Resveratrol Enhances Apoptotic and Oxidant Effects of Paclitaxel through TRPM2 Channel Activation in DBTRG Glioblastoma Cells

Öztürk, Yasin; Günaydın, Caner; Yalçın, Fatma; Nazıroğlu, Mustafa; Braidy, Nady

doi:https://doi.org/10.1155/2019/4619865

Oxidative Medicine and Cellular Longevity

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Abstract Introduction Materials and Methods Results Discussion Abbreviations Data Availability Disclosure Conflicts of Interest Authors’ Contributions Acknowledgments References Copyright Related Articles

Research Article | Open Access

Volume 2019 | Article ID 4619865 | https://doi.org/10.1155/2019/4619865

Resveratrol Enhances Apoptotic and Oxidant Effects of Paclitaxel through TRPM2 Channel Activation in DBTRG Glioblastoma Cells

Yasin Öztürk,¹Caner Günaydın,²Fatma Yalçın,³Mustafa Nazıroğlu,^4,5and Nady Braidy⁶

Academic Editor: Pablo Muriel

Received23 Oct 2018

Revised25 Dec 2018

Accepted03 Jan 2019

Published07 Mar 2019

Abstract

Numerous studies have reported a strong association between increased production of reactive oxygen species (ROS) and the pathobiology of several diseases, and cancer in particular. Therefore, manipulation of cellular oxidative stress levels represents an important therapeutic target. Recently, resveratrol (RESV), a naturally occurring phytochemical, has been shown to sensitize several cell lines to the anticancer effects of other chemotherapeutic agents, including paclitaxel (PAX). However, the molecular mechanisms of action of RESV through oxidative sensitive TRPM2 channel activation remain unclear. The aim of this study was to evaluate the effect of combination therapy of RESV and PAX on activation of TRPM2 in DBTRG glioblastoma cells. DBTRG cells were divided into four treatment groups: control, RESV (50 μM), PAX (50 μM), and PAX + RESV for 24 hours. Our data shows that markers for apoptosis, mitochondrial membrane depolarization and mitochondrial function, intracellular steady-state ROS levels, caspase 3 activity, TRPM2 current density, and Ca²⁺ florescence intensity were significantly increased in DBTRG cells following treatment with PAX and RESV, respectively, although cell viability was also decreased by these treatments. These biochemical markers were further increased to favor the anticancer effects of PAX in DBTRG cells in combination with RESV. The PAX and RESV-mediated increase in current density and Ca²⁺ florescence intensity was decreased with a TRPM2 blocker. This suggests that for this combination therapy to have a substantial effect on apoptosis and cell viability, the TRPM2 channel must be stimulated.

1. Introduction

Gliomas are primary solid tumors of the brain and are induced in the brain by glial cell activation. Glioblastoma multiforme (GBM) is the most aggressive, fast-growing glioma that is formed from glial cells which support the viability of neuronal cells within the central nervous system (CNS) [1]. GBM is defined as a grade IV astrocytoma. Even with optimal therapy, the median duration of survival is between 12 and 15 months, and less than 5% of all patients survive for more than 5 years. Without treatment, survival is often limited to less than 3 months [2]. Since surgery, radiotherapy, and chemotherapy are unlikely to lead to a significant increase in remission of GBM tumors, there is a strong need for the use of new innovative treatments with less adverse effects, when first-line therapy was unsuccessful.

Paclitaxel (PAX) is an effective and widely used anticancer drug isolated from the bark and trunk of Pacific yew [3]. PAX is widely used in clinical practice for the treatment of several types of cancer including GBM [4], lung [5], ovary [6], and breast [7]. Mechanistically, PAX is thought to stimulate and enhance tubulin polymerization, leading to G2/M or G1 cell cycle arrest and apoptosis [8]. PAX has also been shown to induce several factors including reactive oxygen species (ROS) production and apoptosis level in cancer cells [9]. Resistance to PAX-induced apoptosis and oxidative stress production has been previously reported in glioblastoma cells [10]. Therefore, the high mortality rate of glioblastoma cancer can be partly attributed to the unknown molecular pathways of PAX resistance. Recently, it was demonstrated that resveratrol (RESV) could sensitize several cancer cell lines to the anticancer effects of other cancer drugs, including paclitaxel [11–15]. It has been suggested by our group and others that since RESV and PAX have differential effects on apoptosis and cell cycle regulation, their combination may have synergistic anticancer activity.

RESV (trans-3,4,5-trihydroxystilbene) is a naturally occurring phytochemical that is abundant in grapes, peanuts, and red wine. Accumulating evidence suggests that RESV can mediate several health benefits including lifespan extension, anti-inflammation, and protection against cardiovascular and neurodegenerative diseases [16, 17]. In addition to the antioxidant role of RESV, prooxidant and non-antioxidant effects of RESV have been previously reported and are dependent on the cellular model used, treatment conditions, and dosage/formulation/time of delivery [18–25]. In addition, the non-antioxidant role of RESV was also reported in patients with nonalcoholic fatty liver disease [26, 27]. Evidence in support of the chemopreventative effect of RESV in a number of cellular and animal models has been convincing. For instance, one study observed excessive ROS production and apoptosis in cancer cells exposed to RESV [28–30]. RESV also induced oxidative DNA damage in the form of DNA strand breaks in the presence of cupric cations [31]. RESV has also been shown to inhibit cancer cell growth when used alone at high concentrations (>50 μM) or in combination with other anticancer drugs [32–42]. RESV promoted ROS production to induce cellular resistance through the p53-CXCR2 pathway in human osteosarcoma and pulmonary cancer cell lines [43]. Since resistance to PAX in the treatment of GBM cells is a major obstacle, combination with natural phytochemicals such as RESV may improve treatment outcomes. However, the molecular mechanisms underlying RESV and PAX-mediated drug resistance remain to be clarified.

Calcium ion (Ca²⁺) is a major intracellular second messenger signaling cation that regulates many physiological functions including cell migration and apoptosis [44]. Transient receptor potential (TRP) melastatin 2 (TRPM2) is a subfamily member of the TRP superfamily with residual ADP-ribose (ADPR) hydrolase activity [45]. In addition to ADPR, TRPM2 is activated in primary and cancer cells by reactive oxygen species [46–52]. In different cancer cells, an increase in [Ca²⁺]i through activation of TRPM2 channels increased the rate of cell migration, presumably tumor invasion [53]. Hence, TRPM2 channels serve as targets of therapeutic agents to limit tumor growth and tumor-induced Ca²⁺ entry in cancer treatments [54]. Moreover, alpha lipoic acid has been shown to attenuate hypoxia-induced apoptosis, inflammation, and mitochondrial oxidative stress via inhibition of the TRPA1 channel in a human glioblastoma cell line [55].

In this study, we report that PAX and RESV increased intracellular steady-state ROS levels and mitochondrial dysfunction culminating in a decline in cell viability and increased cell death via an apoptotic mechanism. To our knowledge, the cytotoxic effects of RESV on PAX-induced oxidative stress and TRPM2 channel activation in DBTRG cells have not been previously investigated. The aim of this study was to evaluate if RESV treatment could increase PAX-induced oxidative damage in DBTRG glioblastoma cells in vitro. We show that glioblastoma cell apoptosis and mitochondrial oxidative stress in these cells can be modulated by treatment with PAX and RESV. Increased TRPM2 channel activation in these cells may represent an important mechanism for modulating GBM cell death.

2. Materials and Methods

2.1. Cell Culture

The DBTRG cell line was purchased from Şap Institute, Ministry of Agriculture and Forestry (Ankara, Turkey). These cells were cultured in DMEM medium (Invitrogen, Istanbul, Turkey) added with 10% fetal bovine serum (Gibco, Istanbul, Turkey), 1% antibiotic combination (penicillin-streptomycin) (Sigma-Aldrich, Istanbul, Turkey), and 100 μg/ml sodium pyruvate (Sigma-Aldrich, Istanbul, Turkey) at 37°C in a 5% CO₂ incubator (HF90, Heal Force Bio-meditech Holdings Limited, Shanghai, China). Before starting the treatments, the cells were examined within 24 hours after plating onto the coverslips. The cells were counted by using an automatic cell counter (CASY Model TT, Roche, Germany). Cells were seeded in 3-6 flasks at a density of cells per flask (filter cap, sterile, 250 ml, 75 cm²). All cells were cultured at 37°C.

