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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.

1. Introduction

During electrolysis, water (H₂O) weakly dissociates to H⁺ and OH^- in aqueous solution. The hydrogen ions, by receiving an electron on the cathode, are transformed in active and then molecular hydrogen (H₂). Simultaneously, OH^- is oxidized to generate molecular oxygen O₂. For these reasons, the water solution near the cathode is characterized by an alkaline pH, an elevated percentage of dissolved hydrogen and a small amount of platinum (Pt) nanoparticles: this solution is named electrochemical reduced water (ERW) [1]. Reduced water (electrochemical or natural) has been suggested to have beneficial effects on human health [1]. Reducing activity present in natural springs has been described to be beneficial for dermatological and antibacterial treatment [2]. It has been demonstrated that ERW shows reactive oxygen species- (ROS-) scavenging activity that could be useful in the treatment of oxidative stress-related diseases [3, 4]. The first studies to support the use of ERW were performed in Japan in the 1930s and in the 1960s and it was recognized that ERW was effective in chronic diarrhea, gastrointestinal fermentation, and gastric hyperacidity [1]. The antioxidant activity of ERW can be in part due to the extremely low oxidation reduction potential (ORP: average less than -400mV) and the presence of atomic hydrogen [5]. Another factor that could enhance the antioxidant effect of the ERW water is the presence of Pt nanoparticles produced by the electrolysis process in platinum-plated instruments. Pt nanoparticles have demonstrated to scavenge ${O_{2}}^{-}$ , OH^•, and H₂O₂ [6, 7], reducing the damage caused by oxidative stress in cell cultures [8]. In addition, platinum nanoparticles catalyze the process of converting the atomic hydrogen molecule to active atomic hydrogen [1]. It was reported that ERW inhibited the DNA breaking reaction in a dose-dependent manner [9]. ERW was also able to scavenge ROS in rat L6 myotube cells and to enhance sugar uptake [10]. In addition, ERW ameliorated the symptoms of diabetic mice [11–13]. The effects of ERW are due to its rich H₂ content, enabling it (1) to reduce cytotoxic oxygen radicals in cultured cells and protect ischemia-reperfusion injury in rats [14]; (2) to suppress the expression of proinflammatory cytokines by regulating gene expression [15]; (3) to stabilize atherosclerotic plaques [16]; (4) to protect from peroxynitrite derived from nitric oxide [17]; and (5) to reduce the number of injuries caused by hypoxia/reoxygenation [18] and cecal ligation [19]. Regarding the anticancer effects of ERW, it was reported that it reduced tumor angiogenesis by downregulation of VEGF gene transcription and protein secretion through inactivation of ERK [20]; it enhanced apoptosis in human leukemic HL-60 cells [21]; it inhibited colony formation and cell proliferation of human tongue squamous cell carcinoma-derived cell line HSC-4 but not of normal human tongue epithelial-like cells DOK [22]; it inhibited proliferation and invasion of the human fibrosarcoma HT-1080 cells [22]; it strongly prevented (when supplemented with synthesized Pt nanoparticles) the transformation of BALB/c 3T3 cells by 3-methyl cholanthrene as an initiation substance, followed by treatment with phorbol-12-myristate-13-acetate as a promotion substance [23]. While the in vitro results appeared to support the inhibition of cell proliferation by ERW, the analysis of its in vivo effects on tumor growth could better sustain its potential medical applications. The transgenic BALB-neuT mouse represents a valuable tumor model for HER2 breast carcinoma, closely reproducing some features of mammary carcinogenesis in women [24]. Here we evaluated the in vitro and in vivo effects of ERW on cancer cell growth, together with the analysis of involved molecular mechanisms.

2. Materials and Methods

2.1. Equipment

An alkaline ionized, seven electrode plates platinum-plated, water generator was used to produce ERW (Chanson “Miracle Max” Water Ionizer, Taiwan). The generator is provided with high efficiency activated carbon and works with tap water. The ERW produced by the generator has low ORP (-772 ± 51 mV), elevated concentration of dissolved hydrogen (H₂, 1327 ± 158), and an alkaline pH (10.8).

2.2. Reagents

Sulforhodamine B (SRB) was purchased from Sigma-Aldrich (Saint Louis, MO, USA). Antibodies against AKT and phospho-AKT (Ser473) were obtained from Cell Signaling Technology (MA, USA). Antibodies against Bax and Bcl-2 were from BD Pharmigen (BD Biosciences, San Josè, CA, USA). Antibodies against ERK1/2 (C-14), phospho-ERK (E-4), PARP-1, and p53 (DO-1) were obtained from Santa Cruz Biotechnology (Santa Cruz, CA, USA). Anti-ErbB2 antiserum was provided by Dr. M.H. Kraus (University of Alabama, Birmingham, USA). A rabbit polyclonal antibody against actin and goat anti-mouse or anti-rabbit IgG peroxidase-conjugated secondary antibodies were from Sigma-Aldrich.

2.3. Cell Lines and Treatments

BALB-neuT mammary cancer cells (H-2 $^{d}$ ) (TUBO) that overexpress activated rat ErbB2/neu were kindly provided by Professor G. Forni and Professor F. Cavallo (University of Torino, Italy) [25] and were maintained in DMEM (Dulbecco’s modified Eagle’s medium) liquid (Aurogene, Rome, Italy) containing 20% fetal bovine serum, 100 U/ml penicillin and 100 μg/ml streptomycin (complete medium). Human (MCF-7 and MDA-MB-453) breast cancer cell lines were maintained in DMEM liquid (Aurogene, Rome, Italy) containing 10% fetal bovine serum, 100 U/ml penicillin, and 100 μg/ml streptomycin (complete medium). Cells were grown at 37°C in a humidified incubator with an atmosphere of 5% CO₂. During the experiments, cells were cultured with DMEM, high glucose (Gibco, Thermo Fisher Scientific, Waltham, MA, USA) prepared by dilution of 10x DMEM with ERW, designated as ERW treatment (ERW: ORP -450 ± 37 mV, pH 7.3 ± 0.1, H₂ = 751 ± 136), or cultured with DMEM prepared by dilution of 10x DMEM with autoclaved ERW, designated as autoclaved treatment (autoclaved ERW: ORP +50 ± 6 mV, pH 7.3 ± 0.1, H₂ = 0). We used DMEM liquid (Aurogene, Rome, Italy) only as a positive control medium to monitor the cell growth, because breast cancer cells were routinely maintained in this medium (CTR: ORP +50 ± 8 mV, pH 7.3 ± 0.1, H₂ = 0). All culture media were enriched with 10% FBS (MCF-7, MDA-MB-453) or 20% FBS (TUBO). All electrolyzed alkaline water (ERW and autoclaved ERW) was neutralized at pH 7.0-7.4 by adding 3 ml of DMEM 10x, 0.5 ml of 1 M HEPES buffer (pH 5.3, Sigma-Aldrich) and 0.3 ml of penicillin-streptomycin every 27 ml of ERW/autoclaved ERW, before use. Treatments were replenished every 24 hours. We compared through all the experiments the effects of ERW with the effect of autoclaved ERW. Thus, the autoclaved ERW with positive ORP and no concentration of dissolved hydrogen was our control for ERW treatment, since the differences between the effect of ERW and autoclaved ERW can be attributed to the unique characteristics possessed by ERW. Indeed, the ERW treatment possesses a negative ORP and an elevated high concentration of dissolved hydrogen, while the autoclaved ERW treatment possesses a positive ORP and no concentration of dissolved hydrogen.

2.4. Cell Proliferation Analysis by Sulforhodamine B (SRB) Assay

Cells were seeded at 5 × 10³/well in 96-well plates. After 24 hours, cells were treated with ERW, autoclaved ERW and control medium (CTR), and incubated for 24-72 hours. The assay was then performed as previously described [26]. The percentage survival of the cultures treated with ERW or autoclaved ERW was calculated by normalizing their OD values to those of control cultures (CTR) [27]. The experiments were performed in triplicate and repeated six times.

2.5. Cell Viability Analysis by Trypan Blue Exclusion Test

Breast cancer cells (5 × 10⁴ cells/well) were seeded in 24-well plates. After 24 hours, cells were treated with ERW, autoclaved ERW and control medium (CTR), and incubated for 24-72 hours. Media were replaced every 24 hours and cell density was determined. After treatment, adherent and suspended cells were harvested and stained with trypan blue (Sigma-Aldrich) and counted. The experiments were performed in triplicate and repeated six times. The percentage of cell death was determined compared to the total number of cells as previously described [28].

