Abstract
Background
Bladder cancer (BLCA) refers to the malignancy growth that spreads from the bladder linings to the bladder muscles. However, the impact of miR-22-3p and lncRNA TRPM2-AS on this tumor has generated divergent views in the literature. This research aimed to study the effects of lncRNA TRPM2-AS on BLCA and its interaction with miR-22-3p and GINS2 mRNA.
Methods
qRT-PCR was employed to measure the expression of TRPM2-AS, miR-22-3p and GINS2 mRNA in bladder tissues and cells. The subcellular localization of TRPM2-AS in T24 and 5637 cell lines was identified using a cell fractionation system. Luciferase assay, RIP assay and RNA pull-down assay were later performed to validate the direct binding relationship between TRPM2-AS, miR-22-3p and GINS2 mRNA. Several experiments were conducted to determine the viability, proliferation, colony formation and apoptosis of the cell lines.
Results
Findings indicated that TRPM2-AS was significantly upregulated in BLCA tissues and cell lines. Apart from that, it was observed that TRPM2-AS knockdown significantly inhibited the viability, proliferation and colony formation of BCLA cells, but it promoted the apoptosis of the BCLA cells. A significant downstream target of TRPM2-AS, miR-22-3p was found to show a lower expression level in BLCA tissues and cell lines. However, the inhibition of miR-22-3p considerably enhanced BLCA cell phenotypes. As well as discovering that GINS2 mRNA was a downstream target of miR-22-3p and was significantly upregulated in BLCA, experimental results also indicated that the knockdown of GINS2 suppressed BLCA cell phenotypes.
Conclusion
This research confirmed that TRPM2-AS could promote BCLA by binding to miR-22-3p to increase GINS2 expression. This novel interactome in BLCA cell lines might provide more insights into BLCA therapy.
Keywords:
Background
Bladder cancer (BLCA) can be described as the malignancy growth that originates from the bladder cells. This cancer is usually associated with males worldwide, and it is ranked ten among all cancer types.Citation1 Although the occurrence and death rate of BLCA is the highest in South Europe, the incidence rate of BLCA in China has skyrocketed in the last 10 years.Citation1,Citation2 Over the years, several clinical methods have been introduced to treat BLCA, such as surgery, chemotherapy and radiation therapy; nonetheless, the survival rate of BLCA patients has not improved with these methods.Citation3,Citation4 To improve the lives of individuals with BLCA, it is imperative that the underlying molecular mechanism of this tumor be properly understood.
Containing more than 200 bp of nucleotides, long non-coding RNA (lncRNA) has been documented to participate actively in cancer development.Citation5–Citation9 The host gene of TRPM2-AS, which belongs to the lncRNA class, consists of three exons. This RNA gene is also located at chromosome 21q22.3 and was first discovered to be upregulated in melanoma in 2008.Citation10 One research discovered TRPM2-AS to be a cancer-promoting gene in several tumors, including reproductive system tumors, digestive system tumors and respiratory system tumors.Citation11–Citation17 Yet, no study has explored the impact of TRPM2-AS on BLCA.
Besides, in the last 10 years, research has demonstrated that small RNAs could participate in the progression of human neoplasms.Citation18 Small RNAs include miRNAs, with a length of 18–29 nucleotides.Citation19,Citation20 Among them, miRNAs play essential roles in cancer progression. While miR-22-3p’s role has been discovered to act as a tumor suppressor in the neoplasms found in the reproductive system, digestive system and respiratory system,Citation21–Citation27 no research has investigated the effect of miR-22-3p in a lncRNA-related interactome complex on BLCA.
Apart from TRPM2-AS and miR-22-3p, GINS2 (GINS complex subunit 2) has been linked to the development of BLCA. Located on chromosome 16q24.1, GINS2 consists of five exons that belong to the GINS complex family.Citation28 The GINS complex is also a member of the DNA replication helicase family, which participates in the initiation of chromosome replication.Citation29,Citation30 Several studies have documented the inability of GINS2 to promote cancer progression.Citation31–Citation39 However, the function of GINS2 in BLCA has not been studied in the literature.
This research aimed to study the regulatory mechanism of TRPM2-AS, miR-22-3p and GINS2 mRNA in BLCA cell lines. It was hypothesized that TRPM2-AS could promote BLCA by binding miR22-3p to increase GINS2 mRNA expression. Our results might provide a better clinical approach to BLCA treatments.
