Polymorphism of DNA methyltransferase 3B −149C/T and cancer risk: a meta-analysis

DNA methylation is a major epigenetic modification that involves the addition of a methyl group to the 5′ position of a cytosine in a CpG dinucleotide, which is catalyzed by a family of DNA methyltransferases (DNMTs) including three activated forms (DNMT1, DNMT3A and DNMT3B) in human [1, 2]. Aberrant DNA methylation is one of the most consistent epigenetic changes observed in human cancers [3]. DNMT1 is a maintenance DNA methyltransferase, whereas DNMT3A and DNMT3B are considered as de novo methyltransferases because they can methylate unmethylated and hemi-methylated DNA with equal efficiency [4, 5]. A number of studies showed that DNMT3B was up-regulated in several human cancers, demonstrating that DNMT3B may play an important role in tumorigenesis by contributing to the generation of aberrant DNA methylation [6‐8].

The DNMT3B gene is assigned to chromosome 20q11.2 and contains a single C→T transition polymorphism (C46359T) at a novel promoter region, −149 base pairs from the transcription start site, which may result in greatly increased promoter activity of the gene [9]. A number of single-nucleotide polymorphisms (SNP) in the gene have been described in the literature, of which a common SNP −149C/T (rs2424913) in the promoter region of the DNMT3B is known to regulate its expression [10]. Recently, a variety of molecular epidemiological studies have been conducted to examine the association between DNMT3B −149C/T polymorphism and cancer susceptibility [11‐31], but the results remain inconclusive. Therefore, the association between DNMT3B −149C/T polymorphism and cancer risk requires further investigation.

Considering the relatively small sample size in most studies, it is possible to perform a quantitative synthesis of the evidence with rigorous methods. Here, we performed a meta-analysis on 22 published case–controls to derive a more precise evaluation of the association between DNMT3B −149C/T polymorphism and cancer risk.

The present meta-analysis, including 5,903 cancer cases and 8,132 controls from 22 published case–control studies, showed that the DNMT3B −149C/T was not associated with cancer risk. When stratified by different types of cancer, we found an association between DNMT3B −149C/T polymorphism and head and neck cancer risk under heterozygote comparison and dominant model, but there are only two studies in analysis with limited sample size; therefore, the result should be interpreted with caution. Given the important roles of DNMT3B in cancer risk, it was biologically possible that DNMT3B polymorphism is associated with the risk of cancer by increasing DNMT3B promoter activity that modulated an aberrant de novo methylation of CpG islands in some tumor suppressor genes [4]. Studies on the functionality of this polymorphism might contribute to a better understanding of tumor biology and behavior and help us to predict the genetic susceptibility of cancer and choose therapies in an individual manner. However, DNMT3B −149C/T polymorphism did not increase the risk of colorectal cancer, gastric cancer, breast cancer and hepatocellular carcinoma in overall population. The probability may be that different types of cancer may have different mechanism of carcinogenesis. The differences in genetic background and/or environmental exposure may result in different frequency of −149 C/T genotype in healthy individuals from distinct ethnicities; however, in subgroup analysis by ethnicity, we also did not find that DNMT3B −149C/T was associated with ethnicity. It is likely that the small sample size may have insufficient statistical power to detect a real effect. Therefore, more studies based on large population and more different ethnicity should be conducted to further examine this association.

Heterogeneity is a potential problem when interpreting the results of all meta-analysis. Although we minimized the likelihood by performing a careful search for published studies, using strict criteria for study inclusion, precise data extraction and careful data analysis, significant between-study heterogeneity existed in most comparisons. After subgroup analysis by cancer types, ethnicity and source of controls, the heterogeneity was effectively decreased, but significant heterogeneity still existed. Thus, we choose to use random effects model, when I ² value for heterogeneity test is <50 %. The reason might be that different genetic backgrounds and the environment existed among different ethnicities and individuals.

Numbers of SNPs, however, were frequently investigated in the former studies to evaluate the association between DNMT3B polymorphisms and cancer in diverse populations. There might be some other SNPs in DNMT3B associated with risk of cancer. Lee et al. [35] found C alleles of DNMT3B contributed to the susceptibility of lung cancer in Korean population. Some other SNPs of DNMT3B, such as −579 G/T and −283 T/C, were also researched by some studies on their association with cancer risk [11, 12, 14, 19, 36, 37]. However, there were only a very limited number of studies available for some SNPs and therefore not having enough statistical power to explore the real association.

Some other limitations in our meta-analysis should be acknowledged. Firstly, controls were not uniformly defined, while our result was based on unadjusted estimates. Secondly, in the subgroup analyses, the sample size of different types of cancer was relatively small, such as lung cancer, ovarian cancer and prostate cancer not having enough statistical power to explore the real association. Thirdly, only English and Chinese language studies were included in this meta-analysis might have led to publication bias, and the exclusion of unpublished data was generally associated with an overestimation of the true effect.

In conclusion, our meta-analysis suggested that DNMT3B −149C/T polymorphism was not related to overall cancer risk, whereas there was an association between DNMT3B −149C/T polymorphism and head and neck cancer risk under heterozygote comparison and dominant model. Larger samples among different populations, especially more sophisticated gene–gene and gene–environment interactions should be considered in future studies, which should lead to better, comprehensive understanding of the association between DNMT3B −149C/T polymorphism and cancer risk.