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    Correlating interleukin-10 promoter gene polymorphisms with human cerebral infarction onset

    2015-02-07 12:58:29XinhongJiangKexuLinYixianZhangRonghuaChenNanLiu

    Xin-hong Jiang, Ke-xu Lin, Yi-xian Zhang, Rong-hua Chen, Nan Liu,,

    1 Department of Rehabilitation, Union Hospital, Fujian Medical University, Fuzhou, Fujian Province, China

    2 Department of Emergency, Union Hospital, Fujian Medical University, Fuzhou, Fujian Province, China

    3 Department of Neurology, Union Hospital, Fujian Medical University, Fuzhou, Fujian Province, China

    Correlating interleukin-10 promoter gene polymorphisms with human cerebral infarction onset

    Xin-hong Jiang1, Ke-xu Lin2, Yi-xian Zhang1, Rong-hua Chen3, Nan Liu1,3,*

    1 Department of Rehabilitation, Union Hospital, Fujian Medical University, Fuzhou, Fujian Province, China

    2 Department of Emergency, Union Hospital, Fujian Medical University, Fuzhou, Fujian Province, China

    3 Department of Neurology, Union Hospital, Fujian Medical University, Fuzhou, Fujian Province, China

    Evidence suggests that interleukin-10 (IL-10) def ciency exacerbates inf ammation and worsens the outcome of brain ischemia. In view of the critical role of the single nucleotide polymorphic sites -1082 (A/G) and -819 (C/T) in the promoter region of the IL-10 gene, we hypothesized that they are associated with cerebral infarction morbidity in the Chinese Han population. We genotyped these allelic gene polymorphisms by amplif cation refractory mutation system-polymerase chain reaction methods in 181 patients with cerebral infarction (cerebral infarction group) and 115 healthy subjects (control group). We identif ed signif cant dif erences in genotype distribution and allele frequency of the IL-10-1082 A/G allele between cerebral infarction and control groups (χ2= 6.643, P = 0.010). The IL-10-1082 A allele frequency was signif cantly higher in the cerebral infarction group (92.3%) than in the control group (86.1%) (P = 0.015). Moreover, cerebral infarction risk of the AA genotype was 2-fold higher than with the AG genotype (OR = 2.031, 95%CI: 1.134–3.637). In addition, AA genotype together with hypertension was the independent risk factor of cerebral infarction (OR = 2.073, 95%CI: 1.278–3.364). No statistical dif erence in genotype distribution or allele frequency of IL-10-819 C/T was found between cerebral infarction and control groups (P > 0.05). These f ndings suggest that the IL-10-1082 A/G gene polymorphism is involved in cerebral infarction, and increased A allele frequency is closely associated with occurrence of cerebral infarction.

    neural regeneration; IL-10; promoter; gene polymorphisms; ischemic stroke; genetic susceptibility; inf ammation; immune response; ischemia/ reperfusion injury; neural regeneration

    Funding: This study was supported by the National Natural Science Foundation of China, No. 81171867; a grant from the Key Research Program of Fujian Department of Science and Technology of China, No. 2011Y0027.

    Jiang XH, Lin KX, Zhang YX, Chen RH, Liu N (2015) Correlating interleukin-10 promoter gene polymorphisms with human cerebral infarction onset. Neural Regen Res 10(11):1809-1813.

    Introduction

    Cerebral infarction is one of the primary causes of long-term functional disability (Liu et al., 2010, 2013b), and results in residual impairment that diminishes a patient’s independence and quality of life (Nowak, 2008). Despite advances in medical, thrombolytic, and surgical treatments, the treatment of cerebral infarction still lacks an optimal method (Liu et al., 2011b). Recently, the action of non-specif c inf ammation has shed light on ischemia/reperfusion injury (Daemen et al., 1999; Collard and Gelman, 2001; Jong et al., 2003; Yellon and Hausenloy, 2007), and is known to play a critical role during cerebral infarction. Cerebral ischemia induces a strong immune response and consequent inf ammation, which is characterized by activated cytokines, chemokines, adhesion molecules, and proteolytic enzymes that exacerbate tissue damage (del Zoppo et al., 2000; Emsley and Tyrrell, 2002; Wang et al., 2013; Tu et al., 2014). However, the pathogenesis of cerebral infarction is very complicated (Liu et al., 2013a). Interleukin-10 (IL-10) is a pleiotropic cytokine that can exert anti-inf ammatory ef ects during cerebral ischemia injury. The IL-10 gene promoter is highly polymorphic, with multiple single nucleotide polymorphic sites. The most important three sites are -1082 (A/G), -819 (C/T), and -592 (C/A) (Perrey et al., 1999). In this study, we focused on the relationship between IL-10 gene promoter polymorphisms and cerebral infarction. Accordingly, we used amplif cation refractory mutation system-polymerase chain reaction (ARMS-PCR) to detect the distribution frequency of -1082 (A/G) and -819 (C/T) in cerebral infarction. Our study supports the notion that IL-10 gene def ciency determines genetic susceptibility to cerebral infarction.