2.2. Groups

ADP, cumene hydroperoxide (CPx), N-(p-amylcinnamoyl)anthranilic acid (ACA), PAX, and RESV were purchased from Santa Cruz Inc. (Istanbul, Turkey).

The DBTRG cells were divided into four groups as follows: (1) control group which were not incubated with ADPR, cumene hydroperoxide (CPx), ACA, PAX, and RESV but were kept in a flask containing the same cell culture medium and conditions for 24 hours; (2) PAX group in which cells were kept 24 hours in the same culture conditions without treatment and then incubated with PAX (50 μM) for 24 hours [56]; (3) RESV group in which cells were incubated for 24 hours in the same culture condition without treatment and then preincubated with RESV (50 μM) for 24 hours as described in a previous study [57]; and (4) PAX + RESV group in which cells were incubated with PAX (50 μM) and RESV (50 μM) for 24 hours.

2.3. Electrophysiology

Patch-clamp records as whole-cell voltage clamp configuration were obtained from the DBTRG cells at room temperature (°C) (EPC 10 patch-clamp set, HEKA, Lamprecht, Germany). Details of standard intracellular and extracellular buffers were given in previous studies [46, 58]. Na⁺-free solutions were prepared by replacement of 150 mM N-methyl-D-glucamine (NMDG⁺) instead of NaCl. It is well known that the TRPM2 channel is activated by the presence of high intracellular Ca²⁺. Therefore, high intracellular Ca²⁺ concentration (1 μM instead of 100 nM) was used in the patch-clamp experiments. The holding potential of the patch-clamp analyses in the DBTRG was kept as -60 mV. Voltage clamp technique was used in the analyses, and current-voltage (I-V) relationships were obtained from voltage ramps from -150 to +150 mV applied over 200 milliseconds.

In the experiments, TRPM2 was intracellularly gated by ADPR (1 mM) (in a patch pipette), and the channels were extracellularly blocked by ACA (25 μM). The maximal current amplitudes (pA) in a DBTRG were divided by the cell capacitance (pF), a measure of the cell surface. Values of current density were expressed as pA/pF in the patch-clamp experiments.

2.4. Intracellular Ca²⁺ Fluorescence Intensity Measurement through TRPM2 Activation

Intracellular changes in the Ca²⁺ florescence intensity concentration in the DBTRG cell were monitored using 1 μM florescent dye (Fluo3, Calbiochem, Darmstadt, Germany). The cells were treated with the TRPM2 antagonist ACA (25 μM) to inhibit Ca²⁺ entry before stimulation with the TRPM2 channel agonist CPx (1 mM). The cells were analyzed by a laser confocal microscope (LSM 800, Zeiss, Ankara, Turkey) fitted with a 40x oil objective. The results of Fluo3 in 15 μm² of cytosol were indicated as the mean fluorescence intensity as arbitrary unit per cell.

2.5. MTT Assay of Cell Viability

Cell viability was assayed using the 3-(4,5-dimethylthiazol-2yl)-2,5-diphenyltetrazolium bromide colorimetric (MTT) colorimetric assay [59]. Briefly, the culture medium was removed from the cells by washing with 1x PBS, and 100 μl DMEM medium containing 0.5 mg/ml MTT was added. The cells were then incubated for another 4 h. Finally, absorbance values were detected at 490 nm by a microplate reader (Infinite Pro 200; Tecan Austria GmbH, Groedig, Austria) and the ratio of suppression by the DTX and RESV treatments on cell viability was calculated. We performed a total of 6 experiments () for the cell viability assay. The data are presented as fold increase normalized to control.

2.6. Extracellular LDH Activity as a Measurement for Cytotoxicity

The release of lactate dehydrogenase (LDH) into the culture supernatant correlates with the amount of cell death and membrane damage, providing an accurate measure of cellular toxicity. LDH activity was assayed using a standard spectrophotometric technique described by Koh and Choi [60].

2.7. Assay of Apoptosis Level and Caspase 3 and 9 Activities

For determining spectrophotometric (UV-1800, Shimadzu, Kyoto, Japan) analysis apoptosis, we used the Cell APOPercentage Apoptosis kit purchased from Biocolor Ltd. (Northern Ireland) [59]. Briefly, the assay used a dye that is selectively imported by cells that are undergoing apoptosis. Necrotic cells cannot retain the dye and therefore are not stained. The dye that accumulates in 30 minutes within labeled cells is released into solution and the concentration of released intracellular dye measured at 550 nm (or blue-green filter) by a microplate colorimeter (Infinite Pro 200).

The determination of caspase 3 and 9 activities was based on a method previously reported with minor modifications [61]. Caspase 3 (N-acetyl-Asp-Glu-Val-Asp-7-amido-4-methylcoumarin) and 9 (N-acetyl-Leu-Glu- His-Asp-7-amino-4-methylcoumarin) substrates were purchased from Bachem (Bubendorf, Switzerland), and cleavage of the substrates was measured with the microplate reader (Infinite Pro 200) ( and ). The data were calculated as fluorescence units/mg protein and presented as fold increase over the pretreatment level. We performed a total of 6 experiments () for the caspase and apoptosis analyses.

2.8. Measurement of Mitochondrial Membrane Potential (ΔΨm)

5,5,6,6-Tetrachloro-1,1,3,3-tetraethylbenzimidazolylcarbocyanine iodide (JC1) accumulates in mitochondria according to the ΔΨm level and is present either as monomer or as reversible J-aggregate. The JC1 monomer predominating in depolarized mitochondria emits green fluorescence at 530 nm, whereas the oligomer (J-aggregate) forming in mitochondria with negative potentials emits red fluorescence at 590 nm [62]. The mitochondrial membrane potential was assayed using the fluorescent probe JC1 according to the manufacturer’s instruction (Thermo Fisher, Istanbul, Turkey). Briefly, cells were cultured in 96-well plates. After being treated with PAX and RESV, the cells were cultured in the cell culture medium containing the JC1 probe at 37°C for 25 min, then centrifuged for 5 min at 300 at 4°C. The cells were incubated with the JC1 staining buffer for two minutes. Finally, the green fluorescent intensities (JC1 monomer, , ) and red signal (JC1 aggregate, , ) were analyzed, respectively, using the microplate reader (Infinite Pro 200). The ratio of red to green fluorescence intensity is a measure of the mitochondrial membrane potential. The data are presented as fold increase normalized to control.

2.9. XF24 Microplate-Based Respirometry

To determine the effect of PAX and RESV on oxygen consumption rates (OCRs; as indicator of mitochondrial respiration) in DBTRG cells, the Seahorse XF24 extracellular flux analyzer (Seahorse Bioscience, North Billerica, MA, USA) was employed as previously described. Briefly, culture plates were incubated in a CO₂-free incubator at 37°C for 1 hr to equilibrate for temperature and pH. The microplate was then loaded into the XF24 and further incubated for 15 min by a 3 min mix and 2 min wait cycles before commencement of the assay. The XF assay was performed as previously described [63]. After determination of the basal respiration in the cell culture, oligomycin (2 μM), carbonyl cyanide-p-trifluoromethoxyphenylhydrazone (FCCP, 500 nM), and antimycin (3 μM) were sequentially added and the oxygen consumption rates (OCRs) for each culture well were quantified for 2 minutes. This allowed us to determine the basal control ratio (BCR, i.e., basal/maximum respiration) and the uncoupling ratio (UCR, i.e., mitochondrial functional integrity) [64]. Essentially, the BCR is a measurement of how close the basal level of respiration is to the maximum level of respiration (i.e., basal/maximum).

