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Open Access

Peer-reviewed

Research Article

Association of the functionally significant polymorphisms of the MMP9 gene with H. pylori-positive gastric ulcer in the Caucasian population of Central Russia

  • Volodymyr Dvornyk,

    Roles Conceptualization, Methodology, Project administration, Supervision, Writing – review & editing

    Affiliation Department of Life Sciences, College of Science and General Studies, Alfaisal University, Riyadh, Saudi Arabia

  • Irina Ponomarenko,

    Roles Formal analysis, Writing – original draft, Writing – review & editing

    Affiliation Department of Medical Biological Disciplines, Belgorod State University, Belgorod, Russia

  • Oksana Minyaylo,

    Roles Data curation, Methodology, Writing – original draft, Writing – review & editing

    Affiliation Department of Medical Biological Disciplines, Belgorod State University, Belgorod, Russia

  • Evgeny Reshetnikov ,

    Roles Formal analysis, Methodology, Validation, Writing – review & editing

    reshetnikov@bsu.edu.ru

    Affiliation Department of Medical Biological Disciplines, Belgorod State University, Belgorod, Russia

  • Mikhail Churnosov

    Roles Conceptualization, Funding acquisition, Methodology, Project administration, Supervision, Writing – review & editing

    Affiliation Department of Medical Biological Disciplines, Belgorod State University, Belgorod, Russia

Abstract

Background and purpose

The study analyzed the association of functionally significant polymorphisms of matrix metalloproteinases (MMPs) genes with the development of gastric ulcer (GU) in Caucasians from Central Russia.

Methods

The 781 participants, including 434 patients with GU (196 Helicobacter pylori (H. pylori)-positive and 238 H. pylori-negative) and 347 controls (all H. pylori-negative) were recruited for the study. Ten SNPs of the MMP1 (rs1799750), MMP2 (rs243865), MMP3 (rs679620), MMP8 (rs1940475), and MMP9 (rs3918242, rs3918249, rs3787268, rs17576, rs17577, and rs2250889) genes were considered for association with GU using multiple logistic regression. The SNPs associated with GU and loci linked (r2≥0.8) to them were analyzed in silico for their functional assignments.

Results

The SNPs of the MMP9 gene were associated with H. pylori-positive GU: alleles C of rs3918249 (OR = 2.02, pperm = 0.008) and A of rs3787268 (OR = 1.60–1.82, pperm ≤ 0.016), and eight haplotypes of all studied MMP9 gene SNPs (OR = 1.85–2.04, pperm ≤ 0.016) increased risk for H. pylori-positive GU. None of the analyzed SNPs was independently associated with GU and H. pylori-negative GU. Two haplotypes of the MMP9 gene (contributed by rs3918242, rs3918249, rs17576, and rs3787268) increased risk for GU (OR = 1.62–1.65, pperm ≤ 0.006). Six loci of the MMP9 gene, which are associated with H. pylori-positive GU, and 65 SNPs linked to them manifest significant epigenetic effects, have pronounced eQTL (17 genes) and sQTL (6 genes) values.

Conclusion

SNPs of the MMP9 were associated with H. pylori-positive GU but not with H. pylori-negative GU in Caucasians of Central Russia.

Citation: Dvornyk V, Ponomarenko I, Minyaylo O, Reshetnikov E, Churnosov M (2021) Association of the functionally significant polymorphisms of the MMP9 gene with H. pylori-positive gastric ulcer in the Caucasian population of Central Russia. PLoS ONE 16(9): e0257060. https://doi.org/10.1371/journal.pone.0257060

Editor: Kanhaiya Singh, Indiana University Purdue University at Indianapolis, UNITED STATES

Received: April 25, 2021; Accepted: August 21, 2021; Published: September 7, 2021

Copyright: © 2021 Dvornyk et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

Data Availability: All relevant data are within the manuscript and its Supporting Information files.

Funding: The authors received no specific funding for this work.

Competing interests: The authors have declared that no competing interests exist.