Materials and Methods
Bioinformatic Analysis
Gene Expression Profiling Interactive Analysis (GEPIA), an online gene expression profiling interactive analysis tool, was used to analyze the expression of TRPM2-AS and GINS2 mRNA in bladder tissues with and without BLCA. GSE37815 data, which was downloaded from the GEO database, consisted of the mRNA expression profile of BLCA.
The Encyclopedia of RNA Interactomes (ENCORI) was used to study and predict the miRNAs that could bind to TRPM2-AS. The TargetScan Human v7.2 algorithm was later used to predict the target regulatory miRNAs that could bind to the 3ʹUTR of GINS2 mRNA.
Tissue Samples Collection
A total of 38 BLCA tissues, including their corresponding adjacent tissues, were collected from 38 patients diagnosed with BLCA in the last three years at The First Affiliated Hospital of Zhengzhou University. The clinical tissue samples including 6 non-muscular invasive bladder cancer (NMIBC) and 22 muscular invasive bladder cancer (MIBC) were processed according to the ethical standards set out in the Declaration of Helsinki. Besides, this study was approved by the Ethics Committee of the university, and patients who participated in the study were mandated to sign the informed consent form. The clinical characteristics of participants are summarized in .
Quantitative Real-Time Reverse Transcription-Polymerase Chain Reaction (qRT-PCR)
The total miRNAs were first isolated from the tissues using the miRcute miRNA Isolation Kit (DP501, Tiangen Biochemical, China) according to the manufacturer’s guideline. Next, the reverse-transcription of miR-22-3p was conducted using the miRcute miRNA First-strand cDNA Synthesis Kit (KR211, Tiangen Biochemical, China), while that of TRPM2-AS and GINS2 was carried out with the PrimeScript RT reagent Kit (RR037A, Takara, Japan). After performing reverse-transcription, qRT-PCR was performed with TB Green Premix Ex Taq II (RR820A, Takara, Japan). The 2−ΔΔCt method was subsequently used to calculate the RNA levels. While GAPDH was utilized as the reference gene for TRPM2-AS and GINS2 mRNA, U6 was used as the reference gene for miR-22-3p. All the primers were provided by GeneCopoeia (Guangzhou, China), and their sequences are shown in .
Cell Line Acquisition and Cell Culture
Both cancerous and normal cell lines were used in this study. The human BLCA cell lines (RT4, T24, J82 and 5637) and the normal urothelial epithelial cell line (SV-HUC-1) were all acquired from the Institute of Basic Medical Sciences (IBMS) of the Chinese Academy of Medical Sciences (CAMS). They were cultured in RPMI 1640 media with 10% serum and then incubated at 37°C in an atmosphere containing 5% CO2.
Subcellular Fractionation Location
The cytoplasmic and nuclear RNAs of T24 and 5637 cells were separated using the Invitrogen PARIS Kit (ThermoFisher, AM1921, USA). During the experiment, GAPDH and U2 served as the cytoplasmic control and nuclear control, respectively. The expression levels of TRPM2-AS, GAPDH, and U2 were later measured using qPCR. Each experimental procedure was processed at least three times.
Cell Transfection
Genomics materials were acquired from GeneCopoeia (Guangzhou, China), such as negative control (NC) plasmids, miR-22-3p inhibitor, and small interfering RNAs for TRPM2-AS (si-TRPM2-AS) and GINS2 (si-GINS2). The transfection of these materials into T24 and 5637 cells (plated in 6-well plates, 3x104/mL) was performed for 48 hours using Lipofectamine 2000 Reagent (Cat#: 11,668,027, ThermoFisher, USA).
Cell Viability Assay
Cell viability was detected with the WST-8 kit. First, 4800 transfected T24 and 5637 cells were seeded into 96-well plates. They were then grown for 24, 48, 72 hours. After that, 10μL cell counting kit-8 reagent (MedChemExpress, HY-K0301, China) was added to the cells, and the mixture was incubated for 4 h. The optical absorbance of every well was finally read at 450 nm with a microplate reader.
