SOX4 expression is associated with treatment failure and chemoradioresistance in oral squamous cell carcinoma

Background In humans, sex-determining region-Y (SRY) related high-mobility-group box 4 (SOX4) is linked to development and tumorigenesis. SOX4 is over-expressed in several cancers and has prognostic significance. This study evaluated whether SOX4 affects oncogenic behavior and chemoradiotherapy response in head and neck squamous cell carcinoma (HNSCC) cells, and documented the relationship between its expression and prognosis in oral squamous cell carcinoma (OSCC). Methods We used small interfering RNA in HNSCC cells to evaluate the effect of SOX4 on cell proliferation, apoptosis, chemoradiation-induced apoptosis, invasion, and migration. SOX4 expression in OSCC tissues was investigated by immunohistochemistry. Results SOX4 knockdown (KO) decreased cell proliferation and induced apoptosis by activating caspases-3 and −7, and poly-ADP ribose polymerase and suppressing X-linked inhibitor of apoptosis protein in HNSCC cells; it also enhanced radiation/cisplatin-induced apoptosis; and suppressed tumor cell invasion and migration. Immunostaining showed SOX4 protein was significantly increased in OSCC tissues compared with adjacent normal mucosa. SOX4 expression was observed in 51.8 % of 85 OSCC tissues, and was significantly correlated with treatment failure (P = 0.032) and shorter overall survival (P = 0.036) in patients with OSCC. Conclusions SOX4 may contribute to oncogenic phenotypes of HNSCC cells by promoting cell survival and causing chemoradioresistance. It could be a potential prognostic marker for OSCC. Electronic supplementary material The online version of this article (doi:10.1186/s12885-015-1875-8) contains supplementary material, which is available to authorized users.


Background
Oral cavity cancer accounts for approximately 28 % of all head and neck cancers [1]. Squamous cell carcinomas represent about 90 % of oral cavity cancer. Oral squamous cell carcinoma (OSCC) is the sixth most prevalent malignancy worldwide and the third most common cancer in developing nations [1]. Surgery, radiation therapy, chemotherapy or combinations of these modalities are standard options for managing OSCC; therapeutic strategies are based on disease stage [2]. As advancedstage OSCC has a poor prognosis [1], understanding the molecular and biological changes of its progression is critical to development of more effective therapies.
Little is known about the molecular and prognostic significance of SOX4 in OSCC, although one report correlated SOX4 expression with OSCC tumor stage [12]. In the present study, we investigated whether SOX4 affects tumor cell behaviors such as cell proliferation, apoptosis, invasion, migration, and chemoradiation-induced apoptosis in head and neck squamous cell carcinoma (HNSCC) cells to validate its potential as a novel molecular target. We also assessed its prognostic value in OSCC.

Cell culture and transfection
The HNSCC cell lines (PCI 50 and SNU 1041) were kindly provided by Dr. Sung MW (Seoul National University, Seoul, South Korea). The normal immortalized human keratinocyte cell line (HaCaT) was purchased from the American Type Culture Collection (Manassas, VA, USA). Cell lines were cultured in DMEM or RPMI1640 (Hyclone, Logan, UT, USA) supplemented with 10 % fetal bovine serum (Hyclone) in a humidified atmosphere of 5 % CO 2 at 37°C. For transfection, cells were seeded on 6-well plates at 2 × 10 5 cells per well at the time of transfection. Small interfering RNA (siRNA) was used to knock down endogenous SOX4 gene expression in HNSCC cells. Cells were transfected with SOX4-specific siRNA (Bioneer, Daejeon, Korea) or negative control siRNA (Qiagen, Valencia, CA, USA) using Lipofectamine™ 2000 (Invitrogen, Carlsbad, CA, USA) for 48 h. SOX4 knockdown (SOX4-KO) was checked by reverse transcriptionpolymerase chain reaction (RT-PCR) and western blotting.

Protein isolation and western blot analysis
Cells were lysed in RIPA buffer. Resolved proteins were electrophoretically transferred to polyvinylidene fluoride membranes. Specific proteins were sequentially blotted with primary antibodies: SOX4 (Catalogue# ab80261, Abcam, Cambridge, Mass, USA), cleaved caspase-3, cleaved caspase-7, cleaved poly-ADP ribose polymerase (PARP; Cell Signaling Technology, Danvers, MA, USA), X-linked inhibitor of apoptosis protein (XIAP) and polyclonal anti-GAPDH (Santa Cruz Biotechnology, CA, USA). Each membrane was incubated with anti-rabbit or antimouse HRP-conjugated secondary antibody (Santa Cruz Biotechnology). Immunoreactive proteins were visualized on the enhanced chemiluminescence detection system HRP substrate (Millipore, Billerica, MA, USA). The immunoreactive bands were quantified by densitometric analysis using the luminescent image analyzer LAS-4000.

