https://orcid.org/0000-0001-9368-3397
Abstract
Introduction
Laryngeal squamous cell carcinoma (LSCC) is the most common histological subtype of laryngeal cancer. The involved molecular mechanisms and suitable therapeutic targets for LSCC still need to be further investigated. Checkpoint kinase 2 (CHK2) participates in several cellular physiology pathways and plays a role in tumor progression. However, the roles of CHK2 in LSCC remain unclear.
Methods
mRNA expression data were obtained from The Cancer Genome Atlas (TCGA) database, and bioinformatic analysis was performed. Western blot and immunohistochemical analyses were conducted to detect protein expression. MTS assays were performed to examine cell growth of LSCC-derived cell lines.
Results
In the present study, we found that both active form of CHK2 and total CHK2 protein expressions were up-regulated in LSCC tissues. Positive expression of CHK2 was closely associated with advanced clinical features and poor prognosis. Moreover, potential CHK2-involving bioprocesses and signaling pathways were analyzed. In addition, repressed proliferation of LSCC cells was induced by CHK2 inhibitor.
Discussion
Taken together, our findings elucidated that CHK2 may act as an oncogenic factor in LSCC, suggesting a potential target for clinical treatment.
Introduction
Laryngeal cancer is one of the most common malignant tumors of the head and neck region. The most common histological subtype of laryngeal cancer is referred to as laryngeal squamous cell carcinoma (LSCC).Citation1 It was estimated that 177,422 new cases were diagnosed, with approximately 94,771 patients dying from laryngeal cancer in 2018.Citation2 Although surgery is an integral part of treatment for localized laryngeal cancer, nonsurgical options like radiation and systemic therapy have emerged as viable options.Citation3 There are several risk factors implicated in the pathogenesis of laryngeal cancer, including tobacco smoking,Citation4 alcohol consumption,Citation5 dietary factors,Citation6 and human papillomavirus (HPV) infections,Citation7 but the involved molecular mechanisms and suitable therapeutic targets still need further investigation.
In humans, checkpoint kinase 2 (CHK2), which is encoded by CHEK2, is a serine/threonine kinase of 543 residues and participates in series of signaling networks. CHK2 plays multiple roles in nuclear DNA damage repair (DDR). DNA double-strand breaks induce the activation of ATM serine/threonine kinase, which subsequently phosphorylates CHK2 on T68 and results in dimerization and activation of CHK2.Citation8 As a serine/threonine kinase, activated CHK2 phosphorylates its substrates, including BRCA1, E2F1, p53, CDC25A, and CDC25C, to induce the appropriate cellular response.Citation9 In addition, CHK2 mediates stabilization of the FOXM1 transcription factor to stimulate expression of DNA repair genes.Citation10 Besides DDR, CHK2 is also engaged in DNA structure modification and cell cycle progression in normal cellular physiology.
CHK2 also plays a part in tumor progression. CHK2 can prevent tumor progression by averting genomic instability through DNA repair and, if this is not possible, by causing the cell to senesce or die.Citation11 In Hep-2 laryngeal carcinoma cells, down-regulation of Pak4 shows antitumor effects by activation of the ATM/CHK1/2/p53 pathway.Citation12 But, more than a tumor suppressor in the classical sense, increasing evidence supports that CHK2 appears to function like a cancer susceptibility gene.Citation13 For instance, CHK2 is aberrantly and constitutively activated in invasive urinary bladder carcinomas.Citation14 CHK2 overexpresses and mislocalizes within mitotic structures, which enhances chromosomal instability and hepatocellular carcinoma progression.Citation15
The roles of CHK2 in LSCC remain unclear. Previous data showed that the activated CHK2 (T68-phosphorylated CHK2) expression status is a putative indicator of oral cancer risk, and suggested that early therapeutic exploitation of DDR may be of potential benefit in the prevention of oral squamous cell carcinoma, which is another malignant tumor of the head and neck region.Citation16,Citation17 However, a recent study indicated there is no significant relation between CHK2 expression and clinicopathological data or survival in oral squamous cell carcinoma.Citation18 In this research, our data showed that both active form of CHK2 and total CHK2 protein expressions were higher in LSCC tissues than in matched adjacent nontumor tissues. Further, positive expression of CHK2 was closely associated with advanced clinical features and poor prognosis. Moreover, potential CHK2-involving bioprocesses and signaling pathways were analyzed from The Cancer Genome Atlas (TCGA) database. In addition, repressed proliferation of LSCC cells was induced by CHK2 inhibitor. Taken together, our findings elucidated that CHK2 may act as an oncogenic factor in LSCC, suggesting a potential target for clinical treatment.