    Subjects and Methods

    Subjects

    The patients included in this study were inpatients of the Department of Neurology in Union Hospital of Fujian Medical University, China from August 2011 to February 2013. In the cerebral infarction group, there were 181 cases, consisting of 123 males and 58 females, aged 66.1 ± 10.5 years. In the control group, there were 115 healthy subjects, consistingof 68 males and 47 females, aged 65.4 ± 11.6 years. There were no differences in age and gender between the groups (P< 0.05).

    All cerebral infarction patients met the International Classification of Diseases, 10threvision (ICD-10) cerebral infarction classification criteria (Organization, 2004). All healthy control subjects had received a physical examination in Union Hospital of Fujian Medical University, China.

    Patients with any of the following diseases were excluded: cardiac embolism, vasculitis, trauma, thyroid disease, blood disease, use of immunosuppressive agents, cancer, pregnancy, autoimmune diseases, infection, cerebral vascular malformation, or aneurysm.

    The study was approved by the Ethics Committee of Fujian Medical University on the basis of the Declaration of Helsinki-Ethical Principles for Medical Research Involving Human Subjects. All patients provided written informed consent.

    Extraction of genomic DNA

    Two mL samples of fasting antecubital venous blood from both groups were placed in EDTA-Na anticoagulant tubes. Genomic DNA extraction was performed according to the instructions of the DNA extraction kit (Promega Corporation, Madison, WI, USA). The final concentration of DNA working solutions was 0.1 g/L. Working solutions were stored at ?20°C.

    IL-10 promoter polymorphism detection

    Genetic testing primers were synthesized by Shanghai Bioengineering Technology Company (Shanghai, China). PCR amplification was performed (MBI Fermentas, Shanghai, China) according to a previously described method (Perrey et al., 1999). The IL-10-1082 A/G and -819 C/T gene loci primers are:

    IL: Interleukin.

    Gene polymorphisms were genotyped by ARMS (Newton et al., 1989), which was performed in 25 μL volumes containing 25–50 ng genomic DNA, 0.25 mM specif c primers, and0.1 mM internal control primers in the presence of 1.5 mM MgCl2, 0.2 mM each dNTP, 500 mM KCl, 200 mM Tris-HCl, 0.001% gelatin, and 0.5 U Taq DNA polymerase. Internal reference primers were used to identify successful PCR amplif cation, and amplif ed a conserved region of exon 3 of the HLA-DRB1 gene. ARMS-PCR for amplification of the IL-10-1082 G/A and –819 C/T alleles was performed under the following conditions: amplif cation with a 1 minute denaturation step at 95°C, then 10 cycles of 15 seconds at 95°C, 50 seconds at 65°C, and 40 seconds at 72°C, and 20 cycles of 20 seconds at 95°C, 50 seconds at 59°C, and 30 seconds at 72°C, followed by cooling to 4°C (Perrey et al., 1999). After PCR amplif cation, PCR products were resolved by 2% agarose gel electrophoresis and visualized under ultraviolet light, using a 100 bp ladder for sizing. Gene bands from two cases were sequenced by Tiangen Sequencing Biotechnology Co., Ltd. (Beijing, China).

    Table 1 General information for cerebral infarction and control groups

    Table 2 Comparison of interleukin (IL)-10-1082 A/G and -819 C/T genotype frequency [n(%)] between cerebral infarction and control groups

    Table 3 Comparison of interleukin (IL)-10-1082 A/G and -819 C/ T allele frequency [n(%)] between cerebral infarction and control groups

    Table 4 Non-conditional logistic regression analysis of risk factors for cerebral infarction

    Figure 1 Genotyping electrophoresis pattern for the interleukin (IL)-10 promoter region -1082 locus.

