/Invitrogen, Carlsbad, CA, USA), containing 10% FBS in a 5% CO₂ incubator at 37°C.

Exponential growing cells were sealed using parafilm in cell culture flasks (1×10⁶ cells/flask) and immersed in a thermostated water bath at the indicated temperature (43, 45 and 47°C) for 30 min. The control group was treated at 37°C for 30 min. The temperature of the medium increased quickly and reached the set temperatures within 3 min. The temperature in the medium was monitored with a fiber optic thermometer probe (FX-9020; Anritsu Meter Co., Tokyo). After heating, the cells were immediately incubated at 37°C in 5% CO₂.

Cells were incubated for 4 h to restore stability after heating, and then were harvested, counted, and inoculated (at the appropriate concentrations in a volume of 100 μl) into 96-well microtiter plates, 8 replicates were prepared for each group. After different incubation times at 37°C in a humidified 5% CO₂ atmosphere, the MTT assay was performed. MTT (Sigma, St. Louis, MO) was dissolved at a concentration of 5 mg/ml in Hank's salt solution and filtered with a 0.45 μm filter (in order to avoid MTT aggregates). MTT solution (10 ml) was added to each well and also to the control wells without cells. After 4 h of incubation, microtiter plates were centrifuged at 2,000 rpm for 10 min; medium was then removed, and 100 μl of DMSO was added to each well. After thorough mixing with a mechanical plate mixer, absorbance of the wells was read in a scanning well microculture plate reader at test and reference wavelengths of 550 and 620 nm, respectively. Absorbance values from all wells were corrected against the control absorbance levels.

B16F10 cells heated at different temperatures by water bath were allowed to form a monolayer on a fibronectin (5 μg/ml)-coated surface. A wound was made in the monolayer of cells by scratching a line on the monolayer with a pipette tip. Cells were then washed with PBS to remove cell debris and fed with fresh culture medium. Cells were allowed to proliferate and migrate into the wound during the next 24 h. Migration of cells into the wound was observed using a microscope (Olympus BX51, Tokyo, Japan). Three wounds were sampled for each treatment and experiments were carried out in triplicate.

The invasive activity of B16F10 cells after heating at different temperatures was assayed in a Transwell cell culture chamber (6.5 mm, 8 μm Costar, Corning). Polyvinylpyrrolidone-free polycarbonate filters were smeared with 8.0 μg fibronectin (Genscrip cat. no: RP10840) in a volume of 10 μl serum-free DMEM on the reverse side, and dried at room temperature. Matrigel (containing laminin, collagen type IV, heparan sulfate proteoglycan and entactin) (BD Biosciences cat. no: 356230) was diluted to 500 μg/ml with cold phosphate-buffered saline (PBS), applied to the upper surface of the filter (5 μg/filter), and dried at room temperature. B16F10 cells which were heated by water bath for 30 min and then incubated for 2 h at 37°C in 5% CO₂ were harvested with 1 mM EDTA in PBS, washed twice and resuspended to give a final concentration of 2.0×10⁶/ml in serum-free RPMI-1640 with 0.1% bovine serum albumin (BSA). Cell suspensions (100 μl) were added to the upper compartment and the filter chamber was incubated for 24 h at 37°C in a 5% CO₂ atmosphere. The cells on the upper surface of the filters were removed by wiping them with a cotton swab. The filters were then stained with crystal violet for 30 min. The cells that had invaded through Matrigel and reached to the reverse side were counted under a microscope in five predetermined fields at a magnification of ×400. Each assay was performed in triplicate.

B16F10 cells were heated by water bath for 30 min as noted and then incubated for 24 h with serum-free DMEM at 37°C in 5% CO₂. The culture supernatant was collected by centrifugation and then concentrated by lyophilization. The extract was then subjected to zymography on 7.5% SDS-PAGE (sodium dodecyl sulfate polyacrylamide gel electrophoresis) co-polymerized with 0.1% gelatin. Gel was washed in 2.5% Triton X-100 for 30 min to remove SDS and was then incubated overnight in a reaction buffer (50 mM Tris-HCl pH 7.0, 4.5 mM CaCl₂, 0.2 M NaCl). After incubation, the gel was stained with 0.5% Coomassie Blue containing 30% methanol and 10% glacial acetic acid. The bands were visualized by destaining the gel with the solution containing 30% methanol and 10% glacial acetic acid. The experiments were repeated three times under similar conditions, and one experiment was selected for representation.

