Redox Biology
Home The antioxidant response in Barrett's tumorigenesis: A double-edged sword
The antioxidant response in Barrett's tumorigenesis: A double-edged sword
The antioxidant response in Barrett's tumorigenesis: A double-edged sword

Dunfa Peng, Alexander Zaika, Jianwen Que, Wael El-Rifai
https://doi.org/10.1016/j.redox.2021.101894, Volume: 41, Pages: null
Article Type: review-article Article History
Publisher: Elsevier
Abstract

Esophageal adenocarcinoma (EAC) is the dominant form of esophageal malignancies in the United States and other industrialized countries. The incidence of EAC has been rising rapidly during the past four decades. Barrett's esophagus (BE) is the main precancerous condition for EAC, where a metaplastic columnar epithelium replaces normal squamous mucosa of the lower esophagus. The primary risk factor for BE and EAC are chronic gastroesophageal reflux disease (GERD), obesity and smoking. During the BE-dysplasia-EAC sequence, esophageal cells are under a tremendous burden of accumulating reactive oxygen species (ROS) and oxidative stress. While normal cells have intact antioxidant machinery to maintain a balanced anti-tumorigenic physiological response, the antioxidant capacity is compromised in neoplastic cells with a pro-tumorigenic development antioxidant response. The accumulation of ROS, during the neoplastic progression of the GERD-BE-EAC sequence, induces DNA damage, lipid peroxidation and protein oxidation. Neoplastic cells adapt to oxidative stress by developing a pro-tumorigenic antioxidant response that keeps oxidative damage below lethal levels while promoting tumorigenesis, progression, and resistance to therapy. In this review, we will summarize the recent findings on oxidative stress in tumorigenesis in the context of the GERD-BE-EAC process. We will discuss how EAC cells adapt to increased ROS. We will review APE1 and NRF2 signaling mechanisms in the context of EAC. Finally, we will discuss the potential clinical significance of applying antioxidants or NRF2 activators as chemoprevention and NRF2 inhibitors in treating EAC patients.

Keywords
Oxidative stress, Barrett's esophagus, Esophageal adenocarcinoma, Antioxidant response, NRF2, APE1
Peng,Zaika,Que,and El-Rifai: The antioxidant response in Barrett's tumorigenesis: A double-edged sword

Abbreviations

ABSacidic bile salts
AREantioxidant response elements
ALDH1aldehyde dehydrogenase 1
APE1Apurinic/apyrimidinic endonuclease 1
AP-1activator protein-1
ATBCAlpha-Tocopherol Beta Carotene
BEBarrett's esophagus
BERbase excision repair
CATcatalase
CSCcancer stem cell
COSMICCatalogue of Somatic Mutations in Cancers
CREBcAMP response element binding protein
DMFdimethyl fumarate
ERendoplasmic reticulum
EACesophageal adenocarcinoma
GERDgastroesophageal reflux disease
GSK3glycogen synthase kinase-3
GPxglutathione peroxidase
GRglutathione reductase
GSHreduced glutathione
GSSGoxidized glutathione
GSTMglutathione S-transferase mu
GSTTglutathione S-transferase theta
GSTPglutathione S-transferase pi
HO-1heme oxygenase-1
H2O2hydrogen peroxide
4-4-HNEhydroxy-2-nonenal
HIF-1αhypoxia-inducible factor-1α
JNKc-Jun N-terminal kinases
KEAP1kelch‐like‐ECH‐ associated protein 1
MDAmalondialdehyde
NADPHNicotinamide adenine dinucleotide phosphate
NF-κBnuclear factor κB
NRF2nuclear factor erythroid 2‐related factor 2
NFE2L2nuclear factor erythroid 2 like 2
NQO1NAD(P)H quinone oxidoreductase 1
8-OHdG8-hydroxydeoxy-guanosine
ROSreactive oxygen species
RNSreactive nitrogen species
STAT3signal transducer and activator of transcription 3
SODsuperoxide dismutase
CuZn-SODcopper–zinc SOD
Mn-SODmanganese SOD
EC-SODextracellular-SOD
SELECTSelenium and Vitamin E Cancer Prevention Trial
UGTUDP-glucuronosyltransferases
USPSTFU.S. Preventative Services Task Force

Introduction

Oxidative stress results from an imbalance between the production of oxidants that are free radicals and reactive metabolites, including reactive oxygen species (ROS), reactive nitrogen species (RNS), and anti-oxidants that can eliminate ROS or RNS [1]. ROS are products of normal cellular metabolism processes. Mitochondria, where the electron transfer to molecular oxygen occurs at the respiratory chain level, is the site to generate major ROS [2,3], such as superoxide anion (O2 −), hydrogen peroxide (H2O2), hydroxyl radical (OH•-) as well as organic peroxides as normal product of the biological reduction of molecular oxygen. In addition, enzymatic reactions catalyzed by oxidases such as NADPH oxidases, cyclooxygenases, lipooxygenases, and peroxisomal oxidative metabolism, endoplasmic reticulum (ER) stress all generate ROS [2,3]. Under normal physiological conditions, cells have intact anti-oxidant systems to keep ROS tightly controlled at a low level (Fig. 1A). ROS is involved in multiple signaling pathways, such as proliferation and differentiation. ROS plays a vital role in the cellular response to various intracellular environmental stimuli and extra-cellular environmental stimuli [4]. However, accumulation of ROS/RNS causes oxidative stress that poses potential damage to the cells by attacking macromolecules such as DNA, RNA, proteins and lipids. For example, oxidative stress leads to oxidative DNA damage, forming 8-hydroxydeoxy-guanosine (8-OHdG), the hydrolysis product of 8-hydroxyguanosine [5]. The 8-OHdG is a pro-mutagenic lesion that mispairs with adenine, leading to GC to TA transversion [6]. The 8-OHdG is the most widely used oxidative DNA/RNA damage marker [7,8] that has been strongly implicated in carcinogenesis [[9], [10], [11]].

Redox balance in normal, precancerous and neoplastic esophagus.
Fig. 1

Redox balance in normal, precancerous and neoplastic esophagus.

A) ROS are by-products of normal cellular metabolism and activities. The mitochondria is the major site to produce ROS through the respiratory chain reactions (oxidative phosphorylation). Some enzymatic reactions such as NADPH oxidases, cyclooxygenases, lipooxygenases as well as peroxisomal oxidative metabolism, endoplasmic reticulum (ER) stress all generate ROS. However, normal cells have intact antioxidant machinery including antioxidant enzyme systems such as SOD, GPX, CAT, GR and antioxidant metabolites to keep ROS/antioxidants balance in low level. B) Under GERD, Barrett's esophagus (BE) conditions, refluxes of acidic bile salts, inflammatory microenvironment and activation of inflammation promotion signaling pathways like NF-kB, Stat3 result in elevated ROS generation and accumulation. On the other hand, some of antioxidant enzymes, such as GPX3, GPX7 lost partial function. Consequently, oxidative stress often occur that leads to DNA damage and other cellular damage. C), In neoplastic esophagus (high grade dysplasia and EAC), ROS level further elevate due to mainly the activation of oncogenes, growth factors and fully dysfunction of some antioxidant enzymes (GPX3, GPX7). To avoid cell death due to high ROS level, neoplastic cells develop a pro-tumorigenic antioxidant mechanism by constitutively activating APE1-NRF2 master antioxidant machinery. The hijack of NRF2 by tumor cells regain redox balance in higher ROS levels that favors tumor cell survival.

Esophageal Cancer is the 7th most frequent human malignancies and remains the 6th cancer-related death worldwide [12]. There are two major histology types of Esophageal Cancer: Squamous Cell Carcinoma (SCC) and adenocarcinoma [13]. While the incidence of squamous cell carcinoma is declining in the Western world during the past few decades, the prevalence of esophageal adenocarcinoma (EAC) has been rising rapidly in the US and other Western countries, becoming the dominant form of Esophageal Cancer [[14], [15], [16]]. EAC has three major risk factors: gastroesophageal reflux disease (GERD), obesity and smoking [16]. GERD is a condition in which the gastric contents mixed with bile salts reflux into the lower esophagus, causing acute and chronic inflammatory diseases [17]. Chronic GERD leads to Barrett's Esophagus (BE) development, where the original esophageal squamous epithelium is replaced by a specialized metaplastic columnar epithelium [18,19]. BE is the major known precancerous condition with a risk of progression to low-grade dysplasia, high-grade dysplasia and finally, EAC [20,21]. Accumulating lines of evidence indicate that oxidative stress is involved in the GERD-BE-EAC progression cascades [[22], [23], [24]]. We will review oxidative stress in the context of Barrett's related tumorigenesis. We will discuss the regulatory mechanisms and potential clinical significance of antioxidant activators as chemoprevention approach and inhibitors in EAC treatment.