    Figure 3 Genotyping electrophoresis pattern for the interleukin (IL)-10 promoter region -819 locus.

    Figure 4 Reverse sequencing map of the interleukin (IL)-10 promoter region -819 locus (arrows).

    Statistical analysis

    Data analysis was performed using SPSS 13.0 software (SPSS, Chicago, IL, USA). Allele frequency was calculated as: (2 × homozygotes + heterozygotes)/(2 × the number of patients). Representative samples from each group were analyzed using the Hardy-Weinberg balance method. Categorical data [n(%)] were analyzed by chi-square test. Measurement data (mean ± SD) characterized by normal distributions were analyzed by two-sample t-tests. Non-conditional probability logistic regression analysis was used to eliminate the potential inf uence of potential and confounding factors. Values of P < 0.05 were considered statistically signif cant.

    Results

    Demographics between cerebral infarction and control groups There were no signif cant dif erences in age, gender, hyperlipidemia onset, and coronary heart disease onset between cerebral infarction and control groups. The proportion of hypertension and diabetes in the cerebral infarction group was signif cantly higher than in the control group (P < 0.05; Table 1).

    Gene polymorphism analysis of the IL-10-1082 A/G locus The electrophoretic band at 258 bp represented the homozygote alleles, either G (GG) or A (AA). Using the same two pairs of primers, another electrophoretic band at 258 bp represented the heterozygote allele (AG) (Figure 1). Representative sequencing results are shown in Figure 2.

    Gene polymorphism analysis of the IL-10-819 C/T locus The electrophoretic band at 233 bp represented the homozygote alleles, either C (CC) or T (TT). Using the same two pairsof primers, another electrophoretic band at 233 bp represented the heterozygote allele (CT) (Figure 3). Representative sequencing results are shown in Figure 4.

    IL-10-1082 A/G and -819 C/T genotype and allele frequencies

    There were signif cant dif erences in IL-10-1082 A/G genotype distribution frequency between cerebral infarction and control groups [AA: 153 cases (84.5%) vs. 83 cases (72.2%); AG: 28 cases (15.5%) vs. 32 cases (27.8%) (χ2= 6.643, P = 0.010)]. For the IL-10-1082 locus, the A allele frequency in the cerebral infarction group was signif cantly higher than in the control group (92.3% vs. 86.1%; χ2= 5.894, P = 0.015). There were no significant differences in IL-10-1082 A/G and -819 C/T genotype and allele frequencies between both groups (P < 0.05) (Tables 2 and 3).

    Risk factors of cerebral infarction

    To exclude confounding factors, we analyzed possible factors related to cerebral infarction, specif cally, hypertension, diabetes, and IL-10-1082 genotype. Stepwise multiple linear regression and non-conditional logistic regression analyses were performed, in which the three factors served as independent variables and cerebral infarction as the dependent variable. The results were determined using 0.05 and 0.10 as significant standard introducing and eliminating variables, respectively. We found that two independent variables, namely hypertension and 1082 locus genotype, were signif -cantly relevant to cerebral infarction (P < 0.05; Table 4).

    Discussion

    Pathogenesis of ischemic brain damage is complicated, with non-specif c inf ammation mediated by pro-inf ammatory cytokines and chemokines and other inflammatory mediators playing an important role (del Zoppo et al., 2000; Emsley and Tyrrell, 2002; Min et al., 2013; Zhou et al., 2014). Interleukin-10, a pleiotropic anti-inf ammatory factor, plays a protective role in cerebral ischemia models (Moore et al., 2001; Liu et al., 2009). It prevents downregulation of the anti-apoptotic protein Bcl-2 in ischemic brain tissue, and limits excitotoxic damage to the brain through an activin-dependent mechanism (Liu et al., 2007). Ischemic insult and IL-10 administration augments neurogenesis in the rodent brain (Dietrich et al., 1999; Vila et al., 2003; Woiciechowsky et al., 2004; Liu et al., 2007). Hence, these f ndings suggest that IL-10 contributes to reduction of infarct volume and neurological improvement after experimental focal cerebral ischemia. The protective mechanism of IL-10 is achieved by downregulating expression of IL-1β, tumor necrosis factor alpha (TNF-α), P-selectin and other pro-inf ammatory cytokines, and reducing neuronal apoptosis (Liu et al., 2007; Liu et al., 2009). Previous studies have shown a close association between P-selectin, IL-6 promoter polymorphism, and cerebral infarction (Zee et al., 2004; Tong et al., 2010). However, little is known about the association between IL-10 gene polymorphism and cerebral infarction.