2.6. ERW Treatment of BALB-neuT Mice

Transgenic BALB-neuT male mice were mated with BALB/c females (H-2 $^{d}$ ; Charles River, Calco, Italy) in the animal facilities of Tor Vergata University. Founder male BALB-neuT mice were kindly provided by Professor G. Forni and Professor F. Cavallo (University of Turin, Italy) [25]. Progenies (48 mice) were confirmed for the presence of the transgene by PCR [25]. Sixteen individually tagged virgin females were used in this study. Mice were bred under pathogen-free conditions and handled in compliance with European Union and institutional standards for animal research.

Groups of female BALB-neuT mice (8 mice per group) were treated with ERW water or natural water since their weaning and up to 33 weeks of age. The ERW water was changed every three hours during the day while the night was left to mice available ad libitum. Mice were sacrificed at the first signs of distress. Investigation has been conducted in accordance with the ethical standards and according to the Declaration of Helsinki. A veterinary surgeon was present during the experiments. The animal care both before and after the experiments was performed only by trained personnel. The work was conducted with the formal approval of the local animal care committees (institutional and national), and animal experiments have been registered as legislation requires (Authorization from Ministry of Health n° 875/2016-PR, 16/09/16).

2.7. Analysis of ERW Antitumor Activity In Vivo

Mammary glands were checked weekly and tumors recorded at 2-3 mm in diameter. Tumor growth was monitored until all mammary glands displayed a palpable tumor or tumor mass exceeding 20 mm in diameter. At this point mice were sacrificed. The time of tumor appearance was recorded and tumor multiplicity for each treatment group was expressed as mean ± standard deviation (SD) [29].

2.8. Evaluation of Hematological and Clinical Chemistry Parameters

Blood samples were collected in animals under i.p. anesthesia (20 μl/g.b.w. of 1.2% Avertin-2,2,2- tribromoethanol, 2.4% 2-methyl-2-butanol; Sigma-Aldrich). Hematological parameters were analyzed using the commercially available automated cell counter “Drew3” (BPC BioSed, Italy), after collecting 20 μl of whole blood in K2EDTA microvacutainers (Boston, Dickinson and Company, USA). Peripheral blood smears were prepared employing the differential staining Diff-Quick (Dade SpA, Italy) and analyzed for cytomorphological parameters under optical microscopy. The complete blood count (CBC) includes hemoglobin (HGB), hematocrit (HCT), red blood cell (RBC) count, white blood cell (WBC) count, platelet count (PLT), red cell distribution width (RDW), mean corpuscular volume (MCV), mean platelet volume (MPV), mean corpuscular hemoglobin (MCH), mean corpuscular hemoglobin concentration (MCHC), lymphocytes (LYMF), midrange cells (MID), and granulocytes (GRAN). Blood samples were collected in SST microtainers (Serum Separator Tube; Boston, Dickinson and Company) for serum protein electrophoresis and centrifuged at 13.000 rpm for 7 min. For the measurement of blood glucose, mice were placed in fasting three hours before blood sampling. Glucose (GLU) was measured using the automatic analyzer Keylab (BPC BioSed s.r.l., Rome, Italy).

2.9. Western Blotting Analysis

1 × 10⁶ cells were seeded in 100-mm tissue culture dishes 24 hours prior to the addition of ERW and autoclaved ERW treatments. Media were replaced every 24 hours. Western blotting analysis was performed as previously described [26]. 50 μg of cell lysates was resolved in 10% SDS-PAGE and then transferred to nitrocellulose membranes. After blocking, the membranes were incubated with specific primary antibodies at 1-2 μg/ml concentrations overnight at 4°C. After being washed, the filters were incubated with goat anti-mouse or anti-rabbit IgG, peroxidase-conjugated antibodies and developed by chemiluminescence as previously described [30]. A densitometric analysis of autoradiographic bands was performed with Image J software 1.42q (National Institutes of Health, Bethesda, MD, USA) after blot scanning and expressed as bar graphs in the figures.

2.10. Fluorescence-Activated Cell Sorting (FACS) Analysis

Asynchronized, log-phase growing cells (60% confluent, approximately 2.5 × 105/well in 6-well plates) were treated with ERW, autoclaved ERW or control medium (CTR). Media were replaced every 24 hours. Fluorescence-activated cell sorting (FACS) analysis was performed as previously described using a FACSCalibur cytometer with CellQuest Pro 5.2 software (BD Biosciences, San Jose, CA) [26, 31]. A minimum of 20000 events was collected. The experiments were repeated three times

2.11. Statistical Analysis

Data distribution of cell survival, cell death, or FACS analyses was preliminarily verified by the Kolmogorov-Smirnov test, and datasets were analyzed by one-way analysis of variance (ANOVA) followed by Newman-Keuls test as previously described [26, 31]. Differences in the intensity of immunoreactive bands between ERW and autoclaved ERW were evaluated by a two-tailed Student’s t-test. Values with p<0.05 were considered significant. For the hematological and clinical chemistry parameters, only the parameters outside the reference values were analyzed by a two-tailed Student’s t-test comparing those of control mice with the ERW-treated mice. Survival curves and tumor multiplicity were estimated using the Kaplan-Meier method and compared by the log-rank test (Mantel-Cox) with calculation of the SD according to the method of Greenwood. Differences were regarded as significant when p value was <0.05 as previously described [29].

3. Results

3.1. ERW Inhibits Human and Mouse Breast Cancer Cells Survival

We first evaluated the in vitro effect of ERW on the growth of human breast cancer cell lines (MCF-7 and MDA-MB-453), characterized by different expression of estrogen (ER), progesterone (PR), and ErbB2 receptors, and of tumor suppressor p53 [32–36] (Table 1). In addition, we employed the mouse breast cancer cell line TUBO, derived from BALB-neuT mice that overexpresses activated rat ErbB2/neu.

Table 1

Molecular features of employed human breast cancer cell lines.

Cell line	ER ^†	PR	ErbB2	p53	References
MCF-7	+	+	+	+ $^{W T}$	[32–35]
MDA-MB-453	-	-	+/++	+ $^{M}$	[32, 33, 35, 36]

$^{†}$ Estrogen and progesterone receptors (ER/PR) status, ErbB2 expression, p53 protein levels, and mutational status (M: mutated protein; WT: wild-type protein) are indicated.

Cell growth of human (MCF-7, MDA-MB-453) and mouse (TUBO) breast cancer cells was quantified after treatment with ERW, autoclaved ERW, and CTR (used as positive control cultures to monitor the cell growth) for 24, 48, and 72 hours by the SRB assay. The effects of autoclaved ERW achieved statistical significance only at 72 hours compared to CTR treatment in all cell lines (p<0.001). Conversely, the effect of ERW reached statistical significance at all times analyzed as compared to CTR treatment in all cell lines (p<0.001). In addition, ERW treatment had greater cell survival inhibition than autoclaved ERW at all times in all cell lines analyzed (p<0.01) (Figure 1).

[figure omitted; refer to PDF]

The dye exclusion test was used to determine the number of death breast cancer cells after ERW, autoclaved ERW and CTR treatments. The cytotoxic effect of ERW was time-dependent. Autoclaved ERW had no significant effect as compared to CTR. Conversely, the percentage of cell death upon ERW treatment was 22, 34, and 43 for MCF-7 (p<0.001); 16, 22, and 32 for MDA-MB-453 (p<0.001); 26, 36, and 43 for TUBO (p<0.001) cells (Figure 2). In addition, the effects obtained with ERW treatment gained statistical significance as compared to autoclaved ERW treatment at all times analyzed (MCF-7 and TUBO: p<0.001; MDA-MB-453: p<0.01 at 24 h and p<0.001 at 48 and 72 h) (Figure 2).

[figure omitted; refer to PDF]

3.2. ERW Delays Mammary Tumor Growth in BALB-neuT Mice

The in vivo antitumor activity of ERW was analyzed in BALB-neuT mice transgenic for the neu oncogene. This mouse model represents an aggressive ErbB2/neu-mediated mammary carcinogenesis. Indeed, BALB-neuT mice develop atypical hyperplasia of the mammary gland at 6 weeks of age and in situ and invasive carcinoma at 11 and 16 weeks of age, respectively [25]. Groups of female BALB-neuT mice (8 mice per group) were treated with ERW or natural water (control) since their weaning and up to 33 weeks of age.