Increased oxidative stress during GERD-BE-EAC cascades

Recurrent episodes of reflux of gastric juice and bile salts mixture into the lower esophagus are the unique characteristics of GERD-BE and EAC spectrum. We have demonstrated that a short-time exposure of esophageal cells to the acidic bile salts (ABS) to mimic a GERD episode led to significant generation of H2O2 levels and rapid elevation of intracellular ROS levels [22,[25], [26], [27], [28]]. Subsequently, oxidative DNA damage levels (detected by 8-OHdG) and double strand DNA breaks (detected by γH2AX) were significantly increased after ABS exposure [22,25]. EAC is considered a model of oxidative stress and inflammation-driven cancer [29,30]. Chronic GERD induces chronic inflammation (esophagitis) that persists through the BE and EAC progression cascade. During the inflammation process, various inflammatory cells, including mast cells, macrophages and leukocytes, are recruited to the site. As a result, an increased uptake of oxygen, so-called a “respiratory burst,” amplifies the release and accumulation of ROS at the site of damage [1,31].

The inflammatory cells produce various cytokines, chemokines and metabolites as soluble mediators, which promote further recruitment of inflammatory cells to the site of damage with more ROS production. We and others have demonstrated that ABS exposure and inflammatory cytokines and chemokines activate signal transduction cascades such as nuclear factor κB (NF-κB), signal transducer and activator of transcription 3 (STAT3), and hypoxia-inducible factor-1α (HIF-1α) [30,[32], [33], [34]]. Activation of these oncogenic networks contribute to the generation of additional ROS. In line with the experimental observations, the significant increase in ROS levels and oxidative DNA damage in BE-related lesions is confirmed in several experimental animal models [23,35] as well as in human BE and esophageal adenocarcinoma tissue samples [[36], [37], [38]] (Fig. 1).

Dysfunction of anti-oxidant enzymes contributes to oxidative stress in Barrett's tumorigenesis

Normal cells possess intact anti-oxidant machinery to keep ROS level tightly controlled to counteract oxidative stress (Fig. 1A). The balance of oxidants/anti-oxidants is pivotal to maintain normal cellular functions and homeostasis [[39], [40], [41]]. The cellular anti-oxidant defense is comprised of the major enzymatic anti-oxidants that are directly involved in the neutralization of ROS (Fig. 1). Examples include superoxide dismutase (SOD), glutathione peroxidase (GPx), glutathione reductase (GR), and catalase (CAT) [42,43]. SOD is the first characterized anti-oxidant enzyme that includes three types: copper–zinc SOD (CuZn-SOD), manganese SOD (Mn-SOD), and extracellular-SOD (EC-SOD). All of three can catalyze the dismutation of superoxide anion radical (O2 •-) into hydrogen peroxide (H2O2) by reduction [44]. The produced H2O2 is broken into water and oxygen (O2) by catalase (CAT) or glutathione peroxidase (GPx). The GPx enzymes remove H2O2 through oxidizing reduced glutathione (GSH) into oxidized glutathione (GSSG). Glutathione reductase (GR) regenerates GSH from GSSG, using NADPH [42,43].

In addition, some metabolites, such as l-arginine, glutathione, coenzyme Q10, uric acid, lipoid acid, bilirubin, metal-chelating proteins, transferrin, and melatonin also play an essential role in cellular anti-oxidant defense [41,45].

Several genetic variations have been linked to the susceptibility to Barrett's esophagus [[46], [47], [48]]. Among genes encoding anti-oxidant enzymes, variants of GSTP1 (such as rs1695 A>G missense variant), results in reduced enzymatic activity, frequently linked to risks of BE and EAC [49,50]. Variants of GSTT2 were different in African Americans, as compared with European Americans. These different variants are associated with higher expression of the enzyme in African American. The findings may explain the inherent different susceptibility risk to Barrett's esophagus in the population [51]. Furthermore, there are accumulating lines of evidence showing that the cellular anti-oxidants capacity is compromised during BE-EAC tumorigenesis (Fig. 1B) [[52], [53], [54], [55]]. The first line of anti-oxidant enzyme, Mn-SOD, is downregulated in BE and EAC [55]. Several studies have demonstrated a significant reduction in the levels of glutathione contents with major glutathione S-transferases. We have shown frequent DNA hypermethylation and downregulation of multiple anti-oxidant enzymes in BE and EAC. These include glutathione peroxidases (GPX3 and GPX7), glutathione S-transferases (such as GSTM2, GSTM3, GSTM5) [56,57] and metallothionein 3 (MT3) [58]. Dysfunction of these anti-oxidant enzymes makes esophageal cells more sensitive to ABS exposure. It promotes oxidative stress and subsequent DNA damage [25]. Notably, some of these anti-oxidant enzymes such as GPX3 and GPX7 possess unique tumor suppressor functions, in addition to their anti-oxidant properties. For example, GPX3 has a tumor suppressor role in esophageal adenocarcinoma [59], gastric cancer [60,61], breast cancer [62], prostate cancer [63], and colorectal cancer [64]. Similarly, GPX7 has anti-tumorigenic functions in esophageal [57], and gastric adenocarcinomas [65]. Therefore, dysfunction of these antioxidant enzymes not only compromises cellular antioxidant capacity but also favors tumor cell growth, a major contribution to Barrett's tumorigenesis [57,66].

The rebalance of redox signaling in esophageal adenocarcinoma

It is well documented that cancer cells possess higher ROS levels than normal or pre-cancerous cells [1,37,67,68]. Factors contributing to increasing ROS in cancer cells include activation of oncogenes (such as RAS and MYC), inflammatory microenvironments, and dysfunction of normal anti-oxidant enzymes. Other factors include extracellular stimuli such as exposure to reflux conditions, infection with H. pylori, radiation, and drug treatments (Fig. 1 C). However, excessive accumulation of ROS and subsequent oxidative DNA damage will incur serious DNA damage response that is lethal to cancer cells. Cancer cells must evolve to develop pro-tumorigenic anti-oxidant mechanisms that maintain oncogenic activities while keeping ROS and oxidative stress below lethal levels.

Nuclear factor erythroid 2‐related factor 2 (NRF2) is a master antioxidant transcription factor playing a central role in regulating the expression of hundreds of antioxidant genes to defend against toxic and oxidative insults [[69], [70], [71]]. NRF2 is encoded by NFE2L2 (Nuclear Factor, Erythroid 2 Like 2) gene and belongs to the Cap'n’Collar (CNC) subfamily of basic leucine zipper (bZIP) transcription factors. NRF2 is constantly undergoing rapid ubiquitination and proteasomal degradation through its physiological inhibitor, KEAP1 (Kelch‐like‐ECH‐ associated protein 1) [72,73] (Fig. 2A). However, when cells are under oxidative stress, the cysteine residues in KEAP1 are oxidized, leading to KEAP1 conformational changes that result in the release of NRF2 from KEAP1. As a result, the free and newly synthesized NRF2 is protected from KEAP1-mediated ubiquitination and degradation. It accumulates and translocates to the nucleus where it binds to the antioxidant response elements (ARE) on the promoter region of its target genes (Fig. 2B). More than 250 NRF2 target genes were reported, including many genes that directly or indirectly possess antioxidant properties. Examples of NRF2 target genes include aldehyde dehydrogenase 1 (ALDH1), NAD(P)H quinone oxidoreductase 1 (NQO1), glutathione S-transferases (GSTs), UDP-glucuronosyltransferases (UGTs), heme oxygenase-1 (HO-1), and glutathione reductase (GR) [74,75]. In addition to the canonical KEAP1-dependent activation of NRF2, several KEAP1-independent mechanisms regulate NRF2 expression and stability [74,76] (Fig. 2B). GSK3- α/β has been recognized as another NRF2 negative regulator by targeting NRF2 to the SCF/β-TrCP-mediated degradation, which is reported to be more sensitive to metabolic changes [[77], [78], [79]]. HRD1, regulated by XBP1 [80], an endoplasmic reticulum protein, has recently been reported as a novel E3 ubiquitin ligase responsible for compromised NRF2 response during liver cirrhosis [81]. A number of proteins can bind to KEAP1, disrupt the KEAP1-NRF2 complex, leading to accumulation of NRF2, such as p62, an autophagy-related protein [82,83], dipeptidyl peptidase 3 (DPP3) [84], Wilms tumor gene on X chromosome (WTX) [85], and Partner and localizer of BRCA2 (PALB2) [86]. In addition, p21Cip1/WAF1 [87] and BRCA1 [88] can directly interact with NRF2, thereby disrupting the KEAP1-NRF2 complex to activate NRF2.