2.10. Detection of Intracellular Steady-State Reactive Oxygen Species (ROS) Using the DCFH-DA and o- and m-Tyrosine Assays

2,7-Dichlorofluorescin diacetate (DCFH-DA) is a cell-permeable ROS-specific nonfluorescent probe. The DCFH-DA is hydrolysed intracellularly, and later it is oxidized by ROS into 2-7dichlorofluorescein. Intracellular steady-state ROS levels were detected using the DCFH-DA assay (Sigma-Aldrich, Istanbul, Turkey). The cells were treated PAX and RESV for 24 h. After washing the cells, they were incubated with DCFH-DA (10 μM) for 25 min at 37°C in the dark. The cells were washed again and analyzed (, ) using the microplate reader (Infinite Pro 200). The data were presented as fold increase normalized to control.

We also measured o- and m-tyrosine as previously described [65]. Briefly, phenylalanine (313 pmol and 50 nmol) and o- and m-tyrosine (313 fmol to 50 pmol) were used as calibration standards. Labeled [¹³C₆]-phenylalanine was used as an internal standard. Each standard and sample (1 μl) was injected into the GC/MS using a pressure pulsed splitless loading 6890 N gas chromatograph interfaced to a 5973 mass selective detector (Agilent technologies), with methane as the ECNI reagent gas. o- and m-Tyrosine levels were expressed relative to phenylalanine levels.

2.11. Bradford Protein Assay for the Quantification of Total Protein

Enzyme assays were adjusted for variations in cell number using the Bradford protein assay described by Bradford [66].

2.12. Statistical Analyses

The results were presented as deviation (SD). Statistical differences between the mean values for individual groups were assessed using Fisher’s least significant difference (LSD) test in the SPSS program 18.0 (IBM, New York, NY, USA). Statistical significances were determined using a nonparametric test (Mann-Whitney test), and was accepted as significant.

3. Results

3.1. Effects of PAX and RESV on TRPM2 Currents in DBTRG Cells

Results of current density reported as pA/pF in the patch-clamp records are shown in Figure 1. There were no significant currents in the absence of the TRPM2 agonists and antagonists (ADPR and ACA) (Figure 1(a)). The TRPM2 channel in the patch-clamp experiments was gated in the cells by intracellular ADPR, although they were reversibly blocked by ACA and NMDG⁺ (replacement of Na⁺). As expected, the current densities in the DBTRG cells were increased to about 150 pA/pF in the Ctr + ADPR group compared with the Ctr group (5 pA/pF) alone (). However, the current density of TRPM2 was 6-fold () lower in the Ctr + ADPR + ACA group compared to the Ctr + ADPR group (Figure 1(b)). We observed a 10-fold increase in the current densities in DBTRG cells in the PAX + ADPR group compared to the Ctrl + ADPR + ACA group (Figure 1(c)). The TRPM2 currents increased by 1.6-fold in the PAX + RESV + ADPR group as compared to the PAX + ADPR group (Figures 1(d) and 1(e)). These results clearly indicate that PAX induces Ca²⁺ influx through TRPM2 activation. In addition, PAX-induced TRPM2 currents through ROS production were further increased by treatment with RESV.

(a)

(b)

(c)

(d)

(e)

Figure 1

Effect of resveratrol (RESV and 50 μM for 24 hours) and paclitaxel (PAX and 50 μM for 24 hours) incubations on the TRPM2 current densities (pA/pF) in the DBTRG cells ( and ). The TRPM2 currents in the cells were induced by intracellular ADPR (1 mM in patch pipette), but they were blocked by extracellular ACA (25 μM) in the patch-chamber. W.C.: whole cell. (a) Control (Ctr): original recordings from Ctr cell (without ADPR stimulation). (b) Ctr + ADPR group (with ADPR stimulation but not PAX and RESV treatments). (c) Ctr + ADPR + ACA group (with ADPR stimulation and PAX treatment but not RESV treatment). (d) PAX + ADPR group (with ADPR stimulation and PAX plus RESV treatments). (e) Current densities. ( versus control. versus control + ADPR group. versus control + ADPR + ACA group. versus PAX + ADPR group. versus PAX + ADPR + ACA group. versus PAX + RESV + ADPR group).

3.2. Effects of PAX and RESV on Florescence Intensity of Ca²⁺ through TRPM2 Activation in DBTRG Cells

Results of Ca²⁺ florescence intensity in the laser confocal microscopy analyses of four groups are indicated in Figure 2. The Ca²⁺ florescence intensity in the DBTRG cell was 1.3-fold higher in the Ctr + CPx group compared to the Ctr group alone (); however, the Ca²⁺ florescence intensity of TRPM2 was 2-fold () lower in the Ctr + CPx + ACA group compared to the Ctr + CPx group. In addition, the Ca²⁺ florescence intensities were increased in the PAX (4.2- and 3.2-fold), RESV (3.3- and 2.5-fold), PAX + CPx (5- and 3.8-fold), and RESV + CPx (4.3- and 3.3-fold) compared to Ctr and Ctr + CPx groups, respectively (). The Ca²⁺ florescence intensity in the DBTRG cell was further increased in the PAX + RESV group compared to the PAX (2-fold) or RESV (2.5-fold) group (); however, the Ca²⁺ florescence intensity of TRPM2 was significantly () reduced in the ACA treatment groups (PAX + CPx + ACA, RESV + CPx + ACA, and PAX + RESV + CPx + ACA) compared to the CPx (PAX + CPx, RESV + CPx, and PAX + RESV + CPx) groups. PAX and RESV-mediated Ca²⁺ influx through TRPM2 activation was further confirmed by the results of Ca²⁺ florescence intensity.

(a)

(b)

Figure 2

Effect of resveratrol (RESV and 50 μM for 24 hours) and paclitaxel (PAX and 50 μM for 24 hours) incubations on the Ca²⁺ florescence intensity through TRPM2 activation in the DBTRG cells. The cells were stained with Fluo3 calcium dye, and the of fluorescence in 15 mm² of cell as arbitrary unit are presented; independent experiments. The cells were extracellularly stimulated by cumene hydroperoxide (CPx and 1 mM), but they were extracellularly inhibited by ACA (0.025 mM). The samples were analyzed by a laser confocal microscope fitted with a 40x oil objective. ( versus control (Ctr) group. versus Ctr + CPx. versus Ctr + CPx + ACA group. versus RESV + PAX group. versus RESV + CPx and PAX + CPx groups. versus RESV + CPx + ACA and PAX + CPx + ACA groups. versus PAX + RESV group. versus PAX + RESV + CPx group).

3.3. Apoptosis, Caspase, and Cell Viability (MTT) Results

Compared with control, PAX and RESV treatment increased the levels of apoptosis (1.3- and 1.5-fold) (Figure 3(a)) and extracellular LDH activity (1.8- and 2.1-fold) () (Figure 3(b)), although MTT levels were decreased by the treatments (0.8- and 0.7-fold) (Figure 3(c)). More importantly, we found a significant additive effect on apoptosis (1.3- and 1.2-fold) and MTT levels (0.6- and 0.7-fold) and LDH activities (1.9- and 1.6-fold) in the PAX + RESV combination group compared to PAX and RESV treatment alone (). Our data suggests that PAX-induced apoptosis can be further increased by addition of RESV.

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(b)

(c)

3.4. Caspase 3 and 9 Activities

It is well known that mitochondria-dependent intrinsic apoptosis is mediated by excessive Ca²⁺ influx-induced mitochondrial membrane depolarization, leading to activation of caspase 9 and subsequent activation of caspase 3 [46, 58]. After observing increases in Ca²⁺ influx and apoptosis, we decided to measure the activities of intrinsic apoptosis caspase markers, caspase 3 and 9 (Figure 4). Our data shows that caspase 3 but not caspase 9 activity was markedly () increased by 1.25-fold in the PAX and RESV groups compared to the control group. Caspase 3 activity was further increased by 1.28-fold in the PAX + RESV group compared to PAX and RESV groups alone ().

