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Unraveling the Regulatory Mechanisms Underlying Tissue-Dependent Genetic Variation of Gene Expression


It is known that genetic variants can affect gene expression, but it is not yet completely clear through what mechanisms genetic variation mediate this expression. We therefore compared the cis-effect of single nucleotide polymorphisms (SNPs) on gene expression between blood samples from 1,240 human subjects and four primary non-blood tissues (liver, subcutaneous, and visceral adipose tissue and skeletal muscle) from 85 subjects. We characterized four different mechanisms for 2,072 probes that show tissue-dependent genetic regulation between blood and non-blood tissues: on average 33.2% only showed cis-regulation in non-blood tissues; 14.5% of the eQTL probes were regulated by different, independent SNPs depending on the tissue of investigation. 47.9% showed a different effect size although they were regulated by the same SNPs. Surprisingly, we observed that 4.4% were regulated by the same SNP but with opposite allelic direction. We show here that SNPs that are located in transcriptional regulatory elements are enriched for tissue-dependent regulation, including SNPs at 3′ and 5′ untranslated regions (P = 1.84×10−5 and 4.7×10−4, respectively) and SNPs that are synonymous-coding (P = 9.9×10−4). SNPs that are associated with complex traits more often exert a tissue-dependent effect on gene expression (P = 2.6×10−10). Our study yields new insights into the genetic basis of tissue-dependent expression and suggests that complex trait associated genetic variants have even more complex regulatory effects than previously anticipated.


Published in the journal: . PLoS Genet 8(1): e32767. doi:10.1371/journal.pgen.1002431
Category: Research Article
doi: https://doi.org/10.1371/journal.pgen.1002431

Summary

It is known that genetic variants can affect gene expression, but it is not yet completely clear through what mechanisms genetic variation mediate this expression. We therefore compared the cis-effect of single nucleotide polymorphisms (SNPs) on gene expression between blood samples from 1,240 human subjects and four primary non-blood tissues (liver, subcutaneous, and visceral adipose tissue and skeletal muscle) from 85 subjects. We characterized four different mechanisms for 2,072 probes that show tissue-dependent genetic regulation between blood and non-blood tissues: on average 33.2% only showed cis-regulation in non-blood tissues; 14.5% of the eQTL probes were regulated by different, independent SNPs depending on the tissue of investigation. 47.9% showed a different effect size although they were regulated by the same SNPs. Surprisingly, we observed that 4.4% were regulated by the same SNP but with opposite allelic direction. We show here that SNPs that are located in transcriptional regulatory elements are enriched for tissue-dependent regulation, including SNPs at 3′ and 5′ untranslated regions (P = 1.84×10−5 and 4.7×10−4, respectively) and SNPs that are synonymous-coding (P = 9.9×10−4). SNPs that are associated with complex traits more often exert a tissue-dependent effect on gene expression (P = 2.6×10−10). Our study yields new insights into the genetic basis of tissue-dependent expression and suggests that complex trait associated genetic variants have even more complex regulatory effects than previously anticipated.

Introduction

It has become clear that human genetic variants, such as single nucleotide polymorphisms (SNPs), can in cis affect the expression of nearby genes [1], [2]. Many loci exist that contain genetic variants that affect gene expression (expression quantitative loci, eQTL, usually assessed by investigating single nucleotide polymorphisms (SNPs) and expression probes that are within 250 kb up to 1 Mb apart). These cis-eQTL analyses have been performed in many different human tissues and cell types, including lymphoblastoid cell lines (LCL) [3], [4], liver [5][7], blood [8], [9], brain [10], [11], adipose tissues [6], [8], skin [12], [13] and primary fibroblasts [12]. However, considerable heterogeneity of cis-eQTL effects is possible between different tissues: A recent study reported that the proportion of heritability due to gene expression attributable to cis-regulation differs between tissues (37% in blood and 24% in adipose tissue) [14]. By comparing the overlap of significant cis-eQTL at a predefined threshold, estimates on the tissue-dependence of cis-eQTL were between 30% (liver, adipose tissues) and 70–80% (LCLs, fibroblasts, T cells) [8], [9], [15], [16]. However, due to statistical power issues, it is likely that the tissue-dependency of cis-eQTL has been overestimated by studies solely assessing the overlap of cis-eQTL between tissues based on a certain threshold. Realizing this problem, Ding et al. used a refined statistical method to estimate the percentage of overlap by adding a power parameter to the model [12]. They reported that only 30% of cis-eQTL in LCLs were not shared with fibroblast cis-eQTL. Similarly, a recent study by Nica et al. [13] examined the tissue-dependence of cis-eQTL in three human tissues (LCL, skin and fat) in a continuous manner by quantifying the proportion of overlap of cis-eQTL from the enrichment of low P-values. They observed that 29% of cis-eQTL appear to be exclusively tissue-dependent, and also observed that the effect sizes of 10–20% of the cis-eQTL present in multiple tissues differ per tissue type. These observations are in line with a large-scale transcriptomic analysis of 46 human tissues, which found that while only 6.0% of genes were ubiquitously expressed across all the assessed tissues, 3.1% genes were only expressed in a single tissue [17].

To gain a better understanding of this subtle regulation of tissue-dependent regulation and to address the question of how genetic variants mediate tissue-dependent expression, we compared cis-regulation between whole peripheral blood from a large cohort of 1,240 individuals and four smaller primary human tissues (liver, subcutaneous adipose tissue (SAT), visceral adipose tissue (VAT) and skeletal muscle) obtained from a set of 85 subjects. We first applied a robust sampling procedure to estimate accurately how often genes showed different cis-eQTL effects between tissues. We then investigated in what way genes are differently associated with SNPs in different tissues. Finally, we assessed various functional properties for the SNPs involved in tissue-dependent cis-regulation and their association with complex traits.

Results

Cis-eQTL Mapping in Five Primary Tissues

For this study, we collected data for four different tissues from a set of 85 unrelated obese Dutch subjects. We successfully collected data on 74 liver samples, 62 muscle samples, 83 subcutaneous adipose tissue (SAT) samples and 77 visceral adipose tissue (VAT) samples (for 48 individuals all four tissues were available). The fifth tissue, blood, was collected from a different group of 1,240 unrelated Dutch individuals (Table S1). The gene expression levels in all five tissues were profiled using the same Illumina HumanHT12 v3 platform (see Materials and Methods). After normalization, we further removed strong expression differences between these tissues by removing the 50 principal components from this dataset and using the residuals for further analysis (described in [18] and Materials and Methods, Figure S1). We first performed cis-eQTL analysis in each of these datasets separately, by testing the correlation between SNPs and probes that were mapping within 1 Mb distance. At a false-discovery rate (FDR) of 0.05 level, we identified a non-overlapping set of 195,078 probe-SNP pairs that were significant in at least one of the tissues under study: 4,700 probe-SNP pairs were significantly associated in liver, 7,161 pairs significantly in SAT, 5,323 pairs significantly in VAT, 1,971 pairs significantly in muscle, and 190,278 pairs significant in blood (Figure S2). Owing to the much larger sample size, 182,569 probe-SNP pairs (93.6%) were solely detected in blood, while only 601 probe-SNP pairs (0.31%) were significant in each of the five different tissues (Figure S3). Although a previous study showed that the heritability of gene expression levels are higher in blood (37%) compared to adipose tissue (24%) [14], we believe that the large difference in the detected probe-SNP pairs between blood and non-blood tissues is due to statistical power issues that result from substantial sample size differences. As we had initially run cis-eQTL analyses in each of the tissues separately, we subsequently conducted a weighted Z-score meta-analysis across the four non-blood tissues and detected 23,878 probe-SNP pairs at FDR of 0.05. Out of these, 23.2% (5,550 out of 23,878 probe-SNP pairs) had not been identified in any of the single-tissue analyses (Figure S4). In total, the single-tissue analyses and meta-analysis yielded a non-overlapping set of 200,629 significant probe-SNP pairs, corresponding to 103,968 unique expression altering SNPs (eSNPs) and 11,618 probes (eProbes) that represent 8,561 unique genes (eGenes) (Figure S2).