All BALB-neuT mice treated with natural water had palpable tumors by week 16, with a tumor multiplicity of 1.5. By contrast, none of the ERW-treated mice exhibited signs of tumor growth at week 16, indicating specific interference of ERW water with tumor development (p<0.001) (Figures 3(a) and 3(b)). Indeed, in the ERW-treated group palpable tumors appeared and affected all mice only at week 19. In addition, at week 24, when the first control mouse was sacrificed for the excessive size of its tumors, the multiplicity of tumors in control mice was 7.5, while that of ERW-treated mice was 2.63 (p<0.001) (Figures 3(a) and 3(b)). Three and four control mice were euthanized at 25 and 27 weeks, respectively. At 27 weeks of age, when all control mice were sacrificed, ERW mice were still all alive. ERW mice were euthanized for the excessive size of at least one tumor per mice at 30 weeks (2 mice), at 32 weeks (2 mice), and at 33 weeks (4 mice), when the experiment was completed.

[figures omitted; refer to PDF]

Our results indicate that ERW induced a significant prolongation of tumor-free survival and a reduction of tumor multiplicity (Figures 3(a) and 3(b)). Furthermore, our results indicated a specific interference of ERW with tumor growth in BALB-neuT mice (Figure 3(c)). The increase in the median survival of ERW-treated mice was significant compared to control mice (32.5 versus 26 weeks, p=0.0001) (Figure 3(c)). The relative risk of developing tumors in the control mice was 22.25 as compared to ERW-treated mice (Table 2).

Table 2

Analysis of the survival of BALB-neuTmice after treatment with ERW by the log-rank test (Mantel-Cox).

Variable	Contrast	Hazard Ratio	95 $%$ Hazard Ratio Confidence Limits		Median Survival (Weeks)	p Value
			Lower	Upper
Treatment	CTR vs. ERW	22.25	4.577	108.2	26 vs. 32.5	0.0001

CTR: control mice; ERW: mice treated with ERW.

3.3. Hematological and Clinical Chemistry Parameters in Mice Administered with ERW

To determine whether ERW induced changes in hematological and clinical chemistry parameters, we measured complete blood count, cholesterol, triglycerides, serum glutamic oxaloacetic transaminase, serum pyruvic transaminase, glucose, and blood urea nitrogen, in BALB-neuT mice (8 per group) at 7/11/17/23 weeks of age and at the end of the protocol. Values of individual mice were very heterogeneous within each group. No significant differences were observed between the parameters measured in each group of mice at 7 weeks of age. On the other hand, at 11 weeks of age ERW-treated mice showed a decrease in the total number of white blood cells (reference values 5-12 × 10³/mm³; 3.9 versus 7.5, p<0.001), lymphocytes (reference values 4-10 × 10³/mm³; 2.6 versus 4.6, p<0.001), and triglycerides (reference values 80-200 mg/dl; 54.0 versus 122.6, p<0.001) compared to control mice. At this stage, the control mice displayed a slight decreased level of mean corpuscular hemoglobin (reference values 15-19 pg; 13.9 versus 15.4, p<0.001) and mean corpuscular hemoglobin concentration (reference values 34-39 g/dl; 30.4 versus 34.4, p<0.001) compared to ERW-treated mice. Only a significant decrease of triglycerides in control mice compared to ERW-treated mice (52.8 versus 86.7, p<0.05) was observed after 17 weeks of age. In addition, at 23 weeks of age ERW-treated mice displayed a decreased level of mean corpuscular volume (reference values 43-58 μm³; 41.9 versus 44.1, p<0.01) as compared to control mice. It is important to note that control mice showed a marked decrease in the percentage of lymphocytes (reference values 50-75%; 34.2 versus 62.2, p<0.05) and a marked increase in the percentage of granulocytes (reference values 15-40%; 59.1 versus 30.3, p<0.05) as compared to ERW-treated mice, at the end of treatment. Conversely, the percentages of lymphocytes and granulocytes in the ERW-treated mice fell within the reference values (Table 3). Collectively, these results demonstrated that ERW did not affect hematological and clinical chemistry parameters and that the alterations observed in the control and ERW-treated mice are likely associated with tumor growth.

Table 3

Complete blood count (CBC) and clinical chemistry parameters in BALB-neuT mice treated with ERW or natural water (CTR).

CBC	Reference values	7 weeks of age		11 weeks of age		17 weeks of age		23 weeks of age		End of treatment
CBC	Reference values	CTR	ERW	CTR	ERW	CTR	ERW	CTR	ERW	CTR	ERW
WBC (10³/mm³)	5.0-12.0	5.1	5.5	7.5	3.9^#	5.2	5.2	5.3	3.8	5.2	10.5
LYM (10³/mm³)	4.0-10.0	3.2	3.8	4.6	2.6^#	2.9	3.4	3.0	2.1	1.4 $*$	6.5
GRAN (10³/mm³)	0.5-6.0	1.5	1.3	2.2	1.0	1.8	1.4	1.7	1.2	2.9	2.5
MID (10³/mm³)	0-2.0	0.5	0.4	0.6	0.4	0.5	0.5	0.6	0.5	0.4	1.4
LYM (%)	50.0-75.0	63.1	68.4	62.7	66.2	55.5	64.9	57.0	54.3	34.2 $^{x}$	62.2
GRAN (%)	15.0-40.0	28.9	23.6	30.0	26.3	35.4	27.5	33.1	35.0	59.1 $^{x}$	30.3
MID (%)	5.0-15.0	8.0	8.0	7.3	7.5	9.1	7.6	9.9	10.8	6.8	7.6
HCT (%)	35.0-60.0	53.5	52.2	57.8	50.8	54.3	54.6	55.6	47.5	50.2	42.7
MCV (μm³)	43.0-58.0	46.2	46.0	45.7	44.8	45.6	43.1	44.1	41.9 $*$	42.8	39.9
RBC (10⁶/mm³)	6.0-12.0	11.1	11.3	12.0	11.3	11.9	12.0	11.8	11.3	11.7	10.4
HGB (g/dl)	9.0-19.0	16.9	15.4	17.5	17.5	17.3	18.9	18.7	16.6	17.8	15.1
MCH (pg)	15.0-19.0	13.9	13.6	13.9^#	15.4	14.6	15.0	15.3	14.7	15.2	14.5
MCHC (g/dl)	34.0-39.0	29.8	29.6	30.4^#	34.4	32.0	35.2	34.7	35.0	35.5	36.3
RDW (%)	0-99.9	16.4	16.5	15.3	14.5	14.9	15.9	15.9	15.5	15.6	17.9
MPV (μm³)	4.0-7.0	5.8	5.8	5.8	6.0	5.7	5.9	5.8	5.8	6.4	6.2
PLT (10³/mm³)	250-1200	665.0	693.8	796.4	630.3	713.8	923.8	823.0	497.8	860.5	859.0

Clinical Chemistry

CHOL (mg/dl)	50-120	78.5	77.0	75.4	57.0	64.4	68.0	59.2	60.0	68.0	91.7
TRI (mg/dl)	80-200	89.5	104.0	122.6	54.0^#	52.8 $^{x}$	86.7	98.4	89.0	88.0	137.3
GOT (U/l)	20-250	131.0	81.0	82.2	83.0	90.4	65.0	90.0	133.0	67.0	123.3
GPT (U/l)	20-100	47.8	28.9	30.2	30.9	54.2	45.4	46.5	51.4	38.5	31.4
Glucose (mg/dl)	60-120	65.8	92.0	86.6	77.0	84.0	80.0	68.8	99.0	62.0	120.0
BUN (mg/dl)	10-40	28.3	10.0	20.2	22.0	22.0	23.8	23.0	22.5	23.0	22.3

CBC: complete blood count;CTR: control mice;ERW: mice treated with ERW;WBC: white blood cells; LYM: lymphocytes; GRAN: granulocytes; MID: mid-sized cells; HCT: hematocrit; MCV: mean corpuscular volume; RBC: red blood cells; HGB: hemoglobin; MCH: mean corpuscular hemoglobin; MCHC: mean corpuscular hemoglobin concentration; RDW: red cell distribution width; MPV: mean platelet volume; PLT: platelets; CHOL: cholesterol; TRI: triglycerides; GOT: serum Glutamic oxaloacetic transaminase; GPT: serum glutamic pyruvic transaminase; BUN: blood urea nitrogen ( $^{x}$ p ≤ 0.05, $*$ p ≤ 0.01, ^#p ≤ 0.001 compared with the control mice).

