The Potential Role of 8-Oxoguanine DNA Glycosylase-Driven DNA Base Excision Repair in Exercise-Induced Asthma

Belanger, KarryAnne K.; Ameredes, Bill T.; Boldogh, Istvan; Aguilera-Aguirre, Leopoldo

doi:https://doi.org/10.1155/2016/3762561

Mediators of Inflammation

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Review Article | Open Access

Volume 2016 | Article ID 3762561 | https://doi.org/10.1155/2016/3762561

The Potential Role of 8-Oxoguanine DNA Glycosylase-Driven DNA Base Excision Repair in Exercise-Induced Asthma

KarryAnne K. Belanger,^1,2Bill T. Ameredes,^1,2,3,4Istvan Boldogh,^3,4,5and Leopoldo Aguilera-Aguirre⁵

Academic Editor: Helen C. Steel

Received28 Apr 2016

Accepted13 Jun 2016

Published25 Jul 2016

Abstract

Asthma is characterized by reversible airway narrowing, shortness of breath, wheezing, coughing, and other symptoms driven by chronic inflammatory processes, commonly triggered by allergens. In 90% of asthmatics, most of these symptoms can also be triggered by intense physical activities and severely exacerbated by environmental factors. This condition is known as exercise-induced asthma (EIA). Current theories explaining EIA pathogenesis involve osmotic and/or thermal alterations in the airways caused by changes in respiratory airflow during exercise. These changes, along with existing airway inflammatory conditions, are associated with increased cellular levels of reactive oxygen species (ROS) affecting important biomolecules including DNA, although the underlying molecular mechanisms have not been completely elucidated. One of the most abundant oxidative DNA lesions is 8-oxoguanine (8-oxoG), which is repaired by 8-oxoguanine DNA glycosylase 1 (OGG1) during the base excision repair (BER) pathway. Whole-genome expression analyses suggest a cellular response to OGG1-BER, involving genes that may have a role in the pathophysiology of EIA leading to mast cell degranulation, airway hyperresponsiveness, and bronchoconstriction. Accordingly, this review discusses a potential new hypothesis in which OGG1-BER-induced gene expression is associated with EIA symptoms.

1. Introduction

Globally, more than 300 million people suffer from varying severity of asthma and the annual global death rate associated with it exceeds 250,000 [1]. In the United States, the chronic lower respiratory diseases are the third leading cause of death and more than 30 million people including children and adults have been diagnosed with asthma [2]. Exercise-induced asthma (EIA) is a condition involving acute bronchial narrowing (bronchoconstriction) and other asthma-related symptoms triggered by strenuous physical activity [3]. In persons with EIA, bronchial narrowing typically occurs within 5 to 10 minutes after exercise and normally ceases within 30 and 60 minutes and thereafter [3]. The direct impact of bronchoconstriction in pulmonary function is reflected by a decrease (≥10%) in the forced expiratory volume in 1 second (FEV1) [4]. Although the precise prevalence of EIA is not known, some studies suggest that more than 10% of the general population is affected and 90% of asthmatics also show EIA symptoms [3, 5]. This is an important fact to be considered for asthmatics when they engage in sports and conditioning activities.

The etiology of EIA is not yet fully known, but the major theories explaining the characteristic bronchoconstriction after exercise are the osmotic theory and the thermal theory. The first theory proposes that increased ventilation during exercise results in loss of water from the airway cells causing an osmotic imbalance and ultimately stimulating the release of proinflammatory mediators [6–8]. The second theory proposes that a decrease in airway temperature produced by changes in the respiratory air flow during physical activities results in reduction in airway vascular tone and the consequent rebound vasodilation, leading to hyperemia, edema, and airway obstruction [8]. Both mechanisms (osmotic and thermal) are considered stressors that can potentially increase cellular reactive oxygen species (ROS) [9, 10] and trigger various inflammatory responses including mast cell degranulation, release of histamine, and generation of lipoperoxidation products such as leukotriene D4 (LTD4), leading to contractions in airway smooth muscles and ultimately bronchoconstriction [11, 12].