Cis-eQTL Effects Differ per Tissue Type

To assess the tissue-dependency of the cis-eQTL, we compared the Spearman correlation of each probe-SNP pair between tissues. However, due to the small sample sizes of the non-blood datasets we had very limited statistical power to determine whether there were cis-eQTL effect differences between non-blood tissues. We therefore confined ourselves to comparisons between the large blood dataset and each of the smaller non-blood tissues. To correct for sample size differences, we employed a resampling procedure, permitting us to derive an empirical distribution of association Z-scores (calculated based on the Spearman correlation) of each probe-SNP pair in blood of the same sample size as in non-blood tissues (see Materials and Methods; Figure S5). We observed that 18,456 pairs (9.2% of 200,629 probe-SNP pairs) showed a significantly different Z-score between blood and at least one of the non-blood tissues at P<6.23×10−8 (corresponding to a conservative Bonferroni-corrected P<0.05), implying a discordant association between blood and non-blood tissues. The remaining 182,173 probe-SNP pairs, which we called “concordant association”, had similar association Z-scores between the tissues under study (Figure S2). The “discordant associations” accounted for 15.4% of the eSNPs (15,974 out of 103,968 eSNPs), 28.7% of the eProbes (3,330 out of 11,618 eProbes), and 34.1% of the unique eGenes (2,919 out of 8,561 eGenes) (Table S2 and Figure S2). We further assessed for each probe-SNP pair, whether the discordance was detected between blood and multiple non-blood tissues, or only between blood and one specific non-blood tissue. We observed that 14,388 probe-SNP pairs (78.0% of the 18,456 discordant probe-SNP pairs) only showed a discordant effect between blood and one specific non-blood tissue. Only 125 probe-SNP pairs (corresponding to 31 eProbes) showed a discordant association in all four comparisons, suggesting similar regulation in the four non-blood tissues but markedly different regulation in blood (Figure S6). As such these results reveal there are considerable differences in the genetically determined regulation of gene expression between liver, SAT, VAT and muscle tissues, even though the RNA from these tissues had been derived from the same individuals at was collected at exactly the same time.

To ensure that our sampling procedure was robust, we used the same procedure to assess how often our method incorrectly concluded that a probe-SNP Spearman correlation differed between two independent eQTL datasets in the same peripheral blood tissue: We used the 1,240 blood samples as discovery set and used an independent set of 229 blood samples as validation whose expression was profiled using Illumina H8-v2 chips, [18], [19], see Methods and Materials. In this analysis, our method incorrectly deemed that 0.45% of the probe-SNP pairs showed a significant difference at the previously used P<6.23×10−8 level (Figure S7). In our comparisons between blood and non-blood tissues we had observed that 9.2% of the probe-SNP pairs showed a discordant effect, which is substantially higher and indicates that the number of discordant associations that we identified when comparing different tissues are not expected by chance (Fisher's exact test: OR = 20.6 and P<10−300). We also assessed whether imputation accuracy differences between datasets might confound some of the results, but did not find evidence this to be the case (see Materials and Methods).

Properties of eSNPs

For the significant 200,629 probe-SNP pairs, we observed that for 146,480 pairs (73.0%) the eSNPs were located within 250 kb distance of the eProbe while 54,149 probe-SNP pairs (27.0%) mapped between 250 kb and 1 Mb apart. Consistent with a previous study [15], we observed that eSNPs at a larger distance from the probes tend to have smaller effects (Figure S8). However, we realize that due to extensive LD many different SNPs are usually significantly correlated with one single cis-eQTL probe. To address this, we performed step-wise conditional analyses in each tissue type to ascertain whether there were multiple SNPs that independently affected the expression levels of the same probe. We observed this for 26.8% of the eProbes in the large blood dataset (Table S3), (where for 2,794 out 10,443 eProbes we had detected multiple independent eSNPs): We observed that the secondary, tertiary and quaternary eSNPs usually map further away from the probe (Wilcoxon test P = 2.25×10−66, Figure S9), potentially reflecting some regulatory elements such as enhancers that usually reside further away from genes. In the non-blood tissues, we lacked statistical power to detect many secondary and tertiary effects (Table S3).

Interestingly, there was a very high overlap between the discordant eProbes (detected in our comparison across tissues) and the eProbes with multiple independent effects in blood (detected in the aforementioned analysis that solely used blood samples). Out of the 10,443 eProbes in blood, 2,528 eProbes had discordant association and 7,915 eProbes had concordant association. We observed that 47.5% of the discordant eProbes had multiple independent eSNPs present in blood (1,202 out of 2,528); whereas only 20.1% of the concordant eProbes had multiple independent eSNPs (1,592 out of 8,219, Fisher's exact test P = 3.85×10−81). This observation suggests that for eProbes: 1) different independent eSNPs can exist and 2) these independent eSNPs can exert an effect in one tissue while they do not exert an effect in another tissue.

We subsequently analyzed the most significant eSNP per eProbe per tissue and the top eSNP per eProbe from the meta-analysis of four non-blood tissues. In total, we ended up with 13,603 probe-SNP pairs (12,549 top eSNPs, that were affecting 11,575 probes pairs) these six analyses. Among them, 2,612 probe-SNP pairs (19.2%) showed a discordant effect among tissues at P = 6.23×10−8 level (genome-wide test level), accounting for 2,466 (19.7%) unique eSNPs.

We found that the top eSNPs with discordant effect had a significantly higher minor allele frequency (MAF) than the concordant top eSNPs (Wilcoxon test P = 8.27×10−21). The eSNPs at a smaller distance from the eProbe (≤250 kb) were more likely to show a discordant effect compared to the eSNPs at larger distance (250 kb–1 Mb distance, OR = 1.62, P = 3.6×10−22, Figure S10). Although we acknowledge that the top eSNPs do not necessarily reflect the true causal variants, we annotated the functional properties of the top eSNPs to understand the potential roles of the eSNPs (irrespective of whether these reflect concordant or discordant eProbes). We observed that the most of the eSNPs were located in intragenic regions (67.0%) and intronic regions (14.9%), where their function often remains undetermined. Interestingly, eSNPs with discordant effect were (compared to concordant eSNPs) significantly enriched for synonymous-coding SNPs (Fisher's exact P value 9.9×10−4), and more often mapped in the 3′ and 5′ untranslated regions (UTRs, Fisher's exact P values 1.84×10−5 and 4.7×10−4, respectively) (Figure 1).