Whole cell lysates were prepared by lysing the cells on ice with a protein extraction kit (SBS, China) for 20 min. Equal amounts of protein (30 μg/lane) were electrophoresed under non-reducing conditions on 10% acrylamide gels. After SDS-PAGE, proteins were transferred to a polyvinylidene difluoride membrane (Bio-Rad, USA). To block non-specific binding, the membrane was incubated in TBS with 0.1% Tween-20 (TBST) containing 5% nonfat milk for 2 h. Subsequently, the membrane was incubated for 2 h with antibodies against TGF-β₁ and Smad4 (Santa Cruz Biotechnology, Santa Cruz, CA, USA, 1:1000), respectively, in TBST with 5% non-fat milk. After washing in TBST, horseradish peroxidase-conjugated anti-mouse or anti-rabbit IgG (Santa Cruz Biotechnology) was used as a secondary antibody (1:2000 in TBST with 2% BSA, incubated for 1 h). Each sample was also probed with an anti-β-actin antibody (Santa Cruz Biotechnology) as a loading control. Bands were scanned using a densitometer (GS-700, Bio-Rad), and quantification was performed using Quantity One 4.6.2 software (Bio-Rad).

The expression of TGF-β₁ and Smad4 mRNA was analyzed by semi-quantitative RT-PCR. B16F10 cells were heated by water bath for 30 min as noted and then incubated for 24 h. Total RNA was extracted from the cells using TRIzol reagent (Invitrogen) respectively and 5 μg RNA was used to synthesize cDNA using an RT-PCR kit (M-MLV) (KeyGEN, KGA1305) following the manufacturer's protocol. The cDNA was used to amplify the TGF-β₁ and Smad4 mRNA fragment, while the housekeeping gene β-actin was also amplified as an internal standard. The corresponding primer sequences were: β-actin forward, 5′-ACCTTCTACAATGAGCTGCGT-3′ and reverse, 5′-ATAGCACAGCCTGGATAGCAA-3′ (157 bp); TGF-β₁ forward, 5′-GGCCAGATCCTGTCCAAGC-3′ and reverse, 5′-GTGGGTTTCCACCATTAGCAC-3′ (201 bp); Smad4 forward, 5′-GTCTGAGCATTGTGCATAGTTTG-3′ and reverse, 5′-GACGGGCATAGATCACATGAG-3′ (246 bp).

The cycling program was performed as follows: 1 cycle of 94°C for 5 min; 33 cycles of 94°C for 30 sec, 54°C for 45 sec, 72°C for 60 sec; followed by a final elongation step at 72°C for 10 min. Then RT-PCR products were electrophoresed through a 1.5% agarose gel with ethidium bromide. The experiments were repeated three times under similar conditions, and one experiment was selected for representation.

Specific pathogen-free female C57BL/6 mice were purchased from Beijing Center for Disease Control and Prevention (China) and were maintained in our animal facility for at least 2 weeks before use. The mice were housed under specific pathogen-free conditions in a barrier facility with a 12-h light/dark cycle. The mouse model of melanoma was established by transplanting a 0.1-ml cultured B16F10 cell suspension at a concentration of 1×10⁷ cells/ml into the subcutaneous tissue of the back of each mouse. Forty mice were randomized and divided into four groups: 45°C hyperthermia group (H1), 50°C hyperthermia group (H2), magnetic fluid group (M) and control group (C). Orthotopic tumors were staged for 7 days and reached ~0.5 cm³ in size. The tumor-bearing mice of the M group, H1 group and H2 group were locally injected with magnetic fluid in the tumor area, then underwent radiation by an alternating magnetic field (AMF). The magnetic fluid (Fig. 1) was purchased from Anhui Jinke Magnetic Liquids Ltd. and consisted of uncoated and water-based particles of Fe₃O₄ ~10 nm in diameter, and the concentration of the ferrites in aqueous solution was 100 mg/ml. The magnetic field applicator (Fig. 2) was produced by our laboratory at the Department of Engineering Physics, Tsinghua University, and the parameters of the AMF were carefully adjusted until a local tumor temperature (45 or 50°C) was maintained for 30 and 10 min, respectively. After 24 h, 3 mice from each group were sacrificed for anatomy to observe the magnetic fluid distribution and to prepare for the following immunohistochemistry tests.

Tumor growth was monitored at a defined regular interval (2 days) by measuring the diameters using a vernier caliper. Tumor volume was determined based on the following formula: Tumor volume = 0.5 × a × b² (a and b represent the maximal and minimal tumor diameter, respectively). Mice survival times were determined. After a 90-day follow-up period, all mice were sacrificed.

