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    Quercetin exerts anti-inflammatory effects via inhibiting tumor necrosis factor-α-induced matrix metalloproteinase-9 expression in normal human gastric epithelial cells

    2022-03-31 08:07:46HsiLungHsiehMingChinYuLiChingChengMeiYiChuTzuHaoHuangTaSenYehMingMingTsai
    World Journal of Gastroenterology 2022年11期

    Hsi-Lung Hsieh,Ming-Chin Yu, Li-Ching Cheng, Mei-Yi Chu, Tzu-Hao Huang, Ta-Sen Yeh, Ming-Ming Tsai

    Abstract

    Key Words: Anti-inflammatory; Quercetin; Matrix metallopeptidase-9 ; Tumor necrosis factor-α; Normal human gastric epithelial cells

    lNTRODUCTlON

    Gastric diseases are among the most common aliments of the digestive system worldwide and include chronic gastritis, duodenal and gastric ulceration, gastric mucosa-associated lymphoid tissue lymphoma, and gastric cancer (GC)[1 -3 ]. Gastric diseases have multifaceted causes that are related to the growing use of nonsteroidal anti-inflammatory drugs (NSAIDs), pathogen-mediated factors [such asHelicobacter pylori(H. pylori) infection], environmental factors (such as alcohol consumption, salt intake,and cigarette smoking), and host genetic and other factors (such as genetic polymorphisms, psychological stress, oxidative stress, and acidity)[4 ,5 ]. Gastric diseases accompanied by chronic inflammation involve increased neutrophil and mononuclear cell activities and the release of proinflammatory chemokines and cytokines, such as tumor necrosis factor-α (TNF-α)[6 ], interleukin (IL)-1 [7 ], IL-6 , IL-8 ,and IL-10 [8 ], cell adhesion molecules [such as circular dichroism 44 and intercellular adhesion molecule-1 (ICAM-1 )][9 ], and metalloproteinases (MMPs)[10 ]. The induction of MMPs is a major pathological feature and plays a critical role in the progression of gastric diseases[2 ,11 ,12 ]. Among the variants of genetic polymorphisms related to proinflammatory cytokines, those involving ILs and TNF-α are the most extensively studied.

    TNF-α is a multifunctional cytokine that was first identified as a serum factor causing necrosis of transplanted tumors. This cytokine participates in the regulation of immune-inflammatory reactions involved in host defense against infectious, autoimmune, and endocrine diseases and cancer, and its actions help to determine the survival or death of various cells[13 -16 ]. The upregulation of TNF-α and its related pathways is associated with some gastric diseases. Excessive TNF-α expression is associated with tumor promotionviaa strong immune-inflammatory response and angiogenesis, which can modify the risk for gastric, breast, hepatocellular, cervical, or bladder carcinoma[17 -20 ]. Harris et al[21 ]reported thatH. pyloriinfection upregulates TNF-α expression and that this upregulation decreases gastric acid secretion[21 ]. Fan et al[22 ] reported that high expression of TNF-α can stimulate normal gastric epithelial cells to develop into precancerous cells and that these cells may eventually develop into GC. A similar mechanism is also noted in chronic gastritis, intestinal metaplasia, and dysplasia[22 ].

    MMPs are a key group of enzymes that can destroy nearly all elements of the extracellular matrix,including components of the basement membrane[23 ,24 ]. MMP-9 expression damages the extracellular matrix, including components of the basement membrane, inducing gastric disease. MMP-9 is often upregulated or dysregulated in severe gastric disease, where it may accelerate severe gastric inflammation and possibly contribute to the development of GC. High MMP-9 expression is also associated with a poor survival rate in patients with GC[25 -28 ]. MMP-9 is induced in a nuclear factor kappa B (NFκB)-dependent manner[29 ,30 ]. Understanding the roles of inflammatory mediators may provide a basis for new therapeutic approaches for treating gastric inflammatory diseases.

    Recent research suggests that dietary intake may alter the risk of gastric injury[31 ,32 ]. A frequently studied dietary component, quercetin, is a flavonoid polyphenolic compound that is abundant in fruits,red wine, and vegetables. Studies on the bioactivity of quercetin have found that it exerts many favorable effects on human health, such as antioxidant, anti-inflammatory, anticancer, antiallergic,antiviral, free radical-scavenging, and neuroprotective activities[33 ,34 ].

    Quercetin protects gastric mucosal epithelial cells against injury caused by ischemia-reperfusion[35 ],ethanol[36 ], indomethacin[9 ], hydrogen peroxide[10 ], or H. pylori[37 ] in various animal models[38 ].Quercetin also exerts gastroprotective activity against TNF-α-induced injury to the gastric mucosal epithelium, but the mechanisms responsible for this effect remain unknown. Here, we explored whether quercetin protects against TNF-α-induced MMP-9 damage to gastric mucosal epithelial cells. We examined the responses of the human gastric mucosal epithelial cell line GES-1 to challenge with immune-inflammatory reactions mediated by TNF-α and explored the underlying molecular mechanisms.