Fig. 1. Functional Properties of eSNPs with tissue-dependent effect and concordant effect.
Functional Properties of eSNPs with tissue-dependent effect and concordant effect.
The bar plot shows the frequency of the eSNP per function property. The eSNPs were annotated using the web-based tool of SNP Annotation and Proxy Search (SNAP; http://www.broadinstitute.org/mpg/snap/), based on the HapMap CEU population panel (release 22) and genome build 36.3. The asterisks indicate the significance of Fisher's exact test by comparing the eSNPs with concordant effect and with discordant effect, as given in the legend.

As shown before, we observed that SNPs, associated with complex traits and diseases, are more likely to be eSNPs [2], [6], [8], [18], [19]. We subsequently analysed 1,954 trait-associated SNPs (at P<5×10−8, retrieved from the GWAS catalog per 16 September 2011) [20] and observed that 907 trait-associated SNPs (46.4%) were eSNPs. Of these, 261 trait-associated eSNPs (28.7%) showed discordant effects on gene expression, which is significantly higher than what we observed for all 103,968 trait- and non-trait-associated eSNPs (15.4% discordant, Fisher's exact test P = 1.10×10−33) and also significantly higher than if we compare this to only the 12,549 top eSNPs (19.7% discordant, Fisher's exact test P = 2.6×10−10).

Four Categories of Tissue-Dependent Cis-Regulation

As we have shown above, discordant eProbes are more likely to be influenced by multiple independent eSNPs. However, solely assessing the discordance of a single SNP-probe pair does not provide an extensive landscape of the tissue-dependent genetic determinants of gene expression. To gain further insight into this, we created ‘association profiles’ for the discordant eProbes and compared these across tissues. An association profile refers to the association Z-scores of all tested SNPs within 1 Mb distance of the eProbe under study (see Materials and Methods), and takes into account multiple SNPs and linkage disequilibrium. We created such association profiles for 2,007 discordant eProbes 52 (521 eProbes from liver, 708 eProbes from SAT, 526 eProbes from VAT, and 252 eProbes from muscle, Figure S2).

Upon inspection of these association profiles for the discordant eProbes, we identified four main different categories of tissue-dependent genetic regulation of gene expression. If the association profiles for one single eProbe did not correlate at all between two tissues, we further checked whether the eProbe was significant in both tissues: If the probe had a significant association in one tissue but not in the other, we deemed this “specific cis-regulation”. If instead the eProbe was significant in both tissues, but was associated to different (unlinked) eSNPs in the different tissues, we deemed it “alternative cis-regulation” between tissues. For those association profiles where two tissues showed a correlation, we checked the direction and the effect size of allelic effect on gene expression. If the allelic direction was the same and the effect size was different, we concluded the eProbe belonged to the category “different effect size”. If the allelic direction was instead opposite, the probes had tissue-dependent regulation with an “opposite allelic direction” (see Materials and Methods). We discuss each of these four categories in detail below and in Figure 2 and Figure 3.

Fig. 2. cis-regulation of gene expression between tissues.
<i>cis</i>-regulation of gene expression between tissues.
The associated probe-SNP pairs were classified to be concordant or discordant between tissues. The small pie plot shows the proportion of probes that have only concordant association (red part) or at least one discordant association (blue part). The probes with discordant association were under tissue-dependent regulation and we characterized four different mechanisms: specific regulation, alternative regulation, different effect size and opposite effect sizes. Their proportions are shown in the large blue pie plot. The concordant cis-regulation and the four different mechanisms are illustrated by the correlation between SNP genotypes (AA, AG and GG) and gene expression levels in two tissues: brown dots represent the expression of a gene in tissue 1 and purple dots the expression of a gene in tissue 2.

Fig. 3. Case examples for tissue-dependent cis-regulation.
Case examples for tissue-dependent <i>cis</i>-regulation.
(A) The liver-specific regulation of the SORT1 gene. (B) The alternative regulation of the TMEM176A gene in blood and liver. (C) The cis-regulation for the MGMT gene had different effect sizes in blood and SAT. (D) The cis-regulation for the DDT gene show opposite allelic direction between blood and liver. For each gene, the left panel shows the cis-eQTL association profile in the corresponding tissue (liver or SAT, in blue) vs the association profile in blood (red). The x-axis is the genome position based on genome build 36.3 (in Mb). The y-axis at the left is the association strength in terms of Z-score. The Z-score in blood has been weighted by the square root of the sample size, corresponding to the compared tissue. The dashed green line indicates the significance level of association at FDR 0.05. We use the absolute Z-scores to show the association in (A–C), but use the Z-scores in (D) for a better illustration of allelic direction. We assigned the association Z-scores in blood a negative value. If the allelic direction in SAT is the same as that in blood, the Z-score in SAT is negative too; otherwise, the Z-score in SAT is positive. The black line shows the recombination rate at this locus based on the HapMap II CEU panel and the scale is indicated on the right-hand y-axis. The green line with arrow at the bottom shows the genome position of the gene and the arrow indicates the transcription direction. The right panel shows the correlation of the Z-scores between two tissues. The r-value indicates the correlation coefficient of the Pearson correlation.

Specific regulation

Specific cis-regulation refers to a gene that is cis-regulated in only one specific tissue. We found this type of regulation is a common phenomenon as it accounted for on average 33.2% of the discordant eProbes (Figure 2). One well-established example is the SORT1 gene at the 1p13 cholesterol locus, to which SNPs map that affect low-density lipoprotein cholesterol (LDL-C) and the risk of myocardial infarction (MI) in humans [21], [22]. Recently, it was shown that the functional variant rs12740374 alters the binding site for C/EBP transcription factors and consequently alters the hepatic expression of the SORT1 gene [23]. Our data replicated this specific cis-regulation in liver (Figure 3A). The association Z-score for rs12740374 with SORT1 expression variation in liver was 8.24 (N = 74, P = 1.41×10−15) but in blood we observed no effect (Z-score = 0.07, N = 1,240, P = 0.8), nor did we observe any associations in SAT, VAT or muscle, and the association profiles for this gene show no correlation between different tissues (all spearman correlation P values>0.39). Thus, in our data, rs12740374 only exerts an effect on SORT1 gene expression in liver, although we did observe that SORT1 was expressed abundantly in all tissues.

