Genetic association meta-analysis: a new classification to assess ethnicity using the association of MCP-1 -2518 polymorphism and tuberculosis susceptibility as a model

Background In meta-analyses of genetic association studies, ancestry and ethnicity are not accurately investigated. Ethnicity is usually classified using conventional race/ethnic categories or continental groupings even though they could introduce bias increasing heterogeneity between and within studies; thus decreasing the external validity of the results. In this study, we performed a meta-analysis using a novel ethnic classification system to test the association between MCP-1 -2518 polymorphism and pulmonary tuberculosis. Our new classification considers genetic distance, migration and linguistic origins, which will increase homogeneity within ethnic groups. Methods We included thirteen studies from three continents (Asia, Africa and Latin America) and considered seven ethnic groups (West Africa, South Africa, Saharan Africa, East Asia, South Asia, Persia and Latin America). Results The results were compared to the continental group classification. We found a significant association between MCP-1 -2518 polymorphism and TB susceptibility only in the East Asian and Latin American groups (OR 3.47, P = 0.08; OR 2.73, P = 0.02). This association is not observed in other ethnic groups that are usually considered in the Asian group, such as India and Persia, or in the African group. Conclusions There is an association between MCP-1 -2518 polymorphism and TB susceptibility only in the East Asian and Latin American groups. We suggest the use of our new ethnic classification in future meta-analysis of genetic association studies when ancestry markers are not available. This new classification increases homogeneity for certain ethnic groups compared to the continental classification. We recommend considering previous data about migration, linguistics and genetic distance when classifying ethnicity in further studies.


Background
Tuberculosis disease (TB) is a major public health problem worldwide. To create new strategies that will improve TB control, we need a better understanding of the biological, environmental, social, and ethnic factors [1]. One promising route is the study of polymorphisms involved in pulmonary TB susceptibility [2,3]. Several human genes have been associated with TB development [4][5][6], including the monocyte chemoattractant protein 1 (MCP-1), also called CCL2. MCP-1 belongs to a group of CC chemokines located in chromosome 17q11.2. MCP-1 protein interacts with chemokine C-C motif receptor 2 (CCR2) to activate and recruit monocytes, macrophages, CD4+ T cells and immature dendritic cells to the site of infection [7][8][9]. The presence of MCP-1 protein in an adequate concentration is important for granuloma formation and M. tuberculosis clearance [10,11].
Although there are more than ten genetic polymorphisms in the MCP-1 promoter and coding region, only the MCP-1 -2518 A/G allele (reference sequence 1024611) is functional and affects gene expression [10]. A substitution from A to G in -2518 position of the promoter region increases the levels of MCP-1. This action decreases the concentration of IL-12p40, which recruits and activates memory/effector Th1 cells, thus impairing long-term protection to intracellular pathogens [10]. Observational studies have shown that MCP-1 -2518 A/G polymorphism is associated with the development of pulmonary tuberculosis (pTB) and could be a potential marker for latent TB and disease severity [3,12]. However, this association is different among countries such as Persia, India, Korea and China, which share continental groups [13,14].
Geographical distribution by continents is the conventional way to assess ethnicity in meta-analysis of genetic association studies. However, population genetics has demonstrated that ethnic composition is related more with genetic distance, migration and linguistic origins rather than continental groups. In terms of ancestry biomarkers, continental grouping relies on markers such as Y-DNA and mtDNA haplogroups and varies within continents [15,16]. As a consequence, conventional classification might introduce bias and increase heterogeneity between and within studies, decreasing the external validity of the results. Thus, it is questionable if the conventional classification is an appropriate proxy for ethnicity.
In order to have a better understanding of the relationship between ethnicity and the susceptibility to infectious diseases such as TB, we evaluated the association between the MCP-1 -2518 A/G polymorphism and pTB susceptibility using a new multi-factorial ethnic classification and compared it with the conventional approach of continental groups. This new classification is based on previous research on genetic distance, migration and linguistic origins [16][17][18][19], which improves the homogeneity of ethnic groups. We believe that our new classification for ethnicity offers a more robust approach to explain susceptibility to disease, and that it can increase the internal validity of genetic studies when ancestry markers are not available.