The susceptibility of individuals for EIA depends on their genetic background and the environment-modulated epigenetic changes [13, 14]. Initiation, immunopathogenesis, and pathophysiology of EIA result from a highly complex interplay among dysregulated airway epithelial, smooth muscle, and mast cells, and are manifested via a multitude of mediators leading to airway narrowing [15]. These events have also been linked to increased levels of ROS and the use of antioxidants has been shown to reduce exercise-induced bronchoconstriction [16, 17]. In addition, system biology approaches suggested that the repair product of oxidatively damaged DNA by OGG1 induces gene expression associated with airway inflammation, asthma, and EIA related symptoms [18–21]. Thus, this review proposes and discusses a potential role of OGG1-BER induced gene expression in the pathophysiology of EIA.

2. Oxidative Stress and EIA

Oxidative stress is characterized by an imbalance between the production of ROS and the antioxidant defenses, in which the ability of the antioxidant defense to neutralize ROS is overwhelmed. Importantly, ROS are also signaling species that promote airway inflammation and are etiologically linked to exacerbation of asthma by stimulating bronchial hyperreactivity, mast cell degranulation (e.g., release of histamine), generation of mucus, and induction of proinflammatory gene expression [23–25]. As a part of the ROS-driven stress responses and processes within the airway, two of the important redox reactions that can occur and may play a role in EIA are lipid peroxidation and DNA oxidation.

2.1. Lipid Peroxidation

The products of the isoprostane pathway are considered excellent biomarkers of oxidative stress in the airways [26]. A good example of these is 8-epi-prostaglandin F2 alpha (8-epi-PGF2 alpha), which has also been shown to cause contraction of smooth muscle by triggering the thromboxane A2 receptor (TBXA2R) [25, 27], and has been shown to have a role in asthma and EIA [28, 29]. Another important lipid peroxidation pathway associated with EIA is the 5-lipoxygenase (5-LO), which transforms essential fatty acids into leukotrienes. This pathway is the major source of potent proinflammatory leukotrienes (LT), such as LTB4, which is an activator and chemoattractant for leukocytes, and is implicated in several inflammatory diseases [30]. Other leukotrienes, such as LTC4 and LTD4, are potent contracting agents of smooth muscle in airways and can induce epithelial mucus secretion [31]. It has been shown that, in EIA, the ratio between prostaglandin E2 (PGE2) and cysteinyl leukotrienes (CysLTs) becomes imbalanced, favoring the latter. This may be important in EIA because PGE2 normally inhibits mast cell degranulation and promotes relaxation of the airway [32]. In support of this concept, it has been shown that elevated CysLTs contribute to exercise-induced bronchoconstriction (EIB), a hallmark of EIA [33, 34]. Leukotriene receptor antagonists such as montelukast have been successfully used to decrease airway responsiveness to various stimuli [35], supporting that lipid peroxidation is an important factor in asthma, and could be potentially important in EIA, as well.

2.2. DNA Oxidation

ROS induce oxidative modifications to DNA, including single and double strand breaks, preferentially affecting guanine due to its lowest redox potential among other DNA bases [36–38]. Mechanistic studies show that when ^•OH interacts with guanine, it results in a reducing neutral radical that reacts with molecular oxygen (O₂) and, via electron transfer, forms 7,8-dihydro-8-oxoguanine (8-oxoG) [39–41]. To prevent accumulation of oxidized DNA base lesions and their mutagenic effects, eukaryotic cells express DNA repair proteins that are analogous to those from E. coli (e.g., formamidopyrimidine DNA glycosylase: MutM; endonuclease VIII-like DNA glycosylase: Nei; 8-oxo-7,8-dihydrodeoxyguanosine triphosphate GTPase) [42]. OGG1 is an eukaryotic MutM homolog that excises 8-oxoG and its open-ring form FapyG from the 8-oxoG/FapyG:C mispairing [43]. Among oxidized DNA base lesions, 8-oxoG is a biomarker of oxidative damage to DNA [44]. The level of genomic 8-oxoG correlates well with the dose and length of exposure, chemical composition, and physical nature of the inhaled agents/oxidants [45–47]. Furthermore, under chronic inflammatory conditions 8-oxoG is one of the most frequent forms of DNA base damage in the genome [48–53]. Recently, it has been proposed that OGG1-driven DNA base excision repair has a role in asthma pathogenesis [21]. In addition, studies using lungs exposed to the BER product of OGG1 (8-oxoG) revealed a role in various biological processes including innate immune responses and inflammation [18]. Thus, it seems plausible that cellular 8-oxoG levels could be associated with EIA.