Alternative regulation

Alternative regulation between tissues refers to a gene that is cis-associated with a SNP in a particular tissue and associated with a different, independent SNP in another tissue. Such an alternative cis-regulation is also a common phenomenon, as we found it applied to on average 14.5% of the probes with tissue-dependent regulation (Figure 2). One particular example is the trans-membrane gene TMEM176A, also known as hepatocellular carcinoma-associated antigen 112. The expression of TMEM176A was associated with intronic SNP rs714885 in liver (N = 74, P = 5.7×10−6) but with the 19.5 kb upstream SNP rs6464104 in blood (N = 1,240, P = 5.07×10−132) (Figure 3B). These two SNPs are unlinked variants (r2 = 0.002 and D′ = 0.054 based on the HapMap phase II CEU panel). We observed the same alternative association for different probes of TMEM176A in an independent liver eQTL dataset (profiled using a custom ink-jet microarrays [7] and in the aforementioned independent blood eQTL dataset that was profiled using Illumina HumanRef-8 v2 BeadChips) (Table S4) [18], [19]. This clearly shows that 1) multiple, unrelated variants can sometimes affect exactly the same gene, and 2) these independent variants sometimes only exert an effect on the gene expression in a particular tissue.

Different effect size

The different effect size refers to a common phenomenon that a gene is associated with the same SNP with alleles that have the same direction of effect but with a different magnitude in different tissues (Figure 2). For eProbe that showed this, we observed a significantly positive correlation between the association profiles of the tissues. We observed it applies to on average 47.9% of the probes that show tissue-dependent regulation (Figure S2), in line with a previous report [13]. One example is the O-6-methylguanin-DNA-methyltransferase (MGMT) gene that plays an important role in DNA repair and which suppresses tumor development [24]. We observed a cis-eQTL for MGMT across each of the five tissues. However, the effect size in blood was substantially smaller than that in SAT tissues (Figure 3C).

Opposite allelic direction

Surprisingly, we observed that some genes were associated with the same SNPs in different tissues but with alleles having an opposite effect on the gene expression between tissues. For a probe under this regulation, we then also observed a strong negative correlation between its association profiles across different tissues. This “opposite allelic direction” mechanism accounted for on average 4.4% of the probes under tissue-dependent regulation (Figure 2), which is much less common than the three previous mechanisms. However, this is still much more often than would be expected by chance, as determined by a comparison between two blood datasets in which we found the allelic directions were nearly always identical (Figure S7). One striking opposite allelic direction was observed to D-dopachrome tautomerase (DDT), which showed completely opposite effects between blood and liver (Figure 3D). Consistently, we found this opposite effect in the independent liver [7] and blood dataset,(H8v2), even when different probes were assessed. The minor allele rs5751777-C was associated with higher expression in liver (P = 9.95×10−22 in the discovery set and P = 2.86×10−211 in the validation set), but with lower expression in blood (P = 3.98×10−119 in the discovery set and P = 4.37×10−24 in the validation set) (Table S5). Strikingly, this opposite allelic direction was also observed when comparing liver with SAT, VAT and muscle, tissues that were all obtained from exactly the same set of individuals (Figure S11).

Another notable gene with an opposite allelic direction is ORMDL3. Although its function remains unclear, genetic variants near ORMDL3 are associated with various immune-related diseases, including asthma, type 1 diabetes, Crohn's diseases, ulcerative colitis and primary biliary cirrhosis [25][29]. ORMDL3 had a genome-wide significant cis-eQTL in blood and its association in SAT was showing near-genome-wide significance (Figure S12). All disease-associated SNPs in this locus showed association in cis with the expression level of ORMDL3 (Table S6), including the functional variant rs12936231 that has been implicated to play a causal role in chromatin remodeling [30]. The risk alleles for asthma and preventive alleles for other autoimmune diseases showed consistent up-regulation in blood (and were also reported in LCLs) [25], [30]. However, to our surprise, the effect in SAT was completely reversed, leading to down-regulation.

Although we have only provided a few examples here, these observations indicate that conclusions drawn about mechanistic up- or down-regulation from a single tissue cannot necessarily be translated to other tissues, as they may sometimes lead to completely different conclusions depending on the tissues studied. In the supplementary material (Tables S7, S8, S9, S10 and Figures S13, S14, S15, S16), we have summarized the observed tissue-dependent regulation for 156 genes that have been reported to be associated with complex traits at P = 5×10−8 (based on the genes, mentioned in the Catalog of Published Genome-wide Association Studies, as of 16/09/2011). Some of these plots also show that the genetic regulation of gene expression is sometimes even more complicated than what we have described here: some genes can have multiple cis-eQTL that were either shared or specific to the tissues, e.g, the association of MTMR3 gene that was associated with lung cancer [31], Nephrophaty [32], and inflammatory bowel disease [33], [34] (Figure S17).

The four categories of tissue-dependent cis-regulation we have observed can be explained by two molecular models: 1) the tissue-dependent use of the same causal variant, i.e., the same eSNPs tag the same causal variant that is activated differentially by tissue-dependent factors; 2) the tissue-dependent causal variants, i.e., the same or different eSNPs tag different causal variants upon the tissues under study. The extent of the linkage disequilibrium (LD) between the causal variants and tag eSNPs, and the direction of effect of the regulatory factors (e.g., stimulating or suppressing the expression) and the size of their effects could lead to the observations of different categories (Figure 4).

Fig. 4. Molecular models of tissue-dependent cis-regulation.
Molecular models of tissue-dependent <i>cis</i>-regulation.
The observed tissue-dependent cis-regulations can be explained by two molecular models: (A) the tissue-dependent use of the same causal variants, or (B) the use of tissue-dependent causal variants. The ovals indicate the two regulatory factors (e.g., transcription factors) that play regulatory roles in different tissues (brown in tissue 1 and purple in tissue 2). These factors can recognize the same or different cis-elements (the yellow region). The genetic variants are shown as SNPs with A/G alleles. The SNPs in red are causal variants and the SNPs in blue are tag SNPs. The red line between them indicates the linkage disequilibrium. The arrows indicate the effect of regulatory factors, here the up arrows represent expression stimulators and the down arrows expression suppressors. The size of the arrows indicates the size of the differences between the expression of A and G alleles, i.e., the cis-eQTL effect size.

Discussion

Gene expression levels are partly determined by genetic variation, and eQTL mapping in different cell types and tissues has identified many cis-eQTL. However, the effect of cis-eQTL is strongly dependent upon the studied tissue. In this study, we compared the genetic architecture of gene expression regulation in blood and four non-blood primary tissues. We detected that the majority (71.3%) of the detected probes under genetic control (eProbes) show a concordant association across tissues. However, the remaining 28.7% of the eProbes show discordant, tissue-dependent regulation. Strikingly, many of those discordantly associated eProbes are affected by multiple, independent eSNPs. We followed up the genes under tissue-dependent regulation and identified four different mechanisms: specific regulation, alternative regulation, different effect size, and opposite allelic direction. We are the first to provide a comprehensive landscape of the different mechanisms of tissue-dependent cis-regulation. Of the four mechanisms identified, the opposite allelic direction mechanism, where alleles can have opposing effects on gene expression between tissues is of particular interest: Although this mechanism is less common than the other three, it has important implications for inferring the transcriptional effects of alleles from other tissue data, especially on the susceptibility risk alleles for complex diseases. The use of different tissues could result in completely the opposite conclusion! This finding highlights the great importance of investigating disease-relevant tissues in order to correctly characterize the functional effects of disease-associated variants.