    MATERlALS AND METHODS

    Materials

    Roswell Park Memorial Institute (RPMI) 1640 medium, fetal bovine serum (FBS), and TRIzol were purchased from Invitrogen (Carlsbad, CA, United States). Polyvinylidene fluoride (PVDF) membranes,enhanced chemiluminescence (ECL), and Western blot detection systems were obtained from GE Healthcare Biosciences (Chalfont St Giles, Buckinghamshire, United Kingdom). Anti-phospho-c-Src(Cat#2101 ), anti-phospho-ERK1 /2 (Cat#4377 ), anti-phospho-c-Fos (Cat#5348 ), anti-phospho-NF-κB(p65 ) (Cat#3033 ), c-Src (Cat#2109 ), ERK2 (Cat#9108 ), c-Fos (Cat#2250 ), NF-κB (Cat#8242 ), and antiglyceraldehyde-3 -phosphate dehydrogenase (GAPDH) (Cat#2118 ) antibodies were purchased from Cell Signaling Technology (Danvers, MA, United States). Anti-mouse (Cat# 7056 ) and anti-rabbit (Cat# 5054 )horseradish peroxidase-conjugated secondary antibodies were purchased from Santa Cruz Biotechnology (Santa Cruz, CA, United States). 4 ’,6 -Diamidino-2 -phenylindole was purchased from Vector Laboratories (Burlingame, CA, United States). TurboFect Transfection Reagent was purchased from Thermo Fisher Scientific (Waltham, MA, United States). The iScript cDNA Synthesis Kit, SsoFast EvaGreen Supermix, and CFX Connect Real-Time polymerase chain reaction (PCR) detection system were obtained from Bio-Rad Laboratories, Inc. (Hercules, CA, United States). A dual-luciferase reporter system was obtained from Promega (Madison, WI, United States). All inhibitors, including a TNF-α antagonist (SC-356159 ), PP1 (SC-203212 A), U0126 (SC-222395 ), tanshinone IIA (TSIIA) (SC-200932 ), and Bay 11 -7082 (SC-202490 ), were purchased from Santa Cruz Biotechnology. Quercetin was obtained from Biotic Chemical Co., Ltd. (New Taipei City, Taiwan). A stock solution of quercetin was resuspended in a 1 :9 (v/v) solution of dimethyl sulfoxide (DMSO) and 99 % ethanol and diluted to the presented final concentration with culture medium. Human recombinant TNF-α was obtained from R&D Systems(AFL210 ) (Minneapolis, MN, United States). MMP9 inhibitor (MMP9 i) (Cat#15942 -500 ) was purchased from Biomol (Plymouth Meeting, PA, United States). Cell counting Kit-8 (CCK-8 ) kit reagent was obtained from MedChemExpress Ltd. (Hercules, CA, United States). All other enzymes, reagents, and chemicals were obtained from Sigma-Aldrich (St. Louis, MO, United States).

    Cell culture

    GES-1 cells were obtained from Xiamen University in China. The cells were cultured in RPMI 1640 medium containing 10 % FBS, 100 IU/mL penicillin G, 100 mg/mL streptomycin sulfate, and nonessential amino acids at 37 °C in a humidified atmosphere with 5 % CO2 according to a previously described standard protocol[39 ]. The cells were either untreated or treated with quercetin or inhibitors of the TNF-α antagonist, MMP-9 i, c-Src (PP1 ), ERK1 /2 (U0126 ), c-Fos (TSIIA), or NF-κB (BAY). These substances were added to the cell culture 1 h before the addition of TNF-α in all experiments.

    MMP zymography

    Growth-arrested cells were incubated with different treatments for the indicated time intervals. The cells were either untreated or treated with quercetin or inhibitors of TNF-α antagonist, c-Src (PP1 ),ERK1 /2 (U0126 ), c-Fos (TSIIA), or NF-κB (BAY). After treatment, the conditioned media were collected and mixed with 5 × nonreducing sample buffer and analyzed on a 10 % gel containing 0 .15 % gelatin.After electrophoresis, the gel was washed, incubated, stained, and destained. The gelatinolytic activity appeared as parallel white bands on a blue background[40 ].

    CCK-8 assay

    GES-1 cells (5000 cells/well) were seeded into 96 -well plates with serum-free RPMI 1640 medium and cultured for 24 h at 37 °C in a humidified atmosphere with 5 % CO2 . The culture medium was replaced by quercetin diluted in series to concentrations of 0 , 0 .01 , 0 .1 , 1 , 10 , or 100 mg/mL, and the cells were cultured for 24 or 48 h. After incubation with quercetin, 10 mL of the CCK-8 kit reagent was added to each well (100 mL/well), and the incubation was continued for 1 h. The optical density at 450 nm was measured using a multifunction microplate reader (SpectraMax i3 ; Kelowna International Scientific Inc.,New Taipei, Taiwan) using a previously described standard protocol[41 ]. Cell viability is expressed as the percentage of living cells relative to the control.

    Quantitative reverse transcription-PCR

    GES-1 cells were seeded into 9 -cm dishes with serum-free RPMI 1640 medium, cultured for 24 h at 37 °C, and then incubated with TNF-α for 0 , 16 , 20 , or 24 h. Total RNA was extracted using TRIzol reagent,and the concentration of RNA was measured on a Nano100 Micro-Spectrophotometer (CLUBIO; Taipei,Taiwan). cDNA was then synthesized using an iScript cDNA Synthesis Kit and amplified on a spectrofluorometric thermal cycler (iCycler; Bio-Rad Laboratories)[42 ]. To evaluate MMP9 mRNA expression in GES-1 cells, qRT-PCR was performed according to a previously described standard protocol usingGAPDHas the internal control[42 ]. Fluorescence emitted by SsoFast EvaGreen Supermix was measured using the CFX Connect Real-Time PCR detection system. The following primers were used for qRT-PCR: HumanMMP9(sense, 5 ’-AGTTTGGTGTCGCGGAGCAC-3 ’ and antisense, 5 ’-TACAT GAGCGCTTCCGGCAC-3 ’) and human GAPDH (sense, 5 ’-ACAGTCAGCCGCATCTTCTT-3 ’ and antisense, 5 ’-GACAAGCTTCCCGTTCTCAG-3 ’). Relative gene expression is expressed using the Delta-Delta-Ct (ddCt) method, where Ct represents the mean threshold cycle.

    Western blot analysis

    Growth-arrested cells were incubated with different treatments for the indicated time intervals. The cells were either untreated or treated with quercetin or inhibitors of TNF-α antagonist, c-Src (PP1 ),ERK1 /2 (U0126 ), c-Fos (TSIIA), or NF-κB (BAY). After treatment, the cells were washed with PBS,scraped, lysed in lysis buffer, and collected as a whole-cell extract at 4 °C using a previously described standard protocol[42 ]. Samples were loaded onto a 10 % SDS-PAGE gel, electrophoresis was performed,and the bands were transferred to a PVDF membrane. The PVDF membrane was incubated overnight with specific primary antibodies, including anti-phospho-c-Src, anti-phospho-ERK1 /2 , anti-phospho-c-Fos, anti-phospho-NF-κB, or anti-GAPDH. The PVDF membranes were washed and then incubated with anti-mouse or anti-rabbit horseradish peroxidase-conjugated secondary antibody (dilution, 1 :2000 )for 1 h. The relative expression levels of c-Src, ERK1 /2 , c-Fos, and NF-κB were normalized to that of GAPDH. Finally, the immunoreactive bands were incubated in enhanced chemiluminescence reagent,and images were recorded on a UVP BioSpectrum 500 Imaging System (UVP, Inc.; Upland, CA, United States). Densitometry was quantified using UN-SCAN-IT gel software (Silk Scientific, Inc.; Orem, UT,United States).