3.4. ERW Decreases ErbB2/neu Expression and Impairs Phospho-ERK1/ERK2 and AKT Phosphorylation

ErbB2/neu plays a critical role in breast cancer development [37]. Therefore, the interference of ERW treatment to the expression of ErbB2/neu and activation of ErbB2/neu signaling (pERK1/ERK2 and AKT) has been investigated. ERW decreased ErbB2/neu expression in MCF-7 (p=0.008), MDA-MB-453 (p= 0.002), and TUBO cells (p=0.014) as compared to autoclaved ERW (Figures 4 and S1). ERW treatment impaired ERK1 and ERK2 phosphorylation as compared to autoclaved ERW in MCF-7 cells (p=0.002 and p=0.0048, respectively). Conversely, ERW increased ERK1 and ERK2 phosphorylation in MDA-MB-453 (p=0.0001 and p=0.0004) cells and ERK2 in TUBO cells (p=0.006) (Figures 4 and S1). In addition, ERW treatment increased AKT phosphorylation at Ser473 as compared to autoclaved ERW only in MCF-7 (p=0.018) (Figures 4 and S1).

[figures omitted; refer to PDF]

3.5. ERW Induces Apoptosis of Breast Cancer Cell Lines

To determine ERW-mediated effects on cells cycle and apoptosis of breast cancer cells, FACS analysis of DNA content was performed. Figure 5 shows a representative experiment in which the effect of ERW on DNA content was compared to that obtained with autoclaved ERW and with control cultures. The mean results of three independent experiments are reported in Table 4. Our results demonstrated that ERW treatment induced an increase in the percentage of cells in the sub-G1 phase as compared to autoclaved ERW in MCF-7 (p<0.001), MDA-MB-453 (p<0.001), and TUBO (p<0.01) cells. The increase in the percentage of cells in sub-G1 phase was paralleled by the decrease of the percentage of cells in G0/G1 phase in MCF-7 (p<0.01), MDA-MB-453 (p<0.05), and in S and G2/M phases in TUBO cells (p<0.05) (Table 4 and Figure 5). To corroborate that the ERW increase in the percentage of cells in sub-G1 phase was partially caused by the induction of apoptosis, the Bax/Bcl-2 expression ratio was analyzed by Western blotting. ERW treatment increased the Bax/Bcl-2 ratio in both human and mouse cell lines compared to autoclaved ERW treatment (MCF-7, p=0.02; MDA-MB-453, p=0.01; TUBO, p=0.0046) (Figures 6 and S1). In addition, ERW and autoclaved ERW did not modulate the expression of p53 in MCF-7 cell line. Decreased PARP-1 expression upon ERW treatment was detected both in MCF-7 (p=0.001) and MDA-MB-453 (p=0.01) cells as compared to autoclaved ERW treatment (Figures 6 and S1).

Table 4

Effects of ERW on apoptosis and cell cycle distribution of breast cancer cells after 72 hours of treatment.

	Treatment	Sub-G1 ^†		G0/G1		S		G2/M
	Treatment	Mean ± SD	p-value	Mean ± SD	p-value	Mean ± SD	p-value	Mean ± SD	p-value
MCF-7	CTR	$3.08 \pm 0.64$		$61.93 \pm 1.81$		$12.66 \pm 0.64$		$22.70 \pm 1.80$
	Autoclaved ERW	$3.58 \pm 0.10$		$59.59 \pm 0.97$		$13.91 \pm 0.45$		$23.31 \pm 1.42$
	ERW	$19.60 \pm 0.48$	<0.001 ^1,2	$49.34 \pm 1.24$	<0.01 ^1,2	$11.88 \pm 0.54$		$19.57 \pm 1.28$

MDA-MB-453	CTR	$5.16 \pm 0.42$		$69.93 \pm 0.11$		$10.36 \pm 0.98$		$14.97 \pm 1.30$
	Autoclaved ERW	$5.61 \pm 0.35$		$73.60 \pm 2.63$		$9.16 \pm 0.45$		$11.85 \pm 1.81$
	ERW	$16.83 \pm 0.24$	<0.001 ^1,2	$61.18 \pm 2.45$	<0.05 ^1,2	$8.18 \pm 0.92$		$14.07 \pm 1.86$

TUBO	CTR	$6.65 \pm 0.72$		$45.89 \pm 2.95$		$15.13 \pm 1.90$		$32.81 \pm 0.32$
	Autoclaved ERW	$6.04 \pm 0.69$		$35.39 \pm 0.57$	<0.01 ¹	$18.31 \pm 0.89$		$40.75 \pm 2.04$	<0.05 ¹
	ERW	$26.98 \pm 3.95$	<0.01 ^1,2	$31.82 \pm 0.28$	<0.01 ¹	$7.75 \pm 1.79$	<0.05 ^1,2	$33.70 \pm 2.51$	<0.05 ²

$^{†}$ Percentages of cells in the sub-G1, G0/G1, S, and G2/M phase were calculated using Cell Quest Pro 5.2 software. Results represent mean values±standard deviation (SD) from three independent experiments. The statistical significance of the effects obtained with ERW and autoclaved ERW was calculated versus those obtained with ¹positive control medium (CTR) and ²autoclaved ERW.

[figure omitted; refer to PDF]

[figures omitted; refer to PDF]

4. Discussion

ERW has shown to possess (1) suppressive effects against oxidative stress, granting DNA protection [4, 9]; (2) carbon tetrachloride-induced liver damage reduction [38]; (3) alloxan-induced type 1 diabetes modulation [4, 39]; (4) hemodialysis-induced oxidative stress reduction during end-stage renal disease [40, 41]; (5) nephroprotective effects on cisplatin-induced kidney damage in mice [42]; and (6) suppressive effects on lipopolysaccharide-induced neuroinflammation [43]. Furthermore, Pt nanoparticles produced by electrode plates during electrolysis and visualized by transmission electron microscopy [1] can play an additional role in the ROS-scavenging activity of ERW [8].

Previous studies have reported anticancer effects of ERW on human lung adenocarcinoma cell line A549 [20], human leukemic HL-60 cells [21], squamous cell carcinoma-derived cell line HSC-4 [22], fibrosarcoma HT-1080 cells [8, 22, 44], human leukemic monocyte lymphoma cell line U937 [45], and BALB/c 3T3 cells [23]. Despite the possibility that ROS might play an underlying role in the oxidative damage process that is closely related to many chronic and inflammatory diseases including cancer, no effects on tumor growth have been previously studied in in vivo models using ERW water.

The present study has added information of ERW anticancer activity in never before tested human and mouse breast cancer cell lines, including BALB-neuT mammary cancer cells (H-2 $^{d}$ ) (TUBO), MCF-7, and MDA-MB-453. We demonstrated that ERW treatment inhibited cell survival, induced apoptosis of breast cancer cells, decreased ErbB2/neu expression, and impaired pERK1/ERK2 activation, as previously reported in another cell line [20]. The effect on ErbB2/neu expression could be linked to the antioxidant properties of ERW. It has been described that ErbB2 and ErbB3 expression can be induced by ROS and that ErbB2-dependent signaling contributes to antioxidant defenses [46, 47]. In addition, it has been described that flavonoids act as antioxidants and decreases the expression of ErbB2 and ErbB3 proteins in HT-29 human colon cancer [48]. Furthermore, Pt nanoparticles present in ERW can play a synergic effect in the viability reduction of tumor cells [49]. It has been suggested that Pt nanoparticles may serve as a reservoir for Pt ions that can induce DNA damage in cancer cells [50].

In addition, ERK1/2 MAP kinase signaling pathway is abnormally and frequently activated in human cancer [51] and plays a key role in cell proliferation. Here, we demonstrated that ERW down-regulates MAP kinases activity as compared to the autoclaved ERW in MCF-7 cells. The effect of ERW on ERK1/2 was opposite in the other cell lines. This opposite effect might be due to the expression of alternative pathways activation in different cell lines and might mirror the tumor heterogeneity occurring in human tumors. On the other hand, these cell lines were sensitive to the proapoptotic effect of ERW as well, thus suggesting that MAPK activation could trigger apoptosis in these cell lines. Indeed, it was reported that MAPK/ERK activation could protect or contribute to cell death depending on the specific context [52, 53].

In addition, we showed that ERW treatment induced a slight phosphorylation at Ser473 in MCF-7 cells. It has been reported that phosphorylation at Thr308 is necessary and sufficient for AKT activation, but the second phosphorylation at Ser473 is required for maximal activation of AKT [54]. AKT activation plays a key role in cell survival and tumor growth. However, despite AKT phosphorylation, we found that ERW inhibited cells survival, increased cell death, and inhibited ERK activation in this cell line. The contribution of the activation of AKT to cell death is not fully clear. However, a crosstalk between PI3K-AKT and Ras-Raf-MEK-ERK pathways has been reported. AKT inactivated c-Raf and B-Raf by directly phosphorylating them and thus inhibiting the MEK-ERK pathway in different cell lines [55–58]. In addition, different apoptotic stimuli, such as curcumin, taxol, etoposide, and staurosporine, are able to induce apoptosis and at the same time AKT phosphorylation in Ser473 [59]. Furthermore, it has been shown that AKT can induce phosphorylation of histone H2A and CDK2, signals that could favor the activation or maintenance of apoptosis [60, 61].