BrdU Assay
BrdU assay was performed to evaluate the proliferation ability of the cell lines. First, 3×104/mL T24 and 5637 cells were seeded into 96-well plates for 24 h. After that, 10μL BrdU (5-bromo-2ʹ-deoxyuridine, a thymidine analog, Abcam, ab126556, UK) was added to each well for 4 h. Next, a fixing solution was added to each well to denature the cellular DNA. Each well was then aspirated and washed. After that, the anti-BrdU primary antibody (100 μL/well) was added to the wells to allow the mixture to react for 1 h. Each well was aspirated and washed again. After100 μL/well Peroxidase conjugate Goat Anti-Mouse IgG secondary was added, the cell lines were incubated for 0.5 h. Then, 100 µL/well TMB Peroxidase substrate was added to the cells, and the mixture was incubated in the dark for 0.5 h. To further quantify the proliferation, 100 µL of Stop Solution was added to each well. The optical absorbance of each well was then read at 450 nm with a spectrophotometric microtiter plate reader. All procedures were conducted at room temperature, and experiments in each group were repeated at least three times.
Colony Formation Assay
After 48 hours of transfection, the cells were collected and seeded into a 6-well culture plate with a density of 1×103 cells per well. The colony formation was observed after 14 days of culture, and the culture was later terminated when the cells formed visible colonies. After that, the medium was discarded, and the cells were rinsed with phosphate-buffered saline (PBS). Next, 4% paraformaldehyde was added to each well for an incubation period of 15 min. Next, the 0.1% crystal violet dye was added to the cells for an incubation period of 30 min. Finally, the colony formation images were taken with a light microscope (Olympus, Japan).
Flow Cytometry Assay
Flow cytometry was carried out to measure cell death and identify the early and late apoptotic cells. Briefly, 1×105/mL T24 and 5637 cells in every group were rinsed in PBS three times and fixed in cold methanol for 30 min at 4 °C. Subsequently, the cells were suspended in 100 μL 1×binding buffer. PBS was subsequently added to each well to wash the cell for three times. Then, the cells were incubated with 5 μL Annexin V and PI staining solution in the dark for 20 min. After that, the cells were passed through the FACS scan flow cytometer (Cytoflex, Beckman Coulter) in an hour. In this study, both early (Annexin V positive and PI negative populations) and late apoptosis (Annexin V positive and PI positive staining) rates were counted as the apoptosis rate.
Caspase-3 Activation Assay
This assay was conducted to further investigate the apoptosis conditions of the cells in each group. The caspase-3 activation was assessed using a Colorimetric Caspase-3 Assay Kit (Cat#: ab39401, Abcam, UK). First, 1×106 transfected T24 and 5637 cells were suspended in 50 μL cold cell lysis buffer for 10 minutes. The protein concentration was later detected and adjusted to ~150 μg protein/50 μL reaction buffer. Then, 50 μL reaction buffer containing 10 mM DTT and 5 μL 4 mM DEVD-pNA substrate was added to the cell lysates for 1 h. The optical absorbance was finally read at 405 nm with a spectrometer.
Luciferase Reporter Assay
The plasmids containing the wild strains and mutants of TRPM2-AS and GINS2 mRNA, with and without the predicted binding sequences, were constructed by and purchased from GeneCopoeia (China). These plasmids were first transfected into the T24 and 5637 cells using Lipofectamine 2000 Reagent (Cat#: ThermoFisher, 11,668,027, USA). Then, the miR-22-3p mimics or NC were co-transfected into the transfected T24 and 5637 cells using Lipofectamine 2000 Reagent. After 48 h, the cells were gathered and lysed with the lysis buffer. The dual-luciferase reporter assay system (Cat#: LF031, GeneCopoeia, China) was used to analyze the relative luciferase activity.
RNA Immunoprecipitation (RIP)
RIP immunoprecipitation assay was performed using the Magna RIP RNA-Binding Protein Immunoprecipitation Kit (Millipore, 17–700, USA). The BLCA cells were lysed in the RIP lysis buffer that contained magnetic beads conjugated with anti-Argonaute2 (AGO2) or anti-IgG antibodies. After the samples were incubated with Proteinase K, the immunoprecipitated RNA was isolated with TRIzol Reagent (ThermoFisher, 15,596,026, USA). Finally, the enrichment of TRPM2-AS and miR-22-3p was measured using qRT-PCR.
