Aberrant GSTP1 promoter methylation is associated with increased risk and advanced stage of breast cancer: a meta-analysis of 19 case-control studies

Background Glutathione S-transferase P1 (GSTP1) has been reported to function as a tumor suppressor gene in various types of human cancers. Aberrant methylation of tumor-related genes at the promoter regions can inactivate genes, which is important in the carcinogenesis of breast cancer. However, the role of GSTP1 promoter methylation in the occurrence of breast cancer and its relationship with tumor stage and histological grade has not been fully elucidated. Thus, we carried out a meta-analysis to yield a more accurate association. Methods A systematically literature search was made on PubMed, EMBASE and Web of Science databases for eligible studies. The odds ratio (OR) and 95 % confidence interval (95 % CI) were calculated by RevMan 5.2 software. Subgroup and sensitivity analyses were conducted to explore the source of heterogeneity. Results Eventually, 17 articles involving 19 case–control studies were included in the present meta-analysis. Overall, the pooled results indicated that aberrant GSTP1 promoter methylation was significantly associated with the risk of breast cancer (OR = 7.85, 95 % CI = 5.12–12.01; Caucasians OR = 7.23, 95 % CI = 3.76–13.90 and Asians OR = 11.71, 95 % CI = 5.69–24.07). Furthermore, our results revealed that GSTP1 promoter methylation was more often observed in late-stage breast cancer patients compared with early-stage ones (OR = 1.84, 95 % CI = 1.32–2.58). However, no significant association was identified between GSTP1 promoter methylation and histological grade (OR = 0.74, 95 % CI = 0.43–1.26). Conclusions The results indicated that GSTP1 promoter methylation probably plays an important role in breast carcinogenesis, which could serve as an effective biomarker for the diagnosis and monitor of breast cancer. Electronic supplementary material The online version of this article (doi:10.1186/s12885-015-1926-1) contains supplementary material, which is available to authorized users.


Background
Breast cancer, a heterogeneous disease, is by far the most common malignancy that affects females. It has been reported that an estimated 1.7 million new cases of breast cancer were diagnosed with nearly 522,000 related deaths worldwide in 2012 [1]. Moreover, incidence rates differ between regions with a lifetime risk of 1 in 3 women in Asia and 1 in 8 women in the United States [2]. Despite intensive research, the molecular mechanism of cancer development is still not fully understood. Generally, the interplay between genetic and environmental risk factors has played an important role in the etiology of breast cancer [3]. In recent years, increasing evidence has shown that epigenetic changes of tumor-related genes are involved in the pathogenesis and development of breast cancer, and could be used as indicators of cancer diagnosis and treatment [4][5][6].
Glutathione-S-transferases (GSTs) are a family of enzymes involved in the detoxification of carcinogenic and cytotoxic substances by catalyzing their conjugation with reduced glutathione [7,8]. Among the isoenzymes, the pi-class GST (GSTπ) encoded by the GSTP1 gene is implicated in a large variety of detoxification and metabolism reactions, which prevent cells from genome damage and cancer initiation [9,10]. The GSTP1 gene is a tumor suppressor gene and locus on chromosome 11q13 [11]. Aberrant methylation of the GSTP1 often occurs in different cancer types including those of liver, prostate, and breast cancer [12,13]. Moreover, the silencing of GSTP1 gene expression induced by promoter methylation has been found to be implicated in the pathogenesis of breast cancer [14].
To date, several studies have investigated the methylation patterns of the GSTP1 in breast cancer patients, yet the data are greatly variable due to differences among studies. Therefore, we conducted a meta-analysis of the published clinical studies to evaluate the effect of GSTP1 promoter methylation on breast cancer patients.

Eligible criteria
Eligible studies included in this meta-analysis should meet the following standards: (1) assessed the association between GSTP1 promoter methylation and breast cancer; (2) independent case-control studies; (3) all patients met the clear diagnostic criteria for breast cancer; (4) provided sufficient data about the methylation levels of GSTP1 in tissue or blood samples of cancer patients and normal controls; (5) the methylated GSTP1 was detected by polymerase chain reaction (PCR) based methylation assays.

Literature search
This meta-analysis was reported according to the checklist of the Meta-analysis of Observational Studies in Epidemiology (MOOSE) guidelines (Additional file 1: Table S1). We systematically searched related clinical studies regarding the association between GSTP1 promoter methylation and breast cancer via PubMed, EMBASE and Web of Science databases (up to January 31, 2015). The key terms: (breast OR mammary) And (cancer OR neoplasm OR tumor OR carcinoma) And (GSTP1 OR glutathione S-transferase P1) And (methylation OR hypermethylation) were used. The references cited in the selected studies were also scanned for relevant studies.

Data extraction
Data extraction was conducted independently by two reviewers from the included studies. The recorded information for each study contained the following: First author's name, year of publication, patients' ethnicity, sample type, sample size, tumor stage, histological grade, GSTP1 methylation frequencies and the methylation detection methods. All selected studies used normal samples as controls, which were composed of normal breast tissues from breast cancer patients and normal samples from noncancer people. Of these studies, we combined stage 0, I and II as early-stage, stage III and IV as late-stage, which were defined by AJCC staging system [15]. As for histological grade, Grade I and II were defined as low-grade, Grade III was defined as high-grade [16].