We also demonstrated that ERW induces apoptosis both in human and mouse breast cancer cell lines. In particular, we showed that the ERW-mediated increase in the percentage of cells in sub-G1 phase was caused by the induction of apoptosis, as confirmed by the increase in the ratio of the proapoptotic protein Bax to the antiapoptotic protein Bcl-2. It was previously reported that ERW induced apoptosis through the upregulation of Bax and downregulation of Bcl-2 in human leukemic HL-60 cells [21]. Of note, ERW induced apoptosis in both human and mouse breast cancer cell lines and ERW induced apoptosis was not dependent on p53 expression since ERW treatment triggered apoptosis also in MDA-MB-453 carrying mutated p53. In addition, cell death induced by ERW treatment was not dependent on ER and PR status. Our results showed that although the Bax/Blc-2 ratio increased in ERW-treated cultures as compared to autoclaved ERW, we did not observed the cleavage of PARP-1. However, we observed a significant downregulation of the expression of total PARP-1 in MCF-7 and MDA-MB-453 cells. PARP-1 is overexpressed in different types of cancer, including prostate, pancreatic, and breast, and it has been reported that decreased expression of PARP-1 inhibited cell proliferation and induced apoptosis in pancreatic cancer cells [62]. In addition, the degradation of PARP-1 mediated by caspase-independent ubiquitylation which has a role in apoptosis, necrosis, and other cellular processes has been reported [63–66]. Accordingly, the observed decrease of PARP-1 expression might confirm apoptosis activation.

This is the first time that an in vivo mouse model (BALB-neuT) is used to show the direct effects of ERW on cancer. Previous in vivo studies with ERW focused on other factors: nephroprotective effect of ERW against cisplatin-induced kidney toxicity and oxidative damage in mice [42] and antioxidant and anti-inflammatory effects of hydrogen-rich water in alleviating ethanol-induced fatty liver in mice [67]. Our in vivo study showed that BALB-neuT mice that drank ERW delayed the development of tumors compared to the control. In addition, ERW induced a significant prolongation of tumor-free survival and a reduction in tumor multiplicity. The increase in the median survival of ERW-treated mice was highly significant as compared to control mice (p=0.0001) and the relative risk of developing tumors in the control mice was 22.25 as compared to the ERW-treated mice. The observed inhibition of in vivo growth could be due to the direct effect of ERW on ErbB2 receptor that is abnormally activated in this mouse model, the impairment of its downstream effector MAPK ERK, and the induction of apoptosis. The overexpression of ErbB2 was reported to inhibit both the intrinsic and extrinsic pathway of apoptosis in breast cancer [68].

Furthermore, biochemical parameters did not differ significantly between ERW-treated group and control group. However, a slight difference was found on white cells count between day 11 and 17 (most lymphocytes and neutrophils). This modification is likely associated with advanced neoplastic stage in control mice. In fact ERW delayed the appearance of the tumor in the ERW-treated BALB-neuT mice as compared to control mice. A feasible mechanism could be also due to a decrease in the inflammatory state that would guarantee ERW-treated BALB-neuT mice a better immune surveillance towards the onset of the tumor.

Overall, our in vitro and in vivo results suggest a role of ERW in inhibiting cancer cell growth. Further studies are warranted to investigate ERW potential use in breast cancer treatment.

5. Conclusions

In this study, we show that ERW treatment inhibited cell survival, induced cell apoptosis, decreased ErbB2/neu expression, and impaired pERK1/ERK2 activation in breast cancer cells. In addition, our in vivo results showed that ERW induced a significant prolongation of tumor-free survival and a reduction in tumor multiplicity in transgenic BALB-neuT mice. Overall, these results suggest a potential beneficial role of ERW in inhibiting cancer cells growth. Further studies are warranted to investigate ERW potential use in breast cancer treatment.

Ethical Approval

The animal protocol was conducted with the formal approval of the local animal care committees (institutional and national), and animal experiments have been registered as legislation requires (Authorization from Ministry of Health number 875/2016-PR, 16/09/16).

Disclosure

Maurizio Mattei and Roberto Bei are co-last authors.

Conflicts of Interest

The authors declare that there are no conflicts of interest. Dott. Ivan Dus works for Nerò H2O d.o.o, Kraška Ulica 2, 6210 Sežana (SLO). This professional relationship does not, however, influence this author’s scientific neutrality.

Authors’ Contributions

Giovanni Vanni Frajese and Monica Benvenuto contributed equally to this work.

References

[1] S. Shirahata, T. Hamasaki, K. Teruya, "Advanced research on the health benefit of reduced water," Trends in Food Science & Technology, vol. 23 no. 2, pp. 124-131, DOI: 10.1016/j.tifs.2011.10.009, 2012.

[2] S. Giampaoli, F. Valeriani, G. Gianfranceschi, M. Vitali, M. Delfini, M. R. Festa, E. Bottari, V. Romano Spica, "Hydrogen sulfide in thermal spring waters and its action on bacteria of human origin," Microchemical Journal, vol. 108, pp. 210-214, DOI: 10.1016/j.microc.2012.10.022, 2013.

[3] S. Shirahata, Y. Li, T. Hamasaki, "Redox regulation by reduced water as active hydrogen donors and intracellular ROS scavengers for prevention of type 2 diabetes," Cell Technology for Cell Products, pp. 99-101, DOI: 10.1007/978-1-4020-5476-1, 2007.

[4] Y. Li, T. Nishimura, K. Teruya, "Protective mechanism of reduced water against alloxan-induced pancreatic beta-cell damage: Scavenging effect against reactive oxygen species," Cytotechnology, vol. 40, pp. 139-149, 2002.

[5] T. Kashiwagi, H. Yan, T. Hamasaki, "Electrochemically Reduced Water Protects Neural Cells from Oxidative Damage," Oxidative Medicine and Cellular Longevity, vol. 2014,DOI: 10.1155/2014/869121, 2014.

[6] T. Hamasaki, T. Kashiwagi, T. Imada, N. Nakamichi, S. Aramaki, K. Toh, S. Morisawa, H. Shimakoshi, Y. Hisaeda, S. Shirahata, "Kinetic analysis of superoxide anion radical-scavenging and hydroxyl radical-scavenging activities of platinum nanoparticles," Langmuir, vol. 24 no. 14, pp. 7354-7364, DOI: 10.1021/la704046f, 2008.

[7] M. Kajita, K. Hikosaka, M. Iitsuka, A. Kanayama, N. Toshima, Y. Miyamoto, "Platinum nanoparticle is a useful scavenger of superoxide anion and hydrogen peroxide," Free Radical Research, vol. 41 no. 6, pp. 615-626, DOI: 10.1080/10715760601169679, 2007.

[8] T. Hamasaki, G. Harada, N. Nakamichi, S. Kabayama, K. Teruya, B. Fugetsu, W. Gong, I. Sakata, S. Shirahata, "Electrochemically reduced water exerts superior reactive oxygen species scavenging activity in HT1080 cells than the equivalent level of hydrogen-dissolved water," PLoS ONE, vol. 12 no. 2,DOI: 10.1371/journal.pone.017119, 2017.

[9] S. Shirahata, S. Kabayama, M. Nakano, T. Miura, K. Kusumoto, M. Gotoh, H. Hayashi, K. Otsubo, S. Morisawa, Y. Katakura, "Electrolyzed-reduced water scavenges active oxygen species and protects DNA from oxidative damage," Biochemical and Biophysical Research Communications, vol. 234 no. 1, pp. 269-274, DOI: 10.1006/bbrc.1997.6622, 1997.

[10] M. Oda, K. Kusumoto, K. Teruya, "Electrolyzed and natural reduced water exhibit insulin-like activity on glucose uptake into muscle cells and adipocytes," Animal cell technology: products from cells, pp. 425-427, 1999.

[11] D. Jin, S. H. Ryu, H. W. Kim, E. J. Yang, S. J. Lim, Y. S. Ryang, C. H. Chung, S. K. Park, K. J. Lee, "Anti-diabetic effect of alkaline-reduced water on OLETF rats," Bioscience, Biotechnology, and Biochemistry, vol. 70 no. 1, pp. 31-37, DOI: 10.1271/bbb.70.31, 2006.