    The IL-10 gene promoter region is approximately 5 kb and located within the region upstream of the translation initiation site (Turner et al., 1997; D’Alfonso et al., 2000). The IL-10 gene promoter is highly polymorphic with multiple single nucleotide polymorphic sites. The three most important ones are -1082 (A/G), -819 (C/T), and -592 (C/ A) (Perrey et al., 1999). Here, we found that the genotype distribution of the IL-10 promoter in the Chinese Han population is consistent with the results of a previous study (Meenagh et al., 2002). Specif cally, the frequency of G allele carriers of the -1082 locus is signif cantly lower in the Chinese Han population than that in Ireland, Mexico, and other races. Additionally, our data shows that the -1082 locus GG genotype is not detectable in the Chinese Han population, and only the AA and/or AG genotypes are present. These f ndings indicate that gene polymorphisms of some inf ammatory cytokines dif er depending upon ethnicity. Based on the f nding that IL-10 genetic linkage at the single nucleotide polymorphic sites, -819 and -592, are linked (Perrey et al., 1999), we assumed -592 genotypes from -819 genotypes, instead of directly examining IL-10-592 loci polymorphic sites.

    Interleukin-10 gene promoter polymorphisms are closely related to IL-10 expression levels in vivo. Studies indicate that -1082G, -819C, and -592C are highly expressed alleles compared with -1082A, -819T, and -592A (Hoffmann et al., 2001). In the presence of allele -1082A, stimulation of lymphocytes with concanavalin A results in lower IL-10 production than in allele -1082A-negative cells (Turner et al., 1997; Koch et al., 2001). These studies also found that protein production is independent of alleles -819 and -592, suggesting that IL-10 levels are determined mainly by the -1082 genotype. Here, we found a statistical dif erence in distribution of the IL-10-1082 locus between cerebral infarction and control groups, suggesting that cerebral infarction risk is 2-fold higher with the AA genotype than the AG genotype. Therefore, the AA genotype together with hypertension is the independent risk factor of cerebral infarction. Interestingly, our results show that the A allelic gene frequency in cerebral infarction patients (92.3%) is higher than normal controls (86.1%). This was not observed for IL-10-819 C/T and-592 C/A genotype distributions and allele frequencies, suggesting that the incidence of cerebral infarction is related to increased frequency of the IL-10-(-1082 A/G) A allele.

    Cerebral infarction is associated with an extremely high rate of disability (Liu et al., 2011a). For a long time, clinical experts have formed a consensus on its clinical risk factors, i.e., hypertension, diabetes, and hyperlipidemia. Generally, the incidence of cerebral infarction can be signif cantly reduced through ef ective interventions to these risk factors. However, these known risk factors are not found in a considerable proportion of patients, even with a thorough medical history and physical examination. Thus, we found signif cant correlation between the IL-10-1082 gene polymorphism and cerebral infarction. Further studies regarding the IL-10-1082 gene polymorphism are needed, with consideration of a different experimental design. Detection of cerebral infarction susceptibility genes is conducive to identifying populationsat disease risk, and improving the ef ectiveness of primary prevention.

    Acknowledgments: We would like to thank our colleague Xiao-dong Pan for language revision.

    Author contributions: NL had full access to the study concept and design, and supervised the study. XHJ was responsible for study design and wrote the paper. KXL, YXZ, and RHC provided and analyzed the data, and performed the statistical analysis. All authors approved the f nal version of the paper. Conf icts of interest: None declared.

    Plagiarism check: This paper was screened twice using Cross-Check to verify originality before publication.

    Peer review: This paper was double-blinded, stringently reviewed by international expert reviewers.

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    Copyedited by James R, Raye W, Wang J, Li CH, Song LP, Zhao M

    *Correspondence to: Nan Liu, M.D., xieheliunan1984@sina.com.

    orcid: 0000-0003-2901-3721 (Xin-hong Jiang)

    10.4103/1673-5374.170308 http://www.nrronline.org/

    Accepted: 2015-08-11

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