Human cervical cancer cell lines, HeLa and SiHa, were obtained from the American Type Culture Collection (ATCC) and cultured in Dulbecco’s modified Eagle’s medium (DMEM; Invitrogen, Grand Island, NY, USA) supplemented with 10% fetal bovine serum (FBS; Invitrogen), in 5% CO₂ at 37°C. One percent (1%) O₂ with 5% CO₂ and 94% N₂ was used as a hypoxia condition in an airtight anaerobic incubator (Coylab 1 Person Polymer O₂ Control Glove Boxes) (27).

Western blot analysis was performed as previously described (28). Briefly, control and treated cells were lysed in an SDS-PAGE sample buffer. Equal amounts of proteins were fractionated on SDS-PAGE and transferred to polyvinylidene difluoride membranes. After blocking with 5% non-fat dry milk in TBST (Tris-buffered saline containing 0.1% Tween-200), the membrane was incubated overnight at 4°C with primary antibodies against LOX (1:4,000; Novus), E-cadherin (1:1,000; Cell Signaling Technology), α-SMA (1:200; Abcam), vimentin (1:1,000; Cell Signaling Technology), MMP-2 (1:1,000; Boster), MMP-9 (1:1,000; Boster), tubulin (1:5,000; Thermo Scientific IHC, Fremont, CA, USA), GAPDH (1:2,000; Cell Signaling Technology). After washing with TBST three times each for 5 min, membranes were incubated with the corresponding secondary antibody (1:2,000; Cell Signaling Technology) conjugated with horseradish peroxidase for 1 h at room temperature. After washing, blots were developed with an enhanced chemiluminescence system (Molecular Imager ChemiDoc XRS+ System, Bio-Rad). Protein bands were quantitated by the 1D ScanEX software (Scananalytics, Fairfax, VA, USA). Experiments shown here were repeated at least 3 times with reproducible results and a representative one is presented, unless otherwise indicated.

Cervical carcinoma cells in phenol red-free DMEM were incubated in normoxia or hypoxia. The conditioned medium was collected and LOX activity was assayed using diaminopentane as a substrate in the Amplex Red fluorescence assay (29,30). The reaction mixture consisted of 1.2 mol/l urea, 0.05 mol/l sodium borate (pH 8.2), 10 mmol/l diaminopentane, 10 μmol/l Amplex red and 1 U/ml horseradish peroxidase in a final volume of 1 ml. Conditioned medium (500 μl) was added to the reaction mixture in the presence or absence of 0.5 mmol/l aminopropionitrile (BAPN; Sigma), an active site inhibitor of LOX. Samples were incubated at 37°C for 30 min, placed on ice, and then recorded at an excitation wavelength of 563 nm and emission wavelength of 587 nm (31). All enzyme activities were calculated as the increase of fluorescent units above background levels of BAPN controls and normalized to total cell protein (28).

Cells were serum-deprived for 24 h, seeded at a density of 50,000 cells/well on the top of Matrigel-coated filters, moved to chambers containing 600 μl of 10% FBS as a chemo-attractant and incubated under normoxia or oxygen-deprived conditions for 48 h. BAPN (500 μM) was added to the culture 24 h before oxygen deprivation and continued throughout the experiment (19). At the same time, equal cells were plated into 96-well plates for cell number assay (MTT). The cells (treated and untreated) were incubated at 37°C under normoxia or oxygen-deprived conditions for 48 h and then the Matrigel was removed with a cotton bud. The invaded cells were fixed, stained with hematoxylin and counted. The invasiveness of cervical carcinoma cells was determined by the percentage-of-invasion score (invaded cell number/total cell number 100%) (32). Experiments were repeated three times. The in vitro cellular migration assay was based on the described membrane invasion culture system, but differed in the use of filters not Matrigel-coated.

Cell morphology was studied during the indicated time course using an Olympus (Melville, NY, USA) IX71 inverted microscope.

Data are presented as the means ± standard deviation of 3 separate experiments. Significance of the differences between the experimental conditions was determined by one-way ANOVA followed by Bonferroni’s test. A P-value <0.05 was considered to indicate statistically significant differences and a P-value <0.01 was considered to indicate statistically very significant differences.

To explore the effect of hypoxia on LOX protein expression, we performed western blot assays in HeLa and SiHa cells incubated under hypoxic conditions for various time points over a 48-h period. As shown in Fig. 1, hypoxia enhanced LOX protein expression in a time course-dependent manner amounting to 1.48-, 1.74- and 2.07-fold of the control (52.6 density units) for HeLa cells (Fig. 1A), and 1.09-, 1.49- and 2.24-fold of the control (41.0 density units) for SiHa cells (Fig. 1B), respectively, at 12, 24 and 48-h time points. Furthermore, LOX catalytic assays indicated significant increases in the LOX activity by hypoxia in the conditioned media reaching 1.5-, 3.2- and 5.2-fold of the control for HeLa cells and 2.5-, 2.8- and 6.2-fold of the control for SiHa cells, respectively, at the same time points as described (Fig. 1C).