Cell proliferation assay
Cells were seeded in a 96-well plate (5 × 10 3 cells/well), and were transfected with SOX4 siRNA and negative control siRNA the next day. After incubation for 48 h, cell proliferation and viability were measured using the EZ-CyTox (tetrazolium salts, WST-1) cell viability assay kit (Daeil Lab Inc, Seoul, South Korea). After adding WST-1 reagent for 1-2 h at 37°C, absorbance at 460 nm was determined using a microplate reader (Infinite M200; Tecan, Austria GmbH, Austria) with Magellan V6 data analysis software (Tecan). Triplicate wells were used for experimental conditions and all experiments were repeated at least three times.

Apoptosis assay
Apoptosis was determined by an Annexin V-fluorescein isothiocyanate (FITC) assay. Forty-eight hours after transfection, cells transfected with SOX4 siRNA or negative control siRNA were collected using trypsin, washed twice in phosphate buffered saline (PBS), and re-suspended in binding buffer (BD Biosciences, San Diego, CA, USA). Annexin V-FITC and 7-amino-actinomycin D (7-AAD; BD Biosciences) were added to the cells, which were incubated in the dark for 15 min, then re-suspended in 400 ml of binding buffer. Cells were analyzed using a FACSCalibur flow cytometer (Becton Dickinson, San Jose, CA). Data analysis was performed using standard Cell Quest software (Becton Dickinson).

Cell invasion assay
Cell invasion ability was measured by the number of cells that invaded through a transwell invasion apparatus with 8.0-μm pores (Costar, Cambridge, UK). Living cells transfected with SOX4 siRNA or negative control siRNA were seeded at 3 × 10 5 cells in 120 μl of a 0.2 % bovine serum albumin (BSA) suspension in the upper chamber. We then loaded 400 μl of 0.2 % BSA containing 7-μg/ml fibronectin (Calbiochem, La Jolla, CA, USA) into the lower chamber as the chemoattractant. After incubation for 24 h, cells that had moved to the bottom Transwell surface were stained with Diff Quik solution (Sysmex, Kobe, Japan) and calculated in five random squares in the microscopic field of view. Results are shown as mean ± standard error of the number of cells/field in three individual experiments.
Cell migration assay (wound healing assay) Cells transfected with SOX4 siRNA or negative control siRNA were seeded in each well of Culture-Inserts (Ibidi, Bonn, Germany) at 1.5 × 10 5 cells/well. After incubation for 24 h, each insert was detached and the progression of cell migration was ascertained by photography at 0, 4, 8, 12, and 24 h, using an inverted microscope. Distances between gaps were normalized to 1 cm after capture of three random sites.

Patients and tumor specimens
To evaluate SOX4 protein expression, paraffin-embedded tissue sections were collected from 95 patients who had undergone diagnostic biopsy or definitive surgery for OSCC at Chonnam National University Hwasun Hospital (Jeonnam, Korea) between May 2004 and June 2013. None of the collected tissues were obtained after radiotherapy and/or chemotherapy. Ten patients were excluded, because of follow-up loss or palliative treatment intent. Of the 85 remaining patients, 82 patients were treated with definitive surgery with/without adjuvant radiotherapy or cisplatinbased concurrent chemoradiotherapy (CRT). Three patients, who refused surgery, were treated with induction chemotherapy, followed by cisplatin-based concurrent CRT with curative intent. Patients with locoregional recurrence after primary treatment underwent salvage surgery or CRT. Of 85 patients in our study, 50 (58.8 %) underwent chemotherapy and/or radiotherapy. Treatment failure was defined as disease with inoperable locoregional progression or distant metastasis, even through salvage treatment. Patients provided the written informed consents for the surgical procedures, as well as for the use of resected tissue specimens. Patients' clinicopathologic characteristics were reviewed in hospital records. Tumors were staged according to the seventh edition of the American Joint Committee on Cancer staging system [18]. Survival was measured from the date of starting treatment to the date of death or date last seen. This study was approved by the Institutional Review Board of Chonnam National University Hwasun Hospital (CNUHH-2015-028).