RNA Pull-Down Assay
The T24 and 5637 cells (5×106) were treated on ice for 20 minutes with 0.5 mL of 25 mM Tris-HCl, 0.05% NP-40, 70 mM KCl, 2.5 mM EDTA, 80 U/mL RNase inhibitor, and 1×protease inhibitor cocktail. After centrifugation, the supernatant was collected and incubated with biotin-coupled miR-22-3p (bio-miR-22-3p) or biotin-coupled NC (bio-NC) for 2 hours. The cell lysate containing bio-miR-22-3p or bio-NC was then incubated with streptavidin magnetic beads. After 4 h, the beads were washed with reaction buffer to isolate the bound RNAs in the pull-down complex. The expression of pull-down RNA was finally detected using qRT-PCR.
Western Blot Assay
The protein of cells was extracted using RIPA Lysis Buffer that contained 5 mM EDTA and PMSF (P0013B, Beyotime, China). Different groups of proteins were quantified using a spectrophotometer so that the proteins were at the same level. Then, 10% SDS-PAGE gel was used to separate 20μg of the total protein in these groups. The total protein was subsequently transferred onto the PVDF membranes (Millipore, MA, USA) with 5.0% evaporated milk at 37 °C for 1 h. Next, the PVDF membranes were incubated with the primary antibodies against GINS2 (1:500, Cat#: ab197123, Abcam, UK), Bcl-2 (1:2000, Cat#: ab182858, Abcam, UK), Bax (1:5000, Cat#: ab32503, Abcam, UK), Cleaved caspase-3 (1:500, Cat#: ab32042, Abcam, UK) and GAPDH (1:5000, Cat#: ab175781, Abcam, UK) at 4°C overnight. After 24 h, the PVDF membranes were washed three times with PBS and then incubated with Goat Anti-Rabbit IgG H&L secondary antibody (1:5000, Cat#: ab205718, Abcam, UK) at room temperature for 1 h. The ECL Substrate Kit (Cat#: ab133406, Abcam, UK) was subsequently used to strengthen the band signals. FluorChem FC2 software (Media Cybernetics, Inc., Rockville, MD, USA) was used to read the intensities of the protein bands.
Statistical Analyses
The data collected from at least three independent results of every experiment were analyzed using the Graphpad Prism v7.0 software. Data were presented as mean ± SD (standard deviation). The Wilcoxon test method was used to identify the significant differences between two groups, while the one-way ANOVA with the Dunnett’s test was used to identify the significant differences among multiple groups. P-values of less than 0.05 were considered statistically significant.
Results
Identification of Genes of Interest
After interrogating GEPIA database with log2FC >1.5 and adjusted P-value <0.01, findings indicated that lncRNA TRPM2-AS was significantly upregulated (log2FC=1.892, adjusted P-value=1.64×10−6) in BLCA (). This result means that TRPM2-AS was positively associated with BLCA progression. Interestingly, TRPM2-AS has been proved to be a tumor promoter in colon cancer,Citation13 gastric cancer,Citation12 breast cancer,Citation14 and lung cancerCitation17 by interacting with miRNAs; however, it has never been studied in BLCA. The GSE37815 data were also analyzed from the GEO database, and it was found that GINS2 was among the top 5 most differentially expressed genes (DEGs) with log2FC=1.99 and adjusted P value=0.00462 (). Like TRPM2-AS, GINS2 was considered to be a significant tumor promoter in thyroid cancerCitation32 lung cancer,Citation33 cervical cancer,Citation40 ovarian cancer,Citation38 breast cancer,Citation34 triple-negative breast cancer,Citation35 and leukemia.Citation39 Based on these findings, it was hypothesized in this study that GINS2 might be a tumor promoter in BLCA as well. and shows the relative expression of TRPM2-AS and GINS2 in BLCA tissues and healthy tissues. Both TRPM2-AS and GINS2 were found to be significantly upregulated in BLCA tissues. Apart from that, GINS2 was discovered to be upregulated in BLCA tissues based on the TCGA samples (). The predicted targets of TRPM2-AS from ENCORI starbase and those of GINS2 from TargetScan Human 7.2 were intersected to identify the potential bridge miRNA between TRPM2-AS and GINS2 (). Among the top 5 out of the total 13 common miRNAs, miR-22-3p was considered to suppress BLCA.Citation41