Materials and Methods
Tissue Samples
This study was approved by the Human Research Ethics Committee of The First Affiliated Hospital of China Medical University. All patients understood the purpose of this research and signed the informed consent. Nineteen pairs of fresh LSCC tissues and matched adjacent nontumor tissues for Western blot analysis were obtained from laryngeal cancer patients who underwent resection surgery in The First Affiliated Hospital of China Medical University in 2017. The tissues were immediately snap-frozen in liquid nitrogen and stored at −80 °C until protein extraction. Another 64 pairs of formalin-fixed, paraffin-embedded sections were obtained from laryngeal cancer patients who had resection surgery in The First Affiliated Hospital of China Medical University from 2007 to 2012, and the patients were followed up till July 2017. All patients were not pretreated before surgery. The clinicopathological data are listed in .
Table 1 The Clinicopathological Parameters of Patients
Cell Culture
Two human LSCC lines (Hep-2 and Tu212) were obtained from the Cell Bank of the Chinese Academy of Sciences (Shanghai, China). Cells were maintained in Dulbecco’s modified Eagle’s medium (DMEM; Gibco) containing 10% fetal bovine serum (FBS; Gibco) at 37 °C with 5% CO2.
Inhibitor and siRNA
BML-277 was purchased from Selleck (S8632), dissolved in dimethyl sulfoxide (DMSO), and stored at −80 °C in small aliquots. siRNAs were obtained from Sigma, and were transfected by jet-PRIME reagent (Polyplus) following the manufacturer’s instructions. The sequence of CHK2-siRNA is 5′-CCUGUGGAGAGGUAAAGCU-3′ and of control-siRNA is 5′-UUCUCCGAACGUGUCACGU-3′.
Western Blot Analysis
Tissue proteins were prepared by extraction with RIPA lysate. Protein concentration was determined with the BCA protein assay kit, and approximately 25 μg of total protein was loaded. GAPDH was used as internal control. Goat anti-mouse/rabbit IgG (HRP) was obtained from Bethyl Laboratories. Antibodies against CHK2 (#6334, 1:1000 dilution) and T68-phosphorylated CHK2 (#2197, 1:1000 dilution) were obtained from Cell Signaling Technology. Antibody against GAPDH was obtained from KangChen Bio-tech Inc.
Immunohistochemical (IHC) Analysis
The IHC experiment was performed with the following procedures. Tissue sections were dewaxed, rehydrated, eliminated of endogenous peroxidase activity, and boiled for antigen retrieval, followed by incubation with indicated CHK2 antibody (#6334, Cell Signaling Technology, IHC antibody validation, 1:400 dilution) overnight at 4 °C. The sections were then incubated with streptavidin-peroxidase-conjugated secondary antibodies. The signals were visualized with diaminobenzidine and the nuclei were counterstained with hematoxylin (ZSGB-bio).
CHK2 expression was scored as follows: 0, negative; 1, weak; 2, moderate; and 3, strong. The frequency of positive cells was defined as follows: 0, 0%; 1, less than 25%; 2, 26% to 50%; 3, 51% to 75%; and 4, greater than 75%. The final score, which is valued between 0 and 12, was determined by multiplying the staining intensity score by the positive cell frequency score.