3. OGG1-Driven Proinflammatory Signaling through Small GTPases

Unexpectedly, Ogg1^−/− null mice did not show a marked phenotype despite the increased levels of the mutagenic 8-oxoG in their genomic DNA. More strikingly, Ogg1 deficiency in mice resulted in decreased inflammatory responses as shown by decreased accumulation of neutrophils, eosinophils and levels of Th1/Th2 cytokines [54–56]. These findings suggested that the absence of 8-oxoG and/or OGG1 is a missing component of proinflammatory signaling in the Ogg1^−/− null mice, implicating the importance of OGG1-BER in the inflammatory process.

During OGG1-BER, the 8-oxoG base is excised from DNA and released to the cytoplasm where it complexes with a cytoplasmic OGG1. The conformational changes in the OGG1 molecule allow it to interact with, and activate, RAS family small GTPases, including Kirsten (K)-RAS, neuroblastoma RAS viral oncogene homolog (N)-RAS, and Harvey (H)-RAS [57, 58]. In addition, the RAS homology GTPases RHO and RHO family of GTPases (RAC1, RAC2, and RAC3) can be activated by 8-oxoG-bound OGG1 [59–62]. Thus, the complex functions as a guanine nucleotide exchange factor (GEF) in a manner similar to that of other RAS and RAS homology protein-activating factors [57, 58]. The biological significance of small GTPase activations by OGG1-BER is not fully understood at this time. However, those observations also suggested that increased 8-oxoG levels in DNA or in body fluids observed in asthmatics are not only biomarkers of environmental exposures or inflammatory processes, but they may also serve as a second messenger [63]. In fact, it has been shown that OGG1-BER–mediated activation of GTPases (K-RAS, RHOA, and RAC1) plays a role in the innate allergic inflammatory response [18, 64], maintenance of chronic inflammation [21, 64], and airway remodeling [20, 62]. Therefore, we postulated that OGG1-BER-induced cell signaling is also likely to play important roles in the pathogenesis and progression of EIA.

4. Gene Expression Associated with Exercise-Induced Bronchoconstriction

In general, asthma is a multifactorial disease that involves complex cell signaling cascades leading to activation and release of multiple proinflammatory mediators, including cytokines/chemokines, histamine, proteases, and heparin. Despite decades of asthma research, our knowledge about the intricate signaling networks and the fine regulation of gene expression associated with this airway disease remains limited. In the particular case of EIA, there is also limited information on the regulation of global gene expression involved in its pathogenesis. Thus, to gain insight into the gene expression underpinning EIA, it is necessary to compare and integrate available gene expression data with the current next-generation whole-genome RNA-Seq data.

We have recently shown that OGG1-BER signaling induces gene expression associated with typical asthma symptoms [19, 20]. Thus, to elucidate the possible role of OGG1-BER signaling in EIA, we compared our RNA-Seq whole-genome gene expression datasets from mouse lungs exposed to 8-oxoG after single challenge (SC, GEO accession number: GSE61095) or multiple challenges (MC, GEO accession number: GSE65031), to the 48 top-ranked upregulated (≥1.5-fold) genes from individuals with exercise-induced bronchoconstriction characteristics (EIB⁺) and those without it (EIB^-), as a control, after intensive exercise (Table 1) published by Hallstrand et al. (GEO accession number: GSE13785) [22]. Interestingly, most of the top 48 upregulated genes in the EIB⁺ group were also upregulated in the SC group of 8-oxoG challenged lungs (Figure 1, upper cluster). On the other hand, fewer genes were upregulated in the MC group (Figure 1, lower cluster). These observations suggest a link between early gene expression induced in SC group by OGG1-BER cell signaling and the gene expression observed after strenuous exercise in the EIB⁺ group. Interestingly, the few genes induced by repeated stimulation (MC) of OGG1-BER signaling showed association with genes upregulated after exercise in EIB⁺ subjects. Taken together, gene expression profiles induced by both SC and MC might have a role at different stages in the pathogenesis of EIA.