[12] M.-J. Kim, K. H. Jung, Y. K. Uhm, K.-H. Leem, H. K. Kim, "Preservative effect of electrolyzed reduced water on pancreatic β -cell mass in diabetic db/db mice," Biological & Pharmaceutical Bulletin, vol. 30 no. 2, pp. 234-236, DOI: 10.1248/bpb.30.234, 2007.

[13] M.-J. Kim, H. K. Kim, "Anti-diabetic effects of electrolyzed reduced water in streptozotocin-induced and genetic diabetic mice," Life Sciences, vol. 79 no. 24, pp. 2288-2292, DOI: 10.1016/j.lfs.2006.07.027, 2006.

[14] I. Ohsawa, M. Ishikawa, K. Takahashi, M. Watanabe, K. Nishimaki, K. Yamagata, K. Katsura, Y. Katayama, S. Asoh, S. Ohta, "Hydrogen acts as a therapeutic antioxidant by selectively reducing cytotoxic oxygen radicals," Nature Medicine, vol. 13 no. 6, pp. 688-694, DOI: 10.1038/nm1577, 2007.

[15] N. Kamimura, K. Nishimaki, I. Ohsawa, S. Ohta, "Molecular hydrogen improves obesity and diabetes by inducing hepatic FGF21 and stimulating energy metabolism in db/db mice," Obesity, vol. 19 no. 7, pp. 1396-1403, DOI: 10.1038/oby.2011.6, 2011.

[16] G. Song, C. Zong, Z. Zhang, Y. Yu, S. Yao, P. Jiao, H. Tian, L. Zhai, H. Zhao, S. Tian, X. Zhang, Y. Wu, X. Sun, S. Qin, "Molecular hydrogen stabilizes atherosclerotic plaque in low-density lipoprotein receptor-knockout mice," Free Radical Biology & Medicine, vol. 87, pp. 58-68, DOI: 10.1016/j.freeradbiomed.2015.06.018, 2015.

[17] T. Yokota, N. Kamimura, T. Igarashi, H. Takahashi, S. Ohta, H. Oharazawa, "Protective effect of molecular hydrogen against oxidative stress caused by peroxynitrite derived from nitric oxide in rat retina," Clinical & Experimental Ophthalmology, vol. 43 no. 6, pp. 568-577, DOI: 10.1111/ceo.12525, 2015.

[18] J. Yu, W. Zhang, R. Zhang, G. Jiang, H. Tang, X. Ruan, P. Ren, B. Lu, "Molecular hydrogen attenuates hypoxia/reoxygenation injury of intrahepatic cholangiocytes by activating Nrf2 expression," Toxicology Letters, vol. 238 no. 3, pp. 11-19, DOI: 10.1016/j.toxlet.2015.08.010, 2015.

[19] Y. Zhai, X. Zhou, Q. Dai, Y. Fan, X. Huang, "Hydrogen-rich saline ameliorates lung injury associated with cecal ligation and puncture-induced sepsis in rats," Experimental and Molecular Pathology, vol. 98 no. 2, pp. 268-276, DOI: 10.1016/j.yexmp.2015.03.005, 2015.

[20] J. Ye, Y. Li, T. Hamasaki, N. Nakamichi, T. Komatsu, T. Kashiwagi, K. Teruya, R. Nishikawa, T. Kawahara, K. Osada, K. Toh, M. Abe, H. Tian, S. Kabayama, K. Otsubo, S. Morisawa, Y. Katakura, S. Shirahata, "Inhibitory effect of electrolyzed reduced water on tumor angiogenesis," Biological & Pharmaceutical Bulletin, vol. 31 no. 1, pp. 19-26, DOI: 10.1248/bpb.31.19, 2008.

[21] C.-F. Tsai, Y.-W. Hsu, W.-K. Chen, Y.-C. Ho, F.-J. Lu, "Enhanced induction of mitochondrial damage and apoptosis in human leukemia HL-60 cells due to electrolyzed-reduced water and glutathione," Bioscience, Biotechnology, and Biochemistry, vol. 73 no. 2, pp. 280-287, DOI: 10.1271/bbb.80413, 2009.

[22] Y. Saitoh, H. Okayasu, L. Xiao, Y. Harata, N. Miwa, "Neutral pH hydrogen-enriched electrolyzed water achieves tumor-preferential clonal growth inhibition over normal cells and tumor invasion inhibition concurrently with intracellular oxidant repression," Oncology Research : Featuring Preclinical and Clinical Cancer Therapeutics, vol. 17 no. 6, pp. 247-255, DOI: 10.3727/096504008786991620, 2008.

[23] R. Nishikawa, K. Teruya, Y. Katakura, K. Osada, T. Hamasaki, T. Kashiwagi, T. Komatsu, Y. Li, J. Ye, A. Ichikawa, K. Otsubo, S. Morisawa, Q. Xu, S. Shirahata, "Electrolyzed reduced water supplemented with platinum nanoparticles suppresses promotion of two-stage cell transformation," Cytotechnology, vol. 47 no. 1-3, pp. 97-105, DOI: 10.1007/s10616-005-3759-2, 2005.

[24] K. Boggio, G. Nicoletti, E. Di Carlo, F. Cavallo, L. Landuzzi, C. Melani, M. Giovarelli, I. Rossi, P. Nanni, C. De Giovanni, P. Bouchard, S. Wolf, A. Modesti, P. Musiani, P. L. Lollini, M. P. Colombo, G. Forni, "Interleukin 12-mediated prevention of spontaneous mammary adenocarcinomas in two lines of HER-2/neu transgenic mice," The Journal of Experimental Medicine, vol. 188 no. 3, pp. 589-596, DOI: 10.1084/jem.188.3.589, 1998.

[25] S. Rovero, A. Amici, E. Di Carlo, R. Bei, P. Nanni, E. Quaglino, P. Porcedda, K. Boggio, A. Smorlesi, P.-L. Lollini, L. Landuzzi, M. P. Colombo, M. Giovarelli, P. Musiani, G. Forni, "DNA vaccination against rat Her-2/Neu p185 more effectively inhibits carcinogenesis than transplantable carcinomas in transgenic BALB/c mice," The Journal of Immunology, vol. 165 no. 9, pp. 5133-5142, DOI: 10.4049/jimmunol.165.9.5133, 2000.

[26] L. Masuelli, M. Benvenuto, E. Di Stefano, R. Mattera, M. Fantini, G. De Feudis, E. De Smaele, I. Tresoldi, M. G. Giganti, A. Modesti, R. Bei, "Curcumin blocks autophagy and activates apoptosis of malignant mesothelioma cell lines and increases the survival of mice intraperitoneally transplanted with a malignant mesothelioma cell line," Oncotarget, vol. 8 no. 21, pp. 34405-34422, 2017.

[27] L. Masuelli, E. Di Stefano, M. Fantini, R. Mattera, M. Benvenuto, L. Marzocchella, P. Sacchetti, C. Focaccetti, R. Bernardini, I. Tresoldi, V. Izzi, M. Mattei, G. V. Frajese, F. Lista, A. Modesti, R. Bei, "Resveratrol potentiates the in vitro and in vivo anti-tumoral effects of curcumin in head and neck carcinomas," Oncotarget, vol. 5 no. 21, pp. 10745-10762, DOI: 10.18632/oncotarget.2534, 2014.

[28] M. Benvenuto, P. Sileri, P. Rossi, L. Masuelli, M. Fantini, M. Nanni, L. Franceschilli, G. Sconocchia, G. Lanzilli, R. Arriga, G. Faggioni, F. Lista, A. Orlandi, V. Manzari, A. L. Gaspari, A. Modesti, R. Bei, "Natural humoral immune response to ribosomal P0 protein in colorectal cancer patients," Journal of Translational Medicine, vol. 13 no. 1, article 101,DOI: 10.1186/s12967-015-0455-7, 2015.

[29] L. Masuelli, M. Benvenuto, M. Fantini, "Curcumin induces apoptosis in breast cancer cell lines and delays the growth of mammary tumors in neu transgenic mice," Journal of BIOLOGICAL REGULATORS & Homeostatic Agents, vol. 27, pp. 105-119, 2013.

[30] L. Masuelli, A. Budillon, L. Marzocchella, M.-A. Mrozek, D. Vitolo, E. Di Gennaro, S. Losito, P. Sale, F. Longo, F. Ionna, F. Lista, R. Muraro, A. Modesti, R. Bei, "Caveolin-1 overexpression is associated with simultaneous abnormal expression of the E-cadherin/ α - β catenins complex and multiple erbb receptors and with lymph nodes metastasis in head and neck squamous cell carcinomas," Journal of Cellular Physiology, vol. 227 no. 9, pp. 3344-3353, DOI: 10.1002/jcp.24034, 2012.

