A Study on <i>MTHFR</i> C677T Gene Polymorphism and Alcohol Dependence among <i>Meiteis</i> of Manipur, India

Singh, Huidrom Suraj; Salam, Kabita; Saraswathy, Kallur Nava

doi:https://doi.org/10.1155/2014/310241

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Research Article | Open Access

Volume 2014 | Article ID 310241 | https://doi.org/10.1155/2014/310241

A Study on MTHFR C677T Gene Polymorphism and Alcohol Dependence among Meiteis of Manipur, India

Huidrom Suraj Singh,^1,2Kabita Salam,^1,3and Kallur Nava Saraswathy¹

Academic Editor: Ranju Ralhan

Received28 May 2014

Accepted15 Sept 2014

Published01 Oct 2014

Abstract

Chronic alcohol consumption is reported to be associated with increase in plasma homocysteine levels which is further influenced by the polymorphism in methylenetetrahydrofolate reductase (MTHFR) gene. The present study aims to understand the extent of the MTHFR C677T polymorphism in alcohol dependent (AD) cases of Meiteis of Manipur, a Mendelian population of India. MTHFR C677T polymorphism was screened in 313 controls and 139 alcohol dependent (AD) cases who all met DSM-IV criteria for alcohol dependence. Both AD cases and controls were unrelated up to 1st cousin. Among the control group, different drinking patterns like abstainer/nondrinkers (NDs), occasional drinkers (ODs), and moderate drinkers (MDs) are included. Both the groups were found to be in Hardy-Weinberg equilibrium (). Genotypic and allelic frequency distribution of MTHFR C677T polymorphism did not differ significantly between AD cases and controls (). However, individuals carrying mutant (T) allele show more than 1-fold increased risk for AD though not significant (OR = 1.43; 95% CI 0.41–5.01, ). In conclusion, MTHFR C677T polymorphism is not found to be risk marker for AD in present studied population. However, higher prevalence of the mutant T allele may exacerbate deleterious health risk in future especially among alcohol drinkers.

1. Introduction

Alcoholism or alcohol dependence (AD) is a complex trait characterized by a cluster of physiological, behavioural, and cognitive phenomena in which the use of alcohol takes on a much higher priority for a given individual than other behaviours that once had greater value [1]. The World Health Organization (WHO) estimates that about 140 million people throughout the world suffer from AD [2]. Moreover, it is one of the leading health risks and is likely to become world’s third largest risk factor for disease and disability. Approximately 2.5 million deaths each year are attributable to alcohol, resulting in 4% of all deaths worldwide [3].

Several studies show significance of genetic influences in substance abuse and dependence [4, 5]. However, comprehensive molecular and pathophysiological mechanism associated with AD is not completely revealed yet. As genetic predisposition to AD and its related morbidity and mortality is undebatable, the emerging research has picked up momentum targeting various pathways involved in alcohol consumption and metabolism for deeper understanding of the pathophysiology of AD. Recent studies revealed association of gene that encodes the methylenetetrahydrofolate reductase (MTHFR C677T) with AD. However, findings showed inconsistent results [6–8]. Available literature indicates that this polymorphism confers elevation of plasma Hcy levels leading to a condition known as hyperhomocysteinemia [9, 10]. Moreover, chronic alcohol consumption is also often found to be associated with hyperhomocysteinemia [11]. Elevation of Hcy levels may further lead to or be associated with several complex diseases or clinical conditions including cardiovascular diseases, pregnancy complications, neural tube defects, Alzheimer disease, end-stage renal disease, schizophrenia, and noninsulin dependent diabetes, as evidenced from several studies [12, 13].

We therefore believe that studying MTHFR C677T gene polymorphism might possibly be helpful for understanding pathophysiology of AD and its associated complex clinical conditions particularly among those populations where prevalence of alcohol consumption/drinking is very high. But no such trial studies have so far been carried out in any Indian community (according to our knowledge). Thus, in the present study, an attempt is made to understand the extent of MTHFR C677T gene polymorphism in AD cases and controls from Meiteis of Manipur, where prevalence/occurrence of alcohol drinkers is very high [2, 14].