    Cell migration assay

    To evaluate the influence of TNF-α-induced MMP-9 expression on the metastatic activity of GES-1 cells,anin vitroTranswell assay (Becton-Dickinson, Franklin Lakes, NJ, United States) was used. Cells at a concentration of 1 × 105 cells/100 mL in serum-free RPMI 1640 medium were added to the upper chamber, and the Matrigel-uncoated insert was inserted in the lower chamber, which contained 20 %FBS + RPMI 1640 medium. The migration assay was run for 24 h following a previously described standard protocol[39 ,42 ].

    Immunofluorescence

    The influence of TNF-α-induced MMP-9 expression in GES-1 cells and the potential involvement of NFκB/p65 translocation from the cytoplasm into the nucleus in this process were investigated. GES-1 cells were seeded into culture plates with coverslips. The cells were either untreated or treated with quercetin or inhibitors of c-Src (PP1 ), ERK1 /2 (U0126 ), or NF-κB (BAY). After treatment, the cells were washed,fixed, permeabilized, blocked, and stained with anti-NF-κB. The coverslips were affixed to slides with mounting medium and stained with 4 ’,6 -diamidino-2 -phenylindole as previously described[43 ].Fluorescence images were photographed using a fluorescence microscope (Leica Microsystems, Wetzlar,Germany).

    Luciferase assay

    The human AP-1 -Luc and NF-κB-Luciferase (Luc) response element reporter plasmids pGL4 .44 GL4 .44 [luc2P/AP1 RE/Hygro] (No. E411 A; JQ858516 ) and pGL4 .32 [luc2 P/NF-κB-RE/Hygro] (No. E849 A;EU581860 ), and the dual-luciferase reporter system were obtained from Promega (Madison). Two plasmids were transfected into GES-1 cells using TurboFect Transfection Reagent according to a previously reported protocol[44 ]. The cells were either untreated or treated with quercetin or inhibitors of TNF-α antagonist, c-Src (PP1 ), ERK1 /2 (U0126 ), or NF-κB (BAY). After treatment, the cells were collected, lysed, and centrifuged, and aliquots of the supernatants were tested for promoter activity using the dual-luciferase assay system. Firefly luciferase activity was standardized to that ofRenillaluciferase.

    Statistical analysis

    All data were obtained from at least three independent experiments and are presented as the mean ±SEM. The data were analyzed using one-way analysis of variance (ANOVA) followed by Tukey’sposthoctest to identify significant differences between multiple groups. Statistical analyses were performed using GraphPad Prism 6 .0 (GraphPad Software, Inc.; La Jolla, CA, United States). A P value < 0 .05 was considered significant. The statistical methods of this study were reviewed by Dr. Jian-Hao Chen from Estat Statistics Consulting Company (Taipei, Taiwan).

    RESULTS

    Omics approach to identify inflammation-related proteins involved in GC

    To examine the potential roles of inflammation-related proteins in GC, we used an omics approach based on four datasets from the following sources: (1 ) The public Human Protein Atla (https://www.proteinatlas.org); (2 ) The public United States National Center for Biotechnology Information(NCBI) Gene Expression Omnibus (GEO) profiles (https://www.ncbi.nlm.nih.gov/geoprofiles/); (3 )Human cytokine factors (https://www.abcam.com/human-cytokine-antibody-array-membrane-174 -targets-ab193657 .html); and (4 ) NCBI PubMed research “inflammation” papers. The combination of the four datasets revealed significant upregulation ofMMP9in GC relative to paired normal tissues, as shown in Figure 1 A. The NCBI GEO profiles revealed consistent significant MMP9 upregulation(Human, ID: 125276865 ; Mouse, ID:54860954 ) in GC tissues relative to paired normal tissues (Figure 1 B).Therefore, we selectedMMP9for further study.

    Role of MMP-9 expression in TNF-a-induced inflammation in GES-1 cells

    MMP-9 expression is involved in gastric inflammation, may contribute to the development of GC, and is associated with poor survival rates[25 -28 ]. To explore the role of TNF-α-activated MMP-9 in GC, GES-1 cells were treated with different concentrations of TNF-α (10 , 20 , or 30 ng/mL) for designated times (0 ,16 , 20 , or 24 h), and MMP9 mRNA and protein levels were measured. TNF-α at a dose of 10 mg/mL for 16 or 20 h did not affect MMP-9 protein expression in GES-1 cells, but exposure for 24 h increased MMP-9 expression compared with 0 h (P < 0 .05 ). TNF-α at a dose of 20 mg/mL for 24 h significantly increased MMP-9 expression compared with 0 h (P < 0 .05 ). TNF-α at a dose of 30 mg/mL for 20 or 24 h resulted in the highest MMP-9 expression of GES-1 cells compared with 0 h (P < 0 .05 and P <0 .01 , respectively).TNF-α induced MMP-9 enzymatic activity in a time- and concentration-dependent manner (Figure 2 A).qRT-PCR was performed to measure theMMP-9mRNA level in TNF-a-induced GES-1 cells. After TNFα stimulation,MMP-9mRNA was significantly upregulated in a time-dependent manner after 16 , 20 ,and 24 h of incubation compared with 0 h (P < 0 .05 , P < 0 .05 , and P < 0 .001 , respectively) (Figure 2 B).These observations suggest that MMP-9 expression was induced by TNF-α at both the transcriptional and translational levels in GES-1 cells. Therefore, we chose to use 30 ng/mL TNF-α in GES-1 cells for further assessments of TNF-α-induced changes in MMP-9 expression. We explored whether a TNF-α antagonist can repress TNF-α-activated MMP-9 expression in GES-1 cells. The cells were either untreated or treated with a TNF-α antagonist (0 .3 , 1 , and 3 mM) for 1 h before the addition of TNF-α.MMP-9 inhibition significantly repressed TNF-α-activated MMP-9 expression in GES-1 cells in a timedependent manner after 16 and 24 h of incubation compared with 0 h (P < 0 .01 and P < 0 .001 ,respectively) (Figure 2 C).