NRF2 regulatory mechanisms.
Fig. 2

NRF2 regulatory mechanisms.

A) three reported negative regulatory mechanisms of NRF2. KEAP1 is the first and major NRF2 negative regulator in cells. In normal condition, KEAP1 binds to NRF2 and connects NRF2 to Cullin3 E3 ubiquitin ligase, leads to NRF2 degradation in proteasome. In addition, GSK-3α/β kinases can phosphorylate NRF2 which lets it binding to β-TrCP-Cul1 ubiquitin ligase, leads to NRF2 degradation in proteasome. HRD1 is a recently identified E3 ubiquitin ligase which targets NRF2 when activated by XBP1 under ER stress. So far, this regulatory pathway has only been reported during liver cirrhosis. B) NRF2 activation mechanisms. When cells are under stresses such as electrophilic stimuli, cysteine molecules in KEAP1 are modified (oxidized) that leads to release of NRF2 from KEAP1-Cul3-mediated ubiquitination. The free and newly-synthesized NRF2 then accumulates and translocates to nucleus and binds to the ARE on its target genes' promotor and activates its target genes. So far, about 250 target genes have been reported involving Phase I-III metabolism, redox regulation, lipid and carbohydrate metabolism, iron/hemo metabolism and many other cellular processes. In addition to this canonic KEAP1 dependent mechanism, many non-canonic mechanisms have been reported. For example, KEAP1 genetic mutations, promoter hypermethylation which inactivate KEAP1, some proteins binding to KEAP1 to interfere with KEAP-NRF2 interaction, such as p62, PALB2. Genetic mutations of NRF2, epigenetic regulation, phosphorylation and SUMOylation of NRF2 itself activate NRF2. Some proteins such as p21, BRCA1 and APE1 have been reported to bind to NRF2 to interfere with NRF2-KEAP1 interaction. Taken together, the NRF2 is a master transcriptional regulator in cellular antioxidant function and other cellular processes. The regulatory mechanisms are complex and context-dependent.

Although NRF2 activation may reduce cancer risk by suppressing oxidative stress and tumor promoting inflammation, an increase in NRF2 expression and activity level has been observed in several cancer types [71,72,75]. The constitutive activation of NRF2 has been reported in several cancers through NFE2L2 genetic mutations [89,90]. We have shown that transient exposure of EAC cells to reflux conditions induced NRF2 accumulation and activation with upregulation of its target genes [91]. The induction of HO-1 and GR in these cells protect against ABS-induced oxidative DNA damage and apoptosis, in concordance with NRF2 basic antioxidant functions [91]. We observed that NRF2 was constitutively upregulated in neoplastic esophageal cells (dysplasia and EAC) and primary EAC samples. Surprisingly, NRF2 was not constitutively up-regulated in non-neoplastic Barrett's cells and tissues. Our analysis of COSMIC (Catalogue of Somatic Mutations in Cancers) database indicated low incidence of mutation of NFE2L2 and KEAP1 in EAC (NFE2L2 in 6.6% (38/576) whereas KEAP1 in 1.22% (7/576)). Therefore, the frequent constitutive overexpression of NRF2 in EAC is a non-mutational event that is likely independent of canonical KEAP1 mechanisms.

The Apurinic/apyrimidinic endonuclease 1 (APE1) (also known as APEX1 or redox factor 1 (REF1)) is one of the key enzymes of the base excision repair (BER) pathways in mammals. APE1 is the key enzyme required for repair of Apurinic/apyrimidinic (AP) sites, a major type of oxidative DNA damage lesions generated by ROS [[92], [93], [94]]. On the other hand, APE1 possesses redox activity that is required for activation of redox-dependent transcription factors such as HIF-1α (hypoxia inducible factor-1α) [95], NF-κB (nuclear factor-κB (NF-κB) [96], p53, CREB (cAMP response element binding protein) and AP-1 (activator protein-1) [94,97]. Recent studies indicate that APE1 is frequently overexpressed at the protein level in human cancers, including EAC [[98], [99], [100]]. APE1 was also induced in response to ABS exposure in esophageal cells [100]. High levels of APE1 protect Barrett's and EAC cells against oxidative DNA damage and DNA double stand breaks, promoting cell survival by regulating JNK and p38 kinases [100]. We have demonstrated that the APE1 redox activity is required for ABS-induced activation of EGFR-STAT3 signaling axis [33]. Activation of STAT3 is an important molecular landmark in carcinogenesis for many human malignancies [101,102], including gastrointestinal tract cancers [103]. Furthermore, APE1 interacts with ARF6 to enhance MMP14 recycling in a redox-sensitive manner, promoting cell invasion [104]. Of note, our recent work suggests that APE1 may regulate NRF2 protein expression in esophageal epithelial cells through a KEAP1-independent regulation of NRF2 stability, likely dependent on APE1 redox activity in EAC (unpublished data). Based on these multiple lines of evidence, the constitutive upregulation of APE1-NRF2 axis in Barrett's carcinogenesis rebalances redox homeostasis in favor of tumorigenic cell survival, contributing to tumor progression and invasion (Fig. 1 C).

Dual roles of NRF2 in Barrett's tumorigenesis

As we have mentioned above, during GERD-BE-EAC process, episodes of reflux of acidic bile salts and chronic inflammation induce high levels of ROS [24,105]. Oxidative stress leads to oxidative DNA damage in both nuclear and mitochondrial DNA, including DNA strand breaks [25,27,28]. In addition, ROS induces protein oxidation as well as lipid peroxidation, producing mutagenic and carcinogenic reactive aldehydes such as 4-hydroxy-2-nonenal (4-HNE) and malondialdehyde (MDA) [[106], [107], [108]], known to be associated with tumorigenesis [109]. We have demonstrated that upon ABS exposure, esophageal cells respond by transiently activating APE1 and NRF2 pathways to reduce intracellular ROS and subsequent DNA damage [91,100]. Therefore, NRF2 may play a protective tumor suppressor role during the early pre-neoplastic stages of esophageal tumorigenesis (Fig. 3A). This is consistent with early discoveries using NRF2 knockout mice which demonstrated that NRF2 knockout mice were more susceptible to chemical-induced tumorigenesis [110,111].

Potential application of NRF2 activators and inhibitors in GERD-BE-EAC patients.
Fig. 3

Potential application of NRF2 activators and inhibitors in GERD-BE-EAC patients.

A) Based on ROS, APE1 and NRF2 levels in GERD-BE-EAC sequence, it is expected that NRF2 activators may be benefit for the patients with GERD and BE. However, cautions must be taken due to the “Dark Side” of NRF2 in which activated NRF2 may promote tumor growth once tumor initiating cells form. For EAC patients, NRF2 inhibitors may be used as adjuvant therapy or in combination with other therapeutic approaches. B) An assumptive figure to illustrate potential mechanisms of use NRF2 inhibitors (NRF2i) in combination with other therapeutic approaches, particularly those that work on the increase of ROS to kill cancer cells, for example cisplatin. Primary cancer cells usually are heterogeneity in terms of intracellular ROS level. Some cancer cells such as cancer stem cells or senescent cells may possess lower ROS than regular cancer cells. Therefore, single drug therapy may only kill partial cancer cells with higher basal ROS levels. Administration of NRF2 inhibitors (NRF2i) in combination with other chemo-/radio-therapy sensitizes tumor cells to these therapies through obvious increase ROS level to lethal threshold. T1-T5 represent tumor populations with different ROS levels.