2. Methods

2.1. General Characteristics

The present study’s Meitei population consisted of 452 subjects, of which 139 were AD cases and 313 were unrelated, healthy controls matched for ethnicity and geography. All the subjects included in the present study were recruited from four districts of Manipur, namely, Imphal East, Imphal West, Thoubal, and Bishnupur, where Meiteis are the predominant inhabitants. Diagnosis of alcohol dependence was made on the basis of Diagnostic and Statistical Manual IV (DSM-IV) criteria for AD [15]. The selected control group included individuals consuming alcohol (occasional and moderate drinkers) who were not categorized as alcohol dependent according to the DSM-IV criteria; 121 were absolute nondrinkers. The present study was approved by the departmental ethics committee, Department of Anthropology, University of Delhi, India. Informed written consent was obtained from all the subjects before collecting the samples.

2.2. Genetic Analysis

5 mL of intravenous blood samples were collected in ethylenediaminetetraacetic acid coated vacutainers from all the subjects recruited in the present study using disposable single-use syringes. DNA was isolated from the collected samples using standard protocol [17]. Identification of MTHFR C677T polymorphism was performed using previously described protocol using HinfI restriction enzyme digestion [16]. The digested PCR products were observed on a 3% agarose gel electrophoresis stained with ethidium bromide. Positive and negative controls are run along with samples as quality control. Genotyping details of the selected SNP are shown in Table 1.

2.3. Statistical Analysis

Genotypic and allele frequencies were calculated by gene counting method and Hardy-Weinberg equilibrium (HWE) was determined using the goodness-of-fit test using POPGENE 1.31 [18]. Genotypic and allelic frequency distribution was assessed among the studied population and comparison was made between NDs and ODs, NDs and MDs, and NDs and AD cases using test. Association of drinking status as well as MTHFR C677T allelic and genotypic counts with AD was evaluated by Pearson’s -test followed by odds ratio (OR) at 95% confidential interval (CI), using the freely available contingency table [19]. Statistical significance was considered at 5% level. Power of the study was calculated using online available software (http://osse.bii.a-star.edu.sg/index.php).

3. Results

In the present study, a comparative analysis of the selected SNP, MTHFR C677T polymorphism was carried out among alcohol dependent (AD) cases and controls to understand the effects and their outcome. However, the selected control group included nondrinkers (NDs) and individuals consuming alcohol who were not categorized as alcohol dependence as per DSM-IV criteria, rather they were occasional drinkers (ODs) and moderate drinkers (MDs). To control the biasness, selected genetic marker was assessed in the subgroups of controls, that is, NDs, ODs, MDs, and AD cases (see Table 2).

Less than 3% of individuals were found to have MTHFR 677TT mutant homozygous genotype among the studied Meitei population. The genotypic frequency distribution of the MTHFR 667CC, 667CT, and 667TT genotypes were 65.47%, 31.65%, and 2.88%, respectively, among AD cases compared with 72.84%, 24.92%, and 2.24%, respectively, among controls. Both groups, that is, AD cases and controls, were found to be in Hardy-Weinberg equilibrium (). No significant difference is observed between AD cases and combined controls with respect to genotypic and allelic frequency distribution of MTHFR C677T polymorphism (). Relative risk analysis reveals that individuals who carry mutant T allele in both heterozygous or homozygous condition show more than onefold increased risk for AD (OR = 1.43, CI 0.41–5.01 and OR = 1.41, CI 0.91–2.20, resp.); however, the risk was not found to be statistically significant (). Power of the study was found to be <20%, which could possibly be due to smaller sample size of the studied population.