The first step of the cancer metastatic process is cell invasion. To study the effect of LOX inhibition with cervical carcinoma cell behavior, we examined the invasion of HeLa and SiHa cells in vitro. Both cell lines were incubated on Matrigel-coated filters of transwells for 48 h under normoxia or hypoxia in the presence or absence of 500 μM BAPN, an inhibitor of LOX. Following incubation, trans-filter (invasion) cells were stained (Fig. 2A and B) and numbers counted (Fig. 2C and D). As shown, two cell lines showed strong invasion phenomenon under hypoxia in comparison to normoxia. Notably, BAPN that inactivates LOX activity significantly reduced hypoxia-elicited cell invasion in both cell models (Fig. 2A and B). Counting of invasive cell number further illustrated morphological conclusion. As shown (Fig. 2C and D), hypoxia enhanced cancer cell invasion to 220 and 250% of the control, which were suppressed to 50 and 60% of the control in HeLa and SiHa cells, respectively, in the presence of 500 μM BAPN. Thus, LOX plays a key role in the development of invasion of cervical carcinoma cells.

Migration is essential for cancer cell motility and crucial for primary metastatic growth. Using the transwell assay we further evaluated BAPN effects on the migration of cervical carcinoma cells. As shown in morphological studies, enhancement of migration was observed in HeLa (Fig. 3A) and SiHa (Fig. 3B) cells under hypoxic conditions which was antagonized in the presence of 500 μM BAPN. This was confirmed by cell number counting such that hypoxia increased cancer cell migration to 180 and 240% of the control, which were decreased to 60 and 70% of the control in HeLa (Fig. 3C) and SiHa cells (Fig. 3D), respectively, in the presence of 500 μM BAPN. Thus, LOX facilitates hypoxia-induced migration of cervical carcinoma cells.

Phase-contrast microscopy showed morphological alterations in cervical carcinoma cells from the flatting, contacting and spreading form under normoxia to the elongating, spindle shape under hypoxia suggesting the loss of epithelial features and the gain of mesenchymal phenotypes of these cancer cells. Thus, hypoxia may induce EMT in cervical carcinoma cells. To test this possibility, we examined expressions of E-cadherin, α-SMA and vimentin, the EMT molecular markers, by western blotting in our cancer cell models. Consistent with the morphological changes, hypoxia induced downregulation of E-cadherin, an epithelial marker, in HeLa (Fig. 4A) and SiHa cells (Fig. 4B) in a time course-dependent manner. Reductions of E-cadherin in HeLa and SiHa cells amounted to 76, 49 and 3% of the control (142.5 density units) for HeLa cells, and 84, 64 and 21% of the control (128.5 density units) for SiHa cells, respectively, at 12, 24 and 48-h hypoxia incubation. Simultaneously, mesenchymal marker proteins, vimentin and α-SMA were increased to 3.0-, 3.5- and 5.0-fold of the control (19.0 density units), and 1.1-, 1.4- and 2.0-fold of the control (25.1 density units) for HeLa cells (Fig. 4C), and 4.2-, 4.6- and 4.3-fold of the control (51.9 density units), and 1.2-, 1.25- and 20.5-fold of the control (6.3 density units) for SiHa cells (Fig. 4D), respectively, under hypoxia for 12, 24 and 48 h. Thus, downregulation of epithelial marker, E-cadherin, and upregulation of mesenchymal markers, α-SMA and vimentin, were associated with cervical carcinoma cells under hypoxia indicating EMT occurred in such cell models under our experimental conditions.

To answer whether BAPN inhibits hypoxia-induced EMT in cancer cell models, we examined BAPN effects on morphological changes in cervical carcinoma cells under hypoxia with phase contrast microscopy. HeLa and SiHa cells exposed to hypoxia for 48 h displayed morphological changes towards a mesenchymal-like appearance (Fig. 5). Anoxic HeLa and SiHa cells were no longer able to form ‘cobblestone’ clusters typical for epithelial cells, but acquired a more elongated, spindle-like morphology, a critical marker of EMT. These morphological changes were involved in cervical carcinoma cell invasion and migration under hypoxia (33). This is based on findings that BAPN inhibited tumor cell invasion and migration (Figs. 2 and 3) antagonized morphological changes in cancer cells under hypoxia, and reversed cell phenotypes similar to those under normoxia. Thus, BAPN prevented HeLa and SiHa cells from hypoxia-induced morphological changes toward the EMT.

Finally, we detected the effects of BAPN on the expressions of E-cadherin, α-SMA, vimentin, MMP-2 and MMP-9 proteins, the EMT markers, in HeLa and SiHa cells exposed to hypoxia for 48 h. As shown, BAPN effectively prevented hypoxia-induced downregulation of E-cadherin (Fig. 6A and B) and strongly inhibited hypoxia-induced upregulation of α-SMA and vimentin (Fig. 6C and D). Although MMP-2 in HeLa and SiHa cells was not changed significantly under hypoxia or hypoxia plus BAPN, MMP-9 in both cell lines was markedly changed in response to experimental conditions (hypoxia and BAPN treatment). MMP-9 expression was increased by hypoxia in SiHa cells up to 1.65-fold of the control (47.5 density units) and turned to 0.88 of the control (47.5 density units) in the presence of 500 μM BAPN. Furthermore, BAPN also reduced MMP-9 expression to 0.41 of the control (128 density units) in HeLa cells in response to hypoxia. Densitometry data of BAPN effects on EMT marker proteins are presented in Table I. These results are consistent with BAPN effects on tumor cell invasion and migration, strongly supporting the conclusion that LOX is an essential factor for modulation of hypoxia-induced EMT, invasion and migration of cervical cancer cells.