However, in neoplastic esophageal cells (dysplastic and EAC), NRF2 is constitutively overexpressed. High levels of NRF2 in neoplastic cells counteract elevated ROS levels and promotes tumor cell survival [100,105]. The overexpression of NRF2 has been associated with uncontrolled tumor growth, angiogenesis, migration, invasion, metastasis and drug resistance [69,75,112]. Recent discoveries indicate that NRF2 is an important player in reprograming cancer cell metabolism [[113], [114], [115]], cancer stem cell properties [116,117], tumor microenvironment and immune response [[118], [119], [120]]. ALDH1 (Aldehyde dehydrogenase 1), an enzyme normally involved in retinol metabolism catalyzing/oxidizing retinaldehyde to retinoic acid, is found upregulated in many human cancer types including gastrointestinal cancers [121,122] and is associated with poor prognosis [123,124]. More importantly, ALDH1 is regarded as one of the unique cancer stem cell (CSC) markers of many human malignancies, and is required for tumor cells to maintain their stemness [124,125]. Heme oxygenase-1 (HO-1) is a microsomal enzyme which catalyzes the oxidation of heme to biologically active products: carbon monoxide (CO), biliverdin, and ferrous iron [126]. As a NRF2 target gene, we have shown that HO-1 was transiently induced in esophageal epithelial cells in response to ABS exposure conditions that mimic a GERD episode [91]. However, like NRF2, HO-1 is overexpressed in many human cancers [127,128]. Constitutive upregulation of HO-1 in tumor tissues favors tumor cells' survival through various mechanisms that include decreasing intracellular ROS, activating AKT and inhibiting apoptosis pathways [128,129]. NRF2 plays a key role in activation of almost all known hallmarks of cancer [129]. In almost all cancer types, overexpression NRF2 is associated with poor prognosis and drug- or radio-resistance [130,131]. In this context, NRF2 plays an oncogenic role in EAC once tumor initiating cells are formed (Fig. 3A). Based on current lines of evidence, we can speculate that silencing of several genes in the glutathione pathways during Barrett's tumorigenesis is compensated via overexpression of NRF2 and possibly APE1 to promote a tumorigenic anti-oxidant response. This could be especially important with the recent evidence showing that some of the silenced glutathione family members, such as GPX3 and GPX7, possess tumor suppressor functions (discussed above). The molecular switch from transient induction to constitutive overexpression of NRF2 may define a conversion from an anti-tumorigenic to pro-tumorigenic antioxidant response during Barrett's carcinogenesis.

Modulation of oxidants and antioxidants in GERD-BE and EAC

Oxidative stress, associated with tumorigenesis, is linked with aging and many human diseases such as inflammatory diseases, neurodegenerative disorders and other diseases [1,[132], [133], [134]]. Therefore, a great effort has been made to explore various antioxidants for prevention or treatment of oxidative stress-related diseases [40,45,135]. In terms of antioxidants in cancer prevention and treatment, numerous per-clinical investigations and clinical trials have been conducted (https://www.clinicaltrials.gov/). It was expected that anti-oxidants would reduce risks for development of cancers. On the contrary, some trials showed that anti-oxidants increased the risk of developing some cancers such as lung cancer [136] and prostate cancer [137,138]. For example, the Alpha-Tocopherol Beta Carotene (ATBC) Cancer Prevention Study reported that male smokers receiving b-carotene had an 18% increase in lung cancer incidence [136]. The SELECT trial [137,138] was a randomized, double-blind, placebo-controlled trial of older males given vitamin E, selenium, both, or neither for 7–12 years. This large trial reported that men taking vitamin E alone had significantly higher risk to develop prostate cancer. Gill et al. [67] recently summarized randomized, placebo-controlled trials that included more than 10,000 participants. The U.S. Preventative Services Task Force (USPSTF), reviewing many of the available clinical trials, concluded that there was insufficient data for or against the use of most nutrient supplements for cancer prevention [139]. Similarly, clinical trials using anti-oxidants as adjuvant therapy in cancer patients’ treatment showed either no clear benefit or contradictory results [140,141].

As NRF2 is recognized as the master regulator of cellular anti-oxidative properties, numerous efforts have been made in developing NRF2 activators or inhibitors [142]. Hundreds of investigations have conducted in vitro and in vivo to evaluate natural or synthesized compounds as NRF2 activators or inhibitors [69,74,143]. So far, only fumaric acid ester dimethyl fumarate (DMF) (also called BG-12 or Tecfidera, from Biogen) has been FDA approved for treatment of psoriasis for many years [144]. Tecfidera was also approved in 2013 to treat relapsing-remitting multiple sclerosis (MS) [[145], [146], [147]]. Oltipraz (4-methyl-5(pyrazinyl-2)-1-2-dithiole-3-thione) is another promising NRF2 inducer undergoing evaluation in a phase III clinical trial for the treatment of nonalcoholic fatty liver disease [148]. In addition, several natural compounds such as sulforaphane [149,150], curcumin [151,152], and resveratrol [153,154] have been identified as NRF2 activators and are under extensive clinical trials in a wide range of oxidative-stress diseases (https://www.clinicaltrials.gov/). However, in terms of using these NRF2 inducers in cancers, a few have been tested in clinical trial studies. The major concern for modulating NRF2 using NRF2 activators relies on the fact that NRF2 functions are hijacked by tumor cells to favor their growth and progression [70,71,155,156]. This so-called “Dark Side” of NRF2 makes it a double-edged sword: a must-caution before applying these compounds in patients. Once tumor-initiating cells are formed at early stage of tumorigenesis, the administration of these compounds may accelerate tumor progression, even promoting metastasis [157,158] (Fig. 3A). For example, Tao, et al. [159] tested modulation of NRF2 in several in vivo mouse models and demonstrated that NRF2 activation prevented initiation of chemically induced cancer, and promoted progression of pre-existing tumors regardless of a chemical or genetic etiology. On the other hand, because NRF2 is overexpressed in many human cancers and is associated with tumor progression, metastasis, drug- or radio-resistance, and poor survival, targeting NRF2 has become an attractive adventure in cancer therapy. Brusatol (quassinoid, natural) is the first NRF2 inhibitor identified by screening natural product extracts [160]. Brusatol is reported to sensitize cancer cells to chemotherapeutic drugs via inhibition of NRF2 signaling pathway [160,161] (Fig. 3B). Although it has been pointed out that brusatol is a global translation inhibitor, it remains a useful tool to study NRF2 inhibition in cancer. Proteins with short half-life, such as NRF2, are the most susceptible ones to inhibitors of protein translation [162]. Tao et al. [159] reported that once tumors are initiated, NRF2 inhibition by brusatol is effective against chemically and spontaneously induced tumors. In addition to brusatol, other investigational compounds are capable to inhibit NRF2 activity, such as AME1 [163], ML385 [164], trigonelline [165], malabaricone A [166], ochratoxin A [167], and wogonin [168]. However, the molecular mechanisms and biological effects of these compounds need to be further investigated.

In terms of GERD-BE and EAC cascade (Fig. 3), as discussed above, we and others have demonstrated increased oxidative stress in this process. We reported that NRF2 is pivotal for esophageal epithelial cells to battle oxidative stress and protect cells from ABS-induced DNA damage. Therefore, from a hypothetical point of view, NRF2 activators may benefit patients and reduce risks for EAC development. However, a word of caution is due given the pro-tumorigenic functions of NRF2. NRF2 activators may in fact accelerate the progression of pre-neoplastic and neoplastic cells towards EAC. It is worth mentioning that there are reports of a beneficial role of antioxidants, such as manganese superoxide dismutase [169]. Several investigations reported that dietary antioxidants, fruits, and vegetables are inversely associated with BE or EAC risk [170,171], while no association was observed for supplements intake [170]. Of note, an early system review and meta-analysis of 14 randomized trials failed to find significant effects of supplementation with b-carotene, vitamins A, C, E, and selenium (alone or in combination), versus placebo, on esophageal, gastric, colorectal, pancreatic, and liver cancer incidences [172]. Regarding NRF2 activators as chemoprevention for BE and EAC, only few reports are available [173,174]. Some studies suggest that resveratrol [173] or curcumin supplementation [174] may have a chemoprevention role in BE. These findings exemplify the dilemma surrounding antioxidants and NRF2 applications in cancer prevention and treatment. Considering the so-called “Dark Side of NRF2”, there are warranted serious concerns for administering antioxidants or NRF2 activators in Barrett's conditions, where the cellular context may significantly alter the response from an anti-tumorigenic to a pro-tumorigenic outcome. For NRF2 inhibitors in EAC, these have not been fully investigated and there are no FDA approved drugs. In fact, the clinical utility of the pre-clinical studies is limited. These studies provide a proof of concept, not ready for clinical trials due to several limiting properties of the existing inhibitors.