Effects of TRPM2-AS on BLCA Cells
The expression of TRPM2-AS in BLCA tissues collected from participants was first detected to explore the impact of TRPM2-AS on BLCA. The results showed that TRPM2-AS expression increased by 3.6-fold in BLCA tissues compared with normal adjacent tissues (). Furthermore, BLCA tissues were divided into two groups according to the median: the high-expression TRPM2-AS group (N = 19) and the low-expression TRPM2-AS group (N = 19). The data analysis showed that the expression of TRPM2-AS was related to the tumor diameter, histological grade, TNM stage, T stage, N stage, M stage, and lymphatic metastasis (). Similar to BLCA tissues, TRPM2-AS expression was observed to be higher in four BLCA cell lines (RT4, T24, J82 and 5637) than in the normal urothelial epithelial cell line (SV-HUC-1) (). Due to the highest expression of TRPM2-AS in T24 and 5637 cell lines, the T24 and 5637 cell lines were chosen to conduct our study in depth. Then, the subcellular fractionation location assay was employed to observe the TRPM2-AS location in T24 and 5637 cell lines. The results showed that TRPM2-AS was mainly located in the cytoplasm (). The results of the si-TRPM2-AS, which were used to transfect T24 and 5637 cells, indicated that si-TRPM2-AS decreased TRPM2-AS expression in T24 and 5637 cells by 70% compared with the blank group (). The outcomes of the CCK-8 and BrdU assays revealed that cell viability and cell proliferation were suppressed in the si-TRPM2-AS group compared with the blank groups ( and ). Furthermore, the colony-formation assay results showed that the number of colonies decreased by approximately 50% in the cells transfected with si-TRPM2-AS (). Flow cytometry and caspase-3 assay were then employed to observe the effect of si-TRPM2-AS on cell apoptosis in two BLCA cell lines. The flow cytometry assay results demonstrated that the apoptosis rate in the si-TRPM2-AS group rose by approximately 2-fold in the two BLCA cell lines compared with the blank groups (). Besides, the caspase-3 activity in the si-TRPM2-AS group grew by approximately 3-fold in the two BLCA cell lines (). The Western blot assay was used to detect the effect of TRM2-AS downregulation on apoptosis-related proteins in BLCA cells, and the results of this assay showed that compared with the blank group, the protein expression of Bax, cleaved caspase-3 increased in T24 and 5637 cells, while that of Bcl-2 decreased. This outcome further indicated that TRM2-AS knockdown promoted the apoptosis of BLCA cells ().
miR-22-3p: Downstream Target of TRPM2-AS
The binding site between TRPM2-AS and miR-22-3p was discovered after analyzing data with ENCORI starBase (). The results of the luciferase reporter assay demonstrated that the fluorescence intensity decreased by half after co-transfecting TRPM2-AS-wild type and miR-22-3p mimics; however, other groups had no differences in T24 and 5637 cell lines (). After performing the RIP assay, it was discovered that the expression of TRPM2-AS increased by 4.6-fold and 5.1-fold in T24 and 5637 cells, respectively. Put simply, this result confirmed that TRPM2-AS could combine with miR-22-3p (). It was also found that miR-22-3p expression decreased by 65.7% in BLCA tissues compared with normal adjacent tissues () and that TRPM2-AS was negatively associated with miR-22-3p (). The qRT-PCR outcome even showed a more than 50% decrease in miR-22-3p expression in T24 and 5637 cells compared with SV-HUC-1 cells (). Experimental results also showed that si-TRPM2-AS increased miR-22-3p expression by more than 1.5-fold in T24 and 5637 cells ().