3.5. Mitochondrial Depolarization (JC1) and Intracellular Steady-State ROS Levels

PAX and RESV increased overloading Ca²⁺ entry through TRPM2 channel activation to promote cancer cell death. It is well known that the overloading Ca²⁺ entry induces mitochondrial dysfunction and intracellular ROS production [67]. Excessive ROS production is known to increase cellular sensitivity in cancer treatment [68]. To investigate whether RESV enhances the effects of PAX on mitochondrial ROS level, we measured the JC1 level and intracellular steady-state ROS levels using a well-established spectrophotometric assay (Infinite Pro 200). We found that the levels of JC1 (Figure 5(a)), DCFH-DA ROS (Figure 5(b)), and o- and m-tyrosine (Figure 5(c)) were significantly () elevated by about 1.5-fold following treatment with PAX and RESV in DBTRG cells. In addition, the levels of JC1 and ROS were further increased by combination treatment of PAX and RESV (). Similarly, we also observed a significant increase in basal control ratio (BCR) and a decline in uncoupling ratio (UCR) in DBTRG cells after a 24 hr incubation with RESV (1.3- and 0.7-fold) and PAX (1.3- and 0.8-fold), and more so in the RESV + PAX group (1.7- and 0.5-fold) using the Seahorse XF24 (Seahorse Bioscience) (Figure 5(d)), consistent with enhanced mitochondrial dysfunction.

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(d)

4. Discussion

Resistance to chemotherapy is an emerging problem for the treatment of GBMs, and identification of alternative adjuvant antitumoral therapeutic agents is necessary for the treatment of cancers [69–73]. In addition to antioxidant roles in normal cells, the prooxidant role of RESV has been previously reported in cancer cells [29]. RESV selectively triggers death in cancer cells and has been previously used for stimulation of apoptosis, mitochondrial oxidative stress, and Ca²⁺ entry in several cancer cell lines [25, 43, 67]. We provide evidence that PAX induced mitochondrial ROS and apoptosis in the DBTRG cells when the TRPM2 channel is activated. We observed that mitochondrial ROS could also activate TRPM2, resulting in increased apoptosis and caspase 3 activation and reduced cell viability. The prooxidant and apoptotic roles of PAX were further enhanced by RESV treatment. This would contribute to cancer cell death by increasing the influx of Ca²⁺ into the cell through TRPM2 channel activation.

TRPM2 channel activation is very sensitive to mitochondrial oxidative stress [44, 45, 59]. PAX induces mitochondrial ROS production which is cytotoxic to some cancer cells. RESV has antioxidant roles in the treatment of various metabolic and cardiovascular disorders. However, recent data indicates that it exhibits prooxidant roles that are likely to be beneficial for the treatment of cancer cells [13, 18, 68]. In the current study, we observed increased levels of TRPM2 current density and Ca²⁺ florescent intensity in the DBTRG cells. More specifically, we observed activation of the TRPM2 channel by PAX and RESV-induced mitochondrial ROS production. To our knowledge, there is no report on RESV, PAX, and TRPM2 channel in DBTRG glioblastoma cells. Similarly, it was previously reported that TRPM2 knockdown significantly enhances gastric cancer cell sensitivity to PAX which validates its therapeutic potential as an anticancer target [54]. These results are consistent with reports on the benefits of targeting TRPM2 in the treatment of neuroblastoma [49, 74–76] and breast cancer cell lines [77]. Contrary to the current results, MPP⁺ treatment increased the level of ROS-mediated TRPM2 activation, and treatment with resveratrol (RSV) attenuated TRPM2-mediated Ca²⁺ influx, reduced intracellular Ca²⁺ overload, and promoted cell survival [78]. These findings suggest that the effects of RESV on TRPM2 may be cell-specific.

The role of the mitochondria in PAX-induced drug resistance is widely related to their major role as a producer of ROS-mediated molecular injury. Increased mitochondrial membrane depolarization, impaired mitochondrial function, and increased ROS production in PAX-induced cell death have been well documented. However, reports on RESV-induced mitochondrial ROS production are conflicting. RESV has been reported to increase mitochondrial membrane dysfunction to induce cell death by increasing the ROS level in cancer cells [79]. A central regulator of mitochondrial biogenesis is a peroxisome proliferator-activated receptor gamma coactivator-1 (PGC-α), and RESV treatment increased mitochondrial membrane depolarization but decreased mitochondrial gene transcript activity and PGC-α expression in lung, breast epithelial, and breast cancer cell lines [68]. Mitochondrial oxidative stress in cancer cells can be induced by PAX [80–82] and RESV, through alterations in mitochondrial membrane depolarization and ATP production, which leads to increased oxidative phosphorylation through the electron transport chain and hence the formation of JC1 and reduced mitochondrial respiration. Thus, activation of apoptosis by PAX and RESV is likely to increase toxic protein aggregates inhibiting cell survival. In the current study, we observed increased levels of apoptosis, mitochondrial membrane depolarization, and ROS values in DBTRG cells exposed to PAX treatment and the effect was further increased in cells cotreated with RESV. Accordingly, the apoptotic and prooxidant roles of RESV have been previously reported in human multiple myeloma cells [83].

Two main pathways of apoptosis are extrinsic and intrinsic apoptosis. Several proteins act in extrinsic apoptosis; for instance, caspase 8 shears and activates downstream apoptosis-inducing proteins including caspase 3 [84]. Caspase 3 acts through both extrinsic and intrinsic apoptosis pathways [85]. In the current study, caspase 3 but not caspase 9 activity was increased by PAX treatment. The effect of PAX treatment on caspase 3 activation was further increased by RESV treatment. Hence, this combination enhanced apoptotic effects in DBTRG cells. Similarly, another study showed that RESV increased the anticancer effects of PAX through upregulation of apoptosis and caspase 3 in non-small cell lung cancer [86] and HepG2 cancer cell lines [12, 87, 88]. Our data shows that PAX and RESV treatment enhances apoptosis in a caspase-9-independent manner. Impaired caspase-9 activation and resistance to anticancer drugs have been previously shown to be independent of the expression of p53, Bcl-2 family proteins, Fas receptor, and Fas ligand and is likely to induce a higher cellular threshold for PAX- and RESV-mediated cell death in DBTRG cells [89]. However, treatment with higher doses may affect this threshold. For example, one study showed that higher doses of cisplatin doses could overcome this threshold, via an alternate, caspase-9-independent apoptotic pathway [89]. These findings are in support for clinical use of high-dose chemotherapy in patients with chemorefractory tumors [89]. However, further understanding of the exact molecular mechanism of action of PAX and RESV on caspase-9 activation is required to overcome chemoresistance in GBMs.

In summary, we observed that mitochondrial ROS and apoptosis produced by PAX and RESV promote activation of TRPM2 in the DBTRG cell line. Therefore, we observed synergic interactions of RESV on PAX-induced apoptosis and oxidative stress through stimulation of the TRPM2 channel. These changes contribute to GBM cell death by increasing the influx of Ca²⁺ into the cell through the channel. If bioavailable forms are made available, RESV is likely to be useful in combination with chemotherapeutic agents such as PAX to improve the therapeutic effect of chemotherapy in DBTRG glioblastoma cancer cells.

Abbreviations

[Ca²⁺]_i:	Intracellular free Ca²⁺
ACA:	N-(p-Amylcinnamoyl)anthranilic acid
ADPR:	ADP-ribose
Ca²⁺:	Calcium ion
DHR 123:	Dihydrorhodamine-123
GBM:	Glioblastoma multiforme
JC1:	5,6,6-Tetrachloro-1,1,3,3-tetraethylbenzimidazolylcarbocyanine iodide
MTT:	3-[4,5-Dimethyl-2-thiazolyl]-2,5-diphenyl-2-tetrazolium bromide
PAX:	Paclitaxel
PGC-α:	Peroxisome proliferator-activated receptor gamma coactivator-1
RESV:	Resveratrol
ROS:	Reactive oxygen species
TRP:	Transient receptor potential
TRPM2:	Transient receptor potential melastatin 2
W.C:	Whole cell.

Data Availability

The data used to support the findings of this study are available from the corresponding author upon request.

Disclosure

The abstract of the study was published in an abstract book of the 7th Oxidative Stress, Calcium Signaling and TRP Channel World Congress, 20-23 April 2018, Alanya, Antalya, Turkey (http://2018.cmos.org.tr).