Search strategy
A literature search was carried out in NCBI database, Scielo and Lilacs to identify genetic association studies between MCP-1 polymorphism and pTB risk prior to December 2013. We used the following MESH terms: (("Polymorphism, Genetic"[Mesh]) AND "Chemokine CCL2"[Mesh]) AND "Tuberculosis" [Mesh]. Mesh term "MCP-1" gave the result CCL2. "Reference sequence 1024611 A/G" gave zero results. Our selection criteria included: 1) studies evaluating the association between MCP-1-2518 A/G and TB risk, 2) observational studies, 3) pulmonary TB, 4) studies performed in adults and children, 4) patients without HIV or cancer, 5) available allelic and the genotype frequencies to estimate an odds ratio (OR), 6) control groups that met Hardy Weinberg Equilibrium, and 7) articles published until December 2013. Studies that did not meet these criteria were excluded. When original articles included more than one study population, we considered each as an independent study. In case of multiple publications on the same study, we included the study with the larger sample and/or the most recently published. The data search retrieved 23 articles. Ten studies were excluded because they were reviews or meta-analyses, or corresponded to pediatric populations, spinal TB, latent TB, HIV positive individuals or data from controls was inaccessible. At the end, 13 studies (7651 cases and 8056 controls) [3,10,[20][21][22][23][24][25][26][27][28][29][30] (Fig. 1) were considered.

Data collection
All articles were separately extracted, reviewed and collated by two independent reviewers who checked for any discordance and reached a consensus in all items. Authors were contacted by email when we needed more information about an article. The following information was extracted for each study: author, year of publication, country of origin, ethnicity, sample size, type of study population, TB definition, allele and the genotype frequencies in cases, controls and methods. The information was systematically reviewed using STROBE and STREGA parameters [31,32].

Ethnic classification
We proposed a new ethnic classification based on previous information about genetic distance, migration and linguistic origins [16,17,[33][34][35] and compared it to the conventional classification. The new ethnic classification considered previous findings about genetic distance [17]. For this purpose, data such as country of origin was extracted from each study.  Table 1. We hypothesized that the new classification creates ethnic groups that have more homogeneity than the groups obtained by the conventional group classification.

Statistical analysis
For each study, the Hardy Weinberg Equilibrium (HWE) was calculated for the controls using X 2 statistic. Genotypes deviated from HWE if two-sided p values were <0.05. Begg funnel plot and Egger's test indicated publication bias if p value was <0.05. Sensitivity analysis was performed by removing one study at a time to assess the stability of the meta-analysis results.
To prove our hypothesis, we assessed heterogeneity and the magnitude of association for each ethnic group. We assessed heterogeneity by using the χ 2 based Q test and I 2 statistic. P values less than 0.01 were considered significant for heterogeneity. To assess the magnitude of association (pooled OR), in the presence of homogeneity, we used a fixed effects model (inverse variance weighted). Otherwise, we used a random effects model (DerSimonian and Laird, D + L). Pooled OR for the association between MCP-1 -2518 A/G polymorphism and pTB risk was determined in three steps. First, we did an allelic comparison (G vs. A) to determine the pooled OR in the overall data and by ethnic subgroups. Second, using our new ethnic classification, we analyzed four genotype models: a) recessive (GG vs. AG + AA), b) homogenous co-dominant (GG vs. AA), c) heterogeneous co-dominant GA vs. AA) and c) dominant (GG + GA vs. AA). Third, we compared these results to those obtained from the analysis using the conventional classification. Odds ratio estimates were considered significant if P was <0.05, and were expressed using a 95 % confidence interval (CI). When analyzing by ethnicity, we used the groups that had ≥1 degree of freedom. For our analysis, the wild type allele was A, and the risk allele was G. We did not adjust our model for environmental effects. The statistical analysis was performed using STATA 11.0. (STATA Corp, College Station, TX, USA).