    Figure 1 ldentification studies of matrix metallopeptidase-9 , a potential inflammation-related protein involved in gastric cancer. A:Identification of potential inflammation-related proteins involved in gastric cancer (GC) based on an omics approach including four integrated datasets. The strategy included proteomic profiling; B: Relative expression levels of matrix metallopeptidase-9 in paired GC and adjacent normal tissues in humans and mice. A t test was used for comparisons between the two groups. Data are expressed as the mean ± SEM of three independent experiments. aP < 0 .05 , bP < 0 .01 vs controls. GC:Gastric cancer; GEO: Gene Expression Omnibus; MMP-9 : Matrix metallopeptidase-9 ; NCBI: National Center for Biotechnology Information.

    Effects of quercetin on TNF-α-induced MMP-9 expression in GES-1 cells

    Quercetin has anti-inflammatory effects[33 ,34 ]. We first measured the viability of GES-1 cells after quercetin treatment. Quercetin treatment at concentrations of 0 , 0 .01 , 0 .1 , 1 , or 10 mM for 24 to 48 h had almost no effect on GES-1 cell viability (Figure 3 A and B). In contrast, 100 mM quercetin significantly reduced GES-1 cell viability after 48 h compared with 0 mM (P < 0 .01 ). Therefore, quercetin was used at concentrations up to 1 mM in the following experiments to explore whether quercetin represses TNF-αactivated MMP-9 expression in GES-1 cells and its mechanism of action. The cells were either untreated or treated with quercetin (0 , 0 .1 , 0 .3 , or 1 mM) for 1 h. Then, TNF-α was added, and the cells were incubated for 0 , 16 , or 24 h (Figure 3 C). Quercetin significantly repressed TNF-α-activated MMP-9 expression in GES-1 cells at doses of 0 .1 , 0 .3 , and 1 mM and in a time-dependent manner after 16 and 24 h of incubation.

    Involvement of c-Src in TNF-α-induced MMP-9 expression in GES-1 cells

    Kimet al[45 ] reported that TNF-α-induced MMP-9 expression is mediatedviamitogen-activated protein kinase (MAPK) in human GC cells[45 ]. We next explored the pathway through which quercetin reduces TNF-α-induced MMP-9 expression in GES-1 cells. To determine the role of c-Src in TNF-α-induced MMP-9 expression, two inhibitors of TNF-α antagonist or c-Src (PP1 ) were used. GES-1 cells were pretreated with the TNF-α antagonist (1 mM) or PP1 (0 , 0 .3 , 1 , or 3 mM) for 1 h, and the cells were then incubated with TNF-α for 0 , 16 , or 24 h (Figure 4 A). Pretreatment with PP1 significantly attenuated TNF-α-induced MMP-9 expression in cells incubated for 16 or 24 h in a time-dependent manner. This finding suggests that c-Src was involved in these responses. To confirm this effect, Western blot analysis was used to examine the phosphorylation of c-Src in cells exposed to TNF-α for 0 , 5 , 15 , 30 , or 60 min(Figure 4 B and C). Pretreatment with quercetin, PP1 , or TNF-α antagonist blocked TNF-α-activated phosphorylation of c-Src in a time-dependent manner with the exception of incubation with PP1 + TNFα and TNF-α antagonist + TNF-α for 15 min (Figure 4 C). These findings suggest that TNF-α induced MMP-9 expression via TNFR-c-Src in GES-1 cells.

    Involvement of ERK1 /2 in TNF-a-induced MMP-9 expression in GES-1 cells

    Figure 2 Tumor necrosis factor-α induces matrix metallopeptidase-9 expression via tumor necrosis factor-α receptor in normal human gastric mucosa epithelial cells. A: Tumor necrosis factor-α (TNF-α) was used at concentrations of 10 , 20 , and 30 ng/mL to stimulate normal human gastric mucosa epithelial cells (GES-1 ) for 0 , 16 , 20 , or 24 h, and matrix metallopeptidase-9 (MMP-9 ) enzymatic activity was measured by gelatin zymography as described in the Materials and Methods section; B: MMP-9 transcripts were analyzed by quantitative reverse transcription-polymerase chain reaction; C: Cells were either untreated or treated with a TNF-α antagonist (TNFR inhibitor) (1 mM) 1 h before the addition of TNF-α (30 ng/mL). The TNF-α antagonist repressed TNF-α-activated MMP-9 expression in GES-1 cells. One-way ANOVA was used for comparisons among different treatment time points (aP < 0 .05 , bP < 0 .01 vs control cells in 0 h).One-way ANOVA was used for comparisons among different treatments (cP < 0 .05 , dP < 0 .01 vs TNF-α-stimulated cells). Data are expressed as the mean ± SEM of three independent experiments. GAPDH: Glyceraldehyde-3 -phosphate dehydrogenase; GES-1 : Normal human gastric mucosa epithelial cell line; MMP: Matrix metallopeptidase; TNF-α: Tumor necrosis factor-α.

    To evaluate whether ERK1 /2 contributes to TNF-α-induced MMP-9 expression, two inhibitors of TNF-α antagonist or ERK1 /2 (U0126 ) were used. GES-1 cells were pretreated with the TNF-α antagonist (1 mM) or U0126 (0 , 0 .3 , 1 , or 3 mM) for 1 h and then incubated with TNF-α for 0 , 16 , or 24 h (Figure 5 A).Pretreatment with U0126 significantly attenuated TNF-α-induced MMP-9 expression after 16 and 24 h of incubation in a time-dependent manner. This finding suggests that ERK1 /2 is involved in this response.To further explore the effects of quercetin, U0126 , PP1 , or TNF-α antagonist on TNF-α-activated ERK1 /2 phosphorylation, Western blot analysis was used to measure ERK1 /2 phosphorylation after exposure for 0 , 5 , 15 , 30 , or 60 min. Pretreatment with quercetin, U0126 , PP1 , or TNF-α antagonist blocked TNF-αactivated ERK1 /2 phosphorylation in a time-dependent manner (Figure 5 B and C). These data suggest that TNF-α-induced MMP-9 expression may be mediated through TNFR-c-Src-ERK1 /2 in GES-1 cells.