Conflicts of Interest

The authors declare that there are no conflicts of interest.

Authors’ Contributions

MN and NB formulated the present hypothesis and were responsible for writing the report. Experiments were performed in the 2nd International Brain Research School, 6-12 October 2017, Isparta, Turkey by YÖ, CG, and FY (http://www.cmos.org.tr/brs2017/tr/index.php). The laser confocal microscopy analyses of the manuscript were performed by MN.

Acknowledgments

The study was supported by BSN Health, Analysis and Innovation Ltd. Inc. Teknokent, Isparta, Turkey (Project No.: 2018-03). There is no financial disclosure for the current study. The authors wish to thank technician Fatih Şahin (BSN Health, Analysis and Innovation, Goller Bolgesi Teknokenti, Suleyman Demirel University, Isparta, Turkey) for helping in the patch-clamp analyses.

References

A. Salazar-Ramiro, D. Ramírez-Ortega, V. Pérez de la Cruz et al., “Role of redox status in development of glioblastoma,” Frontiers in Immunology, vol. 7, p. 156, 2016.
View at: Publisher Site | Google Scholar
A. Philips, D. L. Henshaw, G. Lamburn, and M. J. O’Carroll, “Brain tumours: rise in glioblastoma multiforme incidence in England 1995-2015 suggests an adverse environmental or lifestyle factor,” Journal of Environmental and Public Health, vol. 2018, Article ID 7910754, 10 pages, 2018.
View at: Publisher Site | Google Scholar
F. Wei, L. Shi, Q. Wang, and Y. Zhao, “Fast and accurate separation of the paclitaxel from yew extracum by a pseudo simulated moving bed with solvent gradient,” Journal of Chromatography. A, vol. 1564, pp. 120–127, 2018.
View at: Publisher Site | Google Scholar
L. P. Ganipineni, B. Ucakar, N. Joudiou et al., “Magnetic targeting of paclitaxel-loaded poly(lactic-co-glycolic acid)-based nanoparticles for the treatment of glioblastoma,” International Journal of Nanomedicine, vol. 13, pp. 4509–4521, 2018.
View at: Publisher Site | Google Scholar
J. Xu, C. Su, F. Zhao et al., “Paclitaxel promotes lung cancer cell apoptosis via MEG3-P53 pathway activation,” Biochemical and Biophysical Research Communications, vol. 504, no. 1, pp. 123–128, 2018.
View at: Publisher Site | Google Scholar
C. M. Ho, F. K. Lee, S. H. Huang, and W. F. Cheng, “Everolimus following 5-aza-2-deoxycytidine is a promising therapy in paclitaxel-resistant clear cell carcinoma of the ovary,” American Journal of Cancer Research, vol. 8, no. 1, pp. 56–69, 2018.
View at: Google Scholar
Y. Zhang, Y. Wang, and J. Xue, “Paclitaxel inhibits breast cancer metastasis via suppression of Aurora kinase-mediated cofilin-1 activity,” Experimental and Therapeutic Medicine, vol. 15, no. 2, pp. 1269–1276, 2018.
View at: Publisher Site | Google Scholar
A. F. Phoa, S. Browne, F. M. S. Gurgis et al., “Pharmacology of novel small-molecule tubulin inhibitors in glioblastoma cells with enhanced EGFR signalling,” Biochemical Pharmacology, vol. 98, no. 4, pp. 587–601, 2015.
View at: Publisher Site | Google Scholar
Y. F. Wang, C. Y. Chen, S. F. Chung, Y. H. Chiou, and H. R. Lo, “Involvement of oxidative stress and caspase activation in paclitaxel-induced apoptosis of primary effusion lymphoma cells,” Cancer Chemotherapy and Pharmacology, vol. 54, no. 4, pp. 322–330, 2004.
View at: Publisher Site | Google Scholar
L. Bui, A. Hendricks, J. Wright et al., “Brain tumor genetic modification yields increased resistance to paclitaxel in physical confinement,” Scientific Reports, vol. 6, no. 1, p. 26134, 2016.
View at: Publisher Site | Google Scholar
M. Fukui, N. Yamabe, and B. T. Zhu, “Resveratrol attenuates the anticancer efficacy of paclitaxel in human breast cancer cells in vitro and in vivo,” European Journal of Cancer, vol. 46, no. 10, pp. 1882–1891, 2010.
View at: Publisher Site | Google Scholar
Q. Jiang, M. Yang, Z. Qu, J. Zhou, and Q. Zhang, “Resveratrol enhances anticancer effects of paclitaxel in HepG2 human liver cancer cells,” BMC Complementary and Alternative Medicine, vol. 17, no. 1, p. 477, 2017.
View at: Publisher Site | Google Scholar
T. Kubota, Y. Uemura, M. Kobayashi, and H. Taguchi, “Combined effects of resveratrol and paclitaxel on lung cancer cells,” Anticancer Research, vol. 23, no. 5A, pp. 4039–4046, 2003.
View at: Google Scholar
J. Meng, F. Guo, H. Xu, W. Liang, C. Wang, and X. D. Yang, “Combination therapy using co-encapsulated resveratrol and paclitaxel in liposomes for drug resistance reversal in breast cancer cells in vivo,” Scientific Reports, vol. 6, no. 1, p. 22390, 2016.
View at: Publisher Site | Google Scholar
A. A. Sprouse and B. S. Herbert, “Resveratrol augments paclitaxel treatment in MDA-MB-231 and paclitaxel-resistant MDA-MB-231 breast cancer cells,” Anticancer Research, vol. 34, no. 10, pp. 5363–5374, 2014.
View at: Google Scholar
T. Ahmed, S. Javed, S. Javed et al., “Resveratrol and Alzheimer’s disease: mechanistic insights,” Molecular Neurobiology, vol. 54, no. 4, pp. 2622–2635, 2017.
View at: Publisher Site | Google Scholar
N. Braidy, B. E. Jugder, A. Poljak et al., “Resveratrol as a potential therapeutic candidate for the treatment and management of Alzheimer’s disease,” Current Topics in Medicinal Chemistry, vol. 16, no. 17, pp. 1951–1960, 2016.
View at: Publisher Site | Google Scholar
K. A. Ahmad, M. V. Clement, and S. Pervaiz, “Pro-oxidant activity of low doses of resveratrol inhibits hydrogen peroxide-induced apoptosis,” Annals of the New York Academy of Sciences, vol. 1010, no. 1, pp. 365–373, 2003.
View at: Publisher Site | Google Scholar
N. M. O. Arcanjo, C. Luna, M. S. Madruga, and M. Estévez, “Antioxidant and pro-oxidant actions of resveratrol on human serum albumin in the presence of toxic diabetes metabolites: glyoxal and methyl-glyoxal,” Biochimica et Biophysica Acta - General Subjects, vol. 1862, no. 9, pp. 1938–1947, 2018.
View at: Publisher Site | Google Scholar
C. A. de la Lastra and I. Villegas, “Resveratrol as an antioxidant and pro-oxidant agent: mechanisms and clinical implications,” Biochemical Society Transactions, vol. 35, Part 5, pp. 1156–1160, 2007.
View at: Publisher Site | Google Scholar
I. E. Dueñas-García, M. E. Heres-Pulido, M. R. Arellano-Llamas et al., “Lycopene, resveratrol, vitamin C and FeSO₄ increase damage produced by pro-oxidant carcinogen 4-nitroquinoline-1-oxide in Drosophila melanogaster: xenobiotic metabolism implications,” Food and Chemical Toxicology, vol. 103, pp. 233–245, 2017.
View at: Publisher Site | Google Scholar
J. Favre, C. Yıldırım, T. A. Leyen et al., “Palmitic acid increases pro-oxidant adaptor protein p66Shc expression and affects vascularization factors in angiogenic mononuclear cells: action of resveratrol,” Vascular Pharmacology, vol. 75, pp. 7–18, 2015.
View at: Publisher Site | Google Scholar
W. Gadacha, M. Ben-Attia, D. Bonnefont-Rousselot, E. Aouani, N. Ghanem-Boughanmi, and Y. Touitou, “Resveratrol opposite effects on rat tissue lipoperoxidation: pro-oxidant during day-time and antioxidant at night,” Redox Report, vol. 14, no. 4, pp. 154–158, 2009.
View at: Publisher Site | Google Scholar
W. Lee and D. G. Lee, “Resveratrol induces membrane and DNA disruption via pro-oxidant activity against Salmonella typhimurium,” Biochemical and Biophysical Research Communications, vol. 489, no. 2, pp. 228–234, 2017.
View at: Publisher Site | Google Scholar
L. A. M. Martins, B. P. Coelho, G. Behr et al., “Resveratrol induces pro-oxidant effects and time-dependent resistance to cytotoxicity in activated hepatic stellate cells,” Cell Biochemistry and Biophysics, vol. 68, no. 2, pp. 247–257, 2014.
View at: Publisher Site | Google Scholar
S. Asghari, M. Rafraf, L. Farzin, M. Asghari-Jafarabadi, S. M. Ghavami, and M. H. Somi, “Effects of pharmacologic dose of resveratrol supplementation on oxidative/antioxidative status biomarkers in nonalcoholic fatty liver disease patients: a randomized, double-blind, placebo-controlled trial,” Advanced Pharmaceutical Bulletin, vol. 8, no. 2, pp. 307–317, 2018.
View at: Publisher Site | Google Scholar
A. Hajighasem, P. Farzanegi, Z. Mazaheri, M. Naghizadeh, and G. Salehi, “Effects of resveratrol, exercises and their combination on Farnesoid X receptor, Liver X receptor and Sirtuin 1 gene expression and apoptosis in the liver of elderly rats with nonalcoholic fatty liver,” PeerJ, vol. 6, article e5522, 2018.
View at: Publisher Site | Google Scholar
M. Elshaer, Y. Chen, X. J. Wang, and X. Tang, “Resveratrol: an overview of its anti-cancer mechanisms,” Life Sciences, vol. 207, pp. 340–349, 2018.
View at: Publisher Site | Google Scholar