Conclusions

The antioxidant response in Barrett's tumorigenesis is a complex molecular process. The observed molecular switch from transient induction of some antioxidant genes in pre-neoplastic conditions to their constitutive overexpression in neoplastic cells highlight different molecular functions and biological outcomes. Antioxidants such as APE1 and NRF2 may function as a double-edged sword where the outcome is context dependent where the stimulus and the cellular state matter. The molecular mechanisms and target genes that alter the anti-versus pro-tumorigenic functions of antioxidant response need to be fully elucidated to determine if and when activators or inhibitors can be utilized in patients with Barrett's or EAC.

Declaration of competing interest

None.

References

    Reuter S.. Oxidative stress, inflammation, and cancer: how are they linked?. Free Radic. Biol. Med.49: 112010. 1603-1616

    Lenaz G.. Mitochondria and reactive oxygen species. Which role in physiology and pathology?. Adv. Exp. Med. Biol.942: 2012. 93-136

    Poyton R.O., Ball K.A., Castello P.R.. Mitochondrial generation of free radicals and hypoxic signaling. Trends Endocrinol Metab20: 72009. 332-340

    Sies H., Jones D.P.. Reactive oxygen species (ROS) as pleiotropic physiological signalling agents. Nat. Rev. Mol. Cell Biol.2020.

    Marnett L.J.. Oxyradicals and DNA damage. Carcinogenesis21: 32000. 361-370

    Moriya M.. Single-stranded shuttle phagemid for mutagenesis studies in mammalian cells: 8-oxoguanine in DNA induces targeted G.C-->T.A transversions in simian kidney cells. Proc. Natl. Acad. Sci. U. S. A.90: 31993. 1122-1126

    Lee S.F., Pervaiz S.. Assessment of oxidative stress-induced DNA damage by immunoflourescent analysis of 8-oxodG. Methods Cell Biol.103: 2011. 99-113

    Guetens G.. Oxidative DNA damage: biological significance and methods of analysis. Crit. Rev. Clin. Lab Sci.39: 4–52002. 331-457

    Tudek B., Speina E.. Oxidatively damaged DNA and its repair in colon carcinogenesis. Mutat. Res.736: 1–22012. 82-92

10 

    Valavanidis A., Vlachogianni T., Fiotakis C.. 8-hydroxy-2' -deoxyguanosine (8-OHdG): a critical biomarker of oxidative stress and carcinogenesis. J. Environ. Sci. Health C Environ. Carcinog. Ecotoxicol. Rev.27: 22009. 120-139

11 

    Loft S., Poulsen H.E.. Cancer risk and oxidative DNA damage in man. J. Mol. Med.74: 61996. 297-312

12 

    Bray F.. Global cancer statistics 2018: GLOBOCAN estimates of incidence and mortality worldwide for 36 cancers in 185 countries. CA A Cancer J. Clin.68: 62018. 394-424

13 

    Coia L.R., Sauter E.R.. Esophageal cancer. Curr. Probl. Canc.18: 41994. 189-247

14 

    Blot W.J., McLaughlin J.K.. The changing epidemiology of esophageal cancer. Semin. Oncol.26: 5 Suppl 151999. 2-8

15 

    Pera M.. Epidemiology of esophageal cancer, especially adenocarcinoma of the esophagus and esophagogastric junction. Recent Results Canc. Res.155: 2000. 1-14

16 

    Coleman H.G., Xie S.H., Lagergren J.. The epidemiology of esophageal adenocarcinoma. Gastroenterology154: 22018. 390-405

17 

    di Pietro M.. Barrett's esophagus and reflux disease. Endoscopy42: 112010. 910-915

18 

    Spechler S.J., Goyal R.K.. Barrett's esophagus. N. Engl. J. Med.315: 61986. 362-371

19 

    Falk G.W.. Barrett's esophagus. Gastrointest Endosc Clin N Am4: 41994. 773-789

20 

    Thrift A.P.. Barrett's esophagus and esophageal adenocarcinoma: how common are they really?. Dig. Dis. Sci.63: 82018. 1988-1996

21 

    Altorki N.K., Skinner D.B.. Adenocarcinoma in Barrett's esophagus. Semin. Surg. Oncol.6: 51990. 274-278

22 

    Song J.H.. Oxidative stress from reflux esophagitis to esophageal cancer: the alleviation with antioxidants. Free Radic. Res.50: 102016. 1071-1079

23 

    Lee J.S.. Involvement of oxidative stress in experimentally induced reflux esophagitis and Barrett's esophagus: clue for the chemoprevention of esophageal carcinoma by antioxidants. Mutat. Res.480–481: 2001. 189-200

24 

    Dvorak K.. Bile acids in combination with low pH induce oxidative stress and oxidative DNA damage: relevance to the pathogenesis of Barrett's oesophagus. Gut56: 62007. 763-771

25 

    Peng D.. Glutathione peroxidase 7 protects against oxidative DNA damage in oesophageal cells. Gut2011.

26 

    Zhou Z.. Activation of EGFR-DNA-PKcs pathway by IGFBP2 protects esophageal adenocarcinoma cells from acidic bile salts-induced DNA damage. J. Exp. Clin. Canc. Res.38: 12019. 13

27 

    Dvorak K.. Bile acids in combination with low pH induce oxidative stress and oxidative DNA damage: relevance to the pathogenesis of Barrett's Oesophagus. Gut2006.

28 

    Dvorak K.. Esophageal acid exposure at pH < or = 2 is more common in Barrett's esophagus patients and is associated with oxidative stress. Dis. Esophagus19: 52006. 366-372

29 

    Picardo S.L.. Barrett's to oesophageal cancer sequence: a model of inflammatory-driven upper gastrointestinal cancer. Dig. Surg.29: 32012. 251-260

30 

    Poehlmann A.. Inflammation and Barrett's carcinogenesis. Pathol. Res. Pract.208: 52012. 269-280

31 

    Coussens L.M., Werb Z.. Inflammation and cancer. Nature420: 69172002. 860-867

32 

    Peng D.F.. Loss of glutathione peroxidase 7 promotes TNF-alpha-induced NF-kappaB activation in Barrett's carcinogenesis. Carcinogenesis35: 72014. 1620-1628

33 

    Bhat A.A.. Exposure of Barrett's and esophageal adenocarcinoma cells to bile acids activates EGFR-STAT3 signaling axis via induction of APE1. Oncogene37: 462018. 6011-6024

34 

    Zhang H.Y.. Cancer-related inflammation and Barrett's carcinogenesis: interleukin-6 and STAT3 mediate apoptotic resistance in transformed Barrett's cells. Am. J. Physiol. Gastrointest. Liver Physiol.300: 32011.

35 

    Inayama M.. Involvement of oxidative stress in experimentally induced reflux esophagitis and esophageal cancer. Hepato-Gastroenterology54: 752007. 761-765

36 

    O'Farrell N.J.. Differential expression profiles of oxidative stress levels, 8-oxo-dG and 4-HNE, in barrett's esophagus compared to esophageal adenocarcinoma. Int. J. Mol. Sci.20: 182019.

37 

    Kauppi J.. Increased oxidative stress in the proximal stomach of patients with barrett's esophagus and adenocarcinoma of the esophagus and esophagogastric junction. Transl Oncol9: 42016. 336-339

38 

    Rasanen J.V.. The expression of 8-hydroxydeoxyguanosine in oesophageal tissues and tumours. Eur. J. Surg. Oncol.33: 102007. 1164-1168

39 

    Jimenez P.. Free radicals and antioxidant systems in reflux esophagitis and Barrett's esophagus. World J. Gastroenterol.11: 182005. 2697-2703

40 

    Valko M.. Free radicals and antioxidants in normal physiological functions and human disease. Int. J. Biochem. Cell Biol.39: 12007. 44-84

41 

    Valko M.. Free radicals, metals and antioxidants in oxidative stress-induced cancer. Chem. Biol. Interact.160: 12006. 1-40

42 

    Halliwell B.. Biochemistry of oxidative stress. Biochem. Soc. Trans.35: Pt 52007. 1147-1150

43 

    Hayes J.D., McLellan L.I.. Glutathione and glutathione-dependent enzymes represent a co-ordinately regulated defence against oxidative stress. Free Radic. Res.31: 41999. 273-300

44 

    McCord J.M., Fridovich I.. Superoxide dismutase. An enzymic function for erythrocuprein (hemocuprein). J Biol Chem244: 221969. 6049-6055