    Involvement of c-Fos in TNF-a-induced MMP-9 expression in GES-1 cells

    AP-1 and NF-κB play important regulatory roles in the human MMP-9 promoter region, where they react with cytokines or growth factors[46 ]. To examine the role of c-Fos in TNF-α-induced MMP-9 expression, two inhibitors of TNF-α antagonist or c-Fos (TSIIA) were used. GES-1 cells were pretreated with TNF-α antagonist (1 mM) or TSIIA (0 , 5 , 10 , or 20 mM) for 1 h and incubated with TNF-α for 0 , 16 ,or 24 h (Figure 6 A). Pretreatment with TSIIA significantly attenuated TNF-α-induced MMP-9 expression after 16 and 24 h of incubation in a time-dependent manner. This finding suggests that c-Fos was involved in these responses. To further explore the effects of quercetin, TSIIA, U0126 , PP1 , and TNF-α antagonist on TNF-α-activated c-Fos phosphorylation, Western blot analysis was used to measure c-Fos phosphorylation in cells incubated for various time intervals (Figure 6 B and C). Pretreatment with quercetin or TSIIA, U0126 , PP1 , or TNF-α antagonist blocked TNF-α-activated phosphorylation of c-Fos in a time-dependent manner. An assay to analyze the activity of human AP-1 -Luc response element reporter plasmids was used to explore whether the quercetin-induced reduction in AP-1 promoter reporter activity occurs through the signaling pathways mentioned above. Quercetin attenuated AP-1 promoter reporter activity (Figure 6 D), and this effect may occur through the TNFR-c-Src-ERK1 /2 -c-Fos pathway. Taken together, these results suggest that quercetin reduces TNF-α-induced MMP-9 expression in GES-1 cells via the TNFR-c-Src-ERK1 /2 -c-Fos pathway.

    Involvement of NF-κB in TNF-a-induced MMP-9 expression in GES-1 cells

    To clarify the role of NF-κB (p65 ) in TNF-α-induced MMP-9 expression, two inhibitors of TNF-α antagonist or NF-κB (p65 ) (BAY) were used. GES-1 cells were pretreated with TNF-α antagonist (1 mM)or BAY (0 , 5 , 10 , or 20 mM) for 1 h before the addition of TNF-α and incubated for 0 , 16 , or 24 h(Figure 7 A). Pretreatment with BAY significantly attenuated TNF-α-induced MMP-9 expression after 16 and 24 h of incubation (P < 0 .01 ; P < 0 .05 ) in a time- and dose-dependent manner. This finding suggests that NF-κB (p65 ) was involved in these responses. To further examine the effects of quercetin, BAY,U0126 , PP1 , or TNF-α antagonist on TNF-α-activated NF-κB (p65 ) phosphorylation, Western blot analysis was used to measure NF-κB (p65 ) phosphorylation in cells incubated for the indicated time intervals. Pretreatment with quercetin, BAY, U0126 , PP1 , or TNF-α antagonist blocked TNF-α-activated phosphorylation of NF-κB (p65 ) in a time-dependent manner (Figure 7 B and C).

    We used immunofluorescence to assess the effects of quercetin on NF-κB translocation from the cytoplasm into the nucleus. Cells were first stimulated with TNF-α (30 ng/mL) for 0 , 5 , 10 , 15 , 30 , or 60 min. The data showed that TNF-α induced NF-κB translocation in cells in a time-dependent manner. A maximal response was achieved within 30 min and sustained over 60 min during the period of observation (Figure 7 D). Quercetin, PP1 , BAY, and U0126 reduced TNF-α-induced NF-κB translocation.PP1 and BAY downregulated MMP9 expression in TNF-α-induced GES-1 cells (Figure 7 E). An assay to measure human NF-κB-Luc response element reporter plasmid activity was used to examine whether quercetin could reduce NF-κB promoter reporter activity through the signaling pathways mentioned above. Quercetin attenuated NF-κB promoter reporter activity, and this effect may occur through the TNFR-c-Src-ERK1 /2 -NF-κB pathway (Figure 7 F). Taken together, these results suggest that quercetin reduced TNF-α-induced MMP-9 expression in GES-1 cells via the TNFR-c-Src-ERK1 /2 -c-Fos and NF-κB pathways.

    In vitro antimetastatic activities of quercetin

    Figure 4 Quercetin suppresses tumor necrosis factor-α-induced matrix metallopeptidase-9 expression via tumor necrosis factor-α antagonist-proto-oncogene tyrosine-protein kinase Src in normal human gastric mucosa epithelial cells. A: Cells were either untreated or treated with PP1 (0 , 0 .3 , 1 , or 3 mM) for 1 h before the addition of tumor necrosis factor-α (TNF-α) (30 ng/mL) and then incubated for 0 , 16 , or 24 h as described in the Materials and Methods section. Matrix metallopeptidase-9 (MMP-9 ) zymogen activity was analyzed by gelatin zymography; B and C: Cells were either untreated or treated with quercetin (B; 0 or 1 mM) or PP1 (C; 0 or 1 mM) or TNF-α antagonist (1 mM) for 1 h before the addition of TNF-α (30 ng/mL) and incubated for 0 , 16 , or 24 h. The phosphorylation of c-Src was measured using Western blot analysis after incubation of cells with TNF-α for 0 , 5 , 15 , 30 , or 60 min. One-way ANOVA was used for comparisons among different treatment time points (aP < 0 .05 , bP < 0 .01 vs control cells in 0 h). One-way ANOVA was used for comparisons among different treatments (cP < 0 .05 , dP < 0 .01 vs TNF-α-stimulated cells). Data are expressed as the mean ± SEM of three independent experiments. c-Src: Proto-oncogene tyrosine-protein kinase Src; GAPDH: Glyceraldehyde-3 -phosphate dehydrogenase; GES-1 : Normal human gastric mucosa epithelial cell line; MMP-9 : Matrix metallopeptidase-9 ; TNF-α: Tumor necrosis factor-α.

    Upregulation of MMP9 is involved in the inflammatory response and cell migration[47 -49 ]. Therefore,we further investigated the effects of quercetin on TNF-α-induced MMP9 -mediated functional changes in GES-1 cells. First, images of GES-1 cell migration were observed 24 h after TNF-α treatment.Pretreatment with quercetin (1 mM or 10 mM), a TNF-α antagonist (1 mM), or MMP9 i (5 mM)significantly blocked TNF-α-induced cell migration (Figure 8 ). This finding suggests that quercetin repressed TNF-α-induced cell migration by reducing MMP-9 expression in GES-1 cells.