To assess the extent of MTHFR C677T polymorphism on different patterns of drinking, mutant homozygous 677TT genotype was further assessed in the three subgroups of controls (NDs, ODs, and MDs) and AD cases. 677TT genotype individuals were found to be lower in NDs (2.48%) as compared to ODs (3.54%) and AD cases (2.88%); the difference was not found to be statistically significant (). Though 677TT genotype is found to be completely absent among MDs. This could possibly be due to smaller sample size among the moderate drinkers (MDs). Distribution of the mutant T allele frequency showed an increasing trend from NDs to ODs to AD cases with slight drop among MDs.

To understand the relative risk of MTHFR 677TT genotype on different patterns of drinking, odds ratio was calculated for ODs, MDs, and AD cases taking NDs as reference group. Except AD cases (OR = 1.47, CI 0.86–2.50), other groups, that is, ODs (OR = 1.10, CI 0.62–1.95) and MDs (OR = 1.01, CI 0.53–1.91) showed more or less than onefold increased risk for alcohol dependence, though risks were not found to be statistically significant () in all the three alcohol drinking categories (Table 3).

4. Discussion

Alcohol is a toxic substance that can affect each and every organ of human body particularly stomach, liver, brain, and heart. Alcohol has been found to interact with MTHFR gene polymorphism as indicated by several literatures in modifying the risk of several complex diseases including cardiovascular diseases, diabetes, colon cancer, breast cancer, and hepatocellular carcinoma [20, 21]. Moreover, previous studies have associated MTHFR gene polymorphism with decreased enzymatic activity and modified homocysteine regulation. Therefore, chronic alcohol consumption may increase the risk of causing/developing total plasma homocysteine levels (i.e., hyperhomocysteinemia) which may further lead to several disease phenotypes in the presence of the reduced MTHFR activity associated with the polymorphic gene. The present study determines and compares MTHFR C677T polymorphism among AD cases and controls among Meiteis of Manipur, which is reported to have higher prevalence of alcohol dependence [2, 14]. One of the contributing factors of alcohol dependence in Manipur has been cited as widely available in every nook and corner despite the fact that it is officially declared “dry” state.

The MTHFR C677T polymorphism has been investigated for its association with several complex diseases in several studies across different populations; however, results are not consistent. One of the possible reasons for this could be attributed to variation in allelic frequency distribution in different population groups. The 677T allele frequency is found to be highest in European populations ranging from 24.1% to 64.3% and, hence, it is presumed to be originated in Europe in the late state of human evolution. However, zero frequency of this allele is reported from African population [22]. In Indian population, distribution of 677T allele ranges from complete absence to 23.7% and highest frequency was reported from North-Indian population. Moreover, frequency of T allele is found to be relatively higher among caste populations as compared to that of tribal populations of India. Linguistically, Indo-European speakers have relatively higher T allele frequency followed by Tibeto-Burman, Dravidian, and Austro-Asiatic speakers [22].

An association study carried out in European Caucasoid population demonstrated significant association of mutant T allele of MTHFR C677T polymorphism with alcoholic patients with a history of withdrawal symptoms (WS) (T allele frequency − controls = 0.28, AD cases = 0.39; ) [6]. Similar findings were also reported by Benyamina et al. suggesting possible role of C677T SNP on the etiology of AD. The MTHFR TT genotype was found to be more prevalent in AD patients with milder alcohol dependence (Babor type A) and with Lesch type 3, associated with depression [8]. In the present study, no association was found between alleles or genotypes of MTHFR C677T polymorphism and AD among Meiteis of Manipur. However, our observation of TT genotype being slightly higher among AD cases (2.88) as compared to controls (2.24) is in concurrence with the above association studies where an excess of mutant homozygotes has been reported among the AD cases. Though, no significant difference was observed in the present study. 677T allele frequency distribution among nondrinkers (NDs) that is 0.14 is in accordance with previous report [23]. Moreover, distribution of the mutant T allele frequency showed an increasing trend in the present study from NDs to ODs to AD cases with slight drop among MDs. Lower frequency of T allele among the MDs could be attributed to smaller sample size as well as complete absence of mutant homozygous TT genotype. Such similar increasing trend of T allele is also reported among different subgroups of alcohol use disorders like from healthy controls (0.28) to alcoholic patients with mild withdrawal symptoms (0.33) up to 0.40 in alcohol dependent patients having withdrawal symptoms [6].