L. Huminiecki and J. Horbanczuk, “The functional genomic studies of resveratrol in respect to Its anti-cancer effects,” Biotechnology Advances, vol. 36, no. 6, pp. 1699–1708, 2018.
View at: Publisher Site | Google Scholar
A. Rauf, M. Imran, M. S. Butt, M. Nadeem, D. G. Peters, and M. S. Mubarak, “Resveratrol as an anti-cancer agent: a review,” Critical Reviews in Food Science and Nutrition, vol. 58, no. 9, pp. 1428–1447, 2018.
View at: Publisher Site | Google Scholar
W. Win, Z. Cao, X. Peng, M. A. Trush, and Y. Li, “Different effects of genistein and resveratrol on oxidative DNA damage in vitro,” Mutation Research/Genetic Toxicology and Environmental Mutagenesis, vol. 513, no. 1-2, pp. 113–120, 2002.
View at: Publisher Site | Google Scholar
V. Aires, E. Limagne, A. K. Cotte, N. Latruffe, F. Ghiringhelli, and D. Delmas, “Resveratrol metabolites inhibit human metastatic colon cancer cells progression and synergize with chemotherapeutic drugs to induce cell death,” Molecular Nutrition & Food Research, vol. 57, no. 7, pp. 1170–1181, 2013.
View at: Publisher Site | Google Scholar
E. L. Donald, L. Stojanovska, V. Apostolopoulos, and K. Nurgali, “Resveratrol alleviates oxidative damage in enteric neurons and associated gastrointestinal dysfunction caused by chemotherapeutic agent oxaliplatin,” Maturitas, vol. 105, pp. 100–106, 2017.
View at: Publisher Site | Google Scholar
G. A. Frampton, E. A. Lazcano, H. Li, A. Mohamad, and S. DeMorrow, “Resveratrol enhances the sensitivity of cholangiocarcinoma to chemotherapeutic agents,” Laboratory Investigation, vol. 90, no. 9, pp. 1325–1338, 2010.
View at: Publisher Site | Google Scholar
J. Gusman, H. Malonne, and G. Atassi, “A reappraisal of the potential chemopreventive and chemotherapeutic properties of resveratrol,” Carcinogenesis, vol. 22, no. 8, pp. 1111–1117, 2001.
View at: Publisher Site | Google Scholar
Y. J. Lee, Y. J. Lee, J. H. Im et al., “Synergistic anti-cancer effects of resveratrol and chemotherapeutic agent clofarabine against human malignant mesothelioma MSTO-211H cells,” Food and Chemical Toxicology, vol. 52, pp. 61–68, 2013.
View at: Publisher Site | Google Scholar
J. A. McCubrey, S. L. Abrams, K. Lertpiriyapong et al., “Effects of berberine, curcumin, resveratrol alone and in combination with chemotherapeutic drugs and signal transduction inhibitors on cancer cells—power of nutraceuticals,” Advances in Biological Regulation, vol. 67, pp. 190–211, 2018.
View at: Publisher Site | Google Scholar
R. Mikstacka and E. Ignatowicz, “Chemopreventive and chemotherapeutic effect of trans-resveratrol and its analogues in cancer,” Polski Merkuriusz Lekarski, vol. 28, no. 168, pp. 496–500, 2010.
View at: Google Scholar
A. Mohan, S. Narayanan, S. Sethuraman, and U. M. Krishnan, “Novel resveratrol and 5-fluorouracil coencapsulated in PEGylated nanoliposomes improve chemotherapeutic efficacy of combination against head and neck squamous cell carcinoma,” BioMed Research International, vol. 2014, Article ID 424239, 14 pages, 2014.
View at: Publisher Site | Google Scholar
S. Pervaiz, “Chemotherapeutic potential of the chemopreventive phytoalexin resveratrol,” Drug Resistance Updates, vol. 7, no. 6, pp. 333–344, 2004.
View at: Publisher Site | Google Scholar
F. Quan, S. Q. Zhang, Y. X. Bai et al., “Resveratrol increases sensitivity of CNE2 cells to chemotherapeutic drugs under hypoxia,” Zhong Xi Yi Jie He Xue Bao, vol. 7, no. 10, pp. 952–957, 2009.
View at: Publisher Site | Google Scholar
C. Zhou, W. Qian, J. Ma et al., “Resveratrol enhances the chemotherapeutic response and reverses the stemness induced by gemcitabine in pancreatic cancer cells via targeting SREBP1,” Cell Proliferation, vol. 52, no. 1, article e12514, 2019.
View at: Publisher Site | Google Scholar
B. Li, D. Hou, H. Guo et al., “Resveratrol sequentially induces replication and oxidative stresses to drive p53-CXCR2 mediated cellular senescence in cancer cells,” Scientific Reports, vol. 7, no. 1, p. 208, 2017.
View at: Publisher Site | Google Scholar
M. Naziroglu, “Activation of TRPM2 and TRPV1 channels in dorsal root ganglion by NADPH oxidase and protein kinase C molecular pathways: a patch clamp study,” Journal of Molecular Neuroscience, vol. 61, no. 3, pp. 425–435, 2017.
View at: Publisher Site | Google Scholar
M. Naziroglu and A. Luckhoff, “A calcium influx pathway regulated separately by oxidative stress and ADP-ribose in TRPM2 channels: single channel events,” Neurochemical Research, vol. 33, no. 7, pp. 1256–1262, 2008.
View at: Publisher Site | Google Scholar
H. Akpınar, M. Nazıroğlu, İ. S. Övey, B. Çiğ, and O. Akpınar, “The neuroprotective action of dexmedetomidine on apoptosis, calcium entry and oxidative stress in cerebral ischemia-induced rats: contribution of TRPM2 and TRPV1 channels,” Scientific Reports, vol. 6, no. 1, article 37196, 2016.
View at: Publisher Site | Google Scholar
P. Kang, W. Zhang, X. Chen et al., “TRPM2 mediates mitochondria-dependent apoptosis of melanocytes under oxidative stress,” Free Radical Biology & Medicine, vol. 126, pp. 259–268, 2018.
View at: Publisher Site | Google Scholar
E. Kheradpezhouh, F. H. Zhou, G. J. Barritt, and G. Y. Rychkov, “Oxidative stress promotes redistribution of TRPM2 channels to the plasma membrane in hepatocytes,” Biochemical and Biophysical Research Communications, vol. 503, no. 3, pp. 1891–1896, 2018.
View at: Publisher Site | Google Scholar
A. Oz and O. Celik, “Curcumin inhibits oxidative stress-induced TRPM2 channel activation, calcium ion entry and apoptosis values in SH-SY5Y neuroblastoma cells: involvement of transfection procedure,” Molecular Membrane Biology, vol. 33, no. 3-5, pp. 76–88, 2016.
View at: Publisher Site | Google Scholar
F. Uslusoy, M. Naziroglu, and B. Cig, “Inhibition of the TRPM2 and TRPV1 channels through Hypericum perforatum in sciatic nerve injury-induced rats demonstrates their key role in apoptosis and mitochondrial oxidative stress of sciatic nerve and dorsal root ganglion,” Frontiers in Physiology, vol. 8, p. 335, 2017.
View at: Publisher Site | Google Scholar
Q. Wang, L. Huang, and J. Yue, “Oxidative stress activates the TRPM2-Ca²⁺-CaMKII-ROS signaling loop to induce cell death in cancer cells,” Biochimica et Biophysica Acta (BBA) - Molecular Cell Research, vol. 1864, no. 6, pp. 957–967, 2017.
View at: Publisher Site | Google Scholar
E. Yüksel, M. Nazıroğlu, M. Şahin, and B. Çiğ, “Involvement of TRPM2 and TRPV1 channels on hyperalgesia, apoptosis and oxidative stress in rat fibromyalgia model: protective role of selenium,” Scientific Reports, vol. 7, no. 1, article 17543, 2017.
View at: Publisher Site | Google Scholar
D. W. Koh, D. P. Powell, S. D. Blake, J. L. Hoffman, M. M. Hopkins, and X. Feng, “Enhanced cytotoxicity in triple-negative and estrogen receptor-positive breast adenocarcinoma cells due to inhibition of the transient receptor potential melastatin-2 channel,” Oncology Reports, vol. 34, no. 3, pp. 1589–1598, 2015.
View at: Publisher Site | Google Scholar
S. Almasi, B. E. Kennedy, M. el-Aghil et al., “TRPM2 channel-mediated regulation of autophagy maintains mitochondrial function and promotes gastric cancer cell survival via the JNK-signaling pathway,” The Journal of Biological Chemistry, vol. 293, no. 10, pp. 3637–3650, 2018.
View at: Publisher Site | Google Scholar
H. A. Deveci, Y. Akyuva, G. Nur, and M. Nazıroğlu, “Alpha lipoic acid attenuates hypoxia-induced apoptosis, inflammation and mitochondrial oxidative stress via inhibition of TRPA1 channel in human glioblastoma cell line,” Biomedicine & Pharmacotherapy, vol. 111, pp. 292–304, 2018.
View at: Publisher Site | Google Scholar
J. H. Lee, K. Na, S. C. Song, J. Lee, and H. J. Kuh, “The distribution and retention of paclitaxel and doxorubicin in multicellular layer cultures,” Oncology Reports, vol. 27, no. 4, pp. 995–1002, 2012.
View at: Publisher Site | Google Scholar
M. Zielińska-Przyjemska, M. Kaczmarek, V. Krajka-Kuźniak, M. Łuczak, and W. Baer-Dubowska, “The effect of resveratrol, its naturally occurring derivatives and tannic acid on the induction of cell cycle arrest and apoptosis in rat C6 and human T98G glioma cell lines,” Toxicology In Vitro, vol. 43, pp. 69–75, 2017.
View at: Publisher Site | Google Scholar
Y. Yazgan and M. Naziroglu, “Ovariectomy-induced mitochondrial oxidative stress, apoptosis, and calcium ion influx through TRPA1, TRPM2, and TRPV1 are prevented by 17β-estradiol, tamoxifen, and raloxifene in the hippocampus and dorsal root ganglion of rats,” Molecular Neurobiology, vol. 54, no. 10, pp. 7620–7638, 2017.