Introduction

Gastric ulcer (GU), a disease occurring in the stomach mucosa, is the mucosal inflammation and necrotic lesion that extend to the underlying smooth muscles and are caused by multiple pathogenic factors [1]. GU is a common disease affecting about 10% of population [2]. Common causes of GU include Helicobacter pylori (H. pylori) infection (70–80% of GU patients), intake of non-steroidal anti-inflammatory drugs (NSAIDs), and the digestion of the gastric mucous by gastric acid/pepsin [3, 4].

The development of GU is a complex process that involves secretion of acids, generation of the reactive oxygen species, inhibition of prostaglandins, and degradation of the extracellular matrix (ECM) [5]. Damage of gastric mucosa is associated with ECM degradation in which matrix metalloproteinases (MMPs) play a key role [6]. MMPs are calcium-dependent endopeptidases involved in various processes, including ECM remodeling, cell proliferation, and inflammation. MMPs are synthesized and secreted by gastric epithelial cells, neutrophils, and macrophages [7]. Remodeling of the ECM by MMPs is thought to be one of the important factors contributing to gastric ulceration [8, 9]. Several animal studies were focused on the role of MMPs in GU [911]. There is evidence that MMP9 is important in the early stage of chronic GU [12].

Genetic variation in the MMP genes may be an important element of a complex genetic risk profile that determines the development of GU in chronic H. pylori infection [13]. H. pylori infection can increase the MMP3, MMP7, and MMP9 levels in the gastric mucosa and sera [1416]. The significantly higher levels of the MMP9 protein were observed in H. pylori-positive GU than in the H. pylori-negative one [17].

Despite the solid evidence for the important role of MMP in GU, an association of MMP polymorphisms with GU has been studied poorly: there are only very few studies on this problem [13, 18]. The lack of experimental evidence about the possible association of the MMPs with GU prompts for filling this gap.

This study analyzed polymorphisms of the MMP1, MMP2, MMP3, MMP8, and MMP9 genes for the association and possible role in the development of GU in a Caucasian sample from Central Russia.

Materials and methods

Study subjects

Given the available data about the allele frequencies of the MMP gene polymorphisms in patients with GU and controls [13], we calculated that sample size of 700 should be sufficient to ensure the statistical power of 0.80 at α = 0.05 significance level. In total, 781 participants, including 434 patients with GU and 347 controls, were recruited for the study. The participants were enrolled according to the inclusion criteria: birthplace in Central Russia and Russian ethnicity (self-reported) [19, 20].

All participants were examined by qualified gastroenterologists. GU and complications (if any) were diagnosed by conventional clinical and endoscopic examinations. The control group consisted of healthy individuals without any symptoms of gastrointestinal disease [21]. Endoscopy was not performed in healthy individuals because of both ethical reasons and the low probability of finding an active ulcer in patients without the symptoms [22]. Patients and control group volunteers having used NSAIDs, corticosteroids, and aspirin for a long-term treatment were excluded.

The H. pylori infection in patients was diagnosed by positive findings on histologic examination of biopsies obtained during endoscopy procedures by a certified pathologist and using the Giemsa stain protocol [23]. Among 434 patients with GU, 196 were H. pylori-positive and 238 were H. pylori-negative. In controls, the presence of H. pylori was determined using a commercial IgG ELISA kit (Plate Helicobacter IgG, Roche). Control group volunteers with the presence of H. pylori infection were excluded.

The study protocol was approved by the Medical Institution Ethics Committee of Belgorod State University. All study participants signed informed consent prior to enrolment in the study. The clinical and endoscopic examination of the participants was conducted at the Gastroenterology Division of Belgorod Regional Clinical Hospital.

DNA isolation and genotyping assay

Whole blood samples (5 mL) were collected from all study participants into EDTA‐containing tubes and maintained at − 20°C until processed [24, 25]. Genomic DNA was extracted from the buffy coat by the phenol/chloroform method as described earlier [26].