Statistical analysis
Odds ratios (ORs) and their 95 % confidence intervals (CIs) were used to evaluate the association. Heterogeneity was quantified by the Cochran Q test with statistical significance set at P < 0.10 and I 2 statistics. If there was no statistical heterogeneity among studies (P ≥ 0.10 and I 2 < 40 %), we used the fixed-effect model to pool the results; otherwise, the random-effects model was applied [17]. Moreover, subgroup analyses, which were stratified according to the patients' ethnicity, sample type and detection methods were performed to explore potential sources of heterogeneity and the differences among them. In the presence of heterogeneity, sensitivity analysis was conducted by omitting a single study in each turn to see whether a particular omission could influence the overall estimate. The funnel plots were applied to assess publication bias if the included number of studies was no less than nine. All above analyses were carried out using the Review Manager 5.2 software (Cochrane Collaboration, Oxford, UK). In addition, the effect of possible publication bias was evaluated using the Egger's test [18] and trim-and-fill method [19] by STATA 12.0 software.

Overall and subgroup analyses
Our results showed that breast cancer exhibited significantly higher frequency of GSTP1 methylation than normal controls (OR = 7.85, 95 % CI = 5.12-12.01, Fig. 2). Moreover, subgroup analyses were performed to identify the influence of abnormal GSTP1 promoter methylation on the risk of breast cancer. Ethnicity-stratified analysis revealed that there were statistical associations between GSTP1 promoter methylation and increased breast cancer risk among both Caucasians (OR = 7.23, 95 % CI = 3.76-13.90) and Asians (OR = 11.71, 95 % CI = 5.69-24.07). After stratified by sample type, we found that aberrant methylation of GSTP1 was correlated with the risk of breast cancer detected in tissue (OR = 10.32, 95 % CI = 5.97-17.85) as well as blood samples (OR = 4.02, 95 % CI = 1.12-14.38). After stratified by method, significant associations between GSTP1 promoter methylation and the risk of breast cancer were observed in all of the subgroups (Quantitative: OR = 4.73, 95 % CI = 1.84-12.12; Semi-quantitative:    Table 2. In addition, eight studies [22,28,29,[33][34][35] comprising 832 patients were pooled for the OR in evaluating the association between GSTP1 methylation and tumor stage. The results revealed that aberrant GSTP1 methylation was more often observed in late-stage patients compared with early-stage ones (OR = 1.84, 95 % CI = 1.32-2.58, Fig. 3). However, the pooled OR of five studies showed that there was no significant association between GSTP1 methylation and histological grade (OR = 0.74, 95 % CI = 0.43-1.26) ( Table 3).

Sensitivity analysis
The results showed that moderate heterogeneity existed in investigating the correlation of GSTP1 methylation and breast cancer risk detected in blood samples and quantitative method by subgroup analysis (Table 2). Then, a sensitive analysis was used to find the heterogeneous study. After removal of the study by Brooks et al. [27], the heterogeneity presented in blood samples was reduced from I 2 = 54 % (P h = 0.07) to I 2 = 0 % (P h = 0.71), the heterogeneity in quantitative method was also reduced from I 2 = 45 % (P h = 0.08) to I 2 = 0 % (P h = 0.43), suggesting it might be the heterogeneous study. However, the pooled ORs were not significantly changed in sensitivity analyses, in which each study was deleted at one time, suggested the stability of our results.

Publication bias
Visual inspection of the funnel plot in Fig. 4 shows an asymmetry, which indicates the presence of publication bias in evaluating GSTP1 methylation and breast cancer risk. Egger's test also display statistical evidence of