View at: Publisher Site | Google Scholar
G. Nur, M. Naziroglu, and H. A. Deveci, “Synergic prooxidant, apoptotic and TRPV1 channel activator effects of alpha-lipoic acid and cisplatin in MCF-7 breast cancer cells,” Journal of Receptor and Signal Transduction Research, vol. 37, no. 6, pp. 569–577, 2017.
View at: Publisher Site | Google Scholar
J. Y. Koh and D. W. Choi, “Quantitative determination of glutamate mediated cortical neuronal injury in cell culture by lactate dehydrogenase efflux assay,” Journal of Neuroscience Methods, vol. 20, no. 1, pp. 83–90, 1987.
View at: Publisher Site | Google Scholar
A. C. Uğuz, M. Nazıroğlu, J. Espino et al., “Selenium modulates oxidative stress-induced cell apoptosis in human myeloid HL-60 cells through regulation of calcium release and caspase-3 and -9 activities,” The Journal of Membrane Biology, vol. 232, no. 1-3, pp. 15–23, 2009.
View at: Publisher Site | Google Scholar
V. C. Keil, F. Funke, A. Zeug, D. Schild, and M. Müller, “Ratiometric high-resolution imaging of JC-1 fluorescence reveals the subcellular heterogeneity of astrocytic mitochondria,” Pflügers Archiv, vol. 462, no. 5, pp. 693–708, 2011.
View at: Publisher Site | Google Scholar
R. A. Schuh, P. Clerc, H. Hwang et al., “Adaptation of microplate-based respirometry for hippocampal slices and analysis of respiratory capacity,” Journal of Neuroscience Research, vol. 89, no. 12, pp. 1979–1988, 2011.
View at: Publisher Site | Google Scholar
D. Pesta and E. Gnaiger, “High-resolution respirometry: OXPHOS protocols for human cells and permeabilized fibers from small biopsies of human muscle,” Methods in Molecular Biology, vol. 810, pp. 25–58, 2012.
View at: Publisher Site | Google Scholar
A. Poljak, R. Pamphlett, M. E. Gurney, and M. W. Duncan, “Measurement of o- and m-tyrosine as markers of oxidative damage in motor neuron disease,” Redox Report, vol. 5, no. 2-3, pp. 137–140, 2000.
View at: Publisher Site | Google Scholar
M. M. Bradford, “A rapid and sensitive method for the quantitation of microgram quantities of protein utilizing the principle of protein-dye binding,” Analytical Biochemistry, vol. 72, no. 1-2, pp. 248–254, 1976.
View at: Publisher Site | Google Scholar
C. T. Madreiter-Sokolowski, B. Gottschalk, W. Parichatikanond et al., “Resveratrol specifically kills cancer cells by a devastating increase in the Ca²⁺ coupling between the greatly tethered endoplasmic reticulum and mitochondria,” Cellular Physiology and Biochemistry, vol. 39, no. 4, pp. 1404–1420, 2016.
View at: Publisher Site | Google Scholar
S. Ji, Z. Zheng, S. Liu et al., “Resveratrol promotes oxidative stress to drive DLC1 mediated cellular senescence in cancer cells,” Experimental Cell Research, vol. 370, no. 2, pp. 292–302, 2018.
View at: Publisher Site | Google Scholar
Y. S. Ko, H. Jin, J. S. Lee et al., “Radioresistant breast cancer cells exhibit increased resistance to chemotherapy and enhanced invasive properties due to cancer stem cells,” Oncology Reports, vol. 40, no. 6, pp. 3752–3762, 2018.
View at: Publisher Site | Google Scholar
N. Rabbani, M. Xue, M. O. Weickert, and P. J. Thornalley, “Multiple roles of glyoxalase 1-mediated suppression of methylglyoxal glycation in cancer biology-involvement in tumour suppression, tumour growth, multidrug resistance and target for chemotherapy,” Seminars in Cancer Biology, vol. 49, pp. 83–93, 2018.
View at: Publisher Site | Google Scholar
W. Tunyapanit, S. Chelae, and K. Laoprasopwattana, “Does ciprofloxacin prophylaxis during chemotherapy induce intestinal microflora resistance to ceftazidime in children with cancer?” Journal of Infection and Chemotherapy, vol. 24, no. 5, pp. 358–362, 2018.
View at: Publisher Site | Google Scholar
J. Yuan, Z. Yin, K. Tao, G. Wang, and J. Gao, “Function of insulin-like growth factor 1 receptor in cancer resistance to chemotherapy,” Oncology Letters, vol. 15, no. 1, pp. 41–47, 2018.
View at: Publisher Site | Google Scholar
J. Zhang, B. Zhao, X. Chen, Z. Wang, H. Xu, and B. Huang, “Silence of long noncoding RNA NEAT1 inhibits malignant biological behaviors and chemotherapy resistance in gastric cancer,” Pathology Oncology Research, vol. 24, no. 1, pp. 109–113, 2018.
View at: Publisher Site | Google Scholar
L. Bao, S. J. Chen, K. Conrad et al., “Depletion of the human ion channel TRPM2 in neuroblastoma demonstrates its key role in cell survival through modulation of mitochondrial reactive oxygen species and bioenergetics,” The Journal of Biological Chemistry, vol. 291, no. 47, pp. 24449–24464, 2016.
View at: Publisher Site | Google Scholar
S. J. Chen, N. E. Hoffman, S. Shanmughapriya et al., “A splice variant of the human ion channel TRPM2 modulates neuroblastoma tumor growth through hypoxia-inducible factor (HIF)-1/2α,” Journal of Biological Chemistry, vol. 289, no. 52, pp. 36284–36302, 2014.
View at: Publisher Site | Google Scholar
I. Hirschler-Laszkiewicz, S. J. Chen, L. Bao et al., “The human ion channel TRPM2 modulates neuroblastoma cell survival and mitochondrial function through Pyk2, CREB, and MCU activation,” American Journal of Physiology-Cell Physiology, vol. 315, no. 4, pp. C571–C586, 2018.
View at: Publisher Site | Google Scholar
A. Sumoza-Toledo, M. I. Espinoza-Gabriel, and D. Montiel-Condado, “Evaluation of the TRPM2 channel as a biomarker in breast cancer using public databases analysis,” Boletín Médico del Hospital Infantil de México, vol. 73, no. 6, pp. 397–404, 2016.
View at: Publisher Site | Google Scholar
Y. Sun, P. Sukumaran, S. Selvaraj et al., “TRPM2 promotes neurotoxin MPP⁺/MPTP-induced cell death,” Molecular Neurobiology, vol. 55, no. 1, pp. 409–420, 2018.
View at: Publisher Site | Google Scholar
T. L. Pan, P. W. Wang, Y. C. Hung, C. H. Huang, and K. M. Rau, “Proteomic analysis reveals tanshinone IIA enhances apoptosis of advanced cervix carcinoma CaSki cells through mitochondria intrinsic and endoplasmic reticulum stress pathways,” Proteomics, vol. 13, no. 23-24, pp. 3411–3423, 2013.
View at: Publisher Site | Google Scholar
N. André, D. Braguer, G. Brasseur et al., “Paclitaxel induces release of cytochrome c from mitochondria isolated from human neuroblastoma cells,” Cancer Research, vol. 60, no. 19, pp. 5349–5353, 2000.
View at: Google Scholar
N. André, M. Carré, G. Brasseur et al., “Paclitaxel targets mitochondria upstream of caspase activation in intact human neuroblastoma cells,” FEBS Letters, vol. 532, no. 1-2, pp. 256–260, 2002.
View at: Publisher Site | Google Scholar
Y. Tian, H. Zhang, Y. Qin et al., “Overcoming drug-resistant lung cancer by paclitaxel-loaded hyaluronic acid-coated liposomes targeted to mitochondria,” Drug Development and Industrial Pharmacy, vol. 44, no. 12, pp. 2071–2082, 2018.
View at: Publisher Site | Google Scholar
Q. Li, Y. Yue, L. Chen et al., “Resveratrol sensitizes carfilzomib-induced apoptosis via promoting oxidative stress in multiple myeloma cells,” Frontiers in Pharmacology, vol. 9, p. 334, 2018.
View at: Publisher Site | Google Scholar
M. Brentnall, L. Rodriguez-Menocal, R. de Guevara, E. Cepero, and L. H. Boise, “Caspase-9, caspase-3 and caspase-7 have distinct roles during intrinsic apoptosis,” BMC Cell Biology, vol. 14, no. 1, p. 32, 2013.
View at: Publisher Site | Google Scholar
A. A. Corbat, K. C. Schuermann, P. Liguzinski et al., “Co-imaging extrinsic, intrinsic and effector caspase activity by fluorescence anisotropy microscopy,” Redox Biology, vol. 19, pp. 210–217, 2018.
View at: Publisher Site | Google Scholar
F. Kong, R. Zhang, X. Zhao, G. Zheng, Z. Wang, and P. Wang, “Resveratrol raises in vitro anticancer effects of paclitaxel in NSCLC cell line A549 through COX-2 expression,” The Korean Journal of Physiology & Pharmacology, vol. 21, no. 5, pp. 465–474, 2017.
View at: Publisher Site | Google Scholar
F. Dai, Q. Wang, G. J. Fan, Y. T. du, and B. Zhou, “ROS-driven and preferential killing of HepG2 over L-02 cells by a short-term cooperation of Cu(II) and a catechol-type resveratrol analog,” Food Chemistry, vol. 250, pp. 213–220, 2018.
View at: Publisher Site | Google Scholar
S. Tomas-Hernández, J. Blanco, C. Rojas et al., “Resveratrol potently counteracts quercetin starvation-induced autophagy and sensitizes HepG2 cancer cells to apoptosis,” Molecular Nutrition & Food Research, vol. 62, no. 5, 2018.
View at: Publisher Site | Google Scholar
T. Mueller, W. Voigt, H. Simon et al., “Failure of activation of caspase-9 induces a higher threshold for apoptosis and cisplatin resistance in testicular cancer,” Cancer Research, vol. 63, no. 2, pp. 513–521, 2003.
View at: Google Scholar