We observed that SNPs at various transcriptional regulatory regions more often than expected exert tissue-dependent regulation, although most of the eSNPs were located at intergenic and gene intronic regions where functions remain undefined. However, we must emphasize that the causal variants remained undefined. Furthermore, because of the LD structure, although the same eSNPs can be associated with the expression of the same gene in different tissues, this does not necessarily mean that the same regulatory variants act in the different tissues. We have proposed two molecular models and suggested that tissue-dependent cis-regulations can be explained by the tissue-dependent use of the same causal variants or by the use of different tissue-dependent causal variants. Further fine-mapping and functional analyses are needed to identify the causal variants and to understand how they are used in different tissues due to the limited resolution of cis-eQTL mapping: It is known that the size of regulatory cis-elements generally is only a few base pairs (i.e., the binding sites of transcription factors or microRNAs), whereas the size of linkage disequilibrium blocks is generally in a range of 10–100 kb [35]. Furthermore, as the molecular models that we have proposed are quite simple, we cannot exclude other molecular mechanisms acting in these processes, e.g., the competition of different regulatory factors and binding sites in different tissues, or the role of tissue-specific methylation [36], [37] and chromatin remodeling [38], etc.

It is well known that trait-associated SNPs are more likely to have effects on gene expression but, to our surprise, we found that they are also more likely to exert tissue-dependent effects. This observation adds an extra layer of complexity to complex traits.

We acknowledge that our study has some limitations: We compared cis-regulation between peripheral blood and four rather small non-blood tissues. We lacked statistical power to compare the cis-regulations between two non-blood tissues well. Secondly, the identified discordant eQTLs are determined by the limited tissues that we studied Thirdly, although we corrected for substantial expression differences across samples by employing principal component analysis, it is still possible that some of the observed tissue-dependent cis-regulation can be due to the tissue heterogeneity (i.e. different proportions of cell types per tissue). Likewise it is also possible that some of the identified discordant cis-eQTL could be due to differences in the base-line expression between tissues. However, we observed this to be the case for both concordant and discordant cis-eQTL when investigating the original (non-PCA corrected) expression data (see Table S11).

Nevertheless our results indicate that natural genetic varation can affect gene expression levels in complex ways. Further analyses using different tissues and specific cell types and using larger sample sizes are required to gain a deeper understanding of the genetic variation of gene expression and to gain better insight into the full complexity of disease.

Materials and Methods

Genotyping and Expression Profiling on Liver, Muscle, and Adipose Fat Tissues from the Same Population

Subjects

From April 2006 to January 2009, 85 morbidly obese Dutch subjects (23 male and 62 female subjects) with a body mass index (BMI) between 35 and 70 were included in the study. They all underwent elective bariatric surgery at the Department of General Surgery, Maastricht University Medical Centre. Patients with acute or chronic inflammatory diseases (e.g., autoimmune diseases), degenerative diseases, reported alcohol consumption (>10 g/day), and/or using anti-inflammatory drugs were excluded. The average age of the subjects was 43.9 with a range of 17 and 67 years. This study was approved by the Medical Ethical Board of Maastricht University Medical Centre, in line with the guidelines of the 1975 Declaration of Helsinki. Informed consent in writing was obtained from each subject personally. The subject information was provided in Table S1.

Genotyping

Venous blood samples were obtained after 8 hours fasting on the morning of surgery. DNA was extracted from this blood using the Chemagic Magnetic Separation Module 1 (Chemagen) integrated with a Multiprobe II Pipeting robot (PerkinElmer). All samples were genotyped using Illumina HumanOmni1-Quad BeadChips that contain 1,140,419 SNPs. Genotyping was performed according to standard protocols from Illumina.

RNA profiling in four tissues

Wedge biopsies of liver, visceral adipose tissue (VAT, omentum majus), subcutaneous adipose tissue (SAT, abdominal), and muscle (musculus rectus abdominis) were taken during surgery. RNA was isolated using the Qiagen Lipid Tissue Mini Kit (Qiagen, Crawley, West Sussex, UK, 74804). Assessment of RNA quality and concentration was done with an Agilent Bioanalyzer (Agilent Technologies, Santa Clara, USA). Starting with 200 ng of RNA, the Ambion Illumina TotalPrep Amplification Kit was used for anti-sense RNA synthesis, amplification, and purification according to the protocol provided by the manufacturer (Ambion, Austin, USA). 750 ng of complementary RNA was hybridized to Illumina HumanHT12 BeadChips and scanned on the Illumina BeadArray Reader. Raw probe intensity data for these samples was extracted using Illumina's BeadStudio Gene expression module v3.2 (No background correction was applied, nor did we remove probes with low expression).

Genotyping and Expression Profiling on Blood

Subjects

The genetical genomics samples for blood were collected from unrelated Dutch individuals in four studies: 324 healthy individuals were collected in the University Medical Centre Utrecht, 414 amyotrophic lateral sclerosis (ALS) patients were collected in the University Medical Centre Utrecht, 49 ulcerative colitis (UC) patients from a part of the inflammatory bowel disease (IBD) cohort of the University Medical Centre Groningen, and 453 patients with chronic obstructive pulmonary disease (COPD) were collected with the NELSON study. All samples were collected after informed consent and approved by local ethical review boards. Individual sample information is provided in Table S1.

Genotyping and imputation

DNA from all samples was hybridized to oligonucleotide arrays from Illumina. 324 healthy individuals and 414 ALS patients were genotyped using the Hap370 platform. The 453 COPD patients and 49 UC patients were genotyped on the 610-Quad platform. Because the subjects with liver, muscle, adipose fat tissues were genotyped using more intensive genotyping platform Illumina HumanOmni1-Quad BeadChips, we further used program IMPUTE v2 to impute the genotypes of SNPs that presented in Omni1-Quad chips but not directly genotyped on Hap370 and 610-Quad platform [39]. The reference panel for imputation was the CEU population from HapMap release 22. The directly genotyped SNPs were coded as 0, 1 or 2, while the imputed SNP dosage values were called at a 0.95 confidence level, ranging between 0 and 2. In this way, we obtained the genotype of the same set of 1,140,419 SNPs for all five tissues under study.

RNA profiling

Anti-sense RNA was synthesized, amplified and purified using the Ambion Illumina TotalPrep Amplification Kit (Ambion, USA) following the manufacturers' protocol. Complementary RNA was hybridized to Illumina HumanHT-12 arrays and scanned on the Illumina BeadArray Reader. Raw probe intensity data for these samples was extracted using Illumina's BeadStudio Gene expression module v3.2 (No background correction was applied, nor did we remove proves with low expression).

Genotyping and Expression Profiling in an Independent Blood Dataset of 229 Samples

Subjects

To ascertain whether our method for identifying tissue-dependent cis-eQTL was robust, we compared the large peripheral blood with an independent blood eQTL dataset that comprised 229 samples. We have described this cohort in previous studies [9], [18]. In brief, this study comprised 111 English celiac disease patients, 59 Dutch amyotrophic lateral sclerosis patients and 59 Dutch health controls. The peripheral blood (2.5 ml) was collected with the PAXgene system (PreAnalytix GmbH, UK).