The paraffin-embedded tumor tissues were sectioned into 5-μm slices, deparaffinized in xylene, rehydrated in graded ethanol concentrations (100, 95, 70, and 50%), and finally submerged in phosphate-buffered saline (PBS). Endogenous peroxidase was blocked by incubation with 0.3% H₂O₂ for 30 min in the dark, and then sections were placed in an autoclave with 0.01 M sodium citrate solution at 121°C for 5 min for antigen retrieval. Immunohistochemical staining was performed using primary antibodies for TGF-β₁. The sections were incubated with antibodies (1:100) overnight at 4°C and then incubated with biotin-labeled anti-rabbit IgG (ZSGB-Bio, Beijing, China) at room temperature for 30 min. The tissue sections were counterstained with hematoxylin, dehydrated in graded ethanol concentrations (50, 70, 95, and 100%) and xylene, covered with glass coverslips, and then observed using a bright field microscope.

Statistical analysis was performed using SPSS (version 13.0). Data are expressed as means ± SD for n replicates as indicated in figure legends. One-way analysis of variance followed by an SNK test was used to assess significant differences between the control and experimental groups.

B16F10 cells treated by water bath at 43, 45 and 47°C for 30 min were then tested by MTT assay and scratch-wounding assays. As shown in Fig. 3, the proliferative ability of the cells after being heated at 45 and 47°C was markedly higher than at 43°C (P<0.05). As shown in Fig. 4, the mobility of B16F10 cells was obviously decreased by heating at 45 and 47°C.

We examined changes in the invasive and metastatic potential of B16F10 cells after hyperthermia treatment using a Matrigel invasion assay. Representative images of the Matrigel invasion assay showed a decrease in the number of invasive B16F10 cells after hyperthermia (x400) (Fig. 5A). Column data showed that hyperthermia decreased the invasiveness of B16F10 cells in a temperature-dependent manner (Fig. 5B). Compared with the control group (37°C), B16F10 cells heated at 43, 45 and 47°C showed significantly lower numbers of invasive cells (P<0.01).

In order to ascertain whether the downregulation of MMP-2 and MMP-9 in B16F10 cells is induced by hyperthermia, we examined the effect of hyperthermia treatment at different temperature points in the secretion and activity of MMP-2 and MMP-9 by gelatin zymographic analysis. As shown in Fig. 6, the white bands were areas degraded by MMP-2 and MMP-9. The corresponding image represents the quantitative analysis of the band intensities using a contour tool by Quantity One-4.6.2 (Basic) which clearly showed that hyperthermia treatment caused significant inhibition of the secretion and activity of MMP-2 and MMP-9 in B16F10 cells (P<0.01) and the decrease appeared to be temperature-dependent.

Western blot analysis (Fig. 7A) was performed to ascertain whether the protein expression of TGF-β₁/Smad4 in B16F10 cells is affected by hyperthermia. Fig. 7B shows the corresponding average optical densities of TGF-β₁ and Smad4 after different temperature treatments. The reduction showed temperature dependence for TGF-β₁, while the upregulation of Smad4 lasted for a short time at 43°C and 45°C but not at 47°C. Moreover, at the higher temperature, the increase in Smad4 protein expression occurred earlier. The bar graph represents the corresponding average optical densities using Quantity One-4.6.2 (Basic).

RT-PCR was performed to ascertain whether the mRNA expression of TGF-β₁ and Smad4 in B16F10 cells is suppressed by hyperthermia. As shown in Fig. 8, the mRNA expression of TGF-β₁ was significantly reduced by hyperthermia when the temperature was above 43°C, while the mRNA level of Smad4 did not change significantly.

MFH at 45°C (H1 group) and 50°C (H2 group) inhibited tumor growth. Compared with 45°C MFH (H1 group), 50°C MFH (H2 group) had a greater inhibitive effect on tumor growth (P<0.05). The survival times of the mice in the 50°C MFH H2 group and 47°C MFH H1 group were longer than that of the control group (P<0.05). Immunohistochemical assay showed that the expression of TGF-β₁ was markedly decreased in the 50°C MFH H2 group compared with the other groups (P<0.05) (Fig. 9).

In the in vivo study, no mice died during the MFH process as described above, and no infiltration of magnetic fluid was found in the surrounding tissue and organs. As shown in Fig. 10, the tumor growth rate of the control group and magnetic fluid group was significantly lower than H1 and H2 groups treated at 45 and 50°C, respectively (P<0.05) and the survival period of the tumor-bearing mice which was observed for 90 days after tumor implantation showed that magnetic fluid hyperthermia (especially for H2 group at 50°C) prolonged the life span of the mouse model significantly.