Figure 1

Comparative gene expression between 8-oxoG challenged- and intensive exercise-exposed airways. The clustered heat map was constructed using the list of the most upregulated genes in airway epithelial cells from EIB positive (EIB⁺) individuals after 30 minutes of intensive exercise, as described in Hallstrand et al. [22]. This list of genes was compared to a list of the same genes from lungs challenged once (SC) or multiple times (MC). Top ranked gene list was obtained using Gene Expression Omnibus (GEO)’s built-in application GEO2R (http://www.ncbi.nlm.nih.gov/geo/geo2r/) and Hallstrand et al. GEO deposited dataset (GSE13785). Hierarchically clustered heat map was generated using GENE-E (Broad Institute, http://www.broadinstitute.org/).

5. Mast Cell Degranulation

Mast cells are one of the most important effector cells involved in elicitation of allergic responses [65]. Antigenic activation of mast cells via the high-affinity receptor for IgE (FcɛRI) mediates exocytosis of cytoplasmic granules containing preformed mediators, secretion of lipid-derived factors, and de novo synthesis of cytokines, chemokines, and growth factors [65–68]. In addition to FcɛRI-mediated signals, exposure to a variety of stimuli including pathogen-associated molecules can lead to the release of mast cell mediators [69].

During allergic and other inflammatory reactions, mast cells are exposed to an oxidative microenvironment milieu made up of ROS produced by various cell types in the surrounding peripheral tissues, as a consequence of their effector function [70]. Accordingly, various studies have shown the relevance of ROS/oxidative stress in mast cell activation [71–73]. For example, we have previously reported that it is not the allergenic proteins in pollen grains, subpollen particles, but ROS (superoxide anion, ) generated by their intrinsic NAD(P)H oxidases that are the primary cause of mast cell degranulation in airways and conjunctiva, during allergen/antigen-induced allergic responses [74–76].

Our studies also showed ROS-enhanced secretion of histamine and serotonin from mast cells, independently from FcɛRI-generated stimuli [77]. The release of biogenic amines in those cells was associated with inhibition of H⁺-ATPase activity within secretory granules, activation of PKC-δ, and microtubule-dependent motility and was independent from intracellular free Ca²⁺ levels. We also observed that IgE-mediated mast cell degranulation and antigen-triggered β-hexosaminidase release was decreased by ROS, while ROS were synergistic with antigen-induced IL-4 production in sensitized cells. Taken together, these data suggest that ROS and probably its downstream effect of cell signaling through OGG1-BER can act independently from antigen, augmenting the release of biogenic amines [77], and the initiation of antigen-independent effects.