Ten SNPs of the MMP genes (rs1799750 MMP1, rs243865 MMP2, rs679620 MMP3, rs1940475 MMP8, rs3918242, rs3918249, rs3787268, rs17576, rs17577, and rs2250889 MMP9) were selected for this study according to the criteria [27, 28]: previously reported associations with digestive diseases (gastric and duodenal ulcer, gastric cancer, etc.), regulatory potential, and MAF > 0.05.

All selected SNPs had significant regulatory potential as evidenced by the HaploReg online tools [29] (S1 Table); eight polymorphisms were associated with digestive diseases (gastric and duodenal ulcer, gastric and esophageal cancer, digestive cancers, gastritis) (including two SNPs associated with the peptic ulcer) in previously published candidate gene association studies (S2 Table). Two SNPs (rs3918249 and rs3787268 MMP9) did not demonstrate a significant association with digestive diseases but had significant regulatory potential (according to HaploReg).

The genotyping was performed using the MassARRAY® 4 System by Agena Bioscience®. Blind replicates were genotyped to control the quality [30]. Laboratory personnel that conducted genotyping was blinded to patients’ information. The repeatability test was performed for 5% of randomly selected samples, yielded 100% reproducibility.

Statistical and functional analysis

The observed allele and genotype frequencies were checked for the correspondence to the Hardy-Weinberg equilibrium using the chi-square test [31]. Associations of the SNPs with GU were analyzed using the logistic regression and assuming dominant, log-additive, and recessive genetic models [32]. The regression analysis was adjusted for covariates: BMI as a quantitative variable, whereas a family history of peptic ulcer, alcohol and tobacco consumption, stress, the presence of cardiovascular and endocrine pathology were applied as qualitative parameters (Table 1). The given sample size (434 patients with GU and 347 controls) was sufficient to detect differences in allelic frequencies between the affected subjects and controls at OR = 1.33–1.82 for the additive model, OR = 1.58–1.86 for the dominant model and OR = 1.61–27.0 for the recessive model (at 80% power, ɑ = 0.05 for 2-sided test). Statistical power for each SNP was estimated using Quanto 1.2.4 [33]. The haplotype blocks were identified using the «Solid Spine» algorithm (D’ > 0.8) as implemented in HaploView v.4.2 [34]. The association analyses and adjustment for multiple comparisons by the adaptive permutation test [35] were conducted using the PLINK v. 2.0 software [36]. The significance value was set at pperm<0.017 (after the Bonferroni correction based on the numbers of paired comparisons, n = 3: GU–control, H. pylori-positive GU—control, and H. pylori-negative GU—control).

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Table 1. Phenotypic characteristics of the study participants.

https://doi.org/10.1371/journal.pone.0257060.t001

The functional importance (missense replacement, eQTLs and sQTLs, regulatory potential) of the genetic variants associated with GU and those linked to them was studied in silico [37, 38]. The SIFT online tool [39] was used to identify missense replacements and predict their functional effects. The SNP epigenetic effects were analyzed using RegulomeDB [40] and HaploReg [29]. The data from the GTExportal browser [41] was used to estimate the influence of the GU-candidate loci on mRNA levels and splicing QTLs. Likewise, regulatory potential, eQTL and sQTL values of polymorphisms in strong linkage disequilibrium (LD, r2≥0.8) with the GU-associated loci were estimated [42, 43]. The linked SNPs were identified using HaploReg [29].

Results

Baseline and clinical characteristics of the participants are presented in Table 1. The GU patients had higher BMI (p = 0.003), higher percentage of positive family history of peptic ulcer (p = 0.0005), alcohol (p = 0.0005) and tobacco (p = 0.001) consumption, stress (p = 0.0005), the presence of cardiovascular (p = 0.0005) and endocrine (p = 0.02) pathology as compared to the healthy participants (the data are shown in Table 1). Therefore, these parameters were used as confounding factors in the logistic regression analyses.