Genotyping and imputation

The samples were genotyped using the Illumina (Illumina, San Diega, USA) HumanHap300 platform. We further used IMPUTE v2 to impute the genotypes of all HapMap II SNPs. The reference panel for imputation was the CEU population from HapMap release 22. The directly genotyped SNPs were coded as 0, 1 or 2, while the imputed SNP dosage values were called at a 0.95 confidence level, ranging between 0 and 2.

RNA profiling

Anti-sense RNA was synthesized amplified and purified using the Ambion Illumina TltalPrep Amplification Kit (Ambion, USA) following the manufacturers' protocol. Complementary RNA was hybridized to Illumina HumanRef-8 v2 arrays (further referred to as H8v2) and scanned on the Illumina BeadArray Reader.

Normalization and PCA Correction

The raw expression intensities from five tissues were jointly quantile normalized and log2 transformed. We further applied a principal component analysis (PCA) on expression correlation matrix and observed that genes are differentially expressed among different tissue types (Figure S1). We argue that the dominant principal components (PCs) will primarily capture sample differences in expression that reflect physiological or environmental variation (e.g., tissue type and phenotype difference) as well as systematic experimental variation (e.g. batch and technical effect). In order to target the difference in the genetic variation of expression among tissues, we removed the global variation in expression among tissues by using the residual expression for each probe in each tissue after removing 50 PCs (identical to what we have described before [18]). Our previous analysis on the same dataset showed that the number of significantly detected cis-eQTL probes increased two-fold when 50 PCs were removed from the expression data (see Figure S7 in ref [18]). For the independent blood dataset with 229 subjects, we followed the same quantile normalized and PCA correction.

Population Stratification and SNP Quality Control

We tested population stratification between the two cohorts using the program PLINK (http://pngu.mgh.harvard.edu/~purcell/plink/strat.shtml). This program uses complete linkage agglomerative clustering, based on pair-wise identity-by-state (IBS) distances. The fact that all the individuals from both cohorts were clustered together indicates there was no population stratification. We also checked the allelic frequencies between the two cohorts by treating the 85 individuals with four tissue samples as cases and the 1,240 individuals for blood samples as controls. For the imputed SNPs, we used the genotype with highest probability as the discrete genotype for QC purposes. We removed SNPs that showed significant differences in allele frequency at P<0.01. Then the SNPs were quality controlled for minor allelic frequency >5%, a call rate >95% and an exact Hardy-Weinberg (HWE) P value>0.001. To make certain on the directions of the allelic effect on gene expression (up-regulating or down-regulating), we further removed SNPs with two types of transversion alleles (A/T and G/C) and confined our analysis to SNPs with transition alleles (A/G or C/T) and other types of transversion alleles (A/C or G/T). This quality control resulted in 710,035 SNPs for further analysis.

eQTL Discovery

In order to detect cis-eQTLs, analysis was confined to those probe-SNP combinations for which the distance from the probe transcript midpoint to SNP genomic location was ≤1 Mb. For each probe-SNP pair, we used Spearman correlation to detect association between SNPs and the variations of the gene expression in liver, SAT, VAT, muscle and blood, respectively. We calculated the Spearman correlation coefficient and corresponding P values and subsequently transformed this into a Z-score. To maximize the power of eQTL discovery in non-blood tissues, we further performed meta-analysis for four non-blood tissues that combines the association signals across the four non-blood tissues under study. An overall, joint P value was calculated using a weighted (square root of the dataset sample number) Z-method. Please see the ref [40] for a comprehensive overview of this method.

To correct for multiple testing, we controlled the false-discovery rate (FDR) at 0.05: the distribution of observed p-values was used to calculate the FDR, by comparison with the distribution obtained from permuting expression phenotypes relative to genotypes 100 times. At FDR = 0.05 level, the significance P value threshold was 1.37×10−5 for significantly associated probe-SNP pairs in liver, 2.07×10−5 for significant association in SAT, 1.54×10−5 for significant association in VAT, 5.64×10−6 for significant association in muscle, 4.8×10−4 for significant association in blood and 1.10×10−4 for significant association in the meta-analysis of four non-blood tissues. For these significant probe-SNP pairs, we termed the corresponding SNP, probe and genes as expression SNP (eSNP), regulated probe (eProbe) and regulated genes (eGenes), respectively.

Conditional Regression Analysis to Detect Independent eSNPs

Due to the linkage disequilibrium among the tested SNPs, we usually found numerous eSNPs for each eProbe. In order to detect independent eSNPs, we performed conditional regression analysis for the eProbes per tissue type. For each eProbe, we first regressed out the main effect of the top eSNP. We then subjected the residuals to eQTL mapping to detect potential secondary, independent eSNPs. We again controlled the false discovery at 0.05 by running 100, as described before in the method section “eQTL discovery”. If secondary eSNPs were present, we repeated the entire procedure to detect tertiary eSNPs by regressing out both the primary and secondary effect (using appropriate multivariate regression analysis). This procedure was repeated until no significant associations were detected any more.

Sampling Approach to Identify Tissue-Dependent eQTL

Comparing blood and non-blood tissues

For each of the 200,629 probe-SNP pairs that was significantly associated at FDR 0.05 level, we further assessed whether the detected Z-scores differed per tissue. We used the Z-scores in blood as a reference because the blood samples were independent from other tissue samples and the sample size was much larger. To correct for the sample size difference, we, out of the 1,240 blood samples, randomly selected without replacement the same number of samples for the comparison with liver (N = 74), SAT (N = 83), VAT (N = 77) and muscle (N = 62). For a certain probe-SNP pair, we re-calculated the association Z-score in blood for the selected sample size. The sampling procedure was repeated 100 times. We subsequently fitted a generalized extreme value distribution (GEVD) for the Z-scores of 100× sampling procedures in blood. GEVD is a flexible model with three parameters: location (γ), scale (β) and shape (α). GEVD can resemble different distributions with different settings of parameters. For example, when α = 0, it resembles the Gumbel types of distributions (Type I); when α>0, it resembles the Frechet types of distributions (Type II); when α<0, it resembles the Weibull types of distributions (Type III). Therefore, fitting the GEVD can permit us to estimate realistic distribution of the Z-scores of this certain probe-SNP pair in blood (Figure S3). We then assessed the deviation of the Z-score of the same probe-SNP pair in the other four tissues from the estimated GEVD in blood and computed P value for the difference of Z-scores between tissues. We did this analysis in R (version 2.10.1) using the package evd: Functions for extreme value distributions (version 2.2–4). This analysis was done for each of the 200,629 probe-SNP pairs and between blood and each of four non-blood tissues. Considering the possible dependence of the eQTL effect among tissues, the significance was controlled at the conserved Bonferroni-corrected 0.05, corresponding to a P value of 6.23×10−8 (0.05/200,629 probe-SNP pairs/4 tissue comparisons). The probe-SNP pairs with a P≤6.23×10−8 were called “discordant associations”, while probe-SNP pairs with P>6.23×10−8 were called “concordant associations”. The expression profiling in all five tissues used the same platform. Therefore, the discordant association cannot be explained by the hybridization efficiency. Because all of the tested SNPs were directly genotyped in non-blood tissues but most of them were imputed in blood, we further checked whether the discordance was caused by the imputation. We did not observe that imputation accuracy might confound our results: 69.3% of the discordant eSNPs were imputed in blood whereas 68.0% of the concordant eSNPs were imputed in blood (Fisher's exact test P value = 0.60). We also assessed whether there was heterogeneity in effect present when comparing the different subgroups of phenotypes. We did not find evidence this to be the case (see Table S6 in ref [18]).