Accordingly, gene expression induced by the most abundant product of DNA oxidative damage/repair (8-oxoG) was associated with mast cell degranulation [77]. To determine the validity of this association, we referenced the human genes database GeneCards® online v 4.0 (http://www.genecards.org/) for a list of 80 genes associated to mast cell degranulation and compared it to our RNA-Seq datasets. A hierarchically clustered heat map (Figure 2(a)) depicts the expression profile of those genes across the datasets from mouse lungs after a SC or a MC with 8-oxoG. This heat map shows an important number of upregulated genes associated with mast cell degranulation in the MC group. The expression at mRNA levels (fold-change) of top upregulated genes is shown in Table 1. Among the highest expressed genes in this group, integrin alpha 6 (Itga6) was increased by nearly 30-fold. Interestingly, studies showed increased expression levels of this gene in airway smooth muscle cells derived from individuals with fatal asthma [78]. In other studies, forkhead box F1 (Foxf1), a transcriptional factor expressed in endothelial and smooth muscle cells in the lungs, was associated with interstitial pneumonia [79]. This gene showed a nearly 20-fold increase. The product of Foxf1 also negatively regulates the expression of mast cell tryptase and the expression of chemoattractants such as CXCL12 which is necessary for mast cell migration [80]. These features make Foxf1 an important factor in the pathogenesis of lung inflammatory responses, and a potentially important factor in EIA. Furthermore, phospholipase C, Gamma 1 (Plcg1) transcript level was increased by over 15-fold; its protein product PLCG1 promotes mast cell activation [81]. The interaction network (Figure 2(b)) depicts the direct and indirect interactions between OGG1 and other differentially expressed genes, with a focus on mast cell modulation. These observations and their further investigation might provide insight on potential targets for development of novel compounds to prevent mast cell degranulation in asthmatics, before performing exercise.

(a)

(b)

Figure 2

OGG1-BER induced gene expression associated to airway mast cell degranulation. Mouse lungs received a single challenge (SC) or multiple challenges (MC) with 8-oxoG. Lungs were collected at 30 and 60 min after challenge and analyzed at whole-transcriptome level by RNA-Seq. (a) Hierarchically clustered heat map was generated using GENE-E online software (Broad Institute, http://www.broadinstitute.org/) considering transcript levels (fold-change). Red represents upregulation and blue represents downregulation. (b) Enrichment interaction network of the known and predicted interactions among the set associated with mast cell degranulation and OGG1. Peripheral nodes represent genes with a direct interaction with OGG1. The modified network was generated with GeneMania online database (http://www.genemania.org/).

6. Airway Hyperresponsiveness

One of the most common features of asthma is airway hyperresponsiveness (AHR) which is defined as an increased sensitivity of the airways to constrictor agonists. According to the World Allergy Organization (WAO), EIA represents a major problem among elite athletes, not just through interfering with their performance, but also through representing a potentially significant health risk, as well as a psychological barrier or disincentive toward pushing the limits of performance.

AHR involves various cytokines/chemokines as well as many other mediators, which are under genetic control, and may have an association with the OGG1-BER pathway. To determine the association of OGG1-BER signaling in AHR and the potential link to EIA, we searched in GeneCards database for a list of genes associated with AHR. GeneCards generated a list of 165 genes which was compared to our RNA-Seq datasets from 8-oxoG challenged lungs. A heat map (Figure 3(a)) shows an increased number of upregulated genes in the MC compared to the SC group. This suggested that upregulation of AHR-associated genes might be due to continuous or repeated oxidative damage to the airways, rather than a single insult. The interaction network depicts the multiple interactions between OGG1 and AHR-associated genes (Figure 3(b)). Among the genes with the highest expression levels, interleukin 10 (Il10) showed over 30-fold increase at 60 min in the MC group and over 6-fold increase at 60 min in the SC group. This cytokine has anti-inflammatory properties and its upregulation is commonly observed after or during inflammation, as a counter-regulatory off-switch that promotes the normal resolution of inflammation [82]. However, asthmatics have been shown to be deficient in airway IL-10 expression [83], for reasons that continue to be unexplained, but this deficiency may be important for the postulate that OGG1-BER is a critical factor in EIA. In support of this idea, protein levels of IL-10 have been observed to be increased in an exercise animal model in which LPS-induced lung neutrophilia was decreased after exercise only in Il10^+/+ but not in Il10^−/− mice [84]. Thus, it can be theorized that exercise may be beneficial in promoting the IL-10 response in normal individuals. However, in asthmatics and specifically in the case of EIA, exercise may induce an inflammatory oxidative stress that cannot be countered by IL-10, due to deficiency in its production. In the case of the postulated OGG1-BER pathway in EIA, this would create a scenario in which the effects of mast cell and/or neutrophil degranulation would be unchecked by the anti-inflammatory effects of IL-10 [82], resulting in the enhancement of AHR and the diminution of exercise performance.