The summary data about the studied SNPs is given in S3 Table. All SNPs corresponded to the HWE (p>0.005, pbonf>0.05). None of the SNPs was independently associated with GU according to any of the genetic models (Table 2). As to H. pylori-positive GU, only loci of the MMP9 gene manifested association with the disease. Allele C at rs3918249 MMP9 locus was associated with H. pylori-positive GU according to the dominant model (OR = 2.02, 95% CI 1.21–3.37, pperm = 0.008, power—94.68%), and allele A at rs3787268 MMP9 was associated with H. pylori-positive GU according to the additive (OR = 1.60 95% CI 1.09–2.34, pperm = 0.016, power = 89.98%) and dominant (OR = 1.82 95% CI 1.14–2.89, pperm = 0.012, power = 91.14%) genetic models (the data are provided in Table 3). Several haplotypes of the studied SNPs MMP9 gene were associated with GU (four SNPs within two haplotypes, OR = 1.62–1.65, pperm ≤ 0.006) and H. pylori-positive GU (all six SNPs within eight haplotypes, OR = 1.85–2.04, pperm ≤ 0.016) (Table 4, Fig 1). None of the SNPs was associated with H. pylori-negative GU either independently or within haplotypes (Table 3).

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Fig 1. Linkage disequilibrium (LD) between SNPs rs3918242, rs3918249, rs17576, rs3787268, rs2250889 and rs17577 of the MMP9 gene in GU patients.

A, summary; B, H. pylori-positive GU patients; C, H. pylori-negative GU patients; D, control group. LD values are given as Lewontin’s standardized coefficient D′ (Figure sections 1) and the square of the Pearson’s correlation coefficient (r2) (Figure sections 2) between SNPs.

https://doi.org/10.1371/journal.pone.0257060.g001

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Table 2. Associations of the MMP gene polymorphisms with GU.

https://doi.org/10.1371/journal.pone.0257060.t002

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Table 3. Associations of the MMP gene polymorphisms with H. pylori-positive and H. pylori-negative GU.

https://doi.org/10.1371/journal.pone.0257060.t003

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Table 4. Significant associations of the MMP9 gene haplotypes with GU and H. pylori-positive GU.

https://doi.org/10.1371/journal.pone.0257060.t004

Functional SNP predictions

Non-synonymous SNPs.

Among the six loci of the MMP9 gene associated with H. pylori-positive GU, three SNPs were missense variant: rs17576 (amino acid change Gln279Arg, SIFT score 0.29, SIFT prediction «tolerated»), rs2250889 (Arg574Pro, SIFT score 1.00, SIFT prediction «tolerated») and rs17577 (Arg668Gln, SIFT score 0.02, SIFT prediction «deleterious»).

Regulatory effects predictions.

According to RegulomeDB and HaploReg, all six SNPs of the MMP9 gene (rs3918242, rs3918249, rs17576, rs3787268, rs2250889 and rs17577) associated with H. pylori-positive GU possess significant regulatory effects. The RegulomeDB suggests the most significant regulatory potential for rs17577 (rank - 2b, score—0.79). The other five H. pylori-positive GU-associated SNPs (rs3918242, rs3918249, rs17576, rs3787268, rs2250889) have RegulomeDB rank = 4–5 and RegulomeDB score = 0.59–0.61. According to the HaploReg database, the above six polymorphisms were located in DNase I hypersensitive sites, five SNPs–in the specific region of DNA binding with modified histone marking promoters (rs3918249, rs17576, rs3787268, rs2250889 and rs17577) and enhancers (rs3918242, rs3918249, rs17576, rs3787268 and rs17577) in various tissues, and in the sixteen motifs to the transcription factors (TFs), three SNPs (rs17576, rs2250889 and rs17577)—in evolutionarily conserved DNA segments, and two SNPs (rs2250889 and rs17577)—in the protein-bound site (S1 Table). Herewith, alleles of the MMP9 gene loci associated with increased risk for H. pylori-positive GU (Table 4) increases affinity to twelve TFs (Ahr:Arnt, HIF1, Myc, Hmx, Hoxb8, HDAC2, Mef2, Pou1f1, Sox, Zfp105, p300, NRSF) and decreases affinity to the four TFs (E2F, Arid3a, Pax-5, Pax-4) (S4 Table).