Immunohistochemistry
Tissue processing and immunohistochemical analysis were performed as previously described [15]. The tissues were incubated with polyclonal rabbit anti-human SOX4 (Abcam). Immunohistochemsitry was performed in five batches, averaging 18 samples, with one positive and one negative control per batch. Negative controls were treated similarly, except that primary antibodies were omitted.
Two independent observers interpreted SOX4 staining of specimens with no knowledge of the clinical information. Intensity was scored as follows: 0, no staning of tumor cells; 1+, weak to comparable staining in cytoplasm and/or the nucleus compared to that of nontumoral cells; 2+, readily appreciable or dark brown staining distinctly marking the tumor cell cytoplasm and/or nucleus [10]. Percentages of stained cells were scored as follows: 0: 0 %; 1: 1-25 %; 2: 26-50 %; 3: 51-75 %; and 4, >75 % [6,7]. Final staining scores were the product of the intensity and percentage scores, with ≤4 defined as low SOX4 expression and >4 defined as high SOX4 expression. Staining scores were discordant between the two pathologists (KHL and JHL) in five cases (5/85, κ = 0.875), which were re-evaluated by the two pathologists, who then reached an agreement for each inconclusive sample.

Statistical analyses
Relationships between SOX4 expression and various clinicopathologic parameters were compared using the

SOX4-KO suppresses tumorigenic activities in HNSCC cells
Initially, SOX4 expression at mRNA and protein levels was evaluated in HNSCC cells and HaCaT cells. Western blot and RT-PCR showed SOX4 to be well-expressed in PCI50 and SNU1041 cells, but negligibly expressed in HaCaT cells relative to HNSCC cells (Fig. 1a). To explore the role of SOX4 on oncogenic activities and treatment response in HNSCC cells, we used siRNA to inhibit endogenous SOX4 expression in HNSCC cell lines including PCI50 and SNU1041 cells. SOX4 mRNA and protein expressions were reduced by SOX4 siRNA in PCI50 and SNU 1041 cells compared with cells treated with negative control siRNA (Fig. 1b).

SOX4-KO decreases cell proliferation in HNSCC cells
Proliferating cells, as determined by absorbance, were significantly decreased in SOX4-KO cells at 48 h and 72 h in PCI50 and SNU1041 cells, as compared with negative control cells (P = 0.002; Fig. 1c).

SOX4-KO enhances apoptosis in HNSCC cells
To evaulate the effect of SOX4 on apoptosis, we used an Annexin V apoptosis assay. SOX4-KO PCI50 and SNU1041 cells displayed greater apoptotic rates than did control cells (Fig. 1d). The proportion of early and late apoptotic cells induced by transfection of SOX4 siRNA was greater than that induced by transfection of negative control siRNA (9.2 % vs. 33.2 % and 7.1 % vs. 38.1 %, respectively) in PCI50 and SNU1041 cells. Next, we investigated apoptosis regulatory proteins after SOX4-KO treatment. Levels of cleaved caspases-3 and −7, and PARP were increased, and the level of XIAP was decreased, in SOX4-KO PCI50 and SNU1041 cells, compared with negative control cells (Fig. 1e). These results suggest that SOX4-KO-induced apoptosis is associated with the modulation of apoptosis regulatory proteins such as caspases-3 and −7, PARP and XIAP.

SOX4-KO suppresses the tumor cell invasion and migration in HNSCC cells
In the cell invasion assay, the invasiveness of SOX4-KO PCI50 cells and SNU1041 cells was significantly decreased (See figure on previous page.) Fig. 3 Effects of SOX4 knockdown (SOX4-KO) on radiosensitivity and cisplatin chemosensitivity in head and neck squamous cell carcinoma cells. a, b Combination treatment of SOX4-KO with 5 Gy radiation or cisplatin resulted in significantly more apoptosis in PCI50 and SNU1041 cells than in control cells treated with 5 Gy radiation or cisplatin treatment alone. c, d SOX4-KO cells showed greater expression of cleaved caspases-3 and −7, and cleaved poly-ADP ribose polymerase (PARP), and less X-linked inhibitor of apoptosis protein (XIAP), than did control cells after 5 Gy radiation or cisplatin treatment ( * P < 0.05). C: negative control siRNA transfected cells; S: SOX4-specific siRNA transfected cells (SOX4-KO); Cis: cisplatin treatment; IR: irradiation  Fig. 2a). In the cell migration assay, the migratory ability of SOX4-KO cells was significantly less than that of negative control cells at 8 h, 12 h, and 24 h in PCI50 cells, and 8 h and 12 h in SNU1041 cells (P < 0.05; Fig. 2b).