However, in contrast to the present study and other association studies reporting association of MTHFR C677T gene polymorphism with AD, Saffroy et al. reported a contradictory result among the Caucasian French populations [7]. In fact, they attempted to understand the prevalence of the MTHFR C677T polymorphism in AD subjects and its influence on symptoms associated with alcoholism among Caucasian French populations. They observed a significant decrease in MTHFR 677TT prevalence among AD cases (9%, 21/242) compared to controls (18%, 17/93) () with an odds ratio of 0.42 for alcoholism in subjects with TT genotype (95% CI 0.21–0.83). They reported that MTHFR 677TT genotype could play a protective role against alcohol dependence, for the first time. They also suggested possibility of influence of MTHFR C677T polymorphism on the development of the dependence process itself. However, more association studies are needed to really understand whether MTHFR C677TT genotype is protective against AD or not. Though no confirmatory studies have been reported till now, one of the possible reasons for such inconsistent results could be attributed to its associations with one-carbon metabolism pathway, as MHFR C677T polymorphism plays an important role in elevation of plasma Hcy levels. Moreover, it is also evident that chronic alcohol consumption is associated with folate deficiency which may further lead to an impaired metabolism of homocysteine via inhibiting methionine synthase resulting in the elevation of Hcy level [24]. Both elevation of Hcy level and deficiency of folate may further influence DNA methylation rate, since folate acts as a methyl donor (via S-adenosylmethionine) for DNA methyltransferase and histone methyltransferase [25]. Aberration in DNA methylation status can lead to alterations in reprogramming of epigenetic patterns thereby affecting gene regulation [26]. Further, it also alters the dopaminergic neurotransmission system in the brain affecting cognitive behaviours and addiction [27]. Therefore, polymorphism in this gene may indirectly propagate the development of alcohol dependence by impairing homocysteine metabolism via inhibiting methionine synthase.

Findings of the present study and available literatures suggest that MTHFR C677T polymorphism influence the etiology of alcohol dependence. However, focusing on the ill effects of MTHFR C677T gene polymorphism and its interaction with alcohol would be more meaningful rather than focusing on the development of alcohol dependence process. However, present study has some major limitations like smaller sample size (low study power) and lack of data on related biochemical variables including homocysteine levels, folate, and vitamin B₁₂. Further studies are required to understand the exact pathophysiological mechanism of the development of alcohol dependence with respect to MTHFR C677T gene polymorphism. Therefore, association of MTHFR 677TT genotype with hyperhomocysteinemia, folate, and vitamin B₁₂ levels could assist physicians in identifying AD patients as well as improvement in addiction management.

5. Conclusions

In brief, to our knowledge, this is the first study attempted to understand the extent of MTHFR C677T gene polymorphism against alcohol dependence in Indian context. The present study indicates that MTHFR C677T polymorphism has no direct significant conferring risk for AD among Meiteis of Manipur. However, the selected polymorphism may directly or indirectly affect the one-carbon metabolism by interacting with environmental risk factors and subsequently progressing towards the development of AD. Higher prevalence of the mutant allele in the studied population may exacerbate deleterious future health risk among alcohol drinkers (especially AD cases). Therefore, the present paper paves a way for further population specific studies specifically interaction of selected SNP with biochemical variables including homocysteine, folate, vitamin B₁₂, liver function test, etc. to understand its relationship and predictive outcomes of health effects as well developing right interventional strategies and therapeutics.

Conflict of Interests

The authors report no conflict of interests.

Acknowledgments

The authors wish to thank all the individuals, who participated and contributed to the successful completion of the present study. They would also like to thank University Grants Commission (UGC), India, for their financial support and Centre for Social Development (CSD), Manipur, for allowing them to collect samples.

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Copyright

Copyright © 2014 Huidrom Suraj Singh 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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