Results
The conventional ethnic analysis found heterogeneity in the three continental study groups for both allelic and genotype analysis. Using our new classification, we found homogeneity for South Asia (India) and West Africa, which were further analyzed with a fixed effects model. We could not improve homogeneity within the rest of the ethnic groups and used a random effects model for their analysis. According to the Begg's funnel plot and Egger's test, we did not find any bias in the analysis of the entire group (t = 1.76, P = 0.1; Fig. 2). Sensitivity analysis did not find any prominent effect of each individual   (Fig. 4). We did not find any association for any of the African groups.

MCP-1 -2518 A/G genotypes and pTB susceptibility
The

Ethnic groups and heterogeneity
We found heterogeneity within the ethnic groups from the conventional classification (I 2 73.1 %, P <0.01, for Africa; I 2 83.8 %, P <0.01, for Asia; I 2 90.7 %, P <0.01, for South America). The new ethnic classification showed homogeneity for West Africa and South Asia (I 2 0 %, P = 0.3; I 2 0 %, P = 0.5, respectively). We found heterogeneity within Arabia, East Asia and Latin America (I 2 93.5 %, P <0.01; I 2 88.7 %, P <0.01; I 2 91.6 %, P <0.01, respectively). We could not obtain results for South Africa and Persia, since there was only one study in each group.