In addition to the six H. pylori-positive GU-related SNPs, regulatory significance was estimated for 65 loci linked to them (the data are provided in S5 Table). Seventeen SNPs have been positioned in evolutionarily conserved DNA regions. Nine SNPs (including four synonymous and five missense replacements) were located in protein-coding regions (exons) of the MMP9 gene, 26 in introns, and 30 in intergenic areas. All 65 SNPs linked to the H. pylori-positive GU-associated SNPs had a significant regulatory potential; several polymorphisms manifested epigenetic effects (S5 Table). For example, rs6073989 (linked to rs3787268, r2 = 0.95) is positioned in the specific area of DNA binding with modified histone marking promoters (H3K4me3, H3K9ac) and enhancers (H3K4me1, H3K27ac) in more than ten tissues/organs, the DNAase I hypersensitive segments in sixteen tissues/organs, and a sites of five regulatory DNA motifs (CAC-binding-protein, EWSR1-FLI1, PRDM1, SP1, TATA). The SNP rs6073991, which also was in linkage disequilibrium with rs3787268 (r2 = 0.95), was located in the hypersensitive region to DNAase-I in 49 (!) tissues/organs, in the protein-bound region (with this DNA region interact three regulatory proteins—NRSF, ZNF143, BCL3), and a putative transcription factor binding sites (SZF1-1, T3R) (S5 Table). Importantly, the epigenetic effects of the H. pylori-positive GU-associated SNPs and 65 polymorphisms linked to them of the MMP9 gene were reported for the target organs of GU, adult stomach mucosa and smooth muscle, fetal stomach.

Expression quantitative trait loci (eQTLs).

Referring to the data of the GTExportal resource, six H. pylori-positive GU-associated polymorphisms MMP9 gene and 61 SNPs linked to them had the eQTL significance (cis-eQTL and trans-eQTL) and correlated with mRNA levels of 17 genes in more than 25 various tissues and organs (NEURL2, SLC12A5, CD40, MMP9, RP3-337O18.9, NTTIP1, PCIF1, SPATA25, RP11-465L10.10, ZSWIM1, RPL13P2, SNX21, WFDC10B, PLTP, SYS1, WFDC3, ZNF335) (S6 and S7 Tables). For example, rs3787268 and rs3918249 (individually associated with H. pylori-positive GU) may affect the expression genes (RP3-337O18.9, PLTP, NEURL2) in the organs of the digestive system (esophagus, various sections of the colon) as well as other tissues/organs related to the development of GU: brain (frontal cortex and pituitary (PLTP)), adipose tissue (visceral and subcutaneous) (NEURL2, SPATA25, PLTP, SLC12A5, CD40, ZSWIM1, RP3-337O18.9), whole blood (ZNF335), thyroid (PLTP, NEURL2), adrenal gland (PLTP, PCIF1, SLC12A5, RP11-465L10.10), etc. Importantly, the risk alleles of the analyzed loci (e.g., A rs3787268 and C rs3918249 C) are usually associated with the lower expression of the genes (S6 Table).

Splicing quantitative trait loci (sQTLs).

Analysis of the GTExportal data suggested that the six GU-associated loci of MMP9 had significant sQTL values and might influence alternative splicing of five genes (SLC12A5, ACOT8, CD40, SNX21, PLTP) in various tissues and organs (the results are shown in S8 Table). These polymorphisms manifested strong linkage to 61 SNPs, which affect splicing QTL of six genes (CD40, SLC12A5, ACOT8, SNX21, PLTP, SLC35C2) in more than 15 organs and tissues (S9 Table). Importantly, the independently associated with H. pylori-positive GU loci rs3787268 and rs3918249 correlate with splicing QTLs of the PLTP gene in subcutaneous adipose tissue and SLC12A5 gene in the various parts of the brain (e.g., cortex and substantia nigra, pituitary), which are known to play a role in the pathogenesis of GU. Interestingly, the GU risk allele, C rs3918249, correlates with the elevated level of in the sQTL of the SLC12A5 gene (β>0) in the substantia nigra and pituitary and with the lower level of the sQTL of the SLC12A5 gene (β<0) in the brain cortex. The GU risk allele A rs3787268 is associated with the higher level of the sQTL of the PLTP gene in the subcutaneous adipose tissue (S8 Table). Besides, rs3787268 and rs3918249 each are in strong LD with eleven sQTL SNPs (S9 Table).