SOX4-KO enhances radiosensitivity and cisplatin chemosensitivity in HNSCC cells
We addressed whether SOX4-KO enhances cisplatin chemosensitivity and radiosensitivity by the induction of apoptosis in PCI50 and SNU1041 cells. Twenty-four hours after transfection with SOX4 siRNA or negative control siRNA, cells were treated with 5 Gy radiation or cisplatin (10 μg/ml for 24 h). The combination of SOX4 siRNA and radiation resulted in significantly greater apoptosis compared with radiation alone (Fig. 3a). The percentages of early and late apoptotic cells induced by SOX4 siRNA + 5 Gy radiation were greater than those seen in negative control cells treated with 5 Gy radiation (23.1 % vs. 47.7 % and 19.7 % vs. 39.8 %, respectively) in PCI50 and SNU1041 cells. Similarly, the combination of SOX4 siRNA + cisplatin resulted in markedly greater apoptosis compared with cells treated with cisplatin alone (Fig. 3b), with larger percentages of early and late apoptotic cells in the SOX4 siRNA + cisplatin-treated cells than in the negative control treated with cisplatin only (18.7 % vs. 51.7 % and 19.0 % vs. 34.4 %, respectively) in PCI50 and SNU1041 cells. Consistently, the SOX4-KO cells showed greater expression of cleaved caspases-3 and −7 and PARP, and less XIAP, after radiation or cisplatin treatment compared with the control cells (Fig. 3c, d). These findings suggest that the combination of SOX4-KO and CRT has synergistic apoptotic effects in HNSCC cells.

SOX4 expression is associated with treatment failure and survival in OSCC SOX4 expression in OSCC tissues
The clinicopathological characteristics of the 85 OSCC patients in this study group are summarized in Table 1.
The patients included 61 men and 24 women, whose mean age was 63.2 ± 12.5 years (± standard deviation), with a range of 26-87 years. Their mean follow-up period was 43.7 ± 27.7 months (range: 3.6-125.3 months). SOX4 protein expression was investigated immunohistochemically in formalin-fixed, paraffin-embedded blocks of specimens from these 85 patients. Immunostaining patterns were heterogenous, with predominantly nuclear and/or cytoplasmic immunostained SOX4 protein in tumor cells, but with weak or no staining in the normal oral mucosa (Fig. 4). Based on our criteria [6,7,10], 44 (51.8 %) of the 85 OSCC specimens showed high SOX4 expression.

Correlation between SOX4 expression and clinicopathologic factors in OSCC tissues
To study the prognostic role of SOX4 in OSCC, we investigated the correlation between SOX4 expression and clinicopathological factors. SOX4 expression in OSCC was not associated with age, sex, location, T stage (tumor invasion), N stage or lymph node metastasis (P > 0.05, Table 1). However, SOX4 expression was correlated with recurrence (P = 0.004) and treatment failure (P = 0.032; Table 1). Moreover, overall survival (OS) and diease specific survival (DSS) of patients with high SOX4 expression was significantly shorter than for those with low SOX4 expression (P = 0.036 and P = 0.007, respectively; Fig. 5a).
In 50 patients who were treated with chemotherapy Fig. 4 Expression of SOX4 protein in oral squamous cell carcinoma (OSCC) specimens. Immunostaining showed SOX4 protein was significantly increased in OSCC tissues (arrow) compared with adjacent normal mucosa (arrow head). (×100, ×200 in the inlet box) and/or radiotherapy, patients with high SOX4 expression had significantly shorter OS and DSS than those with low SOX4 expression (P = 0.007 and P = 0.003, respectively; Fig. 5b).