[31] L. Masuelli, L. Marzocchella, C. Focaccetti, I. Tresoldi, C. Palumbo, V. Izzi, M. Benvenuto, M. Fantini, F. Lista, U. Tarantino, A. Modesti, F. Galvano, R. Bei, "Resveratrol and diallyl disulfide enhance curcumin-induced sarcoma cell apoptosis," Frontiers in Bioscience, vol. 17 no. 2, pp. 498-508, DOI: 10.2741/3940, 2012.

[32] R. M. Neve, K. Chin, J. Fridlyand, J. Yeh, F. L. Baehner, T. Fevr, L. Clark, N. Bayani, J.-P. Coppe, F. Tong, T. Speed, P. T. Spellman, S. DeVries, A. Lapuk, N. J. Wang, W.-L. Kuo, J. L. Stilwell, D. Pinkel, D. G. Albertson, F. M. Waldman, F. McCormick, R. B. Dickson, M. D. Johnson, M. Lippman, S. Ethier, A. Gazdar, J. W. Gray, "A collection of breast cancer cell lines for the study of functionally distinct cancer subtypes," Cancer Cell, vol. 10 no. 6, pp. 515-527, DOI: 10.1016/j.ccr.2006.10.008, 2006.

[33] E. Charafe-Jauffret, C. Ginestier, F. Monville, P. Finetti, J. Adélaïde, N. Cervera, S. Fekairi, L. Xerri, J. Jacquemier, D. Birnbaum, F. Bertucci, "Gene expression profiling of breast cell lines identifies potential new basal markers," Oncogene, vol. 25 no. 15, pp. 2273-2284, DOI: 10.1038/sj.onc.1209254, 2006.

[34] L. B. Eckert, G. A. Repasky, A. S. Ülkü, A. McFall, H. Zhou, C. I. Sartor, C. J. Der, "Involvement of ras activation in human breast cancer cell signaling, invasion, and anoikis," Cancer Research, vol. 64 no. 13, pp. 4585-4592, DOI: 10.1158/0008-5472.CAN-04-0396, 2004.

[35] M. Lacroix, R.-A. Toillon, G. Leclercq, "p53 and breast cancer, an update," Endocrine-Related Cancer, vol. 13 no. 2, pp. 293-325, DOI: 10.1677/erc.1.01172, 2006.

[36] S. Vranic, Z. Gatalica, Z.-Y. Wang, "Update on the molecular profile of the MDA-MB-453 cell line as a model for apocrine breast carcinoma studies," Oncology Letters, vol. 2 no. 6, pp. 1131-1137, DOI: 10.3892/ol.2011.375, 2011.

[37] S. A. Eccles, "The epidermal growth factor receptor/Erb-B/HER family in normal and malignant breast biology," The International Journal of Developmental Biology, vol. 55 no. 7-9, pp. 685-696, DOI: 10.1387/ijdb.113396se, 2011.

[38] C. Tsai, Y. Hsu, W. Chen, W. Chang, C. Yen, Y. Ho, F. Lu, "Hepatoprotective effect of electrolyzed reduced water against carbon tetrachloride-induced liver damage in mice," Food and Chemical Toxicology, vol. 47 no. 8, pp. 2031-2036, DOI: 10.1016/j.fct.2009.05.021, 2009.

[39] Y. Li, T. Hamasaki, N. Nakamichi, T. Kashiwagi, T. Komatsu, J. Ye, K. Teruya, M. Abe, H. Yan, T. Kinjo, S. Kabayama, M. Kawamura, S. Shirahata, "Suppressive effects of electrolyzed reduced water on alloxan-induced apoptosis and type 1 diabetes mellitus," Cytotechnology, vol. 63 no. 2, pp. 119-131, DOI: 10.1007/s10616-010-9317-6, 2011.

[40] K.-C. Huang, C.-C. Yang, K.-T. Lee, C.-T. Chien, "Reduced hemodialysis-induced oxidative stress in end-stage renal disease patients by electrolyzed reduced water," Kidney International, vol. 64 no. 2, pp. 704-714, DOI: 10.1046/j.1523-1755.2003.00118.x, 2003.

[41] M. Nakayama, H. Nakano, H. Hamada, N. Itami, R. Nakazawa, S. Ito, "A novel bioactive haemodialysis system using dissolved dihydrogen (H2) produced by water electrolysis: A clinical trial," Nephrology Dialysis Transplantation, vol. 25 no. 9, pp. 3026-3033, DOI: 10.1093/ndt/gfq196, 2010.

[42] T. C. Cheng, Y. W. Hsu, F. J. Lu, "Nephroprotective effect of electrolyzed reduced water against cisplatin-induced kidney toxicity and oxidative damage in mice," Journal of the Chinese Medical Association, 2017.

[43] S. Spulber, K. Edoff, L. Hong, S. Morisawa, S. Shirahata, S. Ceccatelli, "Molecular hydrogen reduces lps-induced neuroinflammation and promotes recovery from sickness behaviour in mice," PLoS ONE, vol. 7 no. 7,DOI: 10.1371/journal.pone.0042078, 2012.

[44] T. Kinjo, J. Ye, H. Yan, T. Hamasaki, H. Nakanishi, K. Toh, N. Nakamichi, S. Kabayama, K. Teruya, S. Shirahata, "Suppressive effects of electrochemically reduced water on matrix metalloproteinase-2 activities and in vitro invasion of human fibrosarcoma HT1080 cells," Cytotechnology, vol. 64 no. 3, pp. 357-371, DOI: 10.1007/s10616-012-9469-7, 2012.

[45] S. Franceschelli, D. Gatta, M. Pesce, A. Ferrone, A. Patruno, M. de Lutiis, A. Grilli, M. Felaco, F. Croce, L. Speranza, "New Approach in Translational Medicine: Effects of Electrolyzed Reduced Water (ERW) on NF- κ B/iNOS Pathway in U937 Cell Line under Altered Redox State," International Journal of Molecular Sciences, vol. 17 no. 9,DOI: 10.3390/ijms17091461, 2016.

[46] J. He, Q. Xu, Y. Jing, F. Agani, X. Qian, R. Carpenter, Q. Li, X.-R. Wang, S. S. Peiper, Z. Lu, L.-Z. Liu, B.-H. Jiang, "Reactive oxygen species regulate ERBB2 and ERBB3 expression via miR-199a/125b and DNA methylation," EMBO Reports, vol. 13 no. 12, pp. 1116-1122, DOI: 10.1038/embor.2012.162, 2012.

[47] F. Belmonte, S. Das, P. Sysa-Shah, V. Sivakumaran, B. Stanley, X. Guo, N. Paolocci, M. A. Aon, M. Nagane, P. Kuppusamy, C. Steenbergen, K. Gabrielson, "ErbB2 overexpression upregulates antioxidant enzymes, reduces basal levels of reactive oxygen species, and protects against doxorubicin cardiotoxicity," American Journal of Physiology-Heart and Circulatory Physiology, vol. 309 no. 8, pp. H1271-H1280, DOI: 10.1152/ajpheart.00517.2014, 2015.

[48] W. K. Kim, M. H. Bang, E. S. Kim, N. E. Kang, K. C. Jung, H. J. Cho, J. H. Y. Park, "Quercetin decreases the expression of ErbB2 and ErbB3 proteins in HT-29 human colon cancer cells," The Journal of Nutritional Biochemistry, vol. 16 no. 3, pp. 155-162, DOI: 10.1016/j.jnutbio.2004.10.010, 2005.

[49] M. Kutwin, E. Sawosz, S. Jaworski, M. Hinzmann, M. Wierzbicki, A. Hotowy, M. Grodzik, A. Winnicka, A. Chwalibog, "Investigation of platinum nanoparticle properties against U87 glioblastoma multiforme," Archives of Medical Science, vol. 13 no. 6, pp. 1322-1334, DOI: 10.5114/aoms.2016.58925, 2017.

[50] M. Yamada, M. Foote, T. W. Prow, "Therapeutic gold, silver, and platinum nanoparticles," Wiley Interdisciplinary Reviews: Nanomedicine and Nanobiotechnology, vol. 7 no. 3, pp. 428-445, DOI: 10.1002/wnan.1322, 2015.

[51] C. A. Pratilas, D. B. Solit, "Targeting the mitogen-activated protein kinase pathway: Physiological feedback and drug response," Clinical Cancer Research, vol. 16 no. 13, pp. 3329-3334, DOI: 10.1158/1078-0432.CCR-09-3064, 2010.