Discussion

In the present study, we report for the first time the association of the SNPs rs3918249 and rs3787268 of MMP9 with H. pylori-positive GU but not with H. pylori-negative GU in the Caucasian population of Central Russia. Alleles C of rs3918249 MMP9 (OR = 2.02) and A of rs3787268 MMP9 (OR = 1.60–1.82), and eight haplotypes of the six studied SNPs of the MMP9 gene (OR = 1.85–2.04) increased risk for H. pylori-positive GU. None of the MMP gene SNPs was independently associated with GU. Also, two haplotypes of the MMP9 gene (contributed by four SNPs, rs3918242, rs3918249, rs17576, and rs3787268) increased risk for GU (OR = 1.62–1.65). Six loci of the MMP9 gene, which are associated with H. pylori-positive GU, and 65 SNPs linked to them manifest significant epigenetic effects, have pronounced eQTL (17 genes) and sQTL (six genes) values in the organs of the digestive system and the other tissues/organs, which have been suggested to contribute to GU.

Only two genome-wide association studies (GWAS) of the peptic ulcer disease (PUD) have been conducted so far [44, 45]. One of them reported only two SNPs (rs2294008 PSCA and rs505922 ABO) associated with duodenal ulcer in Japanese [44]; another determined eight PUD-associated loci in the MUC1, MUC6, FUT2, PSCA, ABO, CDX2, GAST and CCKBR genes, including the two reported for the Japanese cohort [45]. While the estimated heritability for PUD is about 28% [45], only 6% of the estimated variance in the trait is attributed to genome-wide common SNPs (i.e., SNP-based heritability) [45] that raises a problem of so-called “missing heritability”. This problem may be addressed by studying associations of candidate genes for peptic ulcer. In these terms, the MMPs genes are very good candidates, as they are related to both the pathogenesis of H. pylori-associated gastric ulcer and the inflammatory response of the mucosa [13].

So far, only one study [13] reported a significant association of an MMP9 gene variant with H. pylori-positive GU. The authors analyzed 20 SNPs of the MMP1, 3, 7, and 9 genes in the sample of 599 H. pylori-infected German patients and determined that two SNPs were associated with the disease: the rs17576 polymorphism of the MMP9 gene and another variant in the promoter region of the MMP7 gene. Interestingly, Hellmig S. et al. determined allele A of rs17576 as a risk factor for the disease [13], while our results suggested allele variant G of the same locus (within the significantly associated haplotypes of the MMP9 gene) as the risk factor for the Caucasian population of Central Russia. Yeh et al. [18] did not find any significant association of the above SNP with the disease in a Taiwanese population. Thus, our study is the first that reports the association of rs3918242, rs3918249, rs3787268, rs2250889, rs17577 of the MMP9 gene with H. pylori-positive GU.

There are quite a few studies, which analyzed the association of MMP gene polymorphisms with gastric cancer (S2 Table) and reported such an association for the MMP9 gene SNPs included in our study (rs3918242, rs17576, rs17577). Notably, allele C of rs3918242, a risk factor for H. pylori-positive GU in Caucasians from Central Russia in the present study, also increased the risk for gastric cancer [46, 47] and esophageal cancer [48]. It is thought that H. pylori-associated GU is positively linked to stomach cancer due to the damage of gastric mucosa [49] and the MMP9 gene may be one of the candidate genes involved in both H. pylori-associated GU and gastric cancer [50].