Discussion
GSTP1 is a member of the metabolic enzymes family, which has significant implications in the prevention of cancer initiation upon exposure to carcinogens [11,13]. Absence of GSTP1 expression is found in approximately two thirds of the patients with breast cancer, suggesting it might play an important role in breast carcinogenesis [23]. It has also been demonstrated that the hypermethylation of GSTP1 gene promoter frequently occurs in breast cancer and may result in inactivation of GSTP1 expression, thus lead to cancer progression [13].
The current meta-analysis demonstrated that the methylation level of GSTP1 was significantly higher in breast cancer patients than that in normal controls, which indicated its potential role in the etiology of breast cancer. This was in accordance with the results of previous studies [22][23][24]. We also performed subgroup analyses to further explore the potential effects of the patients' ethnicity, sample type and detection method on the association of GSTP1 promoter methylation with the risk of breast cancer. The results revealed that GSTP1 promoter methylation was closely associated with the risk of breast cancer in both Caucasians (OR = 7.23, 95 % CI = 3.76-13.90) and Asians (OR = 11.71, 95 % CI = 5.69-24.07), whereas, the correlation was stronger in Asians than in Caucasians. The reasons might include differences in genetic backgrounds, environments and sample size. After stratified by sample type, we found that aberrant methylation of GSTP1 was correlated with the risk of breast cancer detected in tissue (OR = 10.32, 95 % CI = 5.97-17.85) as well as blood samples (OR = 4.02, 95 % CI = 1.12-14.38). Moreover, a high concordance between tumor and blood DNA methylation of GSTP1 was reported in studies conducted on paired tumor tissue and blood samples from breast cancer patients [29,33]. Yamamoto et al. compared the gene methylation status in serum DNA before and after surgery in patients with primary breast cancer, and demonstrated that the origin of blood methylated DNA was the tumor tissue because patients with aberrant GSTP1 methylation in serum DNA collected before surgery were found to be negative for gene methylation after surgery [33]. This indicated that blood DNA methylation of GSTP1 could reflect alterations in the tumor and the ease of obtaining blood samples makes it a potential biomarker for diagnosis of breast cancer. In the present meta-analysis, the small number of patients, various ethnicity groups and different time of sample collection may contribute to relatively extended confidence intervals. To date, a diversity of PCR based methylation assays were developed and widely used to measure methylation in clinical specimens, classified as quantitative, semi-quantitative and non-quantitative techniques [37]. Several papers have compared MS-MLPA (semi-quantitative) with pyrosequencing (quantitative) or MSP (non-quantitative) and showed a good concordance between MS-MLPA and pyrosequencing [30,37]. Since different methylation assays were applied to detect the methylation levels of GSTP1 in the studies included in this  meta-analysis, we also performed subgroup analysis based on methods to explore potential sources of heterogeneity and the differences among them. As a result, significant associations were identified as detected by quantitative, semi-quantitative and non-quantitative techniques, suggested these methods have the same effect in GSTP1 methylation detection. However, when only quantitative analyses of GSTP1 promoter methylation in blood DNA are pooled, no significant association was observed (data not shown). It is hypothesized that the small sample size may lead to false-negative results. Furthermore, different patient materials and the choice of different primer sets between different studies may influence the results. Aberrantly methylated genes are frequently found in human cancers but rarely in normal controls, and their presence is not an exclusive attribute of metastatic cancer. Examination of body fluid from patients with early stage or organ-confined tumors may also reveal positive results [28]. Our study showed that the methylation level of GSTP1 increased significantly in late-stage compared to the early stage breast carcinomas, suggested that breast cancer patients with GSTP1 promoter hypermethylation may have a biologically aggressive phenotype. Breast cancer is a complex multifactorial disease that is driven by genetic and epigenetic alterations, which cause aberrant gene function [38]. Previous study declared that the genetic variation of GSTP1 affected its Fig. 4 Funnel plot for evaluating publication bias test for GSTP1 methylation and breast cancer risk. The standard error of log (OR) of each study was plotted against its log (OR) Fig. 5 Funnel plot of publication bias test for GSTP1 methylation and breast cancer risk after trim-and-fill method. Logor natural logarithm of OR, horizontal line mean effect size enzymatic activity and detoxifcation ability, thereby contributing to breast cancer susceptibility [10]. Epigenetic alterations including DNA methylation and histone modifications which occur in transformed cells are identified as an early event during tumor development [35,39]. In breast cancer, hypermethylation of promoter CpG islands has been described as the main epigenetic pathway to inactivate genes involved in various aspects of cellular function [30]. It has been reported that GSTP1 is capable of inhibiting tumor growth by its interaction with the c-Jun N-terminal kinase (JNK1) signaling [11], suggesting its role as a tumor suppressor gene. Additionally, because of its detoxifying effects on the anticancer agents, GSTP1 may also affect the sensitivity of breast tumors to chemotherapy, emerged as a novel therapeutic target [7,9].
To our knowledge, this is the first meta-analysis comprehensively performed to assess the relationship between GSTP1 promoter methylation and the incidence of breast cancer. Nevertheless, a number of potential limitations should be acknowledged. First, the effects of potential risk factors such as age, subtype and hormone receptor status on the current results of this meta-analysis could not be eliminated for lack of detailed information. Second, meta-analysis is a secondary analysis and the heterogeneity is the major issue in genetic studies [40][41][42][43]. Of course, our meta-analysis also suffered this issue and we performed subgroup analyses to explore the origin. The results showed that different methylation methods, source of controls and cut-offs positivity of hypermethylation might contribute to heterogeneity. Third, only published clinical studies were selected in this meta-analysis, some unpublished and negative studies may contribute to publication bias. Since studies with statistically positive results were easier to publish than those with negative results, publication bias is inevitable. However, the estimated OR adjusted for publication bias by trim-and-fill method was not substantially changed. Fourth, although our initial search has no language restrictions, only articles published in English and Chinese finally were reviewed. This due to the language ability and the right to use databases of our team, and also might result in some bias.

Conclusions
In conclusion, our meta-analysis suggested a strong association between GSTP1 promoter methylation and breast cancer risk. Thus, aberrant GSTP1 promoter methylation could be a helpful biomarker for the early screening of breast cancer. However, given the limitations elaborated above, high quality studies with larger sample sizes should be employed in further research.