    Figure 5 Quercetin suppresses tumor necrosis factor-α-induced matrix metallopeptidase-9 expression via tumor necrosis factor-α antagonist-c-Src-extracellular-signal-regulated kinase 1 /2 in normal human gastric mucosa epithelial cells. A: Normal human gastric mucosa epithelial cells (GES-1 ) were either untreated or treated with U0126 (0 , 0 .3 , 1 , or 3 mM) for 1 h before the addition of tumor necrosis factor-α (TNF-α) (30 ng/mL) and incubated for 0 , 16 , or 24 h as described in the Materials and Methods section. Matrix metallopeptidase-9 zymogen activity was measured using gelatin zymography;B and C: Cells were either untreated or treated with quercetin (B; 0 or 1 mM), PP1 (C; 0 or 1 mM), U0126 (0 or 1 mM), or TNF-α antagonist (1 mM) for 1 h before the addition of TNF-α (30 ng/mL) and incubated for 0 , 16 , or 24 h. The phosphorylation of extracellular-signal-regulated kinase 1 /2 was examined by Western blot analysis in cells incubated for 0 , 5 , 15 , 30 , or 60 min. One-way ANOVA was used for comparisons among different treatment time points (aP < 0 .05 , bP < 0 .01 vs control cells in 0 h). One-way ANOVA was used for comparisons among different treatments (cP < 0 .05 , dP < 0 .01 vs TNF-α-stimulated cells). Data are expressed as the mean ± SEM of three independent experiments. ERK: Extracellular-signal-regulated kinase; GAPDH: Glyceraldehyde-3 -phosphate dehydrogenase; GC: Gastric cancer; GES-1 : Normal human gastric mucosa epithelial cell line; MMP-9 : Matrix metallopeptidase-9 ; TNF-α: Tumor necrosis factor-α.

    DlSCUSSlON

    Quercetin belongs to a member of the polyphenolic flavonoid family, which has many favorable effects on human health, such as antioxidant, anti-inflammatory, anticancer, antiallergic, antiviral, free radicalscavenging, and neuroprotective activities[33 ,34 ]. Quercetin was used in this study due to its antiinflammatory and gastroprotective effects.

    Figure 6 Quercetin suppresses tumor necrosis factor-α-induced matrix metallopeptidase-9 expression via tumor necrosis factor-αantagonist-c-Src-extracellular-signal-regulated kinase 1 /2 -c-Fos in normal human gastric mucosa epithelial cells. A: Normal human gastric mucosa epithelial cells (GES-1 ) were either untreated or treated with Tanshinone IIA (TSIIA) (0 , 5 , 10 , or 20 mM) 1 h before the addition of tumor necrosis factor-α(TNF-α) (30 ng/mL) and incubated for 0 , 16 , or 24 h as described in the Materials and Methods section. Matrix metallopeptidase-9 zymogen activity was measured using gelatin zymography; B and C: Cells were either untreated or treated with quercetin (B; 0 or 1 mM), PP1 (C; 0 or 1 mM), U0126 (0 or 1 mM), TSIIA (0 or 10 mM),or TNF-α antagonist (1 mM) for 1 h before the addition of TNF-α (30 ng/mL) and incubated for 0 , 16 , or 24 h. The phosphorylation of c-Fos was measured by Western blot analysis in cells incubated for 0 , 5 , 15 , 30 , or 60 min; D: GES-1 cells were transfected with human AP-1 -Luc response element reporter plasmids containing the dual-luciferase reporter system. The cells were then pretreated with PP1 (0 or 1 mM), U0126 (0 or 1 mM), TSIIA (0 or 10 mM), TNF-α antagonist (1 mM), or quercetin(1 mM) for 1 h and exposed to TNF-α for 1 h, and luciferase activity was measured. Firefly luciferase activity was standardized to Renilla luciferase activity. One-way ANOVA was used for comparisons among different treatment time points (aP < 0 .05 , bP < 0 .01 vs control cells in 0 h). One-way ANOVA was used for comparisons among different treatments (cP < 0 .05 , dP < 0 .01 vs TNF-α-stimulated cells). Data are expressed as the mean ± SEM of three independent experiments. ERK:Extracellular-signal-regulated kinase; AP-1 : Activator protein-1 ; GAPDH: Glyceraldehyde-3 -phosphate dehydrogenase; GES-1 : Normal human gastric mucosaepithelial cell line; Luc: Luciferase; GES-1 : Normal human gastric mucosa epithelial cell line; MMP-9 : Matrix metallopeptidase-9 ; Q: quercetin; TNF-α: Tumor necrosis factor-α; TSIIA: Tanshinone IIA.

    Gastric inflammation is essential to the development of gastric epithelial injury and gastric diseases.Huet al[10 ] reported that quercetin can protect GES-1 cells from hydrogen peroxide-induced production of reactive oxygen species in a mouse model of acute gastric mucosal injury. Quercetin is thought to be protective against oxidative stress, mitochondrial dysfunction, and apoptosis and to be involved in the initiation of an antioxidant defense[10 ]. Quercetin has also been observed to modulate the inflammatory response of gastric mucosal epithelial cells against injury caused by ischemia-reperfusion[35 ], ethanol[36 ,38 ], indomethacin[9 ], and H. pylori[37 ] in animal models. In other cells, quercetin has been reported to inhibit the lipopolysaccharide-induced MMP-9 expression in lung inflammation and the production of proinflammatory cytokines[50 ]. Ying et al[51 ] reported that quercetin inhibits IL-1 b-induced ICAM-1 expression mediated by the MAPK pathway in lung inflammation[51 ,52 ], retinal pigment epithelial cells[53 ], and human endothelial cells[54 ]in vivoandin vitro.

    The mechanism through which quercetin exerts gastroprotective activity against TNF-α-induced injury to gastric mucosal epithelial cells is unknown. Gastric inflammation and injury induced by proinflammatory cytokines, such as TNF-α produced by activated immune cells, depend on NF-κB and MMP-9 activation through the NF-κB pathway[29 ,30 ]. Here, we explored whether quercetin protects against TNF-α-induced MMP-9 damage in GES-1 cells. We challenged these cells by inducing an immune-inflammatory reaction mediated by TNF-α and found that quercetin significantly reduced MMP-9 expression in GES-1 cells. Our findings suggest that quercetin helps to maintain the gastric mucosa and has potential as a treatment for preventing the progression of inflammation.