(a)

(b)

Figure 3

OGG1-BER induced gene expression associated with AHR. Mouse lungs received a single challenge (SC) or multiple challenges (MC) of 8-oxoG and were processed as previously described above. (a) Hierarchically clustered heat map was generated using GENE-E online software (Broad Institute, http://www.broadinstitute.org/) considering transcript levels (fold-change). Red represents upregulation and blue represents downregulation. (b) Enrichment network of the known and predicted interactions among the set of genes associated to airway hyperresponsiveness and OGG1. Peripheral nodes represent genes with a direct interaction with OGG1. The modified network was generated with GeneMania online database (http://www.genemania.org/).

Furthermore, the expression levels of other genes like Cxcl1, Cxcl2, and Tnf were notably increased. This may be important, because the chemokines CXCL1 and CXCL2 are potent neutrophil chemoattractants which play a role in the pathogenesis and progression of asthma that could be associated to EIA. Moreover, the upregulation of Tnf gene expression is again consistent with the upregulation of the il10 gene, as its protein product TNF-α is a major driver of IL-10 release from leukocytes [82] that are either drawn in with inflammation, or perpetually resident, within the airway. In this case, it may be important to consider that IL-10 is self-regulating, in that it normally feeds back to shut down both its own release and that of TNF-α [82]; but, with the IL-10 deficiency of asthma, there would be no brake on TNF-α, which has its own important proinflammatory and pro-AHR effects [85], which could drive EIA. Table 2 shows a complete list of the AHR-associated genes and their expression values.

7. The Potential Role of OGG1-BER Signaling in EIA

Physical exercise renders physiological stress to the body including oxidative stress [86, 87] and potentially affects the activation of transcription factors such as NF-κB and activator protein-1 (AP1) which stimulates the expression of cytokines and chemokines, to promote physiological responses that may be linked to EIA [88]. Physical factors, such as temperature, can also exacerbate the outcomes in EIA, through altering the redox state of the airways. For example, it has been documented that exposure to cold temperatures during exercise increases oxidative stress levels, as determined by increased plasma ROS metabolites and lower levels of antioxidants [89]. At the cellular level, it has been observed that the increased levels of ROS in the airway epithelium can stimulate the production of leukotrienes and other inflammatory mediators, playing a pivotal role in lung inflammation [90]. Although it has long been known that ROS are linked to proinflammatory gene expression, the precise mechanisms are still not completely understood. As outlined above, recent studies suggest that oxidative stress can play an important role in cell signaling through a DNA-BER initiated signaling pathway. Of note, these studies showed that the repair product of oxidatively damaged DNA by OGG1 forms a complex with OGG1 in the cytosol and activates small GTPases [59, 61, 62] and downstream signaling molecules involved in both the NF-κB signaling pathway and the expression of innate immune response genes [18].

Based on the data and previous findings outlined above, we propose a model (Figure 4) that represents the potential role of OGG1-BER signaling in EIA. Within this schema, vigorous exercise results in osmotic and thermal changes in the airways leading to oxidative stress. This condition can be exacerbated by the presence of environmental toxicants that can act as prooxidants, such as ozone and sulfur dioxide [91]. Consequently, DNA in the airway cells is oxidized by ROS and the subsequent 8-oxoG lesions are repaired by OGG1-BER, increasing the levels of cytoplasmic free 8-oxoG leading to the formation of OGG18-oxoG complexes. These complexes activate small GTPases such as RAS, RHO, and RAC, inducing downstream signaling which activates transcription factors leading to EIA-related gene expression. The proinflammatory mediators released by airway epithelial and resident cells, such as dendritic cells and macrophages, can result in the typical EIA symptoms including bronchoconstriction, airway hyperresponsiveness, shortness of breath, wheezing, and coughing. It is important to note that IL-10 is conspicuous by its absence in this scheme of OGG1-BER-associated effects on EIA, because of its deficiency in asthmatics [82, 83]. It is likely to be present in nonasthmatics, in amounts necessary to counter the release and effects of proinflammatory mediators. This may also be why some relief from EIA may be obtained with asthma controller treatment therapies such as inhaled corticosteroids [92, 93], which are known to upregulate IL-10 production, in addition to other important anti-inflammatory effects [94].