Interactions of TRPM2-AS and miR-22-3p on BLCA
Several experiments were performed to explore whether TRPM2-AS could regulate BLCA cells’ malignancy phenotypes by regulating miR-22-3p. Before performing experiments, the transfection efficiency of TRPM2-AS siRNA and the miR-22p-3p inhibitor was confirmed using qPCR (). The CCK-8 assay results displayed that the miR-22-3p inhibitor enhanced cell viability, while si-TRPM2-AS weakened it. When the BLCA cells were co-transfected with the miR-22-3p inhibitor and si-TRPM2-AS, no significant differences in terms of cell viability were observed from the blank group (). The results of the BrdU assay showed that the proliferation ability of the cells in the miR-22-3p inhibitor group increased by nearly 1.5 times, while the proliferation ability of the cells in the co-transfection group was similar to that of the blank group (). Moreover, the colony formation assay results showed that while the miR-22-3p inhibitor increased the number of colonies, the si-TRPM2-AS decreased it. When the miR-22-3p inhibitor and si-TRPM2-AS were co-transfected with BLCA cells, no significant difference was observed in the number of colonies between the co-transfection group and the control group (). As for cell apoptosis, the flow cytometry results revealed that the cell apoptosis rate declined by 60% in the miR-22-3p inhibitor group, while the cell apoptosis rate rose by 2-fold in the si-TRPM2-AS group in T24 and 5637 cell lines. Equally important, the cell apoptosis rate in the co-transfection group was found to be the same as that in blank group (). The caspase-3 assay was employed to further study the effects of loss-of-function of TRPM2-AS and miR-22-3p, and the results showed that the miR-22-3p inhibitor decreased caspase-3 activities by 40% but that si-TRPM2-AS increased the caspase-3 activity in T24 and 5637 cells by 3-fold. When miR-22-3p inhibitor and si-TRPM2-AS were co-transfected into the T24 and 5637 cells, no significant difference was observed between the co-transfection group and the blank group (). The results of the Western blot assay showed that the protein levels of Bax and cleaved caspase-3 decreased in the miR-22-3p inhibitor group, while the Bcl-2 protein level increased in the miR-22-3p inhibitor group. However, the protein levels of the co-transfected group were similar to those of the blank group ().
GINS2: Downstream Target Gene of miR-22-3p
The complementary sequences of GINS2 mRNA 3ʹUTR and miR-22-3p were obtained following the analysis of TargetScan Human 7.2 (). The dual-luciferase reporter gene assay and RNA pull-down assay were later performed to verify the complementary binding relationship. The fluorescence intensity was discovered to be reduced in the GINS2-wild type and miR-22-3p mimic co-transfection group, while no differences in T24 and 5637 cell lines were observed in other groups (). The outcome of the RNA pull-down assay also suggested that miR-22-3p could interact directly with GINS2 mRNA (). Experimental findings also revealed that GINS2 was significantly upregulated in BLCA tissues compared with normal adjacent tissues (), a result that indicated a negative correlation with miR-22-3p expression (). In addition, the expression of GINS2 mRNA increased by 6.2-fold in T24 cells and 5.7-fold in 5637 cells compared to SV-HUC-1 cells (). At the protein level, GINS2 expression was observed to increase by 1.9-fold in T24 cells and 1.7-fold in 5637 cells compared to SV-HUC-1 (). What’s more, the transfection of miR-22-3p mimic decreased GINS2 expression by 50%, while the transfection of miR-22-3p inhibitor increased GINS2 expression in T24 and 5637 cells by 2-fold ().
Suppressive Effects of GINS2 Silence on BLCA Cells
The miR-22-3p inhibitor and si-GINS2 were transfected into T24 and 5637 cells to explore whether the effects of GINS2 on BLCA cells was regulated by miR-22-3p. The transfection efficiency of miR-22-3p and GINS2 siRNA was confirmed using a qPCR system () and a Western blot system. The Western blot results showed that the miR-22-3p inhibitor elevated the expression of GINS2 protein by 1.5-fold, while the expression of GINS2 protein in the si-GINS2 group was suppressed by approximately 50%, thus indicating that the miR-22-3p inhibitor and si-GINS2 were successfully transfected into both cell lines (). Moreover, the CCK-8 assay results showed that the si-GINS2 weakened the viability abilities of T24 and 5637 cells; the co-transfection with the miR-22-3p inhibitor attenuated the effect of si-GINS2 on cell viability in the two cell lines (). As for the BrdU assay, it was observed that the proliferation ability of T24 and 5637 cells was impaired by 50% in the si-GINS2 group; nonetheless, the proliferation ability of the two BLCA cell lines in the co-transfection group was the same as the blank group (). The results of the colony formation assay showed that the knockdown of GINS2 reduced the number of colonies of T24 and 5637 cells, but the co-transfection of miR-22-3p inhibitor impaired the influence of si-GINS2 on the colony formation of BLCA cell lines (). As for cell apoptosis, the flow cytometry results revealed that the apoptosis rate induced by si-GINS2 was raised by 2.3-fold in T24 cells and 1.7-fold in 5637 cells compared to the blank group; however, the apoptosis rate in the co-transfection group showed no significant differences with the blank group (). Furthermore, The caspase-3 activity in the transfected BLCA cells was observed, and findings revealed that the caspase-3 activity was enhanced by si-GINS2 and but that the caspase-3 activity in the co-transfection group did not show a significant difference with the blank group either (). Western blot assay findings demonstrated that downregulation of GINS2 increased the level of Bax and cleaved caspase-3 and decreased the level of Bcl-2; nonetheless, no significant difference was found in the protein expression level between the co-transfection group and the blank group ().