    Investigators have provided evidence that c-Src[55 ], the MAPK family[56 -58 ], and NF-κB[57 ,59 ]participate in pathophysiological processes involved in gastric inflammation and GC. Three major groups of MAPKs have been identified, including ERK1 /2 , p38 , and JNK1 /2 , which play critical roles in cell proliferation, differentiation, and inflammation[60 ]. TNF-α-induced MMP-9 expression is regulated through the MAPK pathway in human trophoblastic cells[61 ], human urinary bladder cancer HT1376 cells[62 ], lung cancer cells[63 ], osteoblasts[64 ], and skeletal muscle cells[65 ]. This evidence suggests that MMP-9 expression induced by inflammatory mediators, such as TNF-α, is associated with MAPKs in diverse cell types. We observed similar results in our studies. We observed thein vitroantimetastatic and anti-inflammatory activities of quercetin in GES-1 cells. Quercetin protected against TNF-α-induced MMP-9 damage in GES-1 cells challenged by induction of the immune-inflammatory reaction mediated by TNF-α. PP1 (c-Src inhibitor), U0126 (ERK1 /2 inhibitor), TSAIIA (c-Fos inhibitor), BAY (NF-κB inhibitor), and TNF-α antagonist (TNFR inhibitor) were used to investigate the interactions of c-Src,ERK1 /2 , c-Fos, NF-κB, and TNFR in the TNF-α-induced response. Using immunofluorescence, we found that TNF-α induced NF-κB (p65 ) phosphorylation and translocation and that NF-κB/p65 -Luc and AP-1 -Luc activities were mediated via the TNFR-c-Src-ERK1 /2 -c-Fos and NF-κB pathways. We also found that quercetin reduced TNF-α-induced MMP-9 expression in GES-1 cellsviathe proinflammatory c-Src-ERK1 /2 -c-Fos and NF-κB pathways. Moreover, quercetin may indeed directly inhibit upstream molecules (such as TNFR or c-Src) and subsequently cause the inhibition of downstream molecules, such as ERK1 /2 , c-Fos, and NF-κB.

    NF-κB plays an important role in the regulation of inflammation. Stimulation of proinflammatory cytokines, such as TNF-α, increases NF-κB activity and involves the phosphorylation and degradation of IκBa, which induces the translocation of active NF-κB to the nucleus and the expression of genes encoding proinflammatory factors, such as cytokines, chemokines, and adhesion molecules[66 -69 ]. In our study, pretreatment with BAY attenuated TNF-α-induced MMP-9 expression in GES-1 cells. MMP-9 is a potential target for new therapies and is being investigated by several research groups[70 -72 ]. A better understanding of the roles of inflammatory mediators will help in the development of new therapeutic approaches for treating gastric inflammatory diseases. Reducing MMP-9 production may help to limit gastric damage in the treatment of gastric diseases. Given the increasing use of NSAIDs worldwide, it is important to identify other agents to control inflammation. Quercetin and a quercetinrich diet may exhibit potential as food supplements for the prevention of early pathological changes associated with gastric inflammation.

    Figure 7 Quercetin suppresses tumor necrosis factor-α-induced tumor necrosis factor-α antagonist-c-Src-extracellular-signal-regulated kinase 1 /2 -nuclear factor kappa B (p65 ) activation in normal human gastric mucosa epithelial cells. A: Normal human gastric mucosa epithelial cells (GES-1 ) were either untreated or treated with BAY (0 , 5 , 10 , or 20 mM) for 0 , 16 , or 24 h; compounds were added 1 h before the addition of tumor necrosis factor-α (TNF-α) (30 ng/mL) as described in the Materials and Methods section. Matrix metallopeptidase-9 zymogen activity was measured by gelatin zymography. B and C: Cells were either untreated or treated with quercetin (B; 0 or 1 mM), PP1 (C; 0 or 1 mM), U0126 (0 or 1 mM), BAY (0 or 10 mM), or TNF-α antagonist (1 mM)for 1 h before the addition of TNF-α (30 ng/mL) and incubated for 0 , 16 , or 24 h. Nuclear factor kappa B (NF-κB) phosphorylation was examined by Western blot analysis; D and E: GES-1 cells were treated with 30 ng/mL TNF-α for 0 , 5 , 10 , 15 , 30 , or 60 min (D) or quercetin (1 mM), PP1 (1 mM), U0126 (1 mM), or BAY (10 mM) for 1 h (E) before exposure to TNF-α (30 ng/mL) for 30 min; F: GES-1 cells were transfected with the human NF-κB-Luc response element reporter plasmids containing the dual-luciferase reporter system. The cells were then pretreated with PP1 (0 or 1 mM), U0126 (0 or 1 mM), BAY (0 or 10 mM), quercetin (1 mM), or TNF-α antagonist (1 mM) for 1 h and exposed to TNF-α for 1 h. Then, luciferase activity was measured. Firefly luciferase activity was standardized to that of Renilla luciferase. One-way ANOVA was used for comparisons among different treatment time points (aP < 0 .05 , bP < 0 .01 vs control cells in 0 h). One-way ANOVA was used for comparisons among different treatments simultaneously (cP < 0 .05 , dP < 0 .01 vs TNF-α-stimulated cells). Data are expressed as the mean ± SEM of three independent experiments. ERK: Extracellular-signal-regulated kinase; GAPDH: Glyceraldehyde-3 -phosphate dehydrogenase; GES-1 : Normal human gastric mucosa epithelial cell line; MMP-9 : Matrix metallopeptidase-9 ; NF-κB: Nuclear factor kappa B; Q: Quercetin; TNF-α: Tumor necrosis factor-α.

    Figure 8 Quercetin exhibit antimetastatic activities in vitro. A: Cells were plated in 24 -well culture plates, grown to confluence, and starved with serumfree medium for 24 h. Cells were pretreated with a tumor necrosis factor-α (TNF-α) antagonist (1 mM), matrix metallopeptidase-9 inhibitor (5 mM), or quercetin (1 or 10 mM) for 1 h, and monolayer cells were incubated with TNF-α (30 ng/mL) for 24 h as described in the Materials and Methods section; B: One-way ANOVA was used for comparisons between the two groups (aP < 0 .05 , bP < 0 .01 vs control cells). One-way ANOVA was used for comparisons among different treatments (cP <0 .05 , dP < 0 .01 vs TNF-α-stimulated cells). Data are expressed as the mean ± SEM of three independent experiments. GES-1 : Normal human gastric mucosa epithelial cell line; MMP-9 : Matrix metallopeptidase-9 ; MMP9 i: MMP-9 inhibitor; TNF-α: Tumor necrosis factor-α.