The MMP9 gene is located on chromosome 20q11.1–13.1. The encoded protein (type IV collagenase, also known as gelatinase B) can degrade various collagen (collagen types IV, V, VII, X, XIV, gelatin) and non-collagen substrates (elastin, aggrecan, fibronectin, nidogen, laminin, etc.) of the extracellular matrix (ECM) [51]. ECM of the gastric mucosa contains a significant proportion of collagen, elastin, fibronectin, laminin, hyaluronic acid, and proteoglycan, and their degradation by MMPs is important for the stability of the cellular microenvironment [13]. MMP9 is a key enzyme implicated in gastric ulcer [52, 53]. ECM degradation by MMPs is apparently a key factor contributing to gastric mucosal damage [6]. The significant elevation of the MMP9 level in gastric ulcer tissues suggested that the enzyme may regulate mucosa lesions in GU by degrading collagens and creating lesions [50]. Also, this enzyme is important in the early phase of chronic GU [12].

The present study reports association of the MMP9 gene polymorphisms with H. pylori-positive GU but not with H. pylori-negative GU. The available literature also suggests that MMP9 gene polymorphisms apparently contribute to a genetic risk profile to develop GU in chronic H. pylori infection [13]. There is evidence that MMPs can be induced by both H. pylori bacterial products and proinflammatory cytokines [54]. MMPs have elevated expression in gastric epithelial cells infected with H. pylori that might contribute to the GU pathogenesis. Li et al. [17] analyzed samples of gastric mucosa from the antrum and ulcer site and found that the higher MMP9 expression was associated with the H. pylori infection and correlated with the level of inflammation determined histologically at the border of the ulcer. Several studies demonstrated a correlation between the elevated serum levels of MMP9 and higher MMP9 activity in antral mucosa of H. pylori-infected patients with gastritis [55, 56]. Antral mucosa of H. pylori-infected subjects demonstrates a 19-fold higher MMP9 protein activity than that of uninfected individuals [55] as H. pylori induces NF-kappaB activation through the intracellular signaling pathway resulting in transcription of the MMP9 gene [15]. Notably, the H. pylori-induced MMP9 up-regulation can be reversed after successful pathogen eradication. If the eradication failed, no difference in the MMP9 protein expression was detected in epithelial cells and fibroblasts before and after the treatment [57]. H. pylori plays an important role not only in gastroduodenal diseases (chronic gastritis, peptic ulcer, gastric cancer, etc.) but also in various extragastric pathologies (cardiovascular, endocrine (insulin resistance, diabetes mellitus), etc.) [58]. Indeed, higher BMI, the higher prevalence of cardiovascular and endocrine pathologies, among GU patients (including 45.16% of H. pylori-positive) as compared to the controls (H. pylori-negative) was documented in the present study (Table 1). Importantly, polymorphisms of the MMP genes (including MMP9) were suggested to determine the susceptibility to cardiovascular diseases and their complications in various populations [5961], including Caucasians of Central Russia [42, 62, 63]. Wu et al. [45] documented significant positive SNP-based genetic correlation (rg) between PUD and BMI, body fat-related traits, and coronary artery disease. The in silico analysis in our study also identified significant expression and splicing QTLs among the H. pylori-positive GU-associated SNPs of the MMP9 gene and their proxies affecting several genes (e.g., PLTP, CD40, SLC12A5, NEURL2, SPATA25, ZSWIM1, RP3-337O18.9) in the adipose tissue (visceral and subcutaneous).

The available literature data suggests that the above genes are involved in biological pathways contributing to pathophysiology of GU. For example, the PLTP gene encodes one of two phospholipid transfer proteins found in human blood plasma. This protein transfers phospholipids and cholesterol between different classes of lipoproteins and was implicated in many disorders, including hyperlipidemia, obesity, metabolic syndrome, type II diabetes, and others [64]. There is evidence that PLTP may play important roles in the nervous system through participation in signal transduction pathways [65], control of vitamin E content [66], and maintenance of blood-brain barrier integrity [67]. Another example is the CD40 gene. It is a member of the tumor necrosis factor receptor superfamily and encodes a protein playing a key role in a broad range of immune and inflammatory responses including T cell activation, immunoglobulin isotype switching and cytokine production [68]. CD40 has been implicated in various disorders, such as atherosclerosis, cardiovascular, metabolic (arterial hypertension, diabetes mellitus, etc.), and the others [68, 69]. Importantly, the CD40 DNA methylation levels [70] and CD40 expression (protein and mRNA) [71] were associated with gastric cancer. The ACOT8 gene encodes a peroxisomal thioesterase (acyl-CoA thioesterase 8) involved in the oxidation of fatty acids [72]. This enzyme is localized ubiquitously throughout all cellular compartments and is among the key enzymes of lipid metabolism [72].