Figure 4

Proposed role for OGG1-BER in asthma and EIA-related gene expression. The large inhaled air volumes during physical activity decrease the temperature and water content of the airway epithelium lining fluid, leading to supraphysiological ROS production by epithelial cells, which can be exacerbated by exposures to environmental pollutants. ROS-induced 8-oxoG lesions in the DNA are repaired by OGG1-BER. In the cytosol, 8-oxoG complexes with OGG1 and acts as a guanine nucleotide exchange factor (GEF), activating small GTPases and initiating a signaling cascade that leads to the translocation of transcription factors (TFs) initiating the transcription of genes associated to AHR, mast cell degranulation, and bronchoconstriction.

8. Conclusions

EIA is an acute condition characterized by reversible bronchoconstriction, wheezing, chest tightening, and shortness of breath, during or after exercise. Despite the high prevalence of these potentially serious symptoms in EIA, there is limited information on the molecular pathogenesis. It is mostly agreed that osmotic/thermal changes and environmental pollutants increase levels of oxidative stress; however, the molecular mechanisms by which reactive species are implicated in the pathogenesis of EIA are not fully known. Thus, this review presents a general overview on the pathogenesis of EIA and discusses its potential link to the present knowledge of cell signaling initiated by repair of oxidatively damaged DNA.

However, the genetic basis of EIA has not been completely elucidated. Therefore, we proposed a novel hypothesis (Figure 4), in which cell signaling induced by the repair of oxidatively damaged DNA by OGG1 during the base excision repair pathway plays a role in the regulation of gene expression associated with common symptoms of EIA. This hypothesis is supported by previous studies from other research groups and from our own research group, showing the involvement of OGG1-BER in gene expression related to airway inflammation and other asthma features [18–20, 56, 95]. It is currently acknowledged that osmotic/thermal changes and environmental pollutants increase levels of oxidative stress; however, the understanding of the molecular mechanisms by which reactive species are implicated in the pathogenesis of EIA require further studies. It is evident from the present analysis that DNA damage/repair could be involved in EIA pathogenesis. Further investigation of DNA damage/induced signaling pathway may result in novel pharmacological targets to prevent or treat EIA.

Abbreviations

8-oxoG:	8-Oxo-7,8-dihydroguanine
AHR:	Airway hyperresponsiveness
BER:	Base excision repair
CysLTs:	Cysteinyl leukotrienes
EIA:	Exercise-induced asthma
EIB:	Exercise-induced bronchoconstriction
FapyG:	2,6-Diamino-4-hydroxy-5-formamidopyrimidine
GEF:	Guanine nucleotide exchange factor
H-Ras:	Harvey rat sarcoma viral oncogene homolog
IL:	Interleukin
K-Ras:	Kirsten rat sarcoma viral oncogene homolog
LPS:	Lipopolysaccharides
N-Ras:	Neuroblastoma RAS viral oncogene homolog
MC:	Multiple challenges
OGG1:	8-Oxoguanine DNA glycosylase-1
PI3K:	Phosphatidyl inositol 3 kinase
RAC1:	Ras-related C3 botulinum toxin substrate 1 GTPase
RHO:	Ras homology (Rho) family of small GTPases
ROS:	Reactive oxygen species
SC:	Single challenge.

Competing Interests

The authors declare that there is no conflict of interests regarding the publication of this paper.

Authors’ Contributions

All authors contributed equally.

Acknowledgments

This work was supported by grants NIEHS R01 ES018948 (Istvan Boldogh), NIAID/AI062885 (Istvan Boldogh), N01HV00245 (Istvan Boldogh, PI/PD: A. Kurosky), and NIEHS T32 ES007254 (KarryAnne K. Belanger and Leopoldo Aguilera-Aguirre, PI/PD: Bill T. Ameredes).

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Copyright © 2016 KarryAnne K. Belanger et al. This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

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