45 

    Willcox J.K., Ash S.L., Catignani G.L.. Antioxidants and prevention of chronic disease. Crit. Rev. Food Sci. Nutr.44: 42004. 275-295

46 

    Findlay J.M., Middleton M.R., Tomlinson I.. Genetic susceptibility to Barrett's oesophagus: lessons from early studies. United European Gastroenterol J4: 42016. 485-492

47 

    Findlay J.M., Middleton M.R., Tomlinson I.. Genetic biomarkers of barrett's esophagus susceptibility and progression to dysplasia and cancer: a systematic review and meta-analysis. Dig. Dis. Sci.61: 12016. 25-38

48 

    Gharahkhani P.. Genome-wide association studies in oesophageal adenocarcinoma and Barrett's oesophagus: a large-scale meta-analysis. Lancet Oncol.17: 102016. 1363-1373

49 

    Casson A.G.. Genetic polymorphisms of microsomal epoxide hydroxylase and glutathione S-transferases M1, T1 and P1, interactions with smoking, and risk for esophageal (Barrett) adenocarcinoma. Canc. Detect. Prev.30: 52006. 423-431

50 

    van Lieshout E.M.. Low glutathione and glutathione S-transferase levels in Barrett's esophagus as compared to normal esophageal epithelium. Jpn. J. Canc. Res.90: 11999. 81-85

51 

    Ferrer-Torres D.. Constitutively higher level of GSTT2 in esophageal tissues from african Americans protects cells against DNA damage. Gastroenterology156: 52019. 1404-1415

52 

    Brabender J.. Glutathione S-transferase-pi expression is downregulated in patients with Barrett's esophagus and esophageal adenocarcinoma. J. Gastrointest. Surg.6: 32002. 359-367

53 

    Cobbe S.C.. Alteration of glutathione S-transferase levels in Barrett's metaplasia compared to normal oesophageal epithelium. Eur. J. Gastroenterol. Hepatol.15: 12003. 41-47

54 

    Peters W.H.. Glutathione and glutathione S-transferases in Barrett's epithelium. Br. J. Canc.67: 61993. 1413-1417

55 

    Thanan R.. Proton pump inhibitors suppress iNOS-dependent DNA damage in Barrett's esophagus by increasing Mn-SOD expression. Biochem. Biophys. Res. Commun.421: 22012. 280-285

56 

    Peng D.F.. DNA hypermethylation regulates the expression of members of the Mu-class glutathione S-transferases and glutathione peroxidases in Barrett's adenocarcinoma. Gut58: 12009. 5-15

57 

    Peng D.. Glutathione peroxidase 7 has potential tumour suppressor functions that are silenced by location-specific methylation in oesophageal adenocarcinoma. Gut63: 42014. 540-551

58 

    Peng D.. Location-specific epigenetic regulation of the metallothionein 3 gene in esophageal adenocarcinomas. PloS One6: 72011.

59 

    Lee O.J.. Hypermethylation and loss of expression of glutathione peroxidase-3 in Barrett's tumorigenesis. Neoplasia7: 92005. 854-861

60 

    Peng D.F.. Silencing of glutathione peroxidase 3 through DNA hypermethylation is associated with lymph node metastasis in gastric carcinomas. PloS One7: 102012.

61 

    Cai M.. Gpx3 prevents migration and invasion in gastric cancer by targeting NFsmall ka, CyrillicB/Wnt5a/JNK signaling. Int. J. Clin. Exp. Pathol.12: 42019. 1194-1203

62 

    Mohamed M.M.. Promoter hypermethylation and suppression of glutathione peroxidase 3 are associated with inflammatory breast carcinogenesis. Oxid Med Cell Longev2014: 2014. 787195

63 

    Yu Y.P.. Glutathione peroxidase 3, deleted or methylated in prostate cancer, suppresses prostate cancer growth and metastasis. Canc. Res.67: 172007. 8043-8050

64 

    Barrett C.W.. Tumor suppressor function of the plasma glutathione peroxidase gpx3 in colitis-associated carcinoma. Canc. Res.73: 32013. 1245-1255

65 

    Chen Z.. Glutathione peroxidase 7 suppresses cancer cell growth and is hypermethylated in gastric cancer. Oncotarget8: 332017. 54345-54356

66 

    Peppelenbosch M.P., Spaander M.C., Bruno M.J.. Glutathione peroxidase 7 prevents cancer in the oesophagus. Gut63: 42014. 537-538

67 

    Gill J.G., Piskounova E., Morrison S.J.. Cancer, oxidative stress, and metastasis. Cold Spring Harbor Symp. Quant. Biol.81: 2016. 163-175

68 

    Hayes J.D., Dinkova-Kostova A.T., Tew K.D.. Oxidative stress in cancer. Canc. Cell2020.

69 

    Leinonen H.M.. Role of the Keap1-Nrf2 pathway in cancer. Adv. Canc. Res.122: 2014. 281-320

70 

    Lau A.. Dual roles of Nrf2 in cancer. Pharmacol. Res.58: 5–62008. 262-270

71 

    Menegon S., Columbano A., Giordano S.. The dual roles of NRF2 in cancer. Trends Mol. Med.22: 72016. 578-593

72 

    Kansanen E.. The Keap1-Nrf2 pathway: mechanisms of activation and dysregulation in cancer. Redox biology1: 12013. 45-49

73 

    McMahon M.. Keap1-dependent proteasomal degradation of transcription factor Nrf2 contributes to the negative regulation of antioxidant response element-driven gene expression. J. Biol. Chem.278: 242003. 21592-21600

74 

    Dodson M.. Modulating NRF2 in disease: timing is everything. Annu. Rev. Pharmacol. Toxicol.59: 2019. 555-575

75 

    Taguchi K., Yamamoto M.. The KEAP1-NRF2 system in cancer. Front Oncol7: 2017. 85

76 

    Silva-Islas C.A., Maldonado P.D.. Canonical and non-canonical mechanisms of Nrf2 activation. Pharmacol. Res.134: 2018. 92-99

77 

    Rada P.. SCF/{beta}-TrCP promotes glycogen synthase kinase 3-dependent degradation of the Nrf2 transcription factor in a Keap1-independent manner. Mol. Cell Biol.31: 62011. 1121-1133

78 

    Cuadrado A.. Structural and functional characterization of Nrf2 degradation by glycogen synthase kinase 3/beta-TrCP. Free Radic. Biol. Med.88: Pt B2015. 147-157

79 

    Rada P.. Structural and functional characterization of Nrf2 degradation by the glycogen synthase kinase 3/beta-TrCP axis. Mol. Cell Biol.32: 172012. 3486-3499

80 

    Yamamoto K.. Human HRD1 promoter carries a functional unfolded protein response element to which XBP1 but not ATF6 directly binds. J. Biochem.144: 42008. 477-486

81 

    Wu T.. Hrd1 suppresses Nrf2-mediated cellular protection during liver cirrhosis. Genes Dev.28: 72014. 708-722

82 

    Jiang T.. p62 links autophagy and Nrf2 signaling. Free Radic. Biol. Med.88: Pt B2015. 199-204

83 

    Lau A.. A noncanonical mechanism of Nrf2 activation by autophagy deficiency: direct interaction between Keap1 and p62. Mol. Cell Biol.30: 132010. 3275-3285

84 

    Lu K.. NRF2 induction supporting breast cancer cell survival is enabled by oxidative stress-induced DPP3-KEAP1 interaction. Canc. Res.77: 112017. 2881-2892

85 

    Camp N.D.. Wilms tumor gene on X chromosome (WTX) inhibits degradation of NRF2 protein through competitive binding to KEAP1 protein. J. Biol. Chem.287: 92012. 6539-6550

86 

    Ma J.. PALB2 interacts with KEAP1 to promote NRF2 nuclear accumulation and function. Mol. Cell Biol.32: 82012. 1506-1517

87 

    Chen W.. Direct interaction between Nrf2 and p21(Cip1/WAF1) upregulates the Nrf2-mediated antioxidant response. Mol. Cell34: 62009. 663-673

88 

    Gorrini C.. BRCA1 interacts with Nrf2 to regulate antioxidant signaling and cell survival. J. Exp. Med.210: 82013. 1529-1544

89 

    Goldstein L.D.. Recurrent loss of NFE2L2 exon 2 is a mechanism for Nrf2 pathway activation in human cancers. Cell Rep.16: 102016. 2605-2617

90 

    Sasaki H.. Genotype analysis of the NRF2 gene mutation in lung cancer. Int. J. Mol. Med.31: 52013. 1135-1138