Discussion
TRPM2-AS was significantly upregulated in BLCA tissues and cells compared with the normal control and was found to be mainly located in the cytoplasm. We found that TRPM2-AS enhanced the viability and proliferation of BLCA cells but impaired the apoptosis of BLCA cells. We also noticed that TRPM2-AS was negatively associated with miR-22-3p. In other words, the expression of miR-22-3p in BLCA tissues and cells was low, thereby acting as a negative regulator of BLCA progression. GINS2, which was validated to be a target gene of miR-22-3p, was found to be upregulated in BLCA tissues and cells and observed to not only promote cell viability and cell proliferation but also inhibit cell apoptosis.
Previous studies have found lncRNA TRPM2-AS to be aberrantly upregulated in a wide spectrum of neoplasms. For instance, in melanoma, TRPM2-AS were over-expressed.Citation10 Its aberrant upregulation led to significant cancer cell phenotypes, and its loss-of-function resulted in reduced cancer phenotypes. Apart from the fact that TRPM2-AS was found to stimulate the progression of prostate cancer, the knockout of TRPM2-AS was documented to induce cell apoptosis by strengthening cell stress and cell cycle arrest.Citation11 Another research reported that TRPM2-AS accelerated the development of gastric cancer and that it had a significant association with invasion depth, lymphatic metastasis, TNM stage and poor 5-year survival rate, at the same time, TRPM2-AS enhanced cell propagation, migration and invasion by inhibiting miR-195 to promote the development of gastric cancer.Citation12 Similarly, TRPM2-AS with higher expression in colorectal cancer cells could strengthen the proliferation ability of colorectal cancer by combining with RNA-binding protein TAF15 and thus stabilizing the TRPM2 mRNA.Citation13 Also reported was the ability of TRPM2-AS to be upregulated in breast cancer and to enhance cell proliferation and weaken cell apoptosis in breast cancer cells by binding with miR-140-3p.Citation14 Besides, TRPM2-AS was upregulated in hepatocellular carcinoma (HCC) tissues than in normal adjacent tissues, and it had a significant correlation with tumor size, differentiation, and the prognosis outcome of HCC patients.Citation16 Our results and those of previous studies produced similar conclusions. In our research, TRPM2-AS was upregulated in BLCA to promote cell viability and cell proliferation and inhibit cell apoptosis. Our study not only identified the significant upregulation of TRPM2-AS in BLCA but also confirmed its promoting effects on BLCA phenotypes. However, we need to collect more clinical data to verify the regulatory association between TRPM2-AS expression and clinical characteristics.
Furthermore, previous studies have investigated the role of miR-22-3p in human neoplasms, including BLCA, and its ability to act as a tumor suppressor. For instance, miR-22-3p was reported to be significantly downregulated in NCI-H446 (a small cell lung cancer cell line); it was also found to enhance cell apoptosis and inhibit cell migration by downregulating WRNIP1.Citation26 Similarly, miR-22-3p was downregulated in HCC, leading to the malignant progression of the carcinoma.Citation27 In another study, miR-22-3p was found to hinder the malignancy phenotypes of BLCA.Citation41 Similar to these findings, we found that miR-22-3p was significantly downregulated in BLCA. Our analysis also revealed that miR-22-3p could inhibit cell viability and cell proliferation but that it could enhance cell apoptosis. After studying the effect of miR-22-3p on BLCA’s cell apoptosis, we detected caspase-3 activities, flow cytometry, and apoptosis-related proteins in BLCA cells. Our study confirmed that miR-22-3p induced apoptosis process. Our finding was similar to that of Zeng et alCitation42, in which the cleaved caspase-3 protein level was reported to be upregulated in T24 and RT4 cell lines after treating miR-22-3p mimic.