Comparing two independent blood datasets

To further validate the tissue-dependent effect we had detected, we compared the cis-eQTL effects between the blood dataset HT12 and H8v2, using the same sampling procedure as described above. Because of the difference of expression platform, we could only make comparisons for those probes that were present in both datasets. We only investigated SNPs that showed similar allele frequencies between the two blood datasets (SNPs with allele frequency P<0.01 were excluded from analysis and as the H8v2 dataset contained 111 celiac disease patients that were nearly all HLA-DQ2.2 or HLA-DQ2.5 positive we also excluded the HLA from this analysis). After filtering we could compare 93,656 probe-SNP pairs.

Enrichment for SNP Properties

The minor allele frequency (MAF) and function properties of eSNPs were annotated by the web-based tool SNP Annotation and Proxy Search (SNAP) (www.broadinstitute.rog/mpg/snap) [41], using the CEU population panel from HapMap release 22. We performed Fisher's exact test to compare the enrichment between eSNPs with a tissue-dependent effect on expression across tissues and eSNPs with a static effect.

Cis-eQTL Analysis of Trait-Associated SNPs

To directly assess the effect of trait-associated SNPs on gene expression, we confined our cis-eQTL analysis to 1,954 SNPs (with alleles A/G) that were associated with complex traits at P<5.0×10−8 in the ‘Catalog of Published Genome-wide Associated Studies’ (per 16 September 2011) [20] and assessed the tissue-dependency of eQTL effect across the tissues, following the same analysis and permutation procedures. The cis-eQTL significance threshold P values were set at P = 4.6×10−3 in blood, 2.6×10−4 in liver, 2.5×10−4 in muscle, 1.8×10−4 in VAT and 3.2×10−5 in SAT, and 1.1×10−3 for the meta-analysis of four non-blood tissue. At these levels, a total of 2,990 probe-SNP pairs were significant in at least one eQTL analysis.

Characterizing the Tissue-Dependent Mechanisms of Cis-Regulation

To characterize the tissue-dependent mechanisms of cis-regulation, we reasoned that comparing the association at a single probe-SNP level cannot provide a complete picture of the tissue-dependent genetic determinants of gene expression. To gain further insight into the tissue-dependent cis-regulation, we extended analysis for the eProbes with discordant cis-eQTL that were determined by single probe-SNP comparison and compared their whole association profiles across tissues. The association profile refers to the set of the absolute Z-scores of all N number of the tested SNPs within 1 Mb distance from the middle point of probe under study: i.e., {|Z1|, |Z2|, |Z3|, … |Zn|}. Such a profile can represent the combined association signals of the multiple independent eSNPs and their linkage disequilibrium. Most of the eProbes only showed significant association in blood and were not significantly associated in the smaller non-blood tissues. For those eProbes, we had limited statistical power to determine whether the association in non-blood tissues is truly absent or is not detected due to power issues. Therefore, we confined our comparison of association profiles to the eProbes that were significantly associated in non-blood tissues and compared them to those in blood. To assess the similarity of association profiles across tissues, we computed Pearson correlations coefficient () of the association profiles between two tissues. Because the SNPs were likely in strong linkage equilibrium, there is strong dependency among the Z-scores within the association profile. To determine the empirical threshold for the significance of the correlation between the association profiles and considering the dependency of the SNPs, we performed permutation analysis by randomly assigning genomes to the individuals per tissue type. We thus obtained the association profiles per probe per tissue for the permuted genotypes. These permuted association profiles retained the same correlation structure among SNPs and the Pearson correlation coefficient between the permuted association profiles (r0) would mainly explain the correlation among SNPs. We repeated this permutation 100 times and determined the empirical threshold rthres = 0.21 at FDR 0.05 level using the model (FDR = n0{r0rthres}/n1{rrthres), where r and r0 refer to the Pearson correlation coefficient of real data and permuted data, respectively; n refers to the number of probes where r≥rthres and n0 refers to the average number of probes where r0≥rthres from 100× permutations.

Based on the correlation of association profiles between tissues, we identified four different categories of tissue-dependent genetic regulation of gene expression. If the association profiles for one single probe did not correlate at all between two tissues (r<0.21), we further checked whether the eProbe was significant in both tissues: if the probe had a significant association in one tissue but not in the other, we deemed this “specific cis-regulation”; if instead the eProbe was significant in both tissues, but was associated to different (unlinked) eSNPs in the different tissues, we deemed it “alternative cis-regulation”. For those association profiles where two tissues showed a correlation (r≥0.21), we checked the direction and the effect size of allelic effect on gene expression: if the allelic direction was the same and the effect size was different, we concluded the eProbe belonged to the category “different effect size”; if the allelic direction was instead opposite, the probes had tissue-dependent regulation with an “opposite allelic direction”.

Differential Expression

For the probes with tissue-dependent cis-regulation, we assessed whether they were also differential expressed between the tissues where they showed different cis-regulation. To do so, we relied upon the quantile-normalized expression intensity before any removal of the first 50 principal components. For each discordant eProbe, we used a Wilcoxon Mann-Whitney U test to assess the differential expression between the tissues. We performed the same analysis for a random set of concordant eProbes, equal in size to the set of discordant eProbes. The significance of differential expression was controlled at a Bonferroni-corrected P value 0.05 level.

Accession Numbers

Expression data for both blood tissue and four non-blood dataset have been deposited in GEO with accession numbers GSE20142 (1,240 peripheral blood samples, hybridized to HT12 arrays) and GSE22070 (subcutaneous adipose, visceral adipose, muscle and liver samples). The expression data of the validation blood eQTL dataset (229 samples) has been deposited in GEO with accession number GSE203332.

Supporting Information

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Zdroje

1. CooksonWLiangLAbecasisGMoffattMLathropM 2009 Mapping complex disease traits with global gene expression. Nat Rev Genet 10 184 194

2. NicolaeDLGamazonEZhangWDuanSDolanME 2010 Trait-associated SNPs are more likely to be eQTLs: annotation to enhance discovery from GWAS. PLoS Genet 6 e1000888 doi:10.1371/journal.pgen.1000888

3. MonksSALeonardsonAZhuHCundiffPPietrusiakP 2004 Genetic inheritance of gene expression in human cell lines. Am J Hum Genet 75 1094 1105

4. CheungVGConlinLKWeberTMArcaroMJenK 2003 Natural variation in human gene expression assessed in lymphoblastoid cells. Nat Genet 33 422 425

5. BullaugheyKChavarriaCICoopGGiladY 2009 Expression quantitative trait loci detected in cell lines are often present in primary tissues. Hum Mol Genet 18 4296 4303

6. ZhongHBeaulaurierJLumPYMolonyCYangX 2010 Liver and adipose expression associated SNPs are enriched for association to type 2 diabetes. PLoS Genet 6 e1000932 doi:10.1371/journal.pgen.1000932