    Figure 9 Schematic representation of the effects of quercetin on tumor necrosis factor-α-induced matrix metallopeptidase-9 expression and cell migration in normal human gastric mucosa epithelial cells. Schematic diagram of the signaling pathways for quercetin-mediated attenuation of tumor necrosis factor-α (TNF-α)-induced inflammation via downregulation of matrix metallopeptidase-9 (MMP-9 ) expression in normal human gastric mucosa epithelial cells. Quercetin attenuates TNF-α-induced MMP-9 expression in normal human gastric mucosa epithelial cells through the proinflammatory TNFR-c-Src-extracellular-signal-regulated kinase 1 /2 -c-Fos and nuclear factor kappa B pathways. AP-1 : Activator protein-1 ; c-Src: Proto-oncogene tyrosine-protein kinase Src; ERK: Extracellular-signal-regulated kinase; GES-1 : Normal human gastric mucosa epithelial cell line; MAPK: Mitogen-activated protein kinase; MMP-9 : Matrix metallopeptidase-9 ; MMP9 i: MMP-9 inhibitor; NF-κB: Nuclear factor kappa B; TNF-α: Tumor necrosis factor-α; TSIIA: Tanshinone IIA.

    We evaluated the effects of different concentrations of quercetin on the normal GES-1 cell line using the cell viability assay (Figure 3 A and B). We found that cells treated with quercetin at concentrations ≤10 mM for 24 to 48 h had almost no effect on GES-1 cell viability. Additionally, many studies have confirmed that the safety and efficacy of quercetin remain inconclusive[73 ]. In 2010 , the American Food and Drug Administration considered that the utilization of high-purity quercetin as a food ingredient in different food products is GRAS (“Generally Recognized As Safe”) (https://www.cfsanappsexternal.fda.gov/scripts/fdcc/index.cfm?set=GRASNotices&sort=GRN_No&order=DESC&startrow=1 &type=basic&search=341 ) (GRN No. 341 ). Based on several published human intervention studies, daily doses of oral quercetin are usually in the range of up to 1000 mg/d (they are the safest at 500 mg/d). Therefore,the daily supplement doses of oral quercetin were noticeably higher than the background daily doses of oral quercetin. Side effects subsequent to supplemental quercetin intake have rarely been described naturally. Moreover, supplemental isolated quercetin at doses clearly exceeding dietary quercetin intake will not aggravate gastric injuries, ulcers, or GC[74 -76 ]. However, based on several publishedin vivodata, quercetin promotes insulin secretion, and insulin can increase tumor growth[77 ]. Oral quercetin products have a few potential crucial safety behaviors[78 ], and potential opposite effects in diabetes. In patients who have developed nephropathy or estrogen-dependent cancer, the use of quercetin should be tracked and researched in the future[79 -82 ].

    CONCLUSlON

    We investigated thein vitroeffects of quercetin on antimetastatic and anti-inflammatory activities in GES-1 cells. Quercetin protected against TNF-α-induced damage caused by MMP-9 in human gastric mucosal epithelial cells (GES-1 ) challenged by TNF-α-mediated immune-inflammatory reactions. PP1 (c-Src inhibitor), U0126 (ERK1 /2 inhibitor), TSAIIA (c-Fos inhibitor), BAY (NF-κB inhibitor), and TNF-α antagonist (TNF-α inhibitor) were used to investigate the roles of c-Src, ERK1 /2 , c-Fos, and NF-κB in the TNF-α-induced response. Quercetin reduces TNF-α-induced MMP-9 expression in GES-1 cellsviathe proinflammatory TNFR-c-Src-ERK1 /2 -c-Fos and NF-κB pathways. We propose that quercetin exhibits potential as a novel therapeutic drug for protecting gastric mucosal epithelial cells from damage caused by disease (Figure 9 ). Quercetin and a quercetin-rich diet may be useful as food supplements for the prevention of early pathological changes associated with gastric inflammation.

    ARTlCLE HlGHLlGHTS

    ACKNOWLEDGEMENTS

    The corresponding author would like to thank theWorld Journal of Gastroenterologyfor the opportunity to present this work and acknowledge the hard work of all supporting authors. The authors wish to thank Dr. Chen QX and Dr. Zhou DW at Xiamen University (China) for providing GES-1 cells.

    FOOTNOTES

    Author contributions:Hsieh HL, Yu MC, and Cheng LC contributed equally to this work; all authors contributed to this paper with conception and design of the study, literature review and analysis, manuscript drafting, critical revision, and editing, and approval of the final version.

    Supported byMinistry of Science and Technology, Taiwan, No. MOST 108 -2320 -B-255 -002 -MY3 and No. MOST 110 -2635 -B-255 -001 ; Chang Gung Medical Research Foundation, Taoyuan, Taiwan, No. CMRPF1 I0031 , No.CMRPF1 L0081 , No. CMRPF1 L0021 , No. CMRPF1 L0041 , and No. CMRPF1 I0042 ; and Chang Gung University of Science and Technology, Taoyuan, Taiwan, No. ZRRPF3 K0111 and No. ZRRPF3 L0091 .

    lnstitutional review board statement:No human specimens were involved in this study.

    Conflict-of-interest statement:All authors have nothing to disclose.

    Data sharing statement:No additional data are available.

    Open-Access:This article is an open-access article that was selected by an in-house editor and fully peer-reviewed by external reviewers. It is distributed in accordance with the Creative Commons Attribution NonCommercial (CC BYNC 4 .0 ) license, which permits others to distribute, remix, adapt, build upon this work non-commercially, and license their derivative works on different terms, provided the original work is properly cited and the use is noncommercial. See: https://creativecommons.org/Licenses/by-nc/4 .0 /

    Country/Territory of origin:Taiwan

    ORClD number:Hsi-Lung Hsieh 0000 -0001 -8302 -2472 ; Ming-Chin Yu 0000 -0002 -6980 -7123 ; Li-Ching Cheng 0000 -0003 -3214 -7798 ; Mei-Yi Chu 0000 -0003 -1264 -7824 ; Tzu-Hao Huang 0000 -0002 -4960 -6789 ; Ta-Sen Yeh 0000 -0002 -1830 -9466 ;Ming-Ming Tsai 0000 -0002 -4495 -6616 .

    S-Editor:Fan JR

    L-Editor:Wang TQ

    P-Editor:Yuan YY

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