Besides, miR-22-3p has been reported to participate in the competitive endogenous RNA (ceRNA) network. For instance, miR-22-3p was reported to be involved in a ceRNA network pathway that included lncRNA NNT-AS1 and YAP1, thus regulating the malignancy phenotypes of NSCLC cells.Citation43 In gastric cancer, miR-22-3p was found to be regulated by lncRNA CTC-497E21.4, thus regulating NET1 expression to suppress the malignant development of gastric cancer.Citation44 By acting through the ceRNA network, LINC00858 suppressed miR-22-3p and thus regulated the down-stream effector (YWHAZ) to strengthen the progression of colorectal cancer.Citation25 We herein validated the regulatory relationship between miR-22-3p and TRPM2-AS and found that the latter promoted BLCA by suppressing the former. Even though the ceRNA network in BLCA involving miR-22-3p has not yet been reported, the present study presented a novel ceRNA network that involved miR-22-3p. We believe this proposal might open a new approach for BLCA therapy.
Furthermore, GINS2 has been preliminarily studied in various human cancers. For instance, GINS2 enhanced cell proliferation and weakened cell apoptosis in thyroid cancer by regulating CITED2 and LOXL2 expression.Citation32 GINS2 was also upregulated in NSCLC (non-small cell lung cancer) tissues and cell lines. Moreover, GINS2 enhanced the propagation, migration, invasion and epithelial–mesenchymal transition (EMT) of NSCLC cells by regulating the phosphorylation of PI3K p85, AKT, MEK and ERK.Citation33 Besides, GINS2 was overexpressed in triple-negative breast cancer (TNBC) cell lines, and it was found to strengthen the aggression of TNBC cells by increasing the level of MMP9.Citation35 What’s more, the GINS2 expression level was found to be higher in cervical cancer tissues and cell lines, and findings revealed that GINS2 could boost cell propagation, migration and invasion.Citation37 In epithelial ovarian cancer, GINS2 with a high level of expression in tissues enhanced cell propagation but mitigated cell cycle arrest in S phase.Citation38 To our knowledge, GINS2 has not yet been studied in BLCA. We herein identified that GINS2 was a validated downstream effector of miR-22-3p. We also discovered in previous studies that GINS2 was an oncogene that promoted the development of BLCA cells, which was consistent with the previous studies on GINS2 in other cancers. In addition to that, we found that the effects of the GINS2 knockdown on BLCA cell phenotypes could be attenuated via miR-22-3p inhibition.
Nonetheless, our study was fraught with several limitations. Even though we verified that the TRPM2-AS/miR-22-3p/GINS2 axis could regulate the viability, proliferation and apoptosis of BLCA cell phenotypes, we did not study the effects of the ceRNA network pathway on BLCA cell aggression phenotypes, such as migration and invasion. Besides, we did not conduct animal models to confirm our experiment results in vitro. Hence, we suggested that future research should investigate the clinical application of our findings. We also recommended that other factors influencing the occurrence and progression of tumors should be explored in future studies to expand the ceRNA network.
Conclusion
Our study suggested that TRPM2-AS was a tumor promoter. More specifically, we found that TRPM2-AS enhanced the progression of BLCA by downregulating miR-22-3p and thus increasing GINS2 expression in vitro. In sum, the TRPM2-AS/miR-22-3p/GINS2 axis could be a potential target of BLCA and might provide invaluable information about BLCA therapy.
Abbreviations
miRNAs, microRNAs; PBS, phosphate-buffered saline; EdU, 5-ethynyl-2′-deoxyuridine; BLCA, bladder cancer; qPCR, quantitative real-time PCR.
Data Sharing Statement
The datasets used during the current study are available from the corresponding author on reasonable request.
Ethics Approval and Consent to Participate
Ethic Committee of The First Affiliated Hospital of Zhengzhou University (Henan, China) approved the study.
Consent for Publication
Informed consent was obtained from all patients.
Disclosure
There is no conflict of interest existed among the authors.
Additional information
Funding
References
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