7. SchadtEEMolonyCChudinEHaoKYangX 2008 Mapping the genetic architecture of gene expression in human liver. PLoS Biol 6 e107 doi:10.1371/journal.pbio.0060107

8. EmilssonVThorleifssonGZhangBLeonardsonASZinkF 2008 Genetics of gene expression and its effect on disease. Nature 452 423 428

9. HeapGATrynkaGJansenRCBruinenbergMSwertzMA 2009 Complex nature of SNP genotype effects on gene expression in primary human leucocytes. BMC Med Genomics 2 1

10. MyersAJGibbsJRWebsterJARohrerKZhaoA 2007 A survey of genetic human cortical gene expression. Nat Genet 39 1494 1499

11. RichardsALJonesLMoskvinaVKirovGGejmanPV 2011 Schizophrenia susceptibility alleles are enriched for alleles that affect gene expression in adult human brain. Mol Psychiatry doi:10.1038/mp.2011.1

12. DingJGudjonssonJELiangLStuartPELiY 2010 Gene expression in skin and lymphoblastoid cells: Refined statistical method reveals extensive overlap in cis-eQTL signals. Am J Hum Genet 87 779 789

13. NicaACPartsLGlassDNisbetJBarrettA 2011 The architecture of gene regulatory variation across multiple human tissues: the MuTHER study. PLoS Genet 7 e1002003 doi:10.1371/journal.pgen.1002003

14. PriceALHelgasonAThorleifssonGMcCarrollSAKongA 2011 Single-Tissue and Cross-Tissue Heritability of Gene Expression Via Identity-by-Descent in Related or Unrelated Individuals. PLoS Genet 7 e1001317 doi:10.1371/journal.pgen.1001317

15. DimasASDeutschSStrangerBEMontgomerySBBorelC 2009 Common regulatory variation impacts gene expression in a cell type-dependent manner. Science 325 1246 1250

16. GerritsALiYTessonBMBystrykhLVWeersingE 2009 Expression quantitative trait loci are highly sensitive to cellular differentiation state. PLoS Genet 5 e1000692 doi:10.1371/journal.pgen.1000692

17. SuAICookeMPChingKAHakakYWalkerJR 2002 Large-scale analysis of the human and mouse transcriptomes. Proc Natl Acad Sci U S A 99 4465 4470

18. FehrmannRSNJansenRCVeldinkJHWestraHArendsD 2011 Trans-eQTLs reveal that independent genetic variants associated with a complex phenotype converge on intermediate genes, with a major role for the HLA. PLoS Genet 7 e1002197 doi:10.1371/journal.pgen.1002197

19. DuboisPCATrynkaGFrankeLHuntKARomanosJ 2010 Multiple common variants for celiac disease influencing immune gene expression. Nat Genet 42 295 302

20. HindorffLASethupathyPJunkinsHARamosEMMehtaJP 2009 Potential etiologic and functional implications of genome-wide association loci for human diseases and traits. Proc Natl Acad Sci U S A 106 9362 9367

21. SchunkertHKönigIRKathiresanSReillyMPAssimesTL 2011 Large-scale association analysis identifies 13 new susceptibility loci for coronary artery disease. Nat Genet 43 333 338

22. TeslovichTMMusunuruKSmithAVEdmondsonACStylianouIM 2010 Biological, clinical and population relevance of 95 loci for blood lipids. Nature 466 707 713

23. MusunuruKStrongAFrank-KamenetskyMLeeNEAhfeldtT 2010 From noncoding variant to phenotype via SORT1 at the 1p13 cholesterol locus. Nature 466 714 719

24. EstellerMGarcia-FoncillasJAndionEGoodmanSNHidalgoOF 2000 Inactivation of the DNA-repair gene MGMT and the clinical response of gliomas to alkylating agents. N Engl J Med 343 1350 1354

25. MoffattMFKabeschMLiangLDixonALStrachanD 2007 Genetic variants regulating ORMDL3 expression contribute to the risk of childhood asthma. Nature 448 470 473

26. MellsGFFloydJABMorleyKICordellHJFranklinCS 2011 Genome-wide association study identifies 12 new susceptibility loci for primary biliary cirrhosis. Nat Genet 43 329 332

27. AndersonCABoucherGLeesCWFrankeAD'AmatoM 2011 Meta-analysis identifies 29 additional ulcerative colitis risk loci, increasing the number of confirmed associations to 47. Nat Genet 43 246 252

28. BarrettJCClaytonDGConcannonPAkolkarBCooperJD 2009 Genome-wide association study and meta-analysis find that over 40 loci affect risk of type 1 diabetes. Nat Genet 41 703 707

29. BarrettJCHansoulSNicolaeDLChoJHDuerrRH 2008 Genome-wide association defines more than 30 distinct susceptibility loci for Crohn's disease. Nat Genet 40 955 962

30. VerlaanDJBerlivetSHunninghakeGMMadoreALarivièreM 2009 Allele-specific chromatin remodeling in the ZPBP2/GSDMB/ORMDL3 locus associated with the risk of asthma and autoimmune disease. Am J Hum Genet 85 377 393

31. HuZWuCShiYGuoHZhaoX 2011 A genome-wide association study identifies two new lung cancer susceptibility loci at 13q12.12 and 22q12.2 in Han Chinese. Nat Genet 43 792 796

32. GharaviAGKirylukKChoiMLiYHouP 2011 Genome-wide association study identifies susceptibility loci for IgA nephropathy. Nat Genet 43 321 327

33. FrankeAMcGovernDPBBarrettJCWangKRadford-SmithGL 2010 Genome-wide meta-analysis increases to 71 the number of confirmed Crohn's disease susceptibility loci. Nat Genet 42 1118 1125

34. ImielinskiMBaldassanoRNGriffithsARussellRKAnneseV 2009 Common variants at five new loci associated with early-onset inflammatory bowel disease. Nat Genet 41 1335 1340

35. International HapMap Consortium 2005 A haplotype map of the human genome. Nature 437 1299 1320

36. LiangPSongFGhoshSMorienEQinM 2011 Genome-wide survey reveals dynamic widespread tissue-specific changes in DNA methylation during development. BMC Genomics 12 231

37. ListerRPelizzolaMDowenRHHawkinsRDHonG 2009 Human DNA methylomes at base resolution show widespread epigenomic differences. Nature 462 315 322

38. EeckhouteJLupienMMeyerCAVerziMPShivdasaniRA 2009 Cell-type selective chromatin remodeling defines the active subset of FOXA1-bound enhancers. Genome Res 19 372 380

39. HowieBNDonnellyPMarchiniJ 2009 A flexible and accurate genotype imputation method for the next generation of genome-wide association studies. PLoS Genet 5 e1000529 doi:10.1371/journal.pgen.1000529

40. WhitlockMC 2005 Combining probability from independent tests: the weighted Z-method is superior to Fisher's approach. J Evol Biol 18 1368 1373

41. JohnsonADHandsakerREPulitSLNizzariMMO'DonnellCJ 2008 SNAP: a web-based tool for identification and annotation of proxy SNPs using HapMap. Bioinformatics 24 2938 2939

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