91 

    Peng D.. NRF2 antioxidant response protects against acidic bile salts-induced oxidative stress and DNA damage in esophageal cells. Canc. Lett.458: 2019. 46-55

92 

    Fung H., Demple B.. A vital role for Ape1/Ref1 protein in repairing spontaneous DNA damage in human cells. Mol. Cell17: 32005. 463-470

93 

    Sung J.S., Demple B.. Roles of base excision repair subpathways in correcting oxidized abasic sites in DNA. FEBS J.273: 82006. 1620-1629

94 

    Evans A.R., Limp-Foster M., Kelley M.R.. Going APE over ref-1. Mutat. Res.461: 22000. 83-108

95 

    Logsdon D.P.. Regulation of HIF1alpha under hypoxia by APE1/ref-1 impacts CA9 expression: dual targeting in patient-derived 3D pancreatic cancer models. Mol. Canc. Therapeut.15: 112016. 2722-2732

96 

    Ando K.. A new APE1/Ref-1-dependent pathway leading to reduction of NF-kappaB and AP-1, and activation of their DNA-binding activity. Nucleic Acids Res.36: 132008. 4327-4336

97 

    Tell G.. The many functions of APE1/Ref-1: not only a DNA repair enzyme. Antioxidants Redox Signal.11: 32009. 601-620

98 

    Yuan C.L.. APE1 overexpression is associated with poor survival in patients with solid tumors: a meta-analysis. Oncotarget8: 352017. 59720-59728

99 

    Wang D.. APE1 overexpression is associated with cisplatin resistance in non-small cell lung cancer and targeted inhibition of APE1 enhances the activity of cisplatin in A549 cells. Lung Canc.66: 32009. 298-304

100 

    Hong J.. APE1-mediated DNA damage repair provides survival advantage for esophageal adenocarcinoma cells in response to acidic bile salts. Oncotarget7: 132016. 16688-16702

101 

    Gu Y., Mohammad I.S., Liu Z.. Overview of the STAT-3 signaling pathway in cancer and the development of specific inhibitors. Oncol Lett19: 42020. 2585-2594

102 

    Jin W.. Role of JAK/STAT3 signaling in the regulation of metastasis, the transition of cancer stem cells, and chemoresistance of cancer by epithelial-mesenchymal transition. Cells9: 12020.

103 

    Li B., Huang C.. Regulation of EMT by STAT3 in gastrointestinal cancer (Review). Int. J. Oncol.50: 32017. 753-767

104 

    Lu H.. APE1 upregulates MMP-14 via redox-sensitive ARF6-mediated recycling to promote cell invasion of esophageal adenocarcinoma. Canc. Res.79: 172019. 4426-4438

105 

    Perez S.. Redox signaling in the gastrointestinal tract. Free Radic. Biol. Med.104: 2017. 75-103

106 

    Zhong H., Yin H.. Role of lipid peroxidation derived 4-hydroxynonenal (4-HNE) in cancer: focusing on mitochondria. Redox Biol4: 2015. 193-199

107 

    Xiao M.. Pathophysiology of mitochondrial lipid oxidation: role of 4-hydroxynonenal (4-HNE) and other bioactive lipids in mitochondria. Free Radic. Biol. Med.111: 2017. 316-327

108 

    Dodson M., Castro-Portuguez R., Zhang D.D.. NRF2 plays a critical role in mitigating lipid peroxidation and ferroptosis. Redox Biol23: 2019. 101107

109 

    Burcham P.C.. Genotoxic lipid peroxidation products: their DNA damaging properties and role in formation of endogenous DNA adducts. Mutagenesis13: 31998. 287-305

110 

    Ramos-Gomez M.. Interactive effects of nrf2 genotype and oltipraz on benzo[a]pyrene-DNA adducts and tumor yield in mice. Carcinogenesis24: 32003. 461-467

111 

    Xu C.. Inhibition of 7,12-dimethylbenz(a)anthracene-induced skin tumorigenesis in C57BL/6 mice by sulforaphane is mediated by nuclear factor E2-related factor 2. Canc. Res.66: 162006. 8293-8296

112 

    DeNicola G.M.. Oncogene-induced Nrf2 transcription promotes ROS detoxification and tumorigenesis. Nature475: 73542011. 106-109

113 

    He F., Antonucci L., Karin M.. NRF2 as a regulator of cell metabolism and inflammation in cancer. Carcinogenesis2020.

114 

    Smolkova K.. Nuclear factor erythroid 2-related factor 2 in regulating cancer metabolism. Antioxidants Redox Signal.2020.

115 

    Wang Y.Y.. Nrf2-Mediated metabolic reprogramming in cancer. Oxid Med Cell Longev2018: 2018. 9304091

116 

    Kahroba H.. The Role of Nrf2 signaling in cancer stem cells: from stemness and self-renewal to tumorigenesis and chemoresistance. Life Sci.239: 2019. 116986

117 

    Ryoo I.G., Lee S.H., Kwak M.K.. Redox modulating NRF2: a potential mediator of cancer stem cell resistance. Oxid Med Cell Longev2016: 2016. 2428153

118 

    Xu X.. NFE2L2/KEAP1 mutations correlate with higher tumor mutational burden value/PD-L1 expression and potentiate improved clinical outcome with immunotherapy. Oncol.2020.

119 

    Best S.A.. Synergy between the KEAP1/NRF2 and PI3K pathways drives non-small-cell lung cancer with an altered immune microenvironment. Cell Metabol.27: 42018. 935-943

120 

    Wang J.. Nrf2 suppresses the function of dendritic cells to facilitate the immune escape of glioma cells. Exp. Cell Res.360: 22017. 66-73

121 

    Chen J.. Prognostic value of cancer stem cell marker ALDH1 expression in colorectal cancer: a systematic review and meta-analysis. PloS One10: 122015.

122 

    Taniguchi H.. Cancer stem cells in human gastrointestinal cancer. Canc. Sci.107: 112016. 1556-1562

123 

    Li X.S.. ALDH1A1 overexpression is associated with the progression and prognosis in gastric cancer. BMC Canc.14: 2014. 705

124 

    Yang L.. ALDH1A1 defines invasive cancer stem-like cells and predicts poor prognosis in patients with esophageal squamous cell carcinoma. Mod. Pathol.27: 52014. 775-783

125 

    Tomita H.. Aldehyde dehydrogenase 1A1 in stem cells and cancer. Oncotarget7: 102016. 11018-11032

126 

    Maines M.D.. Heme oxygenase: function, multiplicity, regulatory mechanisms, and clinical applications. Faseb. J.2: 101988. 2557-2568

127 

    Jozkowicz A., Was H., Dulak J.. Heme oxygenase-1 in tumors: is it a false friend?. Antioxidants Redox Signal.9: 122007. 2099-2117

128 

    Zhu X.. Heme oxygenase-1 system and gastrointestinal tumors. World J. Gastroenterol.16: 212010. 2633-2637

129 

    Rojo de la Vega M., Chapman E., Zhang D.D.. NRF2 and the hallmarks of cancer. Canc. Cell34: 12018. 21-43

130 

    Cloer E.W.. NRF2 activation in cancer: from DNA to protein. Canc. Res.79: 52019. 889-898

131 

    Zimta A.A.. The role of Nrf2 activity in cancer development and progression. Cancers (Basel)11: 112019.

132 

    Kryston T.B.. Role of oxidative stress and DNA damage in human carcinogenesis. Mutat. Res.2011.