Due to their pleiotropism, polymorphisms of the MMP9 genes play a key role in multiple biological pathways and therefore have been implicated not only in peptic ulcer [13, 73, present study], but also in cardiovascular diseases [60, 61] as well as a broad range of other disorders involving processes of synthesis and degradation of extracellular matrix: various cancers, including digestive [4648, 7476], glaucoma [27, 77, 78], and others [7982].

One limitation of this study should be acknowledged though. Like other association studies, our study did not utilize any experimental procedures to test the predictions about the possible functional significance of the H. pylori-positive GU-associated SNPs of the MMP9 gene, because “wet” experiments were beyond the study scope. The predictions were made based solely on the in silico analysis of the available functional genomics databases (HaploReg [29], GTExportal browser [41], SIFT online tool [39], RegulomeDB [40]), which include data of large-scale studies in this area (Genotype-Tissue Expression (GTEx) project, Roadmap Epigenomics and ENCODE projects, etc.).

Conclusions

The MMP9 gene polymorphisms were associated with H. pylori-positive GU but not with H. pylori-negative GU in the Caucasian population of Central Russia. Alleles C rs3918249 MMP9 (OR = 2.02) and A rs3787268 MMP9 (OR = 1.60–1.82), and eight haplotypes of the all studied six SNPs MMP9 gene (OR = 1.85–2.04) increased risk for H. pylori-positive GU. None of the MMPs genes SNPs was independently associated with GU. Also, two haplotypes MMP9 gene (including the following SNPs, rs3918242, rs3918249, rs17576, and rs3787268) increased risk for GU (OR = 1.62–1.65). Six loci of the MMP9 gene associated with H. pylori-positive GU and 65 SNPs linked to them manifest significant epigenetic effects, have noticeable eQTL (17 genes) and sQTL (6 genes) values.

Supporting information

S1 Table. The regulatory potential of the studied SNPs.

https://doi.org/10.1371/journal.pone.0257060.s001

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S2 Table. The literature data about associations of the studied polymorphisms of the ММР genes with some digestive diseases.

https://doi.org/10.1371/journal.pone.0257060.s002

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S3 Table. The allele and genotype frequencies of the studied MMP gene SNPs in the GU patients and control group.

https://doi.org/10.1371/journal.pone.0257060.s003

(DOC)

S4 Table. Effect of the MMP-9 gene polymorphisms on affinity of the DNA regulatory motifs.

https://doi.org/10.1371/journal.pone.0257060.s004

(DOCX)

S5 Table. Regulatory effects of the six H. pylori-positive GU-associated SNPs of the MMP9 gene and SNPs in high LD (r2≥0.80).

https://doi.org/10.1371/journal.pone.0257060.s005

(XLS)

S6 Table. eQTL values of the H. pylori-positive GU-associated SNPs MMP-9 gene.

https://doi.org/10.1371/journal.pone.0257060.s006

(XLS)

S7 Table. Effect of SNPs in high LD (r2≥0.80) with the H. pylori-positive GU-associated polymorphisms MMP-9 gene on gene expression level.

https://doi.org/10.1371/journal.pone.0257060.s007

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S8 Table. sQTL values of the H. pylori-positive GU-associated SNPs MMP-9 gene.

https://doi.org/10.1371/journal.pone.0257060.s008

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S9 Table. Effect of SNPs in high LD (r2≥0.80) with the H. pylori-positive GU-associated polymorphisms MMP-9 gene on alternative splicing level.

https://doi.org/10.1371/journal.pone.0257060.s009

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S1 References. References to S2 Table.

https://doi.org/10.1371/journal.pone.0257060.s010

(DOC)

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