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Copyright © 2019 Yasin Öztürk et al. This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

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Oxidative Medicine and Cellular Longevity

Resveratrol Enhances Apoptotic and Oxidant Effects of Paclitaxel through TRPM2 Channel Activation in DBTRG Glioblastoma Cells

Abstract

1. Introduction

2. Materials and Methods

2.1. Cell Culture

2.2. Groups

2.3. Electrophysiology

2.4. Intracellular Ca2+ Fluorescence Intensity Measurement through TRPM2 Activation

2.5. MTT Assay of Cell Viability

2.6. Extracellular LDH Activity as a Measurement for Cytotoxicity

2.7. Assay of Apoptosis Level and Caspase 3 and 9 Activities

2.8. Measurement of Mitochondrial Membrane Potential (ΔΨm)

2.9. XF24 Microplate-Based Respirometry

2.10. Detection of Intracellular Steady-State Reactive Oxygen Species (ROS) Using the DCFH-DA and o- and m-Tyrosine Assays

2.11. Bradford Protein Assay for the Quantification of Total Protein

2.12. Statistical Analyses

3. Results

3.1. Effects of PAX and RESV on TRPM2 Currents in DBTRG Cells

3.2. Effects of PAX and RESV on Florescence Intensity of Ca2+ through TRPM2 Activation in DBTRG Cells

3.3. Apoptosis, Caspase, and Cell Viability (MTT) Results

3.4. Caspase 3 and 9 Activities

3.5. Mitochondrial Depolarization (JC1) and Intracellular Steady-State ROS Levels

4. Discussion

Abbreviations

Data Availability

Disclosure

Conflicts of Interest

Authors’ Contributions

Acknowledgments

References

Copyright

2.4. Intracellular Ca²⁺ Fluorescence Intensity Measurement through TRPM2 Activation

3.2. Effects of PAX and RESV on Florescence Intensity of Ca²⁺ through TRPM2 Activation in DBTRG Cells