RNA Expression Profiles and Bioinformatic Analysis
The mRNA expression data of CHEK2 in 519 head and neck squamous cell carcinoma (HNSC) cancer samples and 44 normal samples were obtained from TCGA database using Gene Expression Profiling Interactive Analysis (GEPIA).Citation19 A subset of 499 patients with survival data was analyzed by Kaplan–Meier analysis. Correlated genes of CHEK2 in RNA expression profiles of HNSC cancer samples and 184 esophageal carcinoma (ESCA) cancer samples were obtained from TCGA database by LinkedOmics.Citation20 With thresholds of statistical correlation (+0.5 and −0.4 in HNSC, +0.5 and −0.35 in ESCA), we screened the top correlated genes of CHEK2. Based on the overlap of correlated genes in both HNSC and ESCA samples, Gene Ontology (GO) and Kyoto Encyclopedia of Genes and Genomes (KEGG) pathway analyses were conducted via Metascape.Citation21
MTS Assay
Cells (5x103 cells/well) were seeded into 96-well plates and cultured overnight. Then, cells were transfected with siRNA or treated with different concentrations of CHK2 inhibitor for indicated times. Cell viability was determined using the CellTiter 96 aqueous one solution cell proliferation assay (Promega).
Statistical Analysis
Statistical analysis was performed using SPSS 17.0 software. The differences between groups were assessed by Student’s t-test. The survival rates were evaluated by the Kaplan–Meier method and tested by the log-rank test. For IHC, the chi-square test was used to determine the significant difference between immunohistochemical expression of CHK2 and clinicopathological features. P<0.05 was regarded as statistically significant.
Results
CHK2 Expression Is Increased in Human LSCC
First, a publicly available cohort of HNSC from TCGA database was used to validate CHEK2 expression levels. Compared with normal tissues, we found a significant increased mRNA expression of CHEK2 in HNSC tissues (). We then explored the active form of CHK2 protein (T68-phosphorylated CHK2, hereafter abbreviated as p-CHK2) and total CHK2 protein expressions in 19 pairs of LSCC tissues and matched adjacent nontumor tissues by Western blot analysis (). The protein expressions relative to GAPDH showed that p-CHK2 expression in 18 LSCC tissues (94.7%, except sample 9) and CHK2 expression in 14 LSCC tissues (73.7%, except sample 9, 10, 11, 14, and 19) were significantly increased, compared with that in the matched adjacent noncancerous tissues (P<0.05, ), indicating both p-CHK2 and CHK2 levels were up-regulated in LSCC. These data suggested that CHK2 was overexpressed in HNSC and LSCC tissues.
Figure 1 CHK2 is overexpressed in LSCC. (A) The mRNA expression of CHEK2 in HNSC tissues and control normal tissues in TCGA database. *P<0.05. (B) Western blot analysis for CHK2 expression in 19 paired LSCC tissues and matched adjacent nontumor tissues. N, adjacent nontumor tissues; Ca, LSCC tissues. GAPDH was used as the loading control. (C) Data from (B) were quantified by densitometry, with GAPDH as the reference. Student’s t-test was used for statistical significance. Gray lines indicate the samples with higher expression of p-CHK2 or CHK2 in cancer tissues, and black lines indicate the samples with lower expression of CHK2 in cancer tissues. *P<0.05.
The Clinical Relevance of CHK2 in LSCC
We further detected the expression of CHK2 in 64 pairs of LSCC tissues and matched adjacent nontumor tissues by the IHC method. Nuclear staining of CHK2 was detected in cells (). In accordance with the results shown in , positive expression of CHK2 was found in 49 (76.6%) LSCC tissues, but only 19 (29.7%) adjacent nontumor tissues were shown with positive expression of CHK2 (). Moreover, the expression of CHK2 in different clinicopathological features of LSCC was evaluated. Although no significant association between CHK2 expression and age (P=1), gender (P=0.1142) or clinical stage (P=1) was observed, a higher rate of positive-CHK2 expression was significantly associated with positive lymph-node metastasis (P=0.0363) and poor differentiation (P=0.0343) ().
Table 2 Relation Between the Clinicopathological Features and CHK2 Expression in LSCC
Figure 2 CHK2 expression is associated with poor prognosis in LSCC patients. (A) Representative images of CHK2 expression in LSCC tissues and adjacent noncancerous tissues. NE, normal epithelium; BC, basal cells; LSCC, laryngeal squamous cell carcinoma. Scale bar, 200 µm. (B) Kaplan–Meier curve analysis of differential expression of CHK2 mRNA for the overall survival in HNSC patients. FPKM cutoff of 2.11 was chosen to define high expression or low expression of CHK2. (C) Kaplan–Meier curve analysis of differential expression of CHK2 for the overall survival in LSCC patients.