[52] S. Zhuang, R. G. Schnellmann, "A death-promoting role for extracellular signal-regulated kinase," The Journal of Pharmacology and Experimental Therapeutics, vol. 319 no. 3, pp. 991-997, DOI: 10.1124/jpet.106.107367, 2006.

[53] S. Cagnol, J. C. Chambard, "ERK and cell death: Mechanisms of ERK-induced cell death—apoptosis, autophagy and senescence," FEBS Journal, vol. 277 no. 1,DOI: 10.1111/j.1742-4658.2009.07366.x, 2010.

[54] D. Liu, Y. Huang, B. Chen, J. Zeng, N. Guo, S. Zhang, L. Liu, H. Xu, X. Mo, W. Li, "Activation of mammalian target of rapamycin pathway confers adverse outcome in nonsmall cell lung carcinoma," Cancer, vol. 117 no. 16, pp. 3763-3773, DOI: 10.1002/cncr.25959, 2011.

[55] C. Rommel, B. A. Clarke, S. Zimmermann, L. Nuñez, R. Rossman, K. Reid, K. Moelling, G. D. Yancopoulos, D. J. Glass, "Differentiation stage-specific inhibition of the Raf-MEK-ERK pathway by Akt," Science, vol. 286 no. 5445, pp. 1738-1741, DOI: 10.1126/science.286.5445.1738, 1999.

[56] S. Zimmermann, K. Moelling, "Phosphorylation and regulation of Raf by Akt (protein kinase B)," Science, vol. 286 no. 5445, pp. 1741-1744, DOI: 10.1126/science.286.5445.1741, 1999.

[57] K.-L. Guan, C. Figueroa, T. R. Brtva, T. Zhu, J. Taylor, T. D. Barber, A. B. Vojtek, "Negative regulation of the serine/threonine kinase B-Raf by Akt," The Journal of Biological Chemistry, vol. 275 no. 35, pp. 27354-27359, DOI: 10.1074/jbc.M004371200, 2000.

[58] H. P. Reusch, S. Zimmermann, M. Schaefer, M. Paul, K. Moelling, "Regulation of Raf by Akt Controls Growth and Differentiation in Vascular Smooth Muscle Cells," The Journal of Biological Chemistry, vol. 276 no. 36, pp. 33630-33637, DOI: 10.1074/jbc.M105322200, 2001.

[59] D. Tang, H. Okada, J. Ruland, L. Liu, V. Stambolic, T. W. Mak, A. J. Ingram, "Akt Is Activated in Response to an Apoptotic Signal," The Journal of Biological Chemistry, vol. 276 no. 32, pp. 30461-30466, DOI: 10.1074/jbc.M102045200, 2001.

[60] J. H. Park, C. K. Kim, S. B. Lee, K. Lee, S. Cho, J. Ahn, "Akt attenuates apoptotic death through phosphorylation of H2A under hydrogen peroxide-induced oxidative stress in PC12 cells and hippocampal neurons," Scientific Reports, vol. 6 no. 1,DOI: 10.1038/srep21857, 2016.

[61] S. Maddika, S. R. Ande, E. Wiechec, L. L. Hansen, S. Wesselborg, M. Los, "Akt-mediated phosphorylation of CDK2 regulates its dual role in cell cycle progression and apoptosis," Journal of Cell Science, vol. 121 no. 7, pp. 979-988, DOI: 10.1242/jcs.009530, 2008.

[62] Z. Hou, Y. Cui, H. Xing, X. Mu, "Down-expression of poly(ADP-ribose) polymerase in p53-regulated pancreatic cancer cells," Oncology Letters, vol. 15, pp. 1943-1948, DOI: 10.3892/ol.2017.7500, 2018.

[63] C. Guillouf, J.-P. Vit, F. Rosselli, "Loss of the Fanconi anemia group C protein activity results in an inability to activate caspase-3 after ionizing radiation," Biochimie, vol. 82 no. 1, pp. 51-58, DOI: 10.1016/S0300-9084(00)00359-X, 2000.

[64] T. Wang, C. M. Simbulan-Rosenthal, M. E. Smulson, P. B. Chock, D. C. H. Yang, "Polyubiquitylation of PARP-1 through ubiquitin K48 is modulated by activated DNA, NAD+, and dipeptides," Journal of Cellular Biochemistry, vol. 104 no. 1, pp. 318-328, DOI: 10.1002/jcb.21624, 2008.

[65] S. Matsushima, N. Okita, M. Oku, W. Nagai, M. Kobayashi, Y. Higami, "An Mdm2 antagonist, Nutlin-3a, induces p53-dependent and proteasome-mediated poly(ADP-ribose) polymerase1 degradation in mouse fibroblasts," Biochemical and Biophysical Research Communications, vol. 407 no. 3, pp. 557-561, DOI: 10.1016/j.bbrc.2011.03.061, 2011.

[66] W. Nagai, N. Okita, H. Matsumoto, H. Okado, M. Oku, Y. Higami, "Reversible induction of PARP1 degradation by p53-inducible cis-imidazoline compounds," Biochemical and Biophysical Research Communications, vol. 421 no. 1, pp. 15-19, DOI: 10.1016/j.bbrc.2012.03.091, 2012.

[67] C. Lin, W. Chuang, F. Lu, C. Chen, "Anti-oxidant and anti-inflammatory effects of hydrogen-rich water alleviate ethanol-induced fatty liver in mice," World Journal of Gastroenterology, vol. 23 no. 27, pp. 4920-4934, DOI: 10.3748/wjg.v23.i27.4920, 2017.

[68] R. L. Carpenter, H. W. Lo, "Regulation of Apoptosis by HER2 in Breast Cancer," Journal of Carcinogenesis & Mutagenesis,DOI: 10.4172/2157-2518.S7-003, 2013.

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Copyright © 2018 Giovanni Vanni Frajese et al. This is an open access article distributed under the Creative Commons Attribution License (the “License”), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited. Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License. https://creativecommons.org/licenses/by/4.0/

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Electrochemical reduced water (ERW) has been proposed to have beneficial effects on human health due to its rich content of H₂ and the presence of platinum nanoparticles with antioxidant effects. Many studies have demonstrated that ERW scavenging properties are able to reduce the damage caused by oxidative stress in different experimental models. Although few in vivo studies have been reported, it has been demonstrated that ERW may display anticancer effects by induction of tumor cells apoptosis and reduction of both angiogenesis and inflammation. In this study, we show that ERW treatment of MCF-7, MDA-MB-453, and mouse (TUBO) breast cancer cells inhibited cell survival in a time-dependent fashion. ERW decreased ErbB2/neu expression and impaired pERK1/ERK2 and AKT phosphorylation in breast cancer cells. In addition, ERW treatment induced apoptosis of breast cancer cell lines independently of the status of p53 and ER and PR receptors. Our in vivo results showed that ERW treatment of transgenic BALB-neuT mice delayed the development of mammary tumors compared to the control. In addition, ERW induced a significant prolongation of tumor-free survival and a reduction in tumor multiplicity. Overall, these results suggest a potential beneficial role of ERW in inhibiting cancer cells growth.

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Title

Electrochemically Reduced Water Delays Mammary Tumors Growth in Mice and Inhibits Breast Cancer Cells Survival In Vitro

Author

Giovanni Vanni Frajese¹

; Benvenuto, Monica²

; Mattera, Rosanna²

; Giampaoli, Saverio¹; Ambrosin, Elena³; Bernardini, Roberta⁴

; Giganti, Maria Gabriella²; Albonici, Loredana²; Dus, Ivan⁵; Manzari, Vittorio²; Modesti, Andrea²; Mattei, Maurizio⁴

; Bei, Roberto²

¹ Department of Movement, Human and Health Sciences, University of Rome “Foro Italico”, 00135 Rome, Italy
² Department of Clinical Sciences and Translational Medicine, University of Rome “Tor Vergata”, 00133 Rome, Italy
³ Department of Agriculture, Environment and Food, University of Molise, 86100 Campobasso, Italy
⁴ STA, University of Rome “Tor Vergata”, 00133 Rome, Italy
⁵ Nerò H2O d.o.o, Kraška Ulica 2, 6210 Sežana, Slovenia

Editor

Ho Lin

Publication year

2018

Publication date

2018

Publisher

John Wiley & Sons, Inc.

ISSN

1741427X

e-ISSN

17414288

Source type

Scholarly Journal

Language of publication

English

DOI

https://doi.org/10.1155/2018/4753507

ProQuest document ID

2116805769

Electrochemically Reduced Water Delays Mammary Tumors Growth in Mice and Inhibits Breast Cancer Cells Survival In Vitro

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