Discussion
Initiation and progression of cancer are caused by alterations in transcriptional activities, resulting in an imbalance between oncogenes and tumor suppressor genes [19]. Transcription factors are deregulated in their expression and function during tumorigenesis [19]. The SOX transcription factor family plays a key role in many developmental processes by controlling terminal differentiation of a wide variety of cell types and cell fate decisions [20]. Consequently, deregulation of several SOX genes have been implicated in tumorigenesis [20]. SOX4 belongs to the C subgroup of the SOX family. High SOX4 expression has been shown to affect tumor development or progression in gastric cancer, colon cancer, prostate cancer, breast cancer, lung cancer, and endometrial cancer [7-10, 21, 22]. The mechanism by which SOX4 is involved in tumor development and progression in many cancers remains unclear. Tumorigenesis results from an imbalance between cell proliferation and cell death; most of the latter occurs through apoptosis [23]. Therefore, the primary mechanism through which SOX4 affects tumor initiation and progression may be deregulation of apoptosis. SOX4 gene encodes a protein with three distinguishable domains: an HMG box, a serine-rich region, and a glycinerich central domain [24]. The HMG box binds DNA, whereas the central domain is a functional region for regulating apoptotic cell death [24]. Therefore, we evaluated the impact of SOX4 in cell proliferation and b SOX4 expression was associated with significantly worse OS and DSS in patients with OSCC, who were treated with chemotherapy and/or radiotherapy (n = 50, P = 0.007 and P = 0.003, respectively). Solid line: patients with low SOX4 expression; dotted line: patients with high SOX4 expression apoptosis in HNSCC cells. In this study, knocked-down SOX4 induced apoptosis and suppressed cell proliferation, which indicates that SOX4 supresses apoptosis in HNSCC cells. Additionally, SOX4-KO-induced apoptosis was associated with the modulation of apoptosis-related proteins such as caspases-3 and −7, PARP, and XIAP. Our results concord with reports in which SOX4-KO in adenoid cystic carcinoma and prostate cancer cells induced apoptosis [6,7,25]. Therefore, SOX4 exerts its anti-apoptotic function by directly inhibiting caspase activities and up-regulation of anti-apoptotic proteins, thus contributing to tumorigenesis in HNSCC.
Second, the anti-apoptotic function of SOX4 apparently causes resistance to anti-cancer treatement such as CRT. Cancer cells are often characterized by increased resistance to apoptosis [26]. Overcoming apoptotic resistance is important to improve response to tumor treatments, especially CRT. In the present study, knocked-down SOX4 enhanced radiation-or cisplatin-induced apoptosis in HNSCC cells, which were further supported by elevated levels of cleaved caspases-3 and −7, and PARP in SOX4-KO HNSCC cells after radiation or cisplatin treatment. These results suggest that SOX4 inhibits radiation-or cisplatin-induced apoptosis, and contributes to CRT resistance in HNSCC cells. These findings are very important because CRT is used as primary or adjuvant treatment for locally advanced HNSCC (including OSCC), and CRT response is accepted as an important prognostic factor [2,27]. Our findings suggest that SOX4 can serve as a specific predictor for CRT response in HNSCC. Furthermore, a therapy in which SOX4 is targeted in combination with CRT might overcome apoptotic resistance and improve response in HNSCC.
Third, SOX4 appears to aggravate cell invasiveness and migration. HNSCC subtypes, including OSCC, are characterized by a marked propensity for local invasion and lymphatic metastasis. Understanding the molecular mechanisms that mediate tumor invasion and metastasis may enable identification of novel therapeutic targets for management of tumor dissemination. Our study showed that knocked-down SOX4 suppressed tumor cell invasion and migration in HNSCC cells; earlier studies showed it to significantly inhibit invasiveness and migration in prostate cancer cells [7]. These results indicate that SOX4 contributes to tumor progression and metastasis, and imply that SOX4 could be a useful target in cancer therapy.
Finally, SOX4 may serve as a biomarker for poor treatment response and outcome in OSCC. In this study, we found that SOX4 expression was significantly associated with recurrence, treatment failure and shorter OS. These results support our results of in vitro study, which associated SOX4 expression with oncogenic HNSCC phenotypes.
Although several studies have associated SOX4 expression with shorter survival in prostate cancer, gastric cancer, and colon cancer [7,9,10], this is the first to demonstrate the correlation between SOX4 expression and treatment failure in OSCC. More accurate prediction of treatment failure would facilitate earlier recurrence detection and maximize the therapeutic effects of salvage treatment. In particular, among patients with OSCC who received chemotherapy and/or radiotherapy, those with high SOX4 expression had significantly shorter OS. These findings indicate that SOX4-related chemoradioresistance has a pessimistic effect on survival in patients with OSCC.

Conclusions
Taken together, SOX4 may contribute to invasive and oncogenic phenotypes of HNSCC cells by promoting cell survival and causing chemoradioresistance. SOX4 may be a prognostic marker for OSCC survival outcomes and treatment response.