Discussion
We found an association between the MCP-1 -2518 polymorphism and tuberculosis susceptibility in East Asian and Latin American populations [13,14,36]. Previous metaanalyses try to extrapolate this association to the Asian continent. However, since there is ethnic variability within each continent, we cannot generalize this conclusion to every  ethnic group. In this way, our meta-analysis groups study populations by using information about migration and linguistics to make ethnic groups more similar. Using this method, we found that an association does not apply to every country in the same continent.
Our new ethnic classification creates ethnic groups (e.g. West Africa and South Asia) with countries sharing similar characteristics. This new classification must be further evaluated with new studies related to genetic susceptibility for infectious and noninfectious diseases.
Regarding TB susceptibility, our new classification, in contrast to the conventional classification, helped to clarify that the association between MCP-1 -2518 A/G polymorphism and pTB is specific for certain populations such as East Asia and Latin America. To our knowledge, this is the first meta-analysis that uses a model of genetic susceptibility for pTB to assess if a new ethnic classification based on previous findings about genetic distance, migration and linguistic origins, improves homogeneity within each ethnic groups [13]. Thus, we propose our new classification as a good proxy when genetic markers are not available [17,[37][38][39][40][41][42].
Previous meta-analyses that use a continental group classification found an association between the MCP-1-2518 A/G polymorphism and pTB, which is significant for Asia and South America [13,14]. However, these ethnic groups include countries that are different in terms of ancestry and therefore genetic susceptibility. Our new classification helps to improve homogeneity in South Asia and West Africa. However our new classification does not help us with homogeneity in East Asia and Latin America, where we found association between polymorphism MCP-1 -2518 G allele and pTB. Failure to reach homogeneity could be explained because of gene-gene or gene-environmental interactions. It has been reported that people carrying polymorphism MCP-1 -2518 and MMP-1 -1607 have a higher risk to develop severe TB [12]. The high frequency of G allele observed in cases compared to controls in both East Asia and Latin America might support the hypothesis of a similar ancestry between these two groups [43]. New and traditional ethnic classification to assess TB susceptibility in MCP-1 -2518 G allele carriers. We observe that the new classification finds a significant association only for the East Asian and Latin American groups. In South Asia (India), where there is homogeneity between studies, we can rule out that the polymorphism is associated with pulmonary TB Recent studies from Africa show that the G polymorphism is not common among this population [21,24]. Human population started in Africa, which means it is the oldest population, and therefore it has had the opportunity to accumulate genetic changes, such as the accumulation of -2518 MCP-1 A allele in its inhabitants that conferred protection and made it possible to adapt to hazardous environmental conditions [44]. We also have to consider other factors influencing TB susceptibility such as malnourishment, socioeconomic, environmental and health factors. The homogeneity found in West Africa cannot be completely explained in our study. We did not assess homogeneity in South Africa, since we only had one study population [22].
To deal with heterogeneity in Asia, we considered three groups: East Asia, South Asia and the Middle East [37][38][39]. The Asian population started from an "out of Africa" migration 50,000 years ago. It originated from two main migratory routes. The first one moved towards South Asia (India), and the second one to East Asia. Later, Central Asia was populated by Eurasian descendants. This is why we grouped Chinese and Korean populations under the East Asia group, India under the South Asia, and considered Persia under Persia. Also, these study populations have social, educational and mating habits that have that are particular to each group [16,33,34,45]. Our classification groups two similar study populations from India under South Asia. Thus in this setting, it is unlikely that pTB susceptibility is due to the presence of MCP-1 -2518 G polymorphism. In contrast to South Asia, we found an association between this polymorphism and pTB in East Asia where we also found heterogeneity. Interestingly, India (South Asia) and China (East Asia) accounted together for more than 40 % of TB cases worldwide in the last decade [46]. However the implementation of TB control strategies in China has helped decrease prevalence by 50 %, mortality rates by almost 80 % and TB incidence rates by 3.4 % per year between 1990 and 2010 [47]. Thus, even though there is a better control of TB in China, genetic factors might be playing an important role in the development of this disease. In contrast, India maintains its high incidence for the last 10 years, which might be due to a lack of social and public health control rather than genetic factors. It is difficult to assess homogeneity within Persia [48,49] because we only had one study population. In further meta-analyses about genetic susceptibility we recommend to give a special consideration to Central Asian countries since they share European ancestry and therefore different genetic markers compared to East and South Asia [33].
Latin American ethnic groups that originated from a Han Chinese migration to South America 3000 years ago share HLA markers with this population [50]. This similarity might also explain similar frequency of MCP-1 -2518 G allele and other genetic markers between East Asians and Latin Americans. Since Mexico and Peru share migration, common history, language routes and admixture indexes [40,[51][52][53], we decided to maintain them in the same ethnic group as previous meta-analyses. However, we consider that for Latin America, we should consider two groups: one of Andean and another of European origin.
The limitations in our study are very common to metaanalyses about genetic association studies. We could not consider environmental and genetic factors that influence this association because this information was not found in the original articles. Thus, for research in multifactorial diseases such as TB, we strongly recommend future studies to include information about malnourishment, socioeconomic factors, BCG and TST status, which could also help to control for heterogeneity.
We obtained homogeneity within South Asia and West Africa, where we can rule out that MCP-1 -2518 polymorphism is associated to susceptibility. However, despite tuberculosis susceptibility found in Latin America and East Asia due to MCP-1 -2518 polymorphism, the populations within each group are still genetically different.
Genetic association studies in populations from Persia, South Africa, South Asia, East Asia and the Americas, where infectious diseases represent a public health problem, will help assess heterogeneity in order to understand the role of ethnicity in genetic susceptibility to these diseases. In the absence of an adequate classification that groups similar genetic characteristics, suitable for understanding genetic susceptibility, our new classification might be a potential proxy for ethnic classification in meta-analysis of genetic association studies when genetic markers are not available.

Conclusions
In summary, using this novel approach, we found an association between the MCP-1 -2518 polymorphism and pTB susceptibility, specifically in Latin American and East Asian populations not detected by using conventional classification. We encourage the use of our new ethnic classification in further genetic association studies for infectious and non-infectious diseases.

Competing interests
The authors do not disclose any financial and non-financial competing interests.