133 

    Lonkar P., Dedon P.C.. Reactive species and DNA damage in chronic inflammation: reconciling chemical mechanisms and biological fates. International journal of cancer. J. Int. Cancer128: 92011. 1999-2009

134 

    Wei Y.H.. Oxidative stress in human aging and mitochondrial disease-consequences of defective mitochondrial respiration and impaired antioxidant enzyme system. Chin. J. Physiol.44: 12001. 1-11

135 

    Ray G., Husain S.A.. Oxidants, antioxidants and carcinogenesis. Indian J. Exp. Biol.40: 112002. 1213-1232

136 

    Alpha-Tocopherol, B.C.C.P.S.G. The effect of vitamin E and beta carotene on the incidence of lung cancer and other cancers in male smokers. N. Engl. J. Med.330: 151994. 1029-1035

137 

    Lippman S.M.. Effect of selenium and vitamin E on risk of prostate cancer and other cancers: the Selenium and Vitamin E Cancer Prevention Trial (SELECT). JAMA301: 12009. 39-51

138 

    Klein E.A.. Vitamin E and the risk of prostate cancer: the selenium and vitamin E cancer prevention trial (SELECT). JAMA306: 142011. 1549-1556

139 

    Moyer V.A., Force U.S.P.S.T.. Vitamin, mineral, and multivitamin supplements for the primary prevention of cardiovascular disease and cancer: U.S. Preventive services Task Force recommendation statement. Ann. Intern. Med.160: 82014. 558-564

140 

    Jacobs C.. Is there a role for oral or intravenous ascorbate (vitamin C) in treating patients with cancer? A systematic review. Oncol.20: 22015. 210-223

141 

    Yasueda A., Urushima H., Ito T.. Efficacy and interaction of antioxidant supplements as adjuvant therapy in cancer treatment: a systematic review. Integr. Canc. Ther.15: 12016. 17-39

142 

    Sova M., Saso L.. Design and development of Nrf2 modulators for cancer chemoprevention and therapy: a review. Drug Des. Dev. Ther.12: 2018. 3181-3197

143 

    Robledinos-Anton N.. Activators and inhibitors of NRF2: a review of their potential for clinical development. Oxid Med Cell Longev2019: 2019. 9372182

144 

    Hoxtermann S., Nuchel C., Altmeyer P.. Fumaric acid esters suppress peripheral CD4- and CD8-positive lymphocytes in psoriasis. Dermatology196: 21998. 223-230

145 

    Fox R.J.. Placebo-controlled phase 3 study of oral BG-12 or glatiramer in multiple sclerosis. N. Engl. J. Med.367: 122012. 1087-1097

146 

    Gold R.. Placebo-controlled phase 3 study of oral BG-12 for relapsing multiple sclerosis. N. Engl. J. Med.367: 122012. 1098-1107

147 

    Havrdova E.. Oral BG-12 (dimethyl fumarate) for relapsing-remitting multiple sclerosis: a review of DEFINE and CONFIRM. Evaluation of: gold R, Kappos L, Arnold D, et al. Placebo-controlled phase 3 study of oral BG-12 for relapsing multiple sclerosis. N. Engl. J. Med.367: 2012.

148 

    Kim W.. Randomised clinical trial: the efficacy and safety of oltipraz, a liver X receptor alpha-inhibitory dithiolethione in patients with non-alcoholic fatty liver disease. Aliment. Pharmacol. Ther.45: 82017. 1073-1083

149 

    Houghton C.A.. Sulforaphane: its "coming of age" as a clinically relevant nutraceutical in the prevention and treatment of chronic disease. Oxid Med Cell Longev2019: 2019. 2716870

150 

    Yagishita Y.. Broccoli or sulforaphane: is it the source or dose that matters?. Molecules24: 192019.

151 

    Gupta S.C., Patchva S., Aggarwal B.B.. Therapeutic roles of curcumin: lessons learned from clinical trials. AAPS J.15: 12013. 195-218

152 

    Salehi B.. The therapeutic potential of curcumin: a review of clinical trials. Eur. J. Med. Chem.163: 2019. 527-545

153 

    Singh A.P.. Health benefits of resveratrol: evidence from clinical studies. Med. Res. Rev.39: 52019. 1851-1891

154 

    Timmers S., Hesselink M.K., Schrauwen P.. Therapeutic potential of resveratrol in obesity and type 2 diabetes: new avenues for health benefits?. Ann. N. Y. Acad. Sci.1290: 2013. 83-89

155 

    Moon E.J., Giaccia A.. Dual roles of NRF2 in tumor prevention and progression: possible implications in cancer treatment. Free Radic. Biol. Med.79: 2015. 292-299

156 

    Wu S., Lu H., Bai Y.. Nrf2 in cancers: a double-edged sword. Cancer Med8: 52019. 2252-2267

157 

    Lignitto L.. Nrf2 activation promotes lung cancer metastasis by inhibiting the degradation of Bach1. Cell178: 22019. 316-329

158 

    Wang H.. NRF2 activation by antioxidant antidiabetic agents accelerates tumor metastasis. Sci. Transl. Med.8: 3342016.

159 

    Tao S.. The effects of NRF2 modulation on the initiation and progression of chemically and genetically induced lung cancer. Mol. Carcinog.57: 22018. 182-192

160 

    Ren D.. Brusatol enhances the efficacy of chemotherapy by inhibiting the Nrf2-mediated defense mechanism. Proc. Natl. Acad. Sci. U. S. A.108: 42011. 1433-1438

161 

    Xiang Y.. Brusatol enhances the chemotherapy efficacy of gemcitabine in pancreatic cancer via the Nrf2 signalling pathway. Oxid Med Cell Longev2018: 2018. 2360427

162 

    Cai S.J.. Brusatol, an NRF2 inhibitor for future cancer therapeutic. Cell Biosci.9: 2019. 45

163 

    Bollong M.J.. A small molecule inhibits deregulated NRF2 transcriptional activity in cancer. ACS Chem. Biol.10: 102015. 2193-2198

164 

    Singh A.. Small molecule inhibitor of NRF2 selectively intervenes therapeutic resistance in KEAP1-deficient NSCLC tumors. ACS Chem. Biol.11: 112016. 3214-3225

165 

    Arlt A.. Inhibition of the Nrf2 transcription factor by the alkaloid trigonelline renders pancreatic cancer cells more susceptible to apoptosis through decreased proteasomal gene expression and proteasome activity. Oncogene32: 402013. 4825-4835

166 

    Manna A.. The variable chemotherapeutic response of Malabaricone-A in leukemic and solid tumor cell lines depends on the degree of redox imbalance. Phytomedicine22: 7–82015. 713-723

167 

    Limonciel A., Jennings P.. A review of the evidence that ochratoxin A is an Nrf2 inhibitor: implications for nephrotoxicity and renal carcinogenicity. Toxins (Basel)6: 12014. 371-379

168 

    Xu X.. Wogonin reverses multi-drug resistance of human myelogenous leukemia K562/A02 cells via downregulation of MRP1 expression by inhibiting Nrf2/ARE signaling pathway. Biochem. Pharmacol.92: 22014. 220-234

169 

    Martin R.C.. Chemoprevention of carcinogenic progression to esophageal adenocarcinoma by the manganese superoxide dismutase supplementation. Clin. Canc. Res.13: 172007. 5176-5182

170 

    Kubo A.. Dietary antioxidants, fruits, and vegetables and the risk of Barrett's esophagus. Am. J. Gastroenterol.103: 72008. 1614-1623

171 

    Murphy S.J.. Dietary antioxidant and mineral intake in humans is associated with reduced risk of esophageal adenocarcinoma but not reflux esophagitis or Barrett's esophagus. J. Nutr.140: 102010. 1757-1763

172 

    Bjelakovic G.. Antioxidant supplements for prevention of gastrointestinal cancers: a systematic review and meta-analysis. Lancet364: 94412004. 1219-1228

173 

    Woodall C.E.. Chemoprevention of metaplasia initiation and carcinogenic progression to esophageal adenocarcinoma by resveratrol supplementation. Anti Canc. Drugs20: 62009. 437-443

174 

    Rawat N.. Curcumin abrogates bile-induced NF-kappaB activity and DNA damage in vitro and suppresses NF-kappaB activity whilst promoting apoptosis in vivo, suggesting chemopreventative potential in Barrett's oesophagus. Clin. Transl. Oncol.14: 42012. 302-311

Acknowledgements

The research reported in this publication was supported by grants from the 10.13039/100000054National Cancer Institute (R01CA224366) and the U.S. Department of Veterans Affair (1IK6BX003787 and I01BX001179). The contents of this work are solely the responsibility of the authors and do not necessarily represent the official views of the Department of Veterans Affairs, National Institutes of Health, or the University of Miami.

Recommended articles
Oxidative eustress: On constant alert for redox homeostasis
Redox Biology
Sirt3-mediated mitophagy regulates AGEs-induced BMSCs senescence and senile osteoporosis
Redox Biology
Binding of the human antioxidation protein α1-microglobulin (A1M) to heparin and heparan sulfate. Mapping of binding site, molecular and functional characterization, and co-localization in vivo and in vitro
Redox Biology
A matter of concern – Trace element dyshomeostasis and genomic stability in neurons
Redox Biology
Elevated levels of oxidized nucleosides in individuals with the JAK2V617F mutation from a general population study
Redox Biology