In addition, Kaplan–Meier analysis showed that high CHK2 expression was associated with poor overall survival rate in HNSC patients (P=0.038, ). In our cohort of 64 cases, positive expression of CHK2 in LSCC patients also contributed to bad prognosis, although there was no statistical difference (P=0.113, ). Taken together, these data suggested positive CHK2 expression may have an association with lymph-node metastasis, poor differentiation, and poor prognosis in LSCC patients.
Analysis of Potential CHK2 Involving Bioprocesses and Signaling Pathways
The same as LSCC, the most common histological subtype of esophageal carcinoma (ESCA) is also referred to as squamous cell carcinoma.Citation22 To reveal the underlying mechanisms of CHK2 function in squamous cell carcinoma, we further analyzed RNA-Sequence data of HNSC and ESCA from TCGA database. We analyzed the genes whose expressions were correlated with CHEK2 by LinkedOmics.Citation20 We then focused on the top correlated genes with CHEK2 using the values of statistical correlation as cutoffs. There were 121 positively-correlated genes and 297 negatively-correlated genes in HNSC, while 105 positively-correlated genes and 184 negatively-correlated genes were found in ESCA (listed in Supplementary Tables S1–S4). Further, there were 37 overlapped positively-correlated genes and 25 overlapped negatively-correlated genes between HNSC and ESCA (listed in Supplementary Tables S5 and S6). GO (BP) and KEGG enrichment analysis of those overlapped genes were revealed by Metascape.Citation21 As shown in , the positively-correlated genes appeared to be involved in cell cycle, DNA conformation, DNA repair, and so on. The negatively-correlated genes were involved in Th17 cell differentiation, cell junction organization, vesicle organization, and so on (). These data suggested that CHK2 may be active in these bioprocesses and signaling pathways in the pathogenesis and development of squamous cell carcinoma.
Figure 3 Functional analysis of genes correlated with CHK2 in squamous cell carcinoma. (A) Significant bioprocesses and pathways represented the functions of genes positively correlated with CHK2. The horizontal axis and the intensity of color represent corrected P-value. The number of enriched genes is shown behind the columns. (B) Significant bioprocesses and pathways represented the functions of genes negatively correlated with CHK2. The horizontal axis and the intensity of color represent corrected P-value. The number of enriched genes is shown behind the columns.
CHK2 Inhibitor BML-277 Reduced LSCC Cell Proliferation
Given that CHK2 plays a role in LSCC development, we then evaluated the effect of CHK2 on cell growth in Tu212 cells. Transient CHK2 knockdown by siRNA was performed, and CHK2 expression was significantly attenuated (). Further, knockdown of CHK2 suppressed the cell growth ability of Tu212 cells, which also suggested an oncogenic potential of CHK2 (). We then sought to investigate the effects of CHK2 inhibitor on LSCC cells. BML-277 is an ATP competitive CHK2 kinase inhibitor, which binds the ATP binding site of CHK2.Citation23 We evaluated the active and inactive forms of CHK2 expression under BML-277 treatment. The results showed that the level of p-CHK2 was decreased under BML-277 treatment, while total CHK2 expression was not obviously changed (), suggesting that BML-277 repressed CHK2 activity. Moreover, we measured cell proliferation by the MTS method. In Tu212 and HEP-2 cells, BML-277 inhibited proliferation of cells in a dose-dependent manner, with maximum suppression observed at 10 μM (). Further, Tu212 and HEP-2 cells were treated with 5 μM BML-277 for different time intervals, and cell viability was inhibited in a time-dependent manner (). These data suggested that CHK2 inhibition had an anti-growth effect on LSCC cells.
Figure 4 CHK2 inhibition represses LSCC cell proliferation. (A) Tu212 cells were separately transfected with siCHK2 or control siRNA (siCtrl). After 48 hours, cells were harvested, and Western blot analysis was performed with the indicated antibodies. GAPDH was used as internal control. (B) Tu212 cells were separately transfected with siCHK2 or siCtrl. Relative cell numbers were determined using MTS assay by absorbance at 490 nm at indicated times. P-value refers to two-sided Student’s t-test. *P<0.05. (C) Tu212 cells were treated with indicated doses of BML-277 or vehicle. After 24 hours, cells were harvested, and Western blot analysis was performed with the indicated antibodies. GAPDH was used as internal control. (D and F) Tu212 cells or HEP-2 cells were treated with indicated doses of BML-277 or DMSO. After 24 hours, relative cell numbers were determined using MTS assay by absorbance at 490 nm. Data are represented as mean±SD from three independent experiments. P-value refers to two-sided Student’s t-test. *P<0.05. (E and G) Tu212 cells or HEP-2 cells were treated with BML-277 (5 μM) or DMSO. Relative cell numbers were determined at various times using MTS assay by absorbance at 490 nm. Data are represented as mean±SD from three independent experiments. P-value refers to two-sided Student’s t-test. *P<0.05.
Discussion
Distinct oncogenic signaling pathways have been associated with LSCC, and finding new molecular markers for early detection and treatment in LSCC progression is worthy and important.Citation24 Here, we report that CHK2, which is a key mediator of the DNA damage checkpoint in DDR, may act as an oncogenic gene and administration of a CHK2 inhibitor shows antitumor function in LSCC. Our data validate the potential therapeutic targeting of CHK2 in LSCC, which provides a basis for further experimental and clinical research.
CHK2 demonstrated both tumor-suppressor functionsCitation25 and the capacity to promote tumor and cell survival. Overexpression, phosphorylation and mislocalization within the mitotic spindle of CHK2 disrupt the sensitive balance of mitotic proteins, which in turn undermines faithful chromosome segregation and contributes to lagging chromosomes during HCC progression.Citation15 In line with those reports, our data found the expression levels of CHK2 protein were up-regulated in LSCC tissues (). Remarkably, significant differences were discovered between positive and negative CHK2 patients within lymph-node metastasis and differentiation (). More importantly, positive expression of CHK2 in LSCC patients may contribute to bad prognosis (). Our data suggested that CHK2 might act as an oncogenic factor in the progression of LSCC; nevertheless, further research studies are required to clarify the functions of CHK2 in vivo.
Using bioprocess and signaling pathway analyses, the biological functions of CHK2 in LSCC were predicted (). These bioprocesses and pathways are known to be involved in both LSCC progression and CHK2 function, for example, cell cycle and DNA repair.Citation9,Citation26,Citation27 But further experimental research is required for better understanding the key mechanisms responsible for the processes.
CHK2 mutations have been detected with high incidence in a subset of cancers, including breast, prostate, ovarian, colorectal, kidney, thyroid, and bladder cancers and leukemias.Citation28 Mice harboring the mutant CHEK2 allele are not only at an elevated risk for the development of cancer but also this risk can be further increased as a result of environmental exposure.Citation29 In LSCC, it is not known whether CHK2 protein is mutated or its mutation rate, which will necessitate further investigation. Also, the phosphorylation status of CHK2 in LSCC is another valuable issue, which will make it necessary to further evaluate.
A previous study illustrated that CHK2 is overexpressed in diffuse large B-cell lymphoma (DLBCL) and addressed the therapeutic efficacy of combining ERK and CHK2 inhibitors in the setting of DLBCL.Citation30 Our data make it possible to consider the role that CHK2 plays in tumorigenesis, which indicates CHK2 may serve as a target of cancer therapy. BML-277 is an ATP-competitive inhibitor of CHK2.Citation23 In our study, inhibition of CHK2 by BML-277 significantly inhibited LSCC cell viabilities in vitro (). These results prove the possible role of CHK2 in tumorigenesis that consequently functions as a therapeutic target in LSCC. Given that the observed growth inhibition by BML-277 in both lines is modest, future research studies evaluating the interaction between BML-277 and chemotherapy or radiation response are required.
Everything considered, our study indicated that CHK2 expression is up-regulated in LSCC, which associates with advanced clinical features and poor prognosis. Further, inhibition of CHK2 could lead to suppression of proliferation in LSCC cells. Our report provides an insight to support a previously unknown role of CHK2 in LSCC progression and suggests a potential role in the treatment of LSCC. The small sample size, as well as the short-term follow-up, may impose some limitations in our study.
Disclosure
The authors report